WO2010087994A2 - Methods for ligation and uses thereof - Google Patents

Methods for ligation and uses thereof Download PDF

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WO2010087994A2
WO2010087994A2 PCT/US2010/000274 US2010000274W WO2010087994A2 WO 2010087994 A2 WO2010087994 A2 WO 2010087994A2 US 2010000274 W US2010000274 W US 2010000274W WO 2010087994 A2 WO2010087994 A2 WO 2010087994A2
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substituted
unsubstituted
protein
transamidase
acyl
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PCT/US2010/000274
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French (fr)
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WO2010087994A3 (en
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Hidde L. Ploegh
John M. Antos
Maximilian Wei-Lin Popp
Carla Guimaraes
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Whitehead Institute For Biomedical Research
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Priority to US13/145,644 priority Critical patent/US8940501B2/en
Priority to EP10736161.0A priority patent/EP2391714B2/en
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Publication of WO2010087994A3 publication Critical patent/WO2010087994A3/en

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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/14Hydrolases (3)
    • C12N9/48Hydrolases (3) acting on peptide bonds (3.4)
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/14Hydrolases (3)
    • C12N9/78Hydrolases (3) acting on carbon to nitrogen bonds other than peptide bonds (3.5)
    • C12N9/80Hydrolases (3) acting on carbon to nitrogen bonds other than peptide bonds (3.5) acting on amide bonds in linear amides (3.5.1)
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2217/00Genetically modified animals

Definitions

  • the present invention relates to compositions and methods for ligation and uses thereof.
  • the invention provides novel reagents and methods for ligating an acyl donor compound with a nucleophilic acyl acceptor compound to form an amide bond using a transamidase.
  • the invention also relates to novel products, e.g., novel polypeptides, that can be produced using transamidate-mediated ligation.
  • Protein engineering is becoming a widely used tool in many areas of protein biochemistry.
  • One engineering method is controlled protein ligation, and over the past ten years some progress has been made.
  • synthetic-based chemistry allows the joining of synthetic peptides together through native chemical ligation and a 166 amino-acid polymer-modified erythropoiesis protein has been synthesized using this method.
  • native chemical ligation relies on efficient preparation of synthetic peptide esters, which can be technically difficult to prepare for large polypeptides such as proteins.
  • the reaction sometimes is performed in an organic solvent to produce the requisite protein ester for ligation.
  • Other ligation methods not requiring the production of protein esters generate protein thioesters.
  • intein-based protein ligation system was used to generate a protein by thiolysis of a corresponding protein- intein thioester fusion.
  • a prerequisite for this intein- mediated ligation method is that the target protein is expressed as a correctly folded fusion with the intein, and that sufficient spacing between the target and intein is needed to allow formation of the intein-thioester.
  • the intein-fusion proteins can only be obtained from inclusion bodies when expressed in Escherichia coli, which often cannot be refolded. This difficulty significantly limits the application of intein-based protein ligation methods.
  • a tag can be linked to a recombinant protein, and after purification, the tag on the fusion may be cleaved from the target protein by treatment with an exogenously added site-specific protease. Additional chromatographic steps then are required to separate the target protein from the uncleaved fusion, the affinity tag, and the protease.
  • an N-terminal 6x His tag from a recombinant protein may be cleaved by an engineered 6x His-tagged aminoprotease, and a subtractive immobilized metal-ion affinity chromatography (IMAC) step can be used to recover the untagged target.
  • IMAC immobilized metal-ion affinity chromatography
  • Other methods may require two or more chromatography steps and even special treatment of the exogenous protease, such as biotinylation, to facilitate its removal.
  • Target proteins are engineered to contain the sortase A recognition motif (LPXTG) near their C-termini.
  • LPXTG sortase A recognition motif
  • the present invention encompasses the recognition that existing methods of transamidase ligation suffer from competition effects and efficiency issues.
  • the inventors sought to extend the practical applications of sortase-mediated ligation to include ligation/labeling at the polypeptide N-terminus using synthetic peptides containing the LPXTG motif and protein substrates with N-terminal glycine residues.
  • sortase-mediated ligation to include ligation/labeling at the polypeptide N-terminus using synthetic peptides containing the LPXTG motif and protein substrates with N-terminal glycine residues.
  • each successful transfer of an LPXT unit to a target protein releases a stoichiometric amount of a peptide fragment containing an N-terminal glycine.
  • This by-product competes with the protein nucleophile for the same acyl enzyme intermediate, thereby limiting the efficiency of the ligation reaction.
  • the invention provides compositions and methods that facilitate N-terminal ligation using a transamidase, e.g., a sortase.
  • a transamidase e.g., a sortase.
  • the present invention provides methods of ligation utilizing a modified transamidase recognition sequence.
  • a modified transamidase sequence comprises an ester group in place of a C- terminal amino acid residue.
  • the present invention provides a method of ligation comprising the step of contacting an acyl donor compound of formula:
  • a 1 - Transamidase recognition sequence i ⁇ XR 1 wherein the transamidase recognition sequence is any peptide motif recognized by a transamidase enzyme;
  • X is -O-, -NR-, or -S-;
  • R is hydrogen, substituted or unsubstituted aliphatic, or substituted or unsubstituted heteroaliphatic;
  • a 1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label;
  • R 1 is acyl, substituted or unsubstit
  • B 1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; and n is an integer from 0 to 100, inclusive; in the presence of a transamidase enzyme under suitable conditions to form a compound of formula:
  • the recognition sequence is LPXT, wherein X is the amino acid D, E, A, N, Q, K, or R.
  • the present invention provides a ligation method comprising the step of contacting an acyl donor compound of formula:
  • a 1 , X, and R 1 are defined as described above; and R 2 is a natural or unnatural amino acid side chain; with a nucleophilic compound of formula:
  • B , 1 and n are defined as described above; in the presence of a transamidase enzyme under suitable conditions to form a compound of formula:
  • X is -O-.
  • R 1 is Ci -6 aliphatic.
  • R is methyl.
  • R is a natural amino acid side chain.
  • R 2 is the side chain group of arginine.
  • R 2 is the side chain group of glutamic acid.
  • R 2 is the side chain group of lysine.
  • a and B are each selected from the group consisting of an antibody, an antibody chain, an antibody fragment, an antibody epitope, a recombinant protein, a peptide comprising one or more D-amino acids, a branched peptide, a therapeutic protein, an enzyme, a polypeptide subunit of a multisubunit protein, a transmembrane protein, a cell surface protein, a methylated peptide or protein, an acylated peptide or protein, a lipidated peptide or protein, a phosphorylated peptide or protein, and a glycosylated peptide or protein.
  • n is 2. In certain embodiments, n is 4.
  • the transamidase is a sortase.
  • the sortase is sortase A.
  • the sortase is sortase B.
  • Transamidase recognition sequence XR 1 wherein the transamidase recognition sequence, A 1 , X, and R 1 are as defined above and described herein.
  • X is -O- and R 1 is methyl.
  • the present invention provides a compound of formula:
  • a 1 , X, R 1 , and R 2 are as defined above and described herein.
  • the compound is of formula:
  • kits comprising an acyl donor compound as described herein.
  • the kit further comprises a transamidase.
  • the kit further comprises a sortase.
  • the kit provides a nucleophilic acyl acceptor as described herein.
  • One aspect of the instant invention is improved methods for removing sortase from a reaction system in which sortase has been used to perform a transamidation reaction. See Example 1 for exemplary description. It will be appreciated that the methods though described in reference to particular materials, are generalizable to other materials.
  • Other aspects of the invention are methods and compositions related to use of multiple sortases, recognizing different motifs, for multiple labeling of polypeptides and other applications.
  • transamidase recognition sequences and compounds containing them and methods of use thereof e.g., for modifying polypeptides.
  • the invention provides methods and compositions relating to use of transamidase-mediated, e.g., sortase-mediated, transpeptidation for the site-specific attachment of a moiety, e.g., a non-polypeptide polymer, e.g., polyethylene glycol or a derivative thereof, to a protein, e.g., a clinically useful protein, to enhance at least one property of the protein, such as extend the circulating half-life, while maintaining high biological activity, as well as covalently joining the N- and C- termini of the protein, e.g.
  • a moiety e.g., a non-polypeptide polymer, e.g., polyethylene glycol or a derivative thereof
  • a protein e.g., a clinically useful protein
  • inventive methods and compositions combine both of these properties by exploiting two distinct transamidase, e.g., sortase, enzymes and engineering a suitable compound (sometimes referred to herein as a "probe") that allows for site-specific modification (e.g., PEGylation) as well as allowing covalent closure in a second transamidase-mediated reaction.
  • the invention provides a circularized version of a polypeptide, wherein the original C- and N-termini of the polypeptide are joined to each other via a linker peptide, wherein the linker peptide comprises a transamidase recognition sequence.
  • the polypeptide is a four-helix bundle polypeptide, e.g., a four-helix bundle cytokine.
  • the polypeptide is a secreted polypeptide.
  • the polypeptide binds to a cellular receptor.
  • the C-terminus, N-terminus, or both, of the polypeptide are not involved in receptor binding.
  • Figure 1 (a) Optimization of a two-step protocol for lipid ligation followed by removal of the sortase enzyme. Conditions: 77 ⁇ M eGFP-LPETG-His ⁇ , 150 ⁇ M sortase A, 2 mM nucleophile, 1% (w/v) detergent, 50 mM Tris, pH 7.5, 150 mM NaCl, 10 mM CaC12, 3 h at 37 °C. After transpeptidation, Ni-NTA resin was added as a slurry in 1 M NaCl and 40 mM imidazole and incubated for 2 h at room temperature.
  • Figure 3 Association of lipid-modified eGFP with HeLa cells.
  • Cells were incubated with lipid-modified eGFP (2.5 ⁇ g/mL) for 1 h in serum-free medium and then analyzed by flow cytometry. Numbers in parentheses represent the fold enhancement in mean cellular fluorescence relative to that of eGFP-GGG. Histograms for eGFP-GGG (black) and eGFP- 1 -ad (gray) are overlapping.
  • FIG. 4 Subcellular distribution of eGFP-l-C22 and eGFP-2-chol in U373 and HeLa cells.
  • Cells were incubated with lipid-modified eGFP (2.5 ⁇ g/mL) at 37 °C in serum- free medium and then imaged live using spinning disk confocal microscopy. Key: (a) U373 cells, 1 h of incubation, (b) U373 cells, 5 h of incubation, (c) HeLa cells, 1.25 h of incubation, (d) HeLa cells, 5 h of incubation.
  • eGFP-l-C22 is able to access early endosomal compartments as determined by partial colocalization with transferrin- Alexa 647.
  • U373 cells were incubated with eGFP-l-C22 (2.5 ⁇ g/mL) for 5 h in serum-free medium followed by the addition of transferrin- Alexa 647 (100 ⁇ g/mL) during the final 15 min.
  • White arrows indicate vesicles with positive staining for both eGFP-l-C22 and transferrin-Alexa 647.
  • Significant colocalization between eGFP-2-chol and transferrin-Alexa 647 was not observed.
  • Figure 9 (a) Fluorescence gel scan showing robust labeling of CtxB polypeptide containing 3 or 5 glycines, (b) ESI-MS showing labeling of CtxB polypeptide containing 5 glycines.
  • Figure 11 Characterization of lipidated triglycine nucleophiles.
  • Figure 14 (a) Standard curve for estimating the yield of lipid-modified eGFP. (b)
  • Figure 15 Control experiment demonstrating minor increases in cellular fluorescence as a result of incubation with eGFP-GGG in combination with free lipidated triglycine nucleophiles.
  • Figures 19-22 present an overview of biological function of sortase in bacterial cell wall anchoring and examples of C-terminal labeling using sortase.
  • Figure 23 shows a schematic overview of N-terminal labeling using sortase.
  • Figure 24 schematically depicts control of reaction equilibrium using inventive LPXTG mimetics
  • Figure 25 schematically shows transpeptidation reactions involving N and C termini.
  • Figure 26 illustrates cyclization of Cre recombinase.
  • A G-Cre-LPETG-His6 (50 ⁇ m) was incubated with sortase A (50 ⁇ m) in the presence or absence of fluorescent GGG- TMR (10 mm) in sortase reaction buffer (50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12) for 21.5 h at 37 °C.
  • SDS-PAGE revealed the expected C-terminal transpeptidation product when GGG-TMR was included, whereas omission of the triglycine nucleophile resulted in clean conversion to a unique protein species with a lower apparent molecular weight.
  • G-Cre-LPETG-His6 (50 ⁇ m) was circularized by treatment with sortase A (50 ⁇ m) in sortase reaction buffer (50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12) for 21.5 h at 37 °C (lane 1). This reaction mixture was then treated with 10 mm GGG-TMR (lane 3) or simply incubated for an additional 24 h at 37 °C (lane 2). All reactions were analyzed by SDS-PAGE with visualization by Coomassie staining or in-gel fluorescence.
  • sortase reaction buffer 50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12
  • A molecular model of eGFP (generated from PDB code lgfl) (31) showing the proximity relationship between the N and C termini. The N-terminal glycine residue is highlighted in red, and the C-terminal LPET residues are shown in green.
  • B G5-eGFP-LPETG-His6 (50 ⁇ m) was circularized by treatment with sortase A (50 ⁇ m) in sortase reaction buffer (50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12) for 24 h at 37 0 C. Schematic representations to the right of the gel indicate the topology of the protein species produced by transpeptidation.
  • Positions of the N and C termini in the p97 hexamer are suitable for intermolecular cross-linking through sortase-catalyzed transpeptidation.
  • A molecular model of p97 trimer (generated from PDB code 3cfl) (28) showing the relative position of p97 monomers in the hexameric ring. The visible N and C termini from the published p97 trimer structure are indicated in red and green, respectively.
  • B molecular model of G-His6-p97- LPSTG-XX showing the proximity relationship between N and C termini in adjacent p97 monomers. N- and C-terminal residues not visible in the published crystal structure have been modeled onto the existing structure.
  • N-terminal glycine residues are shown in red, and the C- terminal LPST residues are shown in green. For clarity, the C-terminal domains of the outer monomers are hidden, as is the N-terminal domain of the central monomer.
  • C G-His6-p97- LPSTG-XX (1.5 mg/ml) was incubated with sortase A (30 ⁇ m) in sortase reaction buffer (50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12) for the times indicated at 37 °C. After 22 h, diglycine (GG) was added (100 mm final concentration), resulting in disappearance of the covalent oligomers (lane 5). For comparison, a control reaction containing 100 mm diglycine peptide from the outset of the experiment is shown in lane 6.
  • Figure 31 Overview of orthogonal labeling strategies using multiple sortases with distinct recognition motifs (recognition motifs described in Pallen, M. J.; Lam, A. C; Antonio, M.; Dunbar, K. Trends in Microbiology 2001, 9(3), 97-101).
  • Figure 32 N-terminal labeling using SrtA s taph- (a) SrtA st aph catalyzes a transacylation reaction using labeled LPRT methyl esters as substrates.
  • the labeled LPRT fragment is transferred to proteins containing N-terminal glycines in a site-specific fashion, (b) FITC (1) and biotin (2) LPRT methyl esters for N-terminal transacylation. (c) CtxB derivatives (50 ⁇ M) were treated with 500 ⁇ M 1 and 50 ⁇ M SrtA sta ph for 2 h at 37 0 C in 50 mM Tris (pH 7.5), 150 mM NaCl, and 10 mM CaCl 2 . Reactions were analyzed by SDS- PAGE with visualization by coomassie staining and fluorescent gel scanning. [0048] Figure 33. Site-specific N- and C-terminal labeling using multiple sortases.
  • the MTSET reagent used to quench SrtAstrep also modifies the active site cysteine of UCHL3 creating an extra +118 Da signal in the mass spectrum. This modification is easily removed from the final product by brief treatment with DTT.
  • Figure 36 shows a ribbon structure of a representative four helix bundle cytokine (erythropoietin) and its receptor, showing that the N and C termini are located away from the receptor binding domain and in close proximity to each other.
  • Figure 37 shows a scheme for C terminal modification or circularization.
  • Figure 38 shows a nucleotide sequence (SEQ ID NO: 1) encoding an IFN alpha2 variant and corresponding encoded protein (SEQ ID NO: 2). In blue and bold print at the N- terminus of SEQ ID NO: 2 is the initiating methioinine (which gets clipped off when the coding sequence is translated in bacteria), followed by the two glycines used by the transamidase for cyclization.
  • sequences in SEQ ID NO: 1 are shown using the same notation as in SEQ ID NO: 2, i.e., blue and bold print denotes start codon (encoding methionine) followed by codons for two glycines; black (normal text) denotes IFN alpha2 coding sequence; followed by green (underlined) codons encoding two glycines; sequence encoding SrtAstaph recognition sequence is in red italics, foolowed by sequence in blue encoding GSHHHHHH.
  • Figure 39 A shows a Coomassie gel of purified Interferon ⁇ (IFN ⁇ ) variants.
  • the IFN ⁇ variant contain two additional G residues at the C terminus that were introduced during cloning and are not depicted in the legend. Cyclization results in removal of GGHis ⁇ so that the circularized version contains an additional GGLPETGG relative to native IFN ⁇ positioned as follows: -Xaac-GGLPETGG-XaaN-, where Xaac and XaaN represent the C- terminal and N-terminal amino acids, respectively, of native IFN ⁇ .
  • Figure 39B shows MS/MS identification of the junction peptide for the ciruclar interferon alpha.
  • Figure 40 shows results of a Daudi cell proliferation inhibition assay demonstrating that IFN ⁇ variants retain biological activity equivalent to the original protein.
  • IFN ⁇ variants are as shown in Figure 39.
  • standard commercially available IFN ⁇
  • +GG GG-IFN ⁇ -LPETGG-His6
  • circular (see description of Figure 39)
  • delGG IFN ⁇ - LPETGG-His6
  • PEG IFN ⁇ -LPETGGGK-PEG
  • Figure 41 shows serum half life ELISA results for PEGylated vs. linear IFN ⁇ demonstrating that PEGylation significantly prolongs the half-life.
  • the linear IFN ⁇ variant tested in this experiment is the delGG variant (which comprises an LPETGG-His6 moiety at the C-terminus).
  • Figure 42 shows Tm's for a thermal denaturation assay performed on IFN ⁇ variants with lysozyme as a control and shows that the circular variant exhibits significantly enhanced thermal stability relative to the other variants.
  • Figure 43 shows a scheme for scheme for double transpeptidation using two sortases and a probe that contains a masked sortase recognition sequence (masking achieved by using phosphothreonine in the LPXTG motif).
  • Figure 44 shows mass spectrometry results showing sequential transpeptidation using a probe containing a masked sortase recognition sequence.
  • Figure 45 shows a scheme for ligating a first protein or protein domain to a second protein or protein domain using two sortase-mediated reactions.
  • Figure 46 shows a scheme for using transamidase-mediated reaction for detecting cell-cell interactions.
  • Figure 47 shows (A) exemplary C-terminal probe.
  • the transpeptidation reaction results in the ligation of species containing a transamidase recognition sequence with those bearing one or more N-terminal glycine residues.
  • the recognition sequence is an LPXTG motif.
  • a drawback of using such recognition sequences as acyl donors is that the transfer of an LPXT unit to a nucleophilic acyl acceptor releases a stoichiometric amount of a peptide fragment containing an N-terminal glycine. Such by-products compete with the desired acyl acceptor and hinder the progress of the ligation reaction.
  • the present invention provides methods for efficiently linking an acyl donor with a nucleophilic acyl acceptor.
  • the development of these methods is significant as they are widely applicable to many acyl donors and a multitude of different acyl acceptors.
  • the processes are useful for ligating proteins and/or peptides to one another, ligating synthetic peptides to recombinant proteins, linking a reporting molecule to a protein or peptide, joining a nucleic acid to a protein or peptide, conjugating a protein or peptide to a solid support or polymer, and linking a protein or peptide to a label.
  • the ligation products and purified products are useful in diagnostic procedures ⁇ e.g., an antibody that specifically binds to a cancer cell epitope is joined to a radioisotope and the conjugate is administered to a patient to detect the presence or absence of cancer cells).
  • the ligation products and purified products are useful in therapeutic procedures (e.g., an antibody that specifically binds to a cancer cell epitope is joined to a toxin such as ricin A and the conjugate is administered to a patient to selectively treat the cancer).
  • the ligation products and purified products are useful in research methods ⁇ e.g., a NH 2 -CH 2 -derivatized fluorophore and sortase are contacted with fixed cells that express a protein linked to a sortase recognition sequence and the location of the protein is detected by a fluorescence imaging technique).
  • transamidase is an enzyme that can form a peptide linkage ⁇ i.e., amide linkage) between an acyl donor compound and a nucleophilic acyl acceptor containing a NH 2 -CH 2 -moiety.
  • Sortases are enzymes having transamidase activity and have been isolated from Gram- positive bacteria. They have, as part of their cell wall structure, peptidoglycan as well as polysaccharides and/or teichoic acids.
  • Gram- positive bacteria include the following genera: Actinomyces, Bacillus, Bifidobacterium, Cellulomonas, Clostridium, Corynebacterium, Micrococcus, Mycobacterium, Nocardia, Staphylococcus, Streptococcus and Streptomyces.
  • the present invention provides a ligation method comprising the step of contacting an acyl donor compound of formula: O
  • a 1 - Transamidase recognition sequence XR 1 wherein the transamidase recognition sequence is any peptide motif recognized by a transamidase enzyme;
  • X is -O-, -NR-, or -S-;
  • R is hydrogen, substituted or unsubstituted aliphatic, or substituted or unsubstituted heteroaliphatic;
  • a 1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label;
  • R 1 is acyl, substituted or unsubstituted
  • B 1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; and n is an integer from 0 to 100, inclusive; in the presence of a transamidase enzyme under suitable conditions to form a compoundormula:
  • T - XR 1 replaces the C-terminal amino acid of the transamidase recognition sequence.
  • the acyl group is ⁇ ⁇ ⁇ - OR 1 . In some embodiments, the acyl group is
  • the transamidase recognition sequence is LPXT, wherein X is a standard or non-standard amino acid.
  • X is selected from D, E, A, N, Q, K, or R.
  • the recognition sequence is selected from LPXT, LPXT, SPXT, LAXT, LSXT, NPXT, VPXT, IPXT, and YPXR.
  • X is selected to match a naturally occurring transamidase recognition sequence.
  • the transamidase recognition sequence is selected from: LPKT, LPIT, LPDT, SPKT, LAET, LAAT, LAET, LAST, LAET, LPLT, LSRT, LPET, VPDT, IPQT, YPRR, LPMT, LPLT, LAFT, LPQT, NSKT, NPQT, NAKT, and NPQS.
  • the transamidase recognition motif comprises the amino acid sequence X 1 PX 2 X 3 , where X 1 is leucine, isolucine, valine or methionine; X 2 is any amino acid; X 3 is threonine, serine or alanine; P is proline and G is glycine.
  • X 1 is leucine and X 3 is threonine.
  • X 2 is aspartate, glutamate, alanine, glutamine, lysine or methionine.
  • the recognition sequence often comprises the amino acid sequence NPX 1 TX 2 , where X 1 is glutamine or lysine; X 2 is asparagine or glycine; N is asparagine; P is proline and T is threonine.
  • the invention encompasses the recognition that selection of X may be based at least in part in order to confer desired properties on the compound containing the recognition motif.
  • X is selected to modify a property of the compound that contains the recognition motif, such as to increase or decrease solubility in a particular solvent.
  • X is selected to be compatible with reaction conditions to be used in synthesizing a compound comprising the recognition motif, e.g., to be unreactive towards reactants used in the synthesis.
  • X is -O-. In some embodiments, X is -NR-. In some embodiments, X is -NH-. In some embodiments, X is -S-.
  • R 1 is substituted aliphatic. In certain embodiments, R 1 is unsubstituted aliphatic. In some embodiments, R 1 is substituted CM 2 aliphatic. In some embodiments, R 1 is unsubstituted C M2 aliphatic. In some embodiments, R 1 is substituted Ci- 6 aliphatic. In some embodiments, R 1 is unsubstituted Ci -6 aliphatic. In some embodiments, R 1 is Ci -3 aliphatic.
  • R 1 is butyl. In some embodiments, R 1 is /?-butyl. In some embodiments, R 1 is isobutyl. In some embodiments, R 1 is propyl. In some embodiments, R 1 is w-propyl. In some embodiments, R 1 is isopropyl. In some embodiments, R 1 is ethyl. In some embodiments, R 1 is methyl.
  • R 1 is substituted aryl. In certain embodiments, R 1 is unsubstituted aryl. In certain embodiments, R 1 is substituted phenyl. In certain embodiments, R 1 is unsubstituted phenyl.
  • a 1 comprises a protein. In some embodiments, A 1 comprises a peptide.
  • a 1 comprises an element selected from the group consisting of an antibody, an antibody chain, an antibody fragment, an antibody epitope, a recombinant protein, a peptide comprising one or more D-amino acids, a branched peptide, a therapeutic protein, an enzyme, a polypeptide subunit of a multisubunit protein, a transmembrane protein, a cell surface protein, a methylated peptide or protein, an acylated peptide or protein, a lipidated peptide or protein, a phosphorylated peptide or protein, and a glycosylated peptide or protein.
  • a 1 is an amino acid.
  • a 1 comprises a protein.
  • a 1 comprises a peptide.
  • a 1 comprises an antibody.
  • a 1 comprises an antibody fragment.
  • A comprises an antibody epitope.
  • a 1 comprises green fluorescent protein.
  • a 1 comprises a lipid. In some embodiments, A 1 comprises a saturated hydrocarbon. In some embodiments, A 1 comprises a partially unsaturated hydrocarbon. In some embodiments, A 1 comprises a Ci -40 hydrocarbon chain. In some embodiments, A 1 comprises a Ci -30 hydrocarbon chain. In some embodiments, A 1 comprises a Ci -2O hydrocarbon chain. In some embodiments, A 1 comprises a Ci 2-40 hydrocarbon chain. [0076] In some embodiments, A 1 comprises a substituted or unsubstituted Ci -20 aliphatic group. In some embodiments, A 1 comprises an adamantyl group.
  • a 1 comprises a small molecule. In certain embodiments, A 1 comprises a bioactive small molecule. In certain embodiments, A 1 comprises a FDA- approved drug. In certain embodiments, A 1 comprises a cytotoxic agent. In certain embodiments, A 1 comprises a steroid. In certain embodiments, A 1 comprises a steroid analog.
  • a 1 comprises a label. In some embodiments, A 1 comprises a fluorescent label. In certain embodiments, A 1 comprises a radiolabel. In certain embodiments, A 1 comprises a chemiluminescent label. In certain embodiments, A 1 comprises a phosphorescent label.
  • a 1 comprises biotin. In certain embodiments, A 1 comprises streptavidin. In certain embodiments, A 1 comprises fluorescein.
  • a 1 and B 1 groups of the present invention are interchangable. That is, a given group A 1 on an acyl donor could also be used as a group B 1 on a nucleophilic acyl acceptor, and vice versa. Thus, all embodiments and variants of A 1 as described herein are also contemplated as B 1 groups.
  • n is an integer from 0 to 50, inclusive. In certain embodiments, n is an integer from 0 to 20, inclusive. In certain embodiments, n is 0. In certain embodiments, n is 1. In certain embodiments, n is 2. In certain embodiments, n is 3.
  • n is 4. In certain embodiments, n is 5. In certain embodiments, n is
  • the present invention provides a ligation method comprising the step of contacting an acyl donor compound of formula:
  • each of A 1 , X, R, and R 1 is as defined above; and R 2 is a natural or unnatural amino acid side chain; with a nucleophilic compound of formula:
  • R 2 is a natural amino acid side chain.
  • R 2 is the side chain group of aspartic acid, glutamic acid, alanine, asparagine, glutamine, lysine, or arginine.
  • R 2 is the side chain group of arginine.
  • R 2 is the side chain group of glutamic acid.
  • R 2 is the side chain group of lysine.
  • R 2 is the side chain group of aspartic acid.
  • R 2 is the side chain group of alanine.
  • R 2 is the side chain group of asparagine.
  • R 2 is the side chain group of glutamine.
  • R 2 is an unnatural amino acid side chain.
  • the acyl donor compound is of formula:
  • the acyl donor compound is of formula:
  • the acyl donor compound is of formula:
  • the acyl donor compound is selected from:
  • the transamidase is a sortase.
  • Enzymes identified as "sortases” from Gram-positive bacteria cleave and translocate proteins to proteoglycan moieties in intact cell walls.
  • sortases that have been isolated from Staphylococcus aureus, are sortase A (Sit A) and sortase B (Srt B).
  • a transamidase used in accordance with the present invention is a sortase A, e.g., from S. aureus.
  • a transamidase is a sortase B, e.g., from S. aureus.
  • Sortases have been classified into 4 classes, designated A , B, C, and D, based on sequence alignment and phylogenetic analysis of 61 sortases from Gram positive bacterial genomes (Dramsi S, Trieu-Cuot P, Bierne H, Sorting sortases: a nomenclature proposal for the various sortases of Gram-positive bacteria. Res Microbiol.156(3):289-97, 2005. These classes correspond to the following subfamilies, into which sortases have also been classified by Comfort and Clubb (Comfort D, Clubb RT. A comparative genome analysis identifies distinct sorting pathways in gram-positive bacteria.
  • sortase A is used herein to refer to a class A sortase, usually named SrtA in any particular bacterial species, e.g., SrtA from S. aureus.
  • sortase B is used herein to refer to a class B sortase, usually named SrtB in any particular bacterial species, e.g., SrtB from S. aureus.
  • the invention encompasses embodiments relating to a sortase A from any bacterial species or strain.
  • the invention encompasses embodiments relating to a sortase B from any bacterial species or strain.
  • the invention encompasses embodiments relating to a class C sortase from any bacterial species or strain.
  • the invention encompasses embodiments relating to a class D sortase from any bacterial species or strain.
  • Amino acid sequences of Srt A and Srt B and the nucleotide sequences that encode them are disclosed in a number of references cited herein and which are incorporated herein by reference.
  • the amino acid sequences of S. aureus SrtA and SrtB are homologous, sharing, for example, 22% sequence identity and 37% sequence similarity.
  • the amino acid sequence of a sortase-transamidase from Staphylococcus aureus also has substantial homology with sequences of enzymes from other Gram-positive bacteria, and such transamidases can be utilized in the ligation processes described herein.
  • a transamidase bearing 18% or more sequence identity, 20% or more sequence identity, or 30% or more sequence identity with the S. pyogenes, A. naeslundii, S. mutans, E. faecalis or B. subtilis open reading frame encoding a sortase can be screened, and enzymes having transamidase activity comparable to Srt A or Srt B from S. aureas can be utilized (e. g. , comparable activity sometimes is 10% of Srt A or Srt B activity or more).
  • the sortase is a sortase A (SrtA).
  • SrtA recognizes the motif LPXTG, with common recognition motifs being, e.g., LPKTG, LPATG, LPNTG.
  • LPETG is used.
  • motifs falling outside this concensus may also be recognized.
  • the motif comprises an 'A' rather than a 'T' at position 4, e.g., LPXAG, e.g., LPNAG.
  • the motif comprises an 'A' rather than a 'G' at position 5, e.g., LPXTA, e.g., LPNTA.
  • the motif comprises a 'G' rather than 'P' at position 2, e.g., LGXTG, e.g., LGATG.
  • the motif comprises an T rather than 'L' at position 1, e.g., IPXTG, e.g., IPNTG or IPETG.
  • the sortase is a sortase B (SrtB), e.g., a sortase B of S. aureus, B. anthracis, or L. monocytogenes.
  • Motifs recognized by sortases of the B class (SrtB) often fall within the consensus sequences NPXTX, e.g., NP[Q/K]-[T/s]- [N/G/s], such as NPQTN or NPKTG.
  • anthracis cleaves the NPQTN or NPKTG motif of IsdC in the respective bacteria (see, e.g., Marraffini, L. and Schneewind, O., Journal of Bacteriology, 189(17), p. 6425-6436, 2007).
  • Other recognition motifs found in putative substrates of class B sortases are NSKTA, NPQTG, NAKTN, and NPQSS.
  • SrtB from L. monocytogenes recognizes certain motifs lacking P at position 2 and/or lacking Q or K at position 3, such as NAKTN and NPQSS (Mariscotti JF, Garcia-Del Portillo F, Pucciarelli MG.
  • the listeria monocytogenes sortase-B recognizes varied amino acids at position two of the sorting motif. J Biol Chem. 2009 Jan 7. [Epub ahead of print])
  • the sortase is a class C sortase.
  • Class C sortases may utilize LPXTG as a recognition motif.
  • the sortase is a class D sortase.
  • Sortases in this class are predicted to recognize motifs with a consensus sequence NA-[E/A/S/H]-TG (Comfort D, supra).
  • Class D sortases have been found, e.g., in Streptomyces spp., Corynebacterium spp., Tropheryma whipplei, Thermobifida fusca, and Bifidobacterium longhum.
  • LPXTA or LAXTG may serve as a recognition sequence for class D sortases, e.g., of subfamilies 4 and 5, respectively subfamily-4 and subfamily-5 enzymes process the motifs LPXTA and LAXTG, respectively).
  • B. anthracis Sortase C which is a class D sortase, has been shown to specifically cleave the LPNTA motif in B. anthracis Basl and BasH (Marrafini, supra).
  • the invention contemplates use of sortases found in any gram positive organism, such as those mentioned herein and/or in the references (including databases) cited herein.
  • the invention also contemplates use of sortases found in gram negative bacteria, e.g., Colwellia psychrerythraea, Microbulbifer degradans, Bradyrhizobium japonicum, Shewanella oneidensis, and Shewanella putrefaciens. They recognize sequence motifs LP[Q/K]T[A/S]T.
  • a sequence motif LPXT[A/S], e.g., LPXTA or LPSTS may be used.
  • the invention contemplates use of sortase recognition motifs from any of the experimentally verified or putative sortase substrates listed at http://bamics3.cmbi.kun.nl/jos/sortase substrates/help.html, the contents of which are incorporated herein by reference, and/or in any of the above-mentioned references.
  • the sortase recognition motif is selected from: LPKTG, LPITG, LPDTA, SPKTG, LAETG, LAATG, LAHTG, LASTG, LAETG, LPLTG, LSRTG, LPETG, VPDTG, IPQTG, YPRRG, LPMTG, LPLTG, LAFTG, LPQTS, it being understood that in various embodiments of the invention the 5 residue is replaced, as described elsewhere herein.
  • the sequence used may be LPXT, LAXT, LPXA, LGXT, IPXT, NPXT, NPQS, LPST, NSKT, NPQT, NAKT, LPIT, LAET, or NPQS.
  • the invention comprises embodiments in which 'X' in any sortase recognition motif disclosed herein or known in the art is any standard or non-standard amino acid. Each variation is disclosed.
  • X is selected from the 20 standard amino acids found most commonly in proteins found in living organisms.
  • X is D, E, A, N, Q, K, or R.
  • X in a particular recognition motif is selected from those amino acids that occur naturally at position 3 in a naturally occurring sortase substrate.
  • X is selected from K, E, N, Q, A in an LPXTG or LPXT motif where the sortase is a sortase A.
  • X is selected from K, S, E, L, A, N in an LPXTG or LPXT motif and a class C sortase is used.
  • a recognition sequence further comprises one or more additional amino acids, e.g., at the N or C terminus.
  • additional amino acids e.g., at the N or C terminus.
  • amino acids e.g., up to 5 amino acids
  • Such additional amino acids may provide context that improves the recognition of the recognition motif.
  • transamidase recognition sequence may refer to a masked or unmasked transamidase recognition sequence.
  • a unmasked transamidase recognition sequence can be recognized by a transamidase.
  • An unmasked transamidase recognition sequence may have been previously masked, e.g., as described herein.
  • a "masked transamidase recognition sequence” is a sequence that is not recognized by a transamidase but that can be readily modified (“unmasked”) such that the resulting sequence is recognized by a transamidase.
  • At least one amino acid of a masked transamidase recognition sequence has a side chain that comprises a moiety that inhibits, e.g., substantially prevents, recognition of the sequence by a transamidase of interest, wherein removal of the moiety allows the transamidase to recognize the sequence.
  • Masking may, for example, reduce recognition by at least 80%, 90%, 95%, or more (e.g., to undetectable levels) in certain embodiments.
  • a threonine residue in a transamidase recognition sequence such as LPXTG is phosphorylated, thereby rendering it refractory to recognition and cleavage by SrtA.
  • the masked recognition sequence can be unmasked by treatment with a phosphatase, thus allowing it to be used in a SrtA-catalyzed transamidation reaction.
  • the invention provides novel masked transamidase recognition sequences, and compounds comprising them.
  • the transamidase recognition sequence comprises the formula:
  • R 2 is the side chain of any natural or unnatural amino acid, optionally modified or substituted.
  • R B is hydrogen; phosphate; sulfate; an oxygen-protecting group; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl; or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • the transamidase recognition sequence comprises the formula: [00104] .In certain embodiments, the transamidase recognition sequence is of the formula:
  • R 2 is the side chain of any natural or unnatural amino acid, optionally modified or substituted.
  • R B is hydrogen; phosphate; sulfate; an oxygen-protecting group; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • the transamidase recognition sequence is of the formula:
  • R ,2 is the side chain of any natural or unnatural amino acid, optionally modified or substituted; and R B is hydrogen; phosphate; sulfate; an oxygen-protecting group; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 2 is the side chain of a natural amino acid. In certain embodiments, R 2 is the side chain group of aspartic acid, glutamic acid, alanine, asparagine, glutamine, lysine, or arginine. In certain embodiments, R 2 is the side chain group of arginine. In certain embodiments, R 2 is the side chain group of glutamic acid. In certain embodiments, R 2 is the side chain group of lysine. In certain embodiments, R 2 is the side chain group of aspartic acid. In certain embodiments, R is the side chain group of alanine. In certain embodiments, R 2 is the side chain group of asparagine. In certain embodiments, R 2 is the side chain group of glutamine.
  • the side chain of aspartic acid, glutamic acid, alanine, asparagine, glutamine, lysine, arginine, or other amino acid of R 2 is modified so as to mask the recognition sequence of the transamidase.
  • a lysine side chain may be acylated or the terminal amino group may be protected with a nitrogen- protecting group.
  • An aspartic acid or glutamic acid may be esterified or amidated.
  • a threonine, serine, or asparagine may be glycosylated.
  • a threonine, serine, or tyrosine may be phosphorylated or sulfated.
  • An amino acid side chain may also be modified using a photocleavable moiety such as o-nitrobenzyl or dimethoxynitrobenzyl or derivatives thereof.
  • a chemical cleavage method is employed.
  • periodate cleavage can be used to cleave a vicinal diol. See, e.g,. Rodenko B J, lass I major histocompatibility complexes loaded by a periodate trigger. J. Am Chem Soc.;131(34):12305-13, 2009.
  • a masked transamidase recognition sequence may be unmasked by a chemical or biological process that does not adversely affect other moieties of the protein or the protein itself.
  • a phosphatase is used to remove a phosphate group masking a recognition sequence.
  • a sulfatase is used to remove a sulfate group.
  • an esterase or amidase is used to remove an acyl group.
  • a glycosidase e.g., an N-glycosidase, is used to remove a carbohydrate moiety.
  • a photocleavable moiety is removed by exposing the protein or peptide to light.
  • mild alkaline hydrolysis is used to remove a masking moiety.
  • a protecting group is removed using reagents and/or conditions typically used to remove the protecting group. See, e.g., Wuts et al, Greene 's Protective Groups in Organic Synthesis (Wiley-Interscience; 4 edition; October 30, 2006).
  • the unmasked transamidase recognition sequence is of the formula:
  • the masked transamidase recognition sequence is of the formula:
  • the unmasked transamidase recognition sequence is of the formula:
  • the masked transamidase recognition sequence is of the formula:
  • the invention provides compounds, sometimes referred to herein as "probes" that comprise a novel masked transamidase recognition sequence and are of use in a transamidase-mediated reaction.
  • the probe further comprises one or more additional amino acids either N- or C-terminal to the masked transamidase recognition sequence.
  • additional amino acid(s) may be modified with, e.g., carbohydrates, lipids, phosphate groups, labels, tags, other polymers (for example, a non-polypeptide polymer such as polyethylene glycol), and acetyl groups.
  • inventive methods comprise N-terminal and/or C-terminal modification of a polypeptide using an inventive probe.
  • both N- and C-termini are modified (dual modification).
  • the invention provides methods of circularizing a polypeptide using an inventive probe.
  • the invention further provides methods of joining two or more polypeptides using an inventive probe, thereby resulting in insertion of a non-genetically encoded peptide element between the two polypeptides.
  • the non-genetically encoded peptide element in some embodiments comprises a modifying moiety, e.g., an acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a particle, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer (e.g,. a polyethylene glycol), a recognition element, a small molecule, a lipid, or a label.
  • a modifying moiety e.g., an acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl
  • the invention provides methods of using inventive transamidase recognition sequences, and probes containing them, for a variety of purposes.
  • a probe comprising a masked transamidase recognition sequence is used for C-terminal labeling, which in some embodiments is followed by unmasking and cyclization (see, e.g., Figure 43 and discussion below).
  • a probe comprising a masked transamidase recognition sequence is used for transamidase-mediated C-terminal labeling, followed by unmasking, followed by a second transamidase-mediated reaction.
  • the second transamidase-mediated reaction may append a second polypeptide at the C-terminus of the oligopeptide probe.
  • the first transamidase-mediated reaction installs a modifying group near the C-terminus, as shown in Figure 33, wherein the modifying group is denoted as "Label".
  • the first and second polypeptides are often each produced by translation of an RNA, e.g., recombinantly produced.
  • the resulting product comprises two polypeptides joined by a non-genetically encoded element.
  • the inventive method uses an oligopeptide with a nucleophilic amino N-terminus to attack the acyl enzyme and form an amide bond between the protein to be labeled and the oligopeptide.
  • the oligopeptide may have any sequence of natural and/or unnatural amino acids and one or more of the amino acids may be modified or labeled in various embodiments.
  • the label may include a fluorescent tag, a phosphorescent tag, biotin, poly (histi dine) tag, or a radioactive label.
  • the oligopeptide may also be modified with carbohydrates, lipids, phosphate groups, labels, tags, other polymers (for example, a non-polypeptide polymer such as polyethylene glycol), and acetyl groups. Any biological or chemical modification of an amino acid or protein may be incorporated into the oligopeptide to be ligated using a transamidase.
  • the oligopeptide includes a second transamidase recognition sequence or a masked transamidase recognition sequence.
  • the oligopeptide is of the formula:
  • j is an integer between 0 and 10, inclusive
  • k is an integer between 0 and 10, inclusive
  • X is -O-, -NR-, or -S-;
  • R is hydrogen; substituted or unsubstituted aliphatic; or substituted or unsubstituted heteroaliphatic;
  • R 1 is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl; each occurrence of R 3 is independently the side chain of a natural or unnatural amino acid; R 4 is the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acycl
  • the oligopeptide is of the formula:
  • transamidase recognition sequence is a sequence recognized by a transamidase; j is an integer between 0 and 10, inclusive; k is an integer between 0 and 10, inclusive; m is an integer between 0 and 10, inclusive; p is 1 or 2;
  • X is -O-, -NR-, or -S-;
  • R is hydrogen; substituted or unsubstituted aliphatic; or substituted or unsubstituted heteroaliphatic; each occurrence of R 1 is independently hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl; each occurrence of R 3 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched
  • R 4 is the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; each occurrence of R is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl;
  • the transamidase recognition sequence is LPXT, wherein X is a natural or unnatural amino acid.
  • X is selected from D, E, A, N, Q, K, or R.
  • the recognition sequence is selected from LPXT, LPXT, SPXT, LAXT, LSXT, NPXT, VPXT, IPXT, and YPXR.
  • X is selected to match a naturally occurring transamidase recognition sequence.
  • the transamidase recognition sequence is selected from: LPKT, LPIT, LPDT, SPKT, LAET, LAAT, LAET, LAST, LAET, LPLT, LSRT, LPET, VPDT, IPQT, YPRR, LPMT, LPLT, LAFT, LPQT, NSKT, NPQT, NAKT, and NPQS.
  • the transamidase recognition motif comprises the amino acid sequence XiPX 2 X 3 , where Xi is leucine, isolucine, valine or methionine; X 2 is any amino acid; X 3 is threonine, serine, or alanine; P is proline; and G is glycine.
  • Xi is leucine
  • X 3 is threonine
  • X 2 is aspartate, glutamate, alanine, glutamine, lysine, or methionine.
  • the recognition sequence often comprises the amino acid sequence NPXiTX 2 , where Xj is glutamine or lysine; X 2 is asparagine or glycine; N is asparagine; P is proline and T is threonine.
  • the recognition sequence comprises the amino acid sequence LPXiTX 2 , where Xi is selected from D, E, A, N, Q, K, or R; X 2 is alanine or glycine; L is leucine; P is proline and T is threonine.
  • Xi is selected from D, E, A, N, Q, K, or R
  • X 2 is alanine or glycine
  • L is leucine
  • P proline
  • T threonine.
  • for recognition sequence of SrtA sta p h is LPXiTA.
  • for recognition sequence of SrtA sta ph is LPX)TG.
  • the invention encompasses the recognition that selection of X may be based at least in part in order to confer desired properties on the compound containing the recognition motif.
  • X is selected to modify a property of the compound that contains the recognition motif, such as to increase or decrease solubility in a particular solvent.
  • X is selected to be compatible with reaction conditions to be used in synthesizing a compound comprising the recognition motif, e.g., to be unreactive towards reactants used in the synthesis.
  • j is 0. In certain embodiments, j is 1. In certain embodiments, j is 2. In certain embodiments, j is 3. In certain embodiments, j is 4. In certain embodiments, j is 5.
  • k is 0. In certain embodiments, k is 1. In certain embodiments, k is 2. In certain embodiments, k is 3. In certain embodiments, k is 4. In certain embodiments, k is 5.
  • m is 0. In certain embodiments, m is 1. In certain embodiments, m is 2. In certain embodiments, m is 3. In certain embodiments, m is 4. In certain embodiments, m is 5.
  • X is -O-. In certain embodiments, X is -NH-.
  • R 1 is substituted hydrogen. In certain embodiments, R 1 is substituted aliphatic. In certain embodiments, R 1 is unsubstituted aliphatic. In some embodiments, R 1 is substituted Ci -12 aliphatic. In some embodiments, R 1 is unsubstituted Ci-
  • R 1 is substituted Ci -6 aliphatic. In some embodiments, R 1 is unsubstituted Ci -6 aliphatic. In some embodiments, R 1 is Ci -3 aliphatic. In certain embodiments, R 1 is Ci -6 alkyl. In some embodiments, R 1 is butyl. In some embodiments, R 1 is H-butyl. In some embodiments, R 1 is isobutyl. In some embodiments, R 1 is propyl. In some embodiments, R 1 is H-propyl. In some embodiments, R 1 is isopropyl. In some embodiments, R 1 is ethyl. In some embodiments, R 1 is methyl. In certain embodiments, R 1 is substituted aryl. In certain embodiments, R 1 is unsubstituted aryl. In certain embodiments,
  • R 1 is substituted phenyl. In certain embodiments, R 1 is unsubstituted phenyl.
  • -XR 1 is -OCH 3 . In certain embodiments, -XR 1 is -OH.
  • -XR 1 is -NH 2 .
  • R 3 is the side chain of a natural amino acid. In certain embodiments, R 3 is hydrogen. In certain embodiments, R 3 is methyl.
  • R 4 is a modified side chain of a natural amino acid.
  • R 4 is a modified side chain of serine, threonine, lysine, aspartate, glutamate, arginine, asparagine, glutamine, or tyrosine.
  • R 4 is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula: wherein R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R D is of the formula: wherein i is an integer between 1 and 100, inclusive.
  • R 5 is the side chain of a natural amino acid. In certain embodiments, R 5 is hydrogen. In certain embodiments, R 5 is methyl.
  • R 6 is the side chain of a natural amino acid. In certain embodiments, R 6 is hydrogen. In certain embodiments, R 6 is methyl.
  • n 0, and -XR 1 is -OCH 3 . In certain embodiments, m is
  • R 6 is methyl, and -XR 1 is -OH.
  • m is 1
  • R 6 is hydrogen
  • -XR 1 is -OH.
  • the oligopeptide for c-terminal labeling is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R D is of the formula:
  • R D is of the formula:
  • R D is of the formula:
  • inventive methods use an oligopeptide with a transamidase recognition sequence that forms an acyl enzyme.
  • the oligopeptide may have any sequence of natural and/or unnatural amino acids and one or more of the amino acids may be modified or labeled in various embodiments.
  • the label may include a fluorescent tag, a phosphorescent tag, biotin, poly(histidine) tag, or a radioactive label.
  • the oligopeptide may also be modified with carbohydrates, lipids, phosphate groups, labels, tags, other polymers (for example, a non- polypeptide polymer such as polyethylene glycol), and acetyl groups.
  • the oligopeptide includes a second transamidase recognition sequence or a masked transamidase recognition sequence.
  • the oligopeptide is of the formula:
  • transamidase recognition sequence is a sequence recognized by a transamidase; j is an integer between 0 and 10, inclusive; k is an integer between 0 and 10, inclusive; m is an integer between 0 and 10, inclusive; p is 1 or 2;
  • X is -O-, -NR-, or -S-;
  • R is hydrogen; substituted or unsubstituted aliphatic; or substituted or unsubstituted heteroaliphatic;
  • R 4 is the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; each occurrence of R 5 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl
  • the transamidase recognition sequence is LPXT, wherein X is a natural or unnatural amino acid.
  • X is selected from D, E, A, N, Q, K, or R.
  • the recognition sequence is selected from LPXT, LPXT, SPXT, LAXT, LSXT, NPXT, VPXT, IPXT, and YPXR.
  • X is selected to match a naturally occurring transamidase recognition sequence.
  • the transamidase recognition sequence is selected from: LPKT, LPIT, LPDT, SPKT, LAET, LAAT, LAET, LAST, LAET, LPLT, LSRT, LPET, VPDT, IPQT, YPRR, LPMT, LPLT, LAFT, LPQT 5 NSKT, NPQT, NAKT, and NPQS.
  • the transamidase recognition motif comprises the amino acid sequence XiPX 2 X 3 , where Xi is leucine, isolucine, valine or methionine; X 2 is any amino acid; X 3 is threonine, serine, or alanine; P is proline; and G is glycine.
  • Xj is leucine, and X 3 is threonine.
  • X 2 is aspartate, glutamate, alanine, glutamine, lysine, or methionine.
  • the recognition sequence often comprises the amino acid sequence NPXiTX 2 , where Xi is glutamine or lysine; X 2 is asparagine or glycine; N is asparagine; P is proline and T is threonine.
  • the recognition sequence comprises the amino acid sequence LPXiTX 2 , where Xi is selected from D, E, A, N, Q, K, or R; X 2 is alanine or glycine; L is leucine; P is proline and T is threonine.
  • a recognition sequence for SrtA strep is LPXiTG.
  • a recognition sequence for SrtA strep is LPXi TA.
  • a recognition sequence for SrtA stre p is LPETA or LPETG.
  • the recognition sequence comprises the amino acid sequence LPX]TG, where Xi is selected from D, E, A, N, Q, K, or R; X 2 is glycine; L is leucine; P is proline and T is threonine.
  • a recognition sequence for SrtA sta p h is LPETG.
  • a recognition sequence for SrtA stre p is LPXiTA.
  • the invention encompasses the recognition that selection of X may be based at least in part in order to confer desired properties on the compound containing the recognition motif.
  • X is selected to modify a property of the compound that contains the recognition motif, such as to increase or decrease solubility in a particular solvent.
  • X is selected to be compatible with reaction conditions to be used in synthesizing a compound comprising the recognition motif, e.g., to be unreactive towards reactants used in the synthesis.
  • X, e.g., Xi is selected such that the transamidase recognition sequence is masked.
  • j is 0. In certain embodiments, j is 1. In certain embodiments, j is 2. In certain embodiments, j is 3. In certain embodiments, j is 4. In certain embodiments, j is 5.
  • k is 0. In certain embodiments, k is 1. In certain embodiments, k is 2. In certain embodiments, k is 3. In certain embodiments, k is 4. In certain embodiments, k is 5. [00140] In certain embodiments, m is 0. In certain embodiments, m is 1. In certain embodiments, m is 2. In certain embodiments, m is 3. In certain embodiments, m is 4. In certain embodiments, m is 5.
  • p is 1. In certain embodiments, p is 2.
  • X is -O-. In certain embodiments, X is -NH-.
  • R 1 is hydrogen. In certain embodiments, R 1 is substituted aliphatic. In certain embodiments, R 1 is unsubstituted aliphatic. In some embodiments, R 1 is substituted C M2 aliphatic. In some embodiments, R 1 is unsubstituted Ci- i 2 aliphatic. In some embodiments, R 1 is substituted Cj -6 aliphatic. In some embodiments, R 1 is unsubstituted Ci -6 aliphatic. In some embodiments, R 1 is Ci -3 aliphatic. In certain embodiments, R 1 is Ci -6 alkyl. In some embodiments, R 1 is butyl. In some embodiments, R 1 is M-butyl.
  • R 1 is isobutyl. In some embodiments, R 1 is propyl. In some embodiments, R 1 is n-propyl. In some embodiments, R 1 is isopropyl. In some embodiments, R 1 is ethyl. In some embodiments, R 1 is methyl. In certain embodiments, R 1 is substituted aryl. In certain embodiments, R 1 is unsubstituted aryl. In certain embodiments,
  • R 1 is substituted phenyl. In certain embodiments, R 1 is unsubstituted phenyl.
  • -XR 1 is -OCH 3 . In certain embodiments, -XR 1 is -OH.
  • -XR 1 is -NH 2 .
  • R 3 is the side chain of a natural amino acid. In certain embodiments, R is hydrogen. In certain embodiments, R 3 is methyl.
  • R 4 is a modified side chain of a natural amino acid. In certain embodiments, R 4 is a modified side chain of serine, threonine, lysine, aspartate, glutamate, arginine, asparagine, glutamine, or tyrosine.
  • R 4 is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula: wherein R D is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R 4 is of the formula:
  • R D is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
  • R D is of the formula: wherein i is an integer between 1 and 100, inclusive.
  • R 5 is the side chain of a natural amino acid. In certain embodiments, R 5 is hydrogen. In certain embodiments, R 5 is methyl.
  • R 6 is the side chain of a natural amino acid. In certain embodiments, R 6 is hydrogen. In certain embodiments, R 6 is methyl.
  • n 0, and -XR 1 is -OCH 3 . In certain embodiments, m is
  • R 6 is methyl, and -XR 1 is -OH.
  • m is 1, R 6 is hydrogen, and -XR 1 is -OH.
  • the oligopeptide for c-terminal labeling is of the formula:
  • a probe for use in N-terminal labeling comprises a modified transamidase sequence that comprises an ester group in place of a C-terminal amino acid residue.
  • a probe for use in n-terminal labeling comprises an amino acid residue at the C-terminus, e.g., G, GG, GGG, etc.
  • a nucleophile located at the N-terminus of a polypeptide to be labeled comprises at least 2 G residues, e.g., 2, 3, 4, 5, or more G residues.
  • Transamidase fragments having transamidation activity can be utilized in the methods described herein. Such fragments can be identified by producing transamidase fragments by known recombinant techniques or proteolytic techniques, for example, and determining the rate of protein or peptide ligation.
  • the fragment sometimes consists of about 80% of the full-length transamidase amino acid sequence, and sometimes about 70%, about 60%, about 50%, about 40% or about 30% of the full- length transamidase amino acid sequence such as that of S. aureus Sortase A (GenBank Accession number AAD48437).
  • the fragment lacks an N-terminal portion of the full-length sequence, e.g., the fragment lacks the N-terminal portion extending to the end of the membrane anchor sequence.
  • the fragment comprises the C-terminus of a full-length transamidase amino acid sequence.
  • a catalytic core region from a sortase is utilized, e.g., a region is from about position 60 to about position 206 of SrtA, e.g., S. aureus SrtA, or about from position 82 to about position 249 of SrtAstrep.
  • Transamidases from other organisms also can be utilized in the processes described herein.
  • transamidases often are encoded by nucleotide sequences substantially identical or similar to the nucleotide sequences that encode Srt A and Srt B.
  • a similar or substantially identical nucleotide sequence may include modifications to the native sequence, such as substitutions, deletions, or insertions of one or more nucleotides. Included are nucleotide sequences that sometimes are 55%, 60%, 65%, 70%, 75%, 80%, or 85% or more identical to a native nucleotide sequence, and often are 90% or 95% or more identical to the native nucleotide sequence (each identity percentage can include a 1%, 2%, 3% or 4% variance).
  • One test for determining whether two nucleic acids are substantially identical is to determine the percentage of identical nucleotide sequences shared between the nucleic acids.
  • Calculations of sequence identity can be performed as follows. Sequences are aligned for optimal comparison purposes and gaps can be introduced in one or both of a first and a second nucleic acid sequence for optimal alignment. Also, non-homologous sequences can be disregarded for comparison purposes. The length of a reference sequence aligned for comparison purposes sometimes is 30% or more, 40% or more, 50% or more, often 60% or more, and more often 70%, 80%, 90%, 100% of the length of the reference sequence. The nucleotides at corresponding nucleotide positions then are compared among the two sequences.
  • the percent identity between the two sequences is a function of the number of identical positions shared by the sequences, taking into account the number of gaps, and the length of each gap, introduced for optimal alignment of the two sequences. [00163] Comparison of sequences and determination of percent identity between two sequences can be accomplished using a mathematical algorithm.
  • Percent identity between two nucleotide sequences can be determined using the algorithm of Meyers & Miller, CABIOS 4: 11 17 (1989), which has been incorporated into the ALIGN program (version 2.0), using a PAM 120 weight residue table, a gap length penalty of 12 and a gap penalty of 4. Percent identity between two nucleotide sequences can be determined using the GAP program in the GCG software package (available at www.gcg.com), using a NWSgapdna. CMP matrix and a gap weight of 40, 50, 60, 70, or 80 and a length weight of 1, 2, 3, 4, 5, or 6. A set of parameters often used is a Blossum 62 scoring matrix with a gap open penalty of 12, a gap extend penalty of 4, and a frame shift gap penalty of 5.
  • stringent conditions refers to conditions for hybridization and washing. Stringent conditions are known to those skilled in the art and can be found in Ausubel et al. Current Protocols in Molecular Biology (John Wiley & Sons, Inc., New York, 1999). Aqueous and non-aqueous methods are described in that reference and either can be used.
  • stringent conditions is hybridization in 6X sodium chloride/sodium citrate (SSC) at about 45 0 C, followed by one or more washes in 0.2X SSC, 0.1% SDS at 50°C.
  • Another example of stringent conditions are hybridization in 6X sodium chloride/sodium citrate (SSC) at about 45°C, followed by one or more washes in 0.2X SSC, 0.1% SDS at 55°C.
  • a further example of stringent conditions is hybridization in 6X sodium chloride/sodium citrate (SSC) at about 45°C, followed by one or more washes in 0.2X SSC, 0. 1% SDS at 60 0 C.
  • stringent conditions are hybridization in 6X sodium chloride/sodium citrate (SSC) at about 45°C, followed by one or more washes in 0.2X SSC, 0.1% SDS at 65 0 C.
  • stringency conditions include hybridization in 0. 5M sodium phosphate, 7% SDS at 65°C, followed by one or more washes at 0.2X SSC, 1% SDS at 65°C.
  • a variant sequence can depart from a native amino acid sequence in different manners. Amino acid substitutions may be made on the basis of similarity in polarity, charge, solubility, hydrophobicity, hydrophilicity, helix-forming properties and/or amphipathic properties and the resulting variants are screened for antimicrobial activity.
  • negatively charged amino acids include aspartic acid and glutamic acid; positively charged amino acids include lysine and arginine; and amino acids with uncharged polar head groups having similar hydrophilicity values include leucine, isoleucine, valine, glycine, alanine, asparagine, glutamine, serine, threonine, phenylalanine, and tyrosine.
  • conservative substitutions may be made, according to Table A. Amino acids in the same block in the second column and in the same line in the third column may be substituted for one another other in a conservative substitution. Certain conservative substitutions are substituting an amino acid in one row of the third column corresponding to a block in the second column with an amino acid from another row of the third column within the same block in the second column.
  • homologous substitution may occur, which is a substitution or replacement of like amino acids, such as basic for basic, acidic for acidic, polar for polar amino acids, and hydrophobic for hydrophobic, for example.
  • Non-homologous substitutions can be introduced to a native sequence, such as from one class of residue to another (e. g. , a non-hydrophobic to a hydrophobic amino acid), or substituting a naturally occurring amino acid with an unnatural amino acids or non- classical amino acid replacements.
  • acyl donors utilized in the ligation processes described herein include or are modified with an appropriate sortase recognition motif.
  • One or more appropriate sortase recognition sequences can be added to an acyl donor not having one by known synthetic and recombinant techniques.
  • 2, 3, 4, 5, 6, 7, 8, 9, or 10 or more sortase or transamidase recognition sequences are incorporated in an acyl donor.
  • the acyl donor comprises the amino acid sequence XiPX 2 X 3 G, where Xi is leucine, isolucine, valine or methionine; X 2 is any amino acid; X 3 is threonine, serine or alanine; P is proline and G is glycine.
  • Xi is leucine and X 3 is threonine.
  • X 2 is aspartate, glutamate, alanine, glutamine, lysine or methionine.
  • the G is omitted and replaced with a acyl group as described herein.
  • the acyl group as described herein.
  • O acyl donor comprises the sequence LPXT OR 1 5 wherein X is any amino acid and R 1 is as described herein.
  • the acyl donor comprises the amino acid sequence NPXiTX 2 , where Xi is glutamine or lysine; X 2 is asparagine or glycine; N is asparagine; P is proline and T is threonine.
  • Transamidases utilized in the inventive ligation methods described herein sometimes are isolated and incorporated into a kit. Any convenient method known can be utilized to isolate the sortase or transamidase.
  • the transamidase is produced with a N-terminal or C- terminal amino acid sequence that facilitates purification.
  • the transamidase sometimes is produced with a C-terminal or N-terminal polyhistidine sequence, often six histidines, which have affinity and bind to nickel-derivitized solid supports.
  • a transamidase used in accordance with the present invention further comprises an affinity tag.
  • affinity tags include , e.g., His-tag (His6), FLAG, Streptag, HA tag, Myc tag, maltose binding protein, SNUT tag, NusA, T7, thioredoxin, GST, etc.
  • a kit includes a plasmid having a transamidase-encoding nucleotide sequence that the user uses to produce the sortase or transamidase in a cell culture or cell free translation system, and often, then purifies the sortase or transamidase according to instructions provided with the kit.
  • the transamidase, acyl donor, and nucleophilic acyl acceptor are contacted with one another under suitable conditions to effect ligation of the acyl donor to the acyl acceptor.
  • the term "contacting” refers to placing the components of the process in close proximity to one another and allowing the molecules to collide by diffusion. Contacting these components with one another can be accomplished by adding them to one body of fluid and/or in one reaction vessel, for example.
  • the components in the system may be mixed in a variety of manners, such as by oscillating a vessel, subjecting a vessel to a vortex generating apparatus, repeated mixing with a pipette or pipettes, or by passing fluid containing one assay component over a surface having another assay component immobilized thereon, for example.
  • the components may be added in any order to the system.
  • the ligation may be performed in any convenient vessel (e.g., tubes such as microfuge tubes, flask, dish), microtiter plates (e.g., 96-well or 384-well plates), glass slides, silicon chips, filters, or any solid or semisolid support having surface (optionally coated) having molecules immobilized thereon and optionally oriented in an array (see, e.g., U. S. Patent No. 6,261,776 and Fodor, Nature 364: 555-556 (1993)), and microfluidic devices (see, e.g., U. S. Patent Nos. 6,440,722; 6,429,025; 6,379,974; and 6,316,781).
  • the system can include attendant equipment such as signal detectors, robotic platforms, and pipette dispensers.
  • the reaction mixture often is cell free and often does not include bacterial cell wall components or intact bacterial cell walls.
  • the system includes one or more cells or cell wall components, often non-bacterial cells or non-Gram-positive bacterial cells.
  • one or more components often are expressed by one or more recombinant nucleotide sequences in a cell, which nucleotide sequences are integrated into the cell genome or non-integrated (e.g., in a plasmid). Cells in such systems often are maintained in vivo, sometimes ex vivo, and sometimes in vitro.
  • the reaction mixture is maintained at any convenient temperature at which the ligation reaction can be performed.
  • the ligation is performed at a temperature ranging from about 15 0 C to about 50 0 C.
  • the ligation is performed at a temperature ranging from about 23 0 C to about 37 0 C.
  • the temperature is room temperature (e.g., about 25°C). The temperature can be optimized by repetitively performing the same ligation procedure at different temperatures and determining ligation rates. Any convenient assay volume and component ratio is utilized.
  • a component ratio of 1 : 1000 or greater transamidase enzyme to acyl donor is utilized, or a ratio of 1 : 1000 or greater transamidase enzyme to acyl acceptor is utilized.
  • ratios of enzyme to acyl donor or enzyme to acyl acceptor is about 1 :1, including 1 :2 or greater, 1 :3 or greater, 1 :4 or greater, 1 :5 or greater, 1 :6 or greater, 1 :7 or greater, 1 :8 or greater, and 1 :9 or greater.
  • the acyl donor is present at a concentration ranging from about 10 ⁇ M to about 10 mM. In some embodiments, the acyl donor is present at a concentration ranging from about 100 ⁇ M to about 1 mM. In some embodiments, the acyl donor is present at a concentration ranging from about 100 ⁇ M to about 5 mM. In some embodiments, the acyl donor is present at a concentration ranging from about 200 ⁇ M to about 1 mM. In some embodiments, the acyl donor is present at a concentration ranging from about 200 ⁇ M to about 800 ⁇ M. In some embodiments, the acyl donor is present at a concentration ranging from about 400 ⁇ M to about 600 ⁇ M.
  • the nucleophilic acyl acceptor is present at a concentration ranging from about 1 ⁇ M to about 500 ⁇ M. In certain embodiments, the nucleophilic acyl acceptor is present at a concentration ranging from about 15 ⁇ M to about 150 ⁇ M. In certain embodiments, the nucleophilic acyl acceptor is present at a concentration ranging from about 25 ⁇ M to about 100 ⁇ M. In certain embodiments, the nucleophilic acyl acceptor is present at a concentration ranging from about 40 ⁇ M to about 60 ⁇ M. [00179] In certain embodiments, the transamidase is present at a concentration ranging from about 1 ⁇ M to about 500 ⁇ M.
  • the transamidase is present at a concentration ranging from about 15 ⁇ M to about 150 ⁇ M. In certain embodiments, the transamidase is present at a concentration ranging from about 25 ⁇ M to about 100 ⁇ M. In certain embodiments, the transamidase is present at a concentration ranging from about 40 ⁇ M to about 60 ⁇ M.
  • the ligation method is performed in a reaction mixture comprising an aqueous environment.
  • Water with an appropriate buffer and/or salt content often may be utilized.
  • An alcohol or organic solvent may be included in certain embodiments.
  • the amount of an organic solvent often does not appreciably esterify a protein or peptide in the ligation process (e.g., esterified protein or peptide often increase only by 5% or less upon addition of an alcohol or organic solvent).
  • Alcohol and/or organic solvent contents sometimes are 20% or less, 15% or less, 10% or less or 5% or less, and in embodiments where a greater amount of an alcohol or organic solvent is utilized, 30% or less, 40% or less, 50% or less, 60% or less, 70% or less, or 80% or less alcohol or organic solvent is present.
  • the system includes only an alcohol or an organic solvent, with only limited amounts of water if it is present.
  • suitable ligation conditions comprise a buffer.
  • the buffer solution comprises calcium ions.
  • the buffer solution does not contain substances that precipitate calcium ions.
  • the buffer solution does not include phosphate ions.
  • the buffer solution does not contain chelating agents.
  • suitable ligation conditions comprise pH in the range of 6 to 8.5.
  • suitable ligation conditions comprise pH in the range of 6 to 8.
  • suitable ligation conditions comprise pH in the range of 6 to 7.5.
  • suitable ligation conditions comprise pH in the range of 6.5 to 8.5. In some embodiments, suitable ligation conditions comprise pH in the range of 7 to 8.5. In some embodiments, suitable ligation conditions comprise pH in the range of 7.5 to 8.5. In some embodiments, suitable ligation conditions comprise pH in the range of 7.0 to 8.5. In some embodiments, suitable ligation conditions comprise pH in the range of 7.3 to 7.8. [00183] One or more components for ligation or a ligation product may be immobilized to a solid support. The attachment between an assay component and the solid support may be covalent or non-covalent (e.g., U. S. Patent No. 6,022,688 for non-covalent attachments).
  • the solid support may be one or more surfaces of the system, such as one or more surfaces in each well of a microtiter plate, a surface of a glass slide or silicon wafer, Biacore chip, a surface of a particle, e.g., a bead (e.g., Lam, Nature 354: 82-84 (1991)) that is optionally linked to another solid support, or a channel in a microfluidic device, for example.
  • a bead e.g., Lam, Nature 354: 82-84 (1991)
  • Types of solid supports, linker molecules for covalent and non-covalent attachments to solid supports, and methods for immobilizing nucleic acids and other molecules to solid supports are known (e.g., U. S. Patent Nos.
  • any material may be used, e.g., plastic (e.g., polystyrene), metal, glass, cellulose, gels (e.g., formed at least in part from organic polymers such as PDMS), etc.
  • the solid support is semi-solid and/or gel-like, deformable, flexible, or the like.
  • Any protein or peptide may be utilized as an acyl donor or nucleophilic acyl acceptor in the ligation process described herein.
  • the protein or peptide often is isolated when utilized in a cell-free system.
  • the protein or peptide sometimes is a subregion of a protein, such as in the N-terminus, C-terminus, extracellular region, intracellular region, transmembrane region, active site (e.g., nucleotide binding region or a substrate binding region), a domain (e.g., an SH2 or SH3 domain) or a post-translationally modified region (e.g., phosphorylated, glycosylated or ubiquinated region), for example.
  • active site e.g., nucleotide binding region or a substrate binding region
  • a domain e.g., an SH2 or SH3 domain
  • a post-translationally modified region e.g., phosphorylated, glycosylated or ubiquinated
  • Peptides often are 50 amino acids or fewer in length (e.g., 45, 40, 35, 30, 25, 20, or 15 amino acids or fewer in length) and proteins sometimes are 100 or fewer amino acids in length, or 200, 300, 400, 500, 600, 700, or 900 or fewer amino acids in length.
  • the protein or peptide sometimes includes the modification moiety or a portion thereof (e. g. , the glycosyl group or a portion thereof).
  • the protein is a signal transduction factor, cell proliferation factor, apoptosis factor, angiogenesis factor, or cell interaction factor.
  • cell interaction factors include but are not limited to cadherins (e.g., cadherins E, N, BR, P, R, and M; desmocollins; desmogleins; and protocadherins); connexins; integrins; proteoglycans ; immunoglobulins (e.g., ALCAM, NCAM-I (CD56), CD44, intercellular adhesion molecules (e.g., ICAM-I and ICAM-2), LFA-I, LFA-2, LFA-3, LECAM-I, VLA-4, ELAM and N- ⁇ BR> CAM); selectins (e.g., L-selectin (CD62L), E-selectin (CD62e), and P-selectin (CD62P)) ; agrin; CD34; and a cell surface protein that is cyclically internalized or internalized in response to ligand binding.
  • cadherins e.g., cadher
  • signal transduction factors include but are not limited to protein kinases (e.g., mitogen activated protein (MAP) kinase and protein kinases that directly or indirectly phosphorylate it, Janus kinase (JAKl), cyclin dependent kinases, epidermal growth factor (EGF) receptor, platelet-derived growth factor (PDGF) receptor, fibroblast-derived growth factor receptor (FGF), insulin receptor and insulin-like growth factor (IGF) receptor); protein phosphatases (e.g., PTPlB, PP2A and PP2C); GDP/GTP binding proteins (e.g., Ras, Raf, ARF, Ran and Rho); GTPase activating proteins (GAFs); guanine nucleotide exchange factors (GEFs); proteases (e.g., caspase 3, 8 and 9), ubiquitin ligases (e.g., MDM2, an E3 ubiquitin ligase), acety
  • the protein sometimes is a nucleic acid-associated protein (e.g., histone, transcription factor, activator, repressor, co-regulator, polymerase or origin recognition (ORC) protein), which directly binds to a nucleic acid or binds to another protein bound to a nucleic acid.
  • the protein sometimes is useful as a detectable label, such as a green or blue fluorescent protein.
  • a protein is a therapeutically useful protein. Certain proteins of interest are described further in the section entitled "Polypeptides" below.
  • the acyl donor comprises an antibody or antibody chain (heavy or light chain) or a portion thereof comprising an immunoglobulin domain (e.g., constant domain or variable domain).
  • antibodies are IgG, IgM, IgA, or IgE.
  • the antibody may be of any class, subclass, or isotype in various embodiments of the invention.
  • the antibody is of a class or isotype that is secreted. See, e.g., Murphy, K., et al., Janeway's Immunobiology, Garland Science; 7th edition (November 27, 2007).
  • antibodies are polyclonal or monoclonal, and may be chimeric, humanized or bispecific.
  • polyclonal and monoclonal antibodies that bind specific antigens are commercially available, and methods for generating such antibodies are known.
  • polyclonal antibodies are produced by injecting an isolated antigen into a suitable animal (e.g., a goat or rabbit); collecting blood and/or other tissues from the animal containing antibodies specific for the antigen and purifying the antibody.
  • Methods for generating monoclonal antibodies include injecting an animal with an isolated antigen (e.g., often a mouse or a rat); isolating splenocytes from the animal; fusing the splenocytes with myeloma cells to form hybridomas; isolating the hybridomas and selecting hybridomas that produce monoclonal antibodies which specifically bind the antigen (e.g., Kohler & Milstein, Nature 256: 495 497 (1975) and StGroth & Scheidegger, J Immunol Methods 5: 1 21 (1980)).
  • monoclonal antibodies are anti MDM 2 antibodies, anti-p53 antibodies (pAB421, DO 1, and an antibody that binds phosphoryl-serl5), anti- dsDNA antibodies and anti-BrdU antibodies, described hereafter.
  • variable region of an antibody is formed from six complementarity- determining regions (CDRs) in the heavy and light chain variable regions
  • CDRs complementarity- determining regions
  • one or more CDRs from one antibody can be substituted (e.g., grafted) with a CDR of another antibody to generate chimeric antibodies.
  • humanized antibodies are generated by introducing amino acid substitutions that render the resulting antibody less immunogenic when administered to humans.
  • the acyl donor comprises an antibody fragment, such as a Fab, Fab', F(ab)'2, Dab, Fv or single-chain Fv (ScFv) fragment, and recombinant methods for generating antibody fragments are known (e.g., U. S. Patent Nos. 6,099,842 and 5,990,296 and PCT/GBOO/04317).
  • single-chain antibody fragments are constructed by joining a heavy chain variable region with a light chain variable region by a polypeptide linker (e.g., the linker is attached at the C-terminus or N- terminus of each chain), and such fragments often exhibit specificities and affinities for an antigen similar to the original monoclonal antibodies.
  • Bifunctional antibodies sometimes are constructed by engineering two different binding specificities into a single antibody chain and sometimes are constructed by joining two Fab'regions together, where each Fab'region is from a different antibody (e.g., U.S. Patent No. 6,342,221).
  • Antibody fragments often comprise engineered regions such as CDR-grafted or humanized fragments.
  • the binding partner is an intact immunoglobulin, and in other embodiments the binding partner is a Fab monomer or a Fab dimer.
  • Acyl donors comprising proteins and peptides may chemically synthesized using known techniques (e.g., Creighton, 1983 Proteins. New York, N. Y.: W. H. Freeman and Company; and Hunkapiller et al, (1984) Nature July 12-18; 310 (5973): 105-11).
  • a peptide can be synthesized by a peptide synthesizer.
  • non-classical amino acids or chemical amino acid analogs can be introduced as a substitution or addition into the fragment sequence.
  • Non-classical amino acids include but are not limited to D- isomers of the common amino acids, 2, 4-diaminobutyric acid, a-amino isobutyric acid, 4- aminobutyric acid, Abu, 2-amino butyric acid, g-Abu, e-Ahx, 6-amino hexanoic acid, Aib, 2- amino isobutyric acid, 3 -amino propionic acid, ornithine, norleucine, norvaline, hydroxyproline, sarcosine, citrulline, homocitrulline, cysteic acid, t-butylglycine, t- butylalanine, phenylglycine, cyclohexylalanine, b-alanine, fluoroamino acids, designer amino acids such as b-methyl amino acids, Ca-methyl amino acids, Na-methyl amino acids, and amino acid analogs in general. Each amino acid in the peptide often is L (le
  • Native protein and peptide sequences sometimes are modified. For example, conservative amino acid modifications may be introduced at one or more positions in the amino acid sequences of target polypeptides.
  • a "conservative amino acid substitution” is one in which the amino acid is replaced by another amino acid having a similar structure and/or chemical function. Families of amino acid residues having similar structures and functions are well known.
  • amino acids with basic side chains e.g., lysine, arginine, histidine
  • acidic side chains e.g., aspartic acid, glutamic acid
  • uncharged polar side chains e.g., glycine, asparagine, glutamine, serine, threonine, tyrosine, cysteine
  • nonpolar side chains e.g., alanine, valine, leucine, isoleucine, proline, phenylalanine, methionine, tryptophan
  • beta-branched side chains e.g., threonine, valine, isoleucine
  • aromatic side chains e.g., tyrosine, phenylalanine, tryptophan, histidine
  • Non-essential amino acid is one that can be altered without abolishing or substantially altering the biological function of a target polypeptide, whereas altering an "essential” amino acid abolishes or substantially alters the biological function of a target polypeptide.
  • Amino acids that are conserved among target polypeptides typically are essential amino acids.
  • Proteins or peptides of an acyl donor may exist as chimeric or fusion polypeptides.
  • a "chimeric polypeptide" or “fusion polypeptide” includes a protein or peptide linked to a different polypeptide. The different polypeptide can be fused to the N- terminus or C-terminus of the target polypeptide.
  • Fusion polypeptides can include a moiety having high affinity for a ligand.
  • the fusion polypeptide can be a GST-target fusion polypeptide in which the protein or peptide sequences are fused to the C-terminus of the GST sequences, or a polyhistidine-target fusion polypeptide in which the protein or peptide is fused at the N-or C-terminus to a string of histidine residues (e.g., sometimes three to six histidines).
  • Such fusion polypeptides can facilitate purification of recombinant protein or peptide.
  • Fusion polypeptides are commercially available that already encode a fusion moiety, and a nucleotide sequence encoding the peptide or polypeptide can be cloned into an expression vector such that the fusion moiety is linked in-frame to the target polypeptide.
  • the fusion polypeptide can be a protein or peptide containing a heterologous signal sequence at its N- terminus.
  • expression, secretion, cellular internalization, and cellular localization of a target polypeptide can be increased through use of a heterologous signal sequence.
  • Fusion polypeptides sometimes include all or a part of a serum polypeptide (e.g., an IgG constant region or human serum albumin).
  • Suitable systems for producing polypeptides in prokaryotic and eukaryotic systems are well known in the art and are of use in the invention.
  • One of skill in the art will select an appropriate system (e.g., appropriate cell type and appropriate vector for inserting a nucleic acid encoding the protein).
  • a host cell is transformed to contain a vector that encodes a polypeptide whereby the polypeptide is produced in the cell.
  • a host cell can be prokaryotic or eukaryotic cell, e.g., bacterial, fungal, plant, or animal (e.g., insect or mammalian).
  • Exemplary host cells include bacterial cells (e.g., Gram-negative bacteria such as E. coli or Gram-positive bacteria such as B.
  • subtilis or Lactococcus lactis insect cells
  • insect cells e.g., Sf9
  • mammalian cells e.g., CHO cells, COS cells, SP2/0 and NS/0 myeloma cells, human embryonic kidney (e.g., HEK 293) cells, baby hamster kidney (BHK) cell, human B cells, seed plant cells
  • Ascomycete cells e.g., Neurospora, Aspergillus and yeast cells; e.g., yeast of the genera Saccharomyces, Pichia, Hansenula, Schizosaccharomyces, Kluyveromyces, Yarrowia, and Candida.
  • yeast species include S.
  • a cell type capable of performing such glycosylation can be selected.
  • a suitable signal sequence may be included at the N-terminus.
  • the nucleophilic residue(s), e.g., G or GG, and optional masking residues are located C-terminal to the signal sequence, so that they are located at the N-terminus of the mature, secreted polypeptide.
  • a secretion signal sequence whose cleavage generates an N-terminal nucleophilic residue e.g., an A or G
  • cleavage of the H-2kb secretion sequence generates an N- terminal glycine.
  • the protein sequence of the H-2kb secretion signal sequence is MVPCTLLLLLAAALAPTQTRA-GG (SEQ ID NO: 3). It gets cleaved at the dash to leave the GG at the N-terminus).
  • An exemplary nucleotide sequence encoding this sequence is: atggtaccgt gcacgctgct cctgctgttg g cggccgccc tggctcgac tcagacccgc gcg (SEQ ID NO: 4).
  • a secretion signal sequence is selected such that, when cleaved, it leaves a masked nucleophilic residue near the N-terminus.
  • the acyl donor or acyl acceptor is modified by a process or with a moiety not typically incorporated into a protein during translation.
  • the acyl donor or acyl acceptor comprises one or more moieties selected from an alkyl moiety (e.g., methyl moiety), an alkanoyl moiety (e.g., an acetyl group (e.g., an acetylated histone)), an alkanoic acid or alkanoate moiety (e.g., a fatty acid), a glyceryl moiety (e.g., a lipid), a phosphoryl moiety, a glycosyl moiety (e.g., N-linked or O-linked carbohydrate chains) or an ubiquitin moiety.
  • an alkyl moiety e.g., methyl moiety
  • an alkanoyl moiety e.g., an acetyl group (e.g., an acetylated his
  • any of numerous chemical modifications may be carried out by known techniques, including but not limited to specific chemical cleavage by cyanogen bromide, trypsin, chymotrypsin, papain, V8 protease, NaBH 4 ; acetylation, formylation, oxidation, reduction; metabolic synthesis in the presence of tunicamycin; and the like.
  • the N-terminal and/or C-terminal ends may be processed (e.g., the N-terminal methionine may not be present due to prokaryotic expression of the protein or peptide) and chemical moieties may be attached to the amino acid backbone.
  • Proteins and peptides sometimes are modified with a detectable label, such as an enzymatic, fluorescent, isotopic or affinity label to allow for detection and isolation of the polypeptide.
  • a detectable label such as an enzymatic, fluorescent, isotopic or affinity label to allow for detection and isolation of the polypeptide.
  • a recognition sequence can be removed in a native amino acid sequence by synthesizing it without the recognition sequence or by modifying some and/or all amino acids in the nucleotide sequence encoding the amino acid recognition sequence by known recombinant techniques.
  • the recognition sequence when a recognition sequence and non-native sequence useful for purification are introduced to the native protein or peptide amino acid sequence, the recognition sequence is incorporated closer such that the non-native sequence useful for purification is cleaved from the acyl donor during ligation.
  • the transamidase also is modified with the non-native sequence and the ligated product is purified away from the reactants when contacted with a solid support that binds the non-native sequence.
  • acyl donor is modified with a detectable label or homing sequence for a detectable label
  • sequences often are incorporated closer to the N-terminus than the recognition sequence so they are not cleaved from the protein or peptide in the ligation process.
  • the present invention provides an acyl donor compound of formula:
  • Transamidase recognition sequence XR 1 wherein the transamidase recognition sequence, X, R 1 , and A 1 are as defined above.
  • the present invention provides an acyl donor compound of formula:
  • any acyl donor compound described herein for use in methods of ligation is similarly provided by the present invention.
  • the transamidase catalyzes formation of an amide linkage between a NH 2 -CH 2 -moiety, which is joined to and/or is in the acyl acceptor, and an acyl moiety in the acyl donor.
  • Suitable NH 2 -CH 2 -moieties are known and can be determined by performing the linkage processes described herein in a routine manner. Where an acyl acceptor does not include a suitable NH 2 -CH2-moiety, one or more NF ⁇ -CF ⁇ -moieties are joined to the molecule.
  • NH 2 -CH 2 -moieties utilized in the methods described herein are present as one or more glycine amino acids in attached to a B 1 group.
  • a B 1 group is derivitized with three glycines.
  • the nucleophilic acyl acceptor can be any molecule that leads to a useful ligated conjugate.
  • the nucleophilic acyl acceptor comprises a protein or peptide.
  • the nucleophilic acyl acceptor comprises an antibody epitope, an antibody, a recombinant protein, a synthetic peptide or polypeptide, a peptide comprising one or more D-amino acids, a peptide comprising all D-amino acids, a peptide comprising one or more unnatural or non-classical amino acids (e. g. , ornithine), a peptide mimetic, or a branched peptide.
  • the nucleophilic acyl acceptor comprises a peptide that confers enhanced cell penetrance to the acyl donor (e.g., a greater amount of the acyl donor compound conjugated to the acyl acceptor is translocated across a cell membrane in a certain time frame as compared to the acyl donor not conjugated to the acyl acceptor), which is referred to herein as a "protein transduction domain (PTD)" peptide or "transduction peptide.”
  • PTD protein transduction domain
  • Any PTD can be conjugated to a protein or peptide using the methods described herein.
  • PTD peptides are known, and include amino acid subsequences from HIV-tat (e.g., U. S. Patent No.
  • sequences from a phage display library e.g., U. S. 20030104622
  • sequences rich in amino acids having positively charged side chains e.g., guanidino-, amidino-and amino-containing side chains; e.g., U. S. Patent No. 6,593,292
  • the PTD peptide sometimes is branched.
  • the appended peptides promote cellular uptake and in some cases, cell-type specificity.
  • Organelle-specific PTDs have also been generated, providing a means to target specific subcellular sites. See, e.g., Stewart KM, Horton KL, Kelley SO. Cell-penetrating peptides as delivery vehicles for biology and medicine. Org Biomol Chem.
  • moieties that enhance stability of a second moiety such as a polypeptide, when conjugated thereto.
  • moieties may increase the half-life of a compound in vivo.
  • examples include non-polypeptide polymers such as polyethylene glycol and derivatives thereof.
  • a polymer is biocompatible.
  • a polymer is biodegradable.
  • the nucleophilic acyl acceptor comprises a detectable moiety. Any known and convenient detectable moiety can be utilized.
  • avidin, streptavidin, a fluorescent molecule, or a radioisotope is linked to the acyl donor.
  • biotin or another vitamin, such as thiamine or folate is linked to the acyl donor.
  • detectable moieties include various enzymes, prosthetic groups, fluorescent materials, luminescent materials, bioluminescent materials, and radioisotopes.
  • suitable enzymes include horseradish peroxidase, alkaline phosphatase, p-galactosidase, or acetylcholinesterase;
  • suitable prosthetic group complexes include streptavidin/biotin and avidin/biotin;
  • suitable fluorescent materials include umbelliferone, fluorescein, fluorescein isothiocyanate, rhodamine, dichlorotriazinylamine fluorescein, dansyl chloride or phycoerythrin;
  • an example of a luminescent material includes luminol;
  • examples of bioluminescent materials include luciferase, luciferin, and aequorin, and examples of suitable radioisotopes include 125 1, 131 I, 35 S or 3 H.
  • the radioisotope sometimes is selected based upon its appropriate use in a nuclear medicinal procedure, such as Be-7, Mg-28, Co-57, Zn-65, Cu-67, Ge-68, Sr-82, Rb-83, Tc- 95m, Tc-96, Pd- 103, Cd- 109, and Xe- 127, to name but a few.
  • Conjugates between an acyl donor and a detectable label are useful in diagnostic procedures. Diagnostic procedures include, for example, nuclear medicinal procedures for locating diseased locations of a subject, and procedures for detecting specific components or pathogens in a biological sample from a subject.
  • the conjugates also are useful as research tools. For example, the conjugates are useful in flow cytometry techniques and for detecting a cellular location of a specific protein or peptide in a cell.
  • a NH 2 -CH 2 -derivitized fluorophore and a transamidase are contacted with cells that express a protein linked to a sortase recognition sequence.
  • the transamidase joins the fluorophore to the protein and allows detection of the cell, protein in the cell, or protein on the cell surface.
  • the transamidase is expressed by a nucleotide sequence that encodes it in the cell (e.g., the nucleotide sequence sometimes is in a plasmid), and in other embodiments useful for detecting a protein on a cell surface or in a fixed cell, exogenous transamidase protein, often isolated protein, is contacted with the cell.
  • the location of a protein in a cell sometimes is detected by a fluorescence imaging technique in cells fixed to a solid support.
  • Imaging techniques include, for example, using a standard light microscope or a confocal microscope (e.g., U. S. Patent Nos. 5,283,433 and 5,296,703 (Tsien)).
  • Appropriate light microscopes are commercially available and are useful for probing cells in two dimensions (/. e., the height of a cell often is not resolved), and confocal microscopy is useful for probing cells in three-dimensions.
  • Many microscopy techniques are useful for determining the location of a protein in a cell (e.g., in the nucleus, cytoplasm, plasma cell membrane, nucleolus, mitochondria, vacuoles, endoplasmic reticulum or Golgi apparatus).
  • Some microscopic techniques are useful for determining the location of molecular antigens in groups of cells, tissue samples, and organs. Cellular locations often are visualized by counter-staining for subcellular organelles.
  • cells expressing the protein are subjected to a known flow cytometry procedure, such as flow microfluorimetry (FMF) and fluorescence activated cell sorting (FACS); U. S. Patent Nos. 6,090,919 (Cormack, et al.) ; 6,461,813 (Lorens); and 6,455,263 (Payan)).
  • FMF flow microfluorimetry
  • FACS fluorescence activated cell sorting
  • the nucleophilic acyl acceptor comprises a polymer or a small molecule.
  • Polymers can be useful for enhancing protein or peptide solubility, stability and circulating time, and/or for decreasing immunogenicity when the protein or peptide is administered to a subject.
  • the polymer is a water soluble polymer such as polyethylene glycol, ethylene glycol/propylene glycol copolymers, carboxymethylcellulose, dextran, polyvinyl alcohol and the like, for example.
  • the acyl donor may include one, two, three or more attached polymer moieties after ligation.
  • the polymer may be of any molecular weight, and may be branched or unbranched.
  • the molecular weight often is between about 1 kDa and about 100 kDa (the term "about” indicating that in preparations of polyethylene glycol, some molecules will weigh more, some less, than the stated molecular weight).
  • Other sizes may be used, depending on a desired therapeutic profile ⁇ e.g., the duration of sustained release desired, the effects if any on biological activity, the ease in handling, the degree or lack of antigenicity and other known effects of the polyethylene glycol to a therapeutic protein or analog).
  • Any small molecule derivatized with or having a NH 2 -CH 2 -moiety can be linked to an acyl donor having a transamidase recognition site.
  • the small molecule is known to be bioactive.
  • Such small molecules can be obtained using any of the numerous approaches in combinatorial library methods known in the art, including: biological libraries; peptoid libraries (libraries of molecules having the functionalities of peptides, but with a novel, non-peptide backbone which are resistant to enzymatic degradation but which nevertheless remain bioactive (see, e.g., Zuckermann et al. , J. Med. Chem. 37 : 2678-85 (1994)); spatially addressable parallel solid phase or solution phase libraries; synthetic library methods requiring deconvolution; "one-bead one-compound” library methods; and synthetic library methods using affinity chromatography selection.
  • Biolibrary and peptoid library approaches are typically limited to peptide libraries, while the other approaches are applicable to peptide, non-peptide oligomer or small molecule libraries of compounds (Lam, Anticancer Drug Des. 12: 145, (1997)).
  • Examples of methods for synthesizing molecular libraries are described, for example, in De Witt et al. , Proc. Natl. Acad. Sci. U. S. A. 90: 6909 (1993); Erb et al, Proc. Natl. Acad. Sci. USA 91 : 1 1422 (1994); Zuckermann et al, J. Med. Chem.
  • Small molecules include, but are not limited to, peptides, peptidomimetics (e. g. , peptoids), amino acids, amino acid analogs, polynucleotides, polynucleotide analogs, nucleotides, nucleotide analogs, organic or inorganic compounds (i. e.
  • the small molecule folate, spermine or puromycin is a component of an acyl donor.
  • the small molecule is a modification moiety described above, such as a phosphoryl moiety, ubiquitin moiety or a glycosyl moiety, for example.
  • the acyl acceptor comprises is a nucleic acid, such as a deoxyribonucleic acid, a ribonucleic acid, nucleic acid derivatives, and a modified nucleic acid.
  • the nucleic acid may comprise or consist of DNA nucleotide sequences (e.g., genomic DNA (gDNA) and complementary DNA (cDNA)) or RNA nucleotide sequences (e.g., mRNA, tRNA, and rRNA).
  • the nucleic acid sometimes is about 8 to about 50 nucleotides in length, about 8 to about 35 nucleotides in length, and sometimes from about 10 to about 25 nucleotides in length.
  • Nucleic acids often are 40 or fewer nucleotides in length, and sometimes are 35 or fewer, 30 or fewer, 25 or fewer, 20 or fewer, and 15 or fewer nucleotides in length.
  • Synthetic oligonucleotides can be synthesized using standard methods and equipment, such as by using an ABI3900 High Throughput DNA Synthesizer, which is available from Applied Biosystems (Foster City, CA).
  • a nucleic acid sometimes is an analog or derivative nucleic acid, which can include backbone/linkage modifications (e.g., peptide nucleic acid (PNA) or phosphothioate linkages) and/or nucleobase modifications. Examples of such modifications are set forth in U. S. Patent No. 6,455,308 (Freier et al.) ; in U. S. Patent Nos.
  • backbone/linkage modifications e.g., peptide nucleic acid (PNA) or phosphothioate linkages
  • nucleic acids may be modified by chemical linkages, moieties, or conjugates that enhance activity, cellular distribution, or cellular uptake of nucleic acid, and examples of modifications in modified nucleic acids are in U. S. Patent Nos. 6,455,308 (Freier), 6,455,307 (McKay et al. ), 6,451,602 (Popoff et al.), and 6,451,538 (Cowsert).
  • the acyl acceptor comprises a toxin.
  • any toxin may be selected, and often is selected for high cytotoxic activity.
  • Proteins or peptides ligated to a toxin often are useful as therapeutics.
  • a protein or peptide antibody or receptor that specifically binds to a cancer cell when linked to a toxin such as ricin is useful for treating cancer in subjects.
  • the toxin is selected from the group consisting of abrin, ricin A, pseudomonas exotoxin and diphtheria toxin.
  • the acyl acceptor comprises a solid support.
  • the solid support often is derivitized with multiple NH 2 -CH 2 -moieties, such as triglycine moieties.
  • the solid support may be any described herein.
  • the solid support is a glass slide, a glass bead, an agarose bead, a magnetic bead, a silicon wafer or a resin.
  • a resin such as EAH Sepharose is derivitized with triglycine moieties using a FMOC/EDC derivitization procedure.
  • the solid support is a particle, e.g., a microparticle (e.g. a particle having an average diameter or smallest cross- sectional length greater than about 1 micron) or nanoparticle (average diameter or smallest cross-sectional length equal to or less than about 1 micron), liposome, etc.
  • the acyl acceptor comprises a phage that expresses a NH 2 - CH 2 -moiety on the surface.
  • the phage expresses a protein or peptide comprising one or more N- terminal glycines, sometimes three or five glycines at the N- terminus, and the phage expressing such a protein is contacted with a protein or peptide containing a transamidase recognition motif and a transamidase, thereby producing a phage/protein or phage/peptide conjugate.
  • a protein or peptide expressed at the phage surface comprises the transamidase recognition motif, and the phage is contacted with an acyl acceptor comprising a NH2-CH 2 -moiety and a transamidase, thereby producing a conjugate between the phage and the acyl acceptor.
  • an acyl acceptor comprising a NH2-CH 2 -moiety and a transamidase, thereby producing a conjugate between the phage and the acyl acceptor.
  • Methods also are available for linking the test polypeptide to the N-terminus or the C-terminus of the phage coat protein.
  • the original phage display system was disclosed, for example, in U. S. Patent Nos. 5,096,815 and 5,198,346. This system used the filamentous phage M13, which required that the cloned protein be generated in E. coli and required translocation of the cloned protein across the E. coli inner membrane. Lytic bacteriophage vectors, such as lambda, T4 and T7 are more practical since they are independent of E. coli secretion.
  • a protein or peptide comprising a NH 2 -CH 2 -moiety or a transamidase recognition sequence can be expressed on the surface of any other phage or virus, including but not limited to, murine leukemia virus (MLV), mouse mammary tumor virus (MMTV), Rous sarcoma virus (RSV), Fujinami sarcoma virus (FuSV), Moloney murine leukemia virus (Mo-MLV), FBR murine osteosarcoma virus (FBR MSV), Moloney murine sarcoma virus (Mo-MSV), Abelson murine leukemia virus (A-MLV), Avian myelocytomatosis virus- 29 (MC29), and Avian erythroblastosis virus (AEV), human immunodeficiency virus (HIV), simian immunodefic
  • the acyl donor or acyl acceptor comprises a cleavable moiety, e.g., Ai or B 1 comprises a cleavable moiety.
  • the acyl donor or acyl acceptor comprises a cleavage site for a protease (e.g., a polypeptide sequence that is recognized by a protease and cleaved).
  • a cleavage reagent e.g., a protease, may be used to cleave the product of a transamidation reaction.
  • the cleavable moiety may be positioned at any desired location, e.g., between a sortase recognition sequence and a moiety of interest such as a tag, label, etc.
  • a number of proteases that cleave polypeptides at particular sequences are known in the art. Examples of sequences having peptidase activity are known (e. g., cysteine-type endopeptidases, aspartic-type endopeptidases, elastases, metalloendopeptidases, mitochondrial inner membrane peptidases, serine-type endopeptidases, threonine endopeptidases, thrombin and other proteases involved in the coagulation and/or clotting cascade or other biological cascades.
  • the cleavable moiety is photocleavable.
  • the cleavage site is located at a position 1,2, 3,4, 5,6, 7, 8,9 or 10 amino acids away from an end of the recognition sequence, and sometimes at a position 15 or fewer, 20 or fewer, 50 or fewer or 100 or fewer amino acids away from the an end of the recognition sequence or, in some embodiments, from an N- or C-terminal end of a polypeptide comprising a recognition sequence or that acts as a nuclephile in a method described herein.
  • the acyl donor or acyl acceptor comprises a linker sequence, also referred to as a "spacer".
  • a linker sequence may be, e.g., 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 25 or fewer, 30 or fewer, 40 or fewer, 50 or fewer, 60 or fewer, 70 or fewer, 80 or fewer, 90 or fewer or 100 or fewer amino acids in length.
  • the linker may be positioned at any desired location, e.g., between a sortase recognition sequence and a moiety of interest such as a tag, label, etc.
  • the invention provides kits comprising one or more acyl donor compounds as described above.
  • a kit comprises a compound of formula:
  • kits comprises a compound of formula:
  • a kit comprises a compound comprising a masked transamidase recognition sequence, e.g., any of the inventive probes described herein.
  • the kit further comprises a transamidase.
  • the kit further comprises a sortase.
  • the kit further comprises sortase A, e.g., SrtA sta p h , SrtA stre p, or both.
  • a kit comprises an enzyme or other reagent for unmasking a masked transamidase recognition sequence.
  • the kit further comprises instructions for ligation with a nucleophilic compound.
  • a kit provides a nucleophilic compound of formula:
  • the invention encompasses the recognition that transamidases can be used to circularize polypeptides with high efficiency.
  • the invention provides a method of circularizing a polypeptide comprising contacting the polypeptide with a transamidase, e.g., sortase, wherein the polypeptide comprises one or more nucleophilic residue(s) at its N- terminus and a transamidase recognition sequence (e.g., LPXTG) at or near its C-terminus, under suitable conditions such that circularization occurs.
  • a transamidase e.g., sortase
  • a transamidase recognition sequence e.g., LPXTG
  • the transamidase is S. aureus SrtA
  • the N-terminus can comprise one or more G residues (e.g., 1, 2, 3, 4, 5, etc.)
  • the transamidase recognition sequence can comprise LPXTG.
  • the resulting circular polypeptide comprises a transamidase recognition sequence positioned between the original C- and N- termini of the polypeptide.
  • circularization can proceed with high efficiency, thus making the transamidase-mediated circularization reaction a feasible means of producing circular proteins with yield and purity compatible with the needs of large-scale and/or commercially feasible production.
  • at least 30%, 40%, 50%, 60%, 70%, 80%, 90%, or more of the starting polypeptide is converted to circular form.
  • the invention provides a circular variant of a polypeptide of interest, wherein the original N- and C-terminal amino acids of the polypeptide of interest are joined together via a linker oligopeptide that comprises or consists of a transamidase recognition sequence.
  • the circular polypeptide comprises the sequence Xaac-(Xaa)k-
  • k and m are each independently between 0 and 5 (e.g., 0, 1, or 2), or between 0 and 10. In some embodiments, k+m is between 0 and 5, between 0 and 10, or between 0 and 20.
  • the transamidase recognition sequence is LPXTG, e.g., LPETG.
  • the circular polypeptide comprises Xaac-LPXTG-XaaN; Xaac-LPXTGG-Xaa N ; Xaac-GLPXTGG-Xaa N ; Xaac-GGLPXTGG-Xaa N .
  • X is E.
  • the invention provides means for purifying a circularized polypeptide away from a starting linear polypeptide.
  • the method comprises (i) providing a polypeptide of interest that comprises one or more nucleophilic residue(s) at its N-terminus and a sequence comprising a transamidase recognition sequence (e.g., LPXTG) and a peptide that serves as an affinity tag at or near its C-terminus; and (ii) contacting the polypeptide of interest with a transamidase under conditions suitable for transamidation reaction to occur.
  • the sequence at or near the C-terminus of the polypeptide of interest can comprise His6, e.g., LPXTGG-His6.
  • the transamidase in some embodiments also comprises a tag, which may be the same or different from the tag present in the polypeptide of interest.
  • transamidase-mediated circularization removes a portion of the C-terminal sequence comprising the tag.
  • the reaction mixture can then be contacted with a moiety that binds to the tag(s).
  • the circular polypeptide will not be bound and can be conveniently separated from the starting linear polypeptide and/or transamidase.
  • the reaction mixture can be contacted with a resin that binds to the tag (e.g., by passing the material through a column containing the resin).
  • the circular polypeptide does not bind to the resin, flows through the column, and can thus be easily purified.
  • the invention provides purified preparations of a circularized polypeptide as described above, wherein the circularized polypeptide is at least 50%, 60%, 70%, 80%, 90%, 95%, 96%, 97%, 98%, 99%, or more of the polypeptide material in the preparation by dry weight.
  • the circularized polypeptide is at least 50%, 60%, 70%, 80%, 90%, 95%, 96%, 97%, 98%, 99%, or more of the material in the preparation by dry weight (optionally excluding counterions that may be present).
  • a polypeptide preparation comprises at least 10 mg, at least 100 mg, or at least 1 g of polypeptide by dry weight.
  • a circularized polypeptide of the invention displays at least one enhanced property relative to a non-circular form.
  • the polypeptide displays increased stability, e.g., increased resistance to exoprotease(s), increased thermal stability, increased circulating time in vivo, increased biological half-life, less propensity to aggregate, and/or increased rate of refolding.
  • increased stability e.g., increased resistance to exoprotease(s), increased thermal stability, increased circulating time in vivo, increased biological half-life, less propensity to aggregate, and/or increased rate of refolding.
  • the invention provides methods for modifying a polypeptide at both the N- and C-termini.
  • the inventive methods make use of two transamidases, e.g., sortases, that recognize distinct transamidase recognition sequences.
  • a first transamidase is able to recognize a first TRS but is not able to significantly recognize a second TRS, while the second transamidase is able to recognize the second TRS but is not able to significantly recognize the first TRS.
  • the transamidase reactions can be carried out sequentially (in either order) or simultaneously in various embodiments.
  • the inventive methods make use of two transamidases, e.g., sortases, wherein the first transamidase is able to recognize a first TRS but is not able to recognize a second TRS, and the second transmidase is able to recognize both the first TRS and a second TRS.
  • sortases Streptococcus pyogenes Sortase A (SrtAstrep) will accept di-alanine based nucleophiles. This sortase will efficiently cleave LPXTA between theronine and alanine and install modified alanine-based nucleophiles.
  • SrtAstrep will also recognize and cleave LPXTG motifs, albeit with reduced efficiency. SrtAstaph will not significantly cleave LPXTA motifs or accept alanine based nucleophiles.
  • a polypeptide is contacted with SrtAstrep and an alanine-containing nucleophile comprising the desired modifying moiety.
  • the polypeptide comprises a TRS that can recognized by SrtA strep at or near its C-terminus and one or more amino acids capable of serving as a nucleophile for a SrtAstaph-mediated reaction at or near its N-terminus (e.g., (G)n, where n is between 1 and 10, e.g., between 1 and 5).
  • a SrtAstaph-mediated reaction at or near its N-terminus
  • the nucleophilic amino acid(s) are masked, so that they are not recognized by SrtA stre p .
  • a sequence that can be cleaved by a protease can be positioned so that cleavage exposes the nucleophilic amino acid(s). In the absence of such cleavage, the nucleophilic residue cannot participate in a sortase-mediated reaction.
  • a sequence that contains two amino acids in suitable context for cleavage by a protease is referred to as a "protease recognition site" herein.
  • the protease recognition sequence serves to mask the nucleophilic amino acid. Additional amino acids may be present N-terminal of the protease recognition site.
  • the protease recognition site is a thrombin recognition site.
  • the thrombin recognition site comprises the sequence LVPRG, LVPRGG or LVPRGS, wherein thrombin cleaves between R and G.
  • PreScission Protease a genetically engineered fusion protein consisting of human rhino virus 3 C protease and GST, is used.
  • proteases that cleave between a first amino acid and a second amino acid, wherein the second amino acid can serve as a nucleophile for a transamidase, can be used.
  • One of skill in the art will be able to select an appropriate protease to cleave C- terminal to a nucleophilic amino acid of interest.
  • the protease and/or cleavage conditions can be selected such that minimal or no undesired cleavage within the polypeptide occurs.
  • the cleaving conditions and agent e.g., protease
  • the protease may be removed or the protein isolated from the reaction mixture in which cleavage was performed.
  • the protease can comprise a tag for convenient removal after cleavage.
  • the protease is immobilized, e.g., on a solid or semisolid support, e.g., particles.
  • the polypeptide is contacted with the protease to expose the N-terminal nucleophilic amino acid.
  • the polypeptide is contacted with a second transamidase and an appropriate probe for N-terminal modification.
  • An exemplary strategy for dual-terminus labeling is outlined in Figures 33b and 34.
  • the invention also encompasses use of chemical agents for cleavage to expose a nucleophilic amino acid.
  • Polypeptides comprising a masked nucleophilic amino acid usable by a transamidase and appropriate cleavable masking sequence (often positioned near the N-terminus of the polypeptide) and a transamidase recognition sequence at or near the C-terminus are an aspect of the invention and have a variety of uses.
  • Site-Specific Modification and Circular ization of Polypeptides [00226] The invention provides methods for both circularizing and site-specifically modifying a polypeptide.
  • modification is performed using an oligonucleotide probe comprising a TRS, which in some embodiments is a masked TRS.
  • the TRS comprises a side chain comprising a modifying moiety of interest.
  • Figure 43 shows a schematic diagram of an inventive approach according to this aspect of the invention.
  • a polypeptide is equipped with a nucleophilic residue at or near the N-terminus and a first TRS at or near its C-terminus.
  • the nucleophilic residue may be masked, e.g., with a protease recognition sequence that, when cleaved, exposes a nucleophilic residue.
  • the polypeptide is contacted with a transamidase and an inventive oligonucleotide probe comprising a second TRS (which is masked in some embodiments and/or is different in sequence to the first TRS in some embodiments) and an amino acid having a modifying moiety (e.g., a label) attached thereto.
  • the transamidase appends the oligonucleotide probe at the C-terminus of the polypeptide.
  • the second TRS in the probe
  • the polypeptide is contacted with an agent or condition (phosphatase, light, etc.) that unmasks the TRS.
  • the polypeptide is also contacted with an agent that unmasks it (e.g., a protease).
  • the polypeptide is contacted with a second transamidase, which catalyzes a second transamidase reaction, which circularizes the polypeptide.
  • the sequence of the polypeptide between the original N- and C-terminal amino acids can be unchanged relative to the original sequence.
  • the N- and C-termini of the polypeptide are joined in the circularized version by a short linker peptide that comprises at least one TRS.
  • the linker peptide comprises two TRSs. It should be noted that the probe depicted in Fig. 43 is exemplary.
  • a probe comprises two or more lysine residues (or other residues having a readily modifiable side chain), wherein at least two moieties are attached to the side chains.
  • the probe comprises two or more different modifying moieties, which are optionally attached to different amino acids.
  • a polypeptide circularized using an inventive probe comprises the following sequence: — lpetAAGKGLPETgg — wherein lpet in lower case is from the C-terminus of the polypeptide. The AAGKGLPET is from the probe.
  • a circularized polypeptide comprises the sequence (Xaa)c — TRS1-SP-TRS2 — (Xaa)N , wherein TRSl is a first TRS, TRS2 is a second TRS, SP is a spacer peptide comprising sequences from the probe (e.g.,GKG), and each — represents one or more optionally present amino acid residues.
  • a circularized version of an original (e.g., naturally occurring) polypeptide comprises the sequence (Xaa)clpetAAGKGLPETgg(Xaa)N, wherein (Xaa)c is from the C-terminus of the original polypeptide, and (Xaa) N is from the N-terminus of the original polypeptide.
  • a moiety e.g., a PEG, is attached to the lysine side chain in some embodiments.
  • one or more of the G residues in the probe (and thus the circularized polypeptide) is omitted.
  • the invention provides methods of covalently linking two or more polypeptides using an inventive olignucleotide probe, which in some embodiments comprises a TRS, e.g., a masked TRS.
  • Figure 45 is a schematic diagram showing certain embodiments of the inventive approach.
  • the probe comprises a moiety of interest such as PEG, a detectable label, etc.
  • at least one of the polypeptides comprises a targeting or delivery domain.
  • a delivery domain facilitates delivery of a compound, e.g,. a polypeptide, to a site of interest, e.g., a site in the body.
  • a targeting domain (which can function as a delivery domain in some embodiments) specifically binds to a molecule of interest, such as a receptor.
  • a targeting domain can be an an antibody, antibody chain, antibody fragment, e.g., a single-chain antibody or an antigen-binding portion thereof.
  • one of the polypeptides comprises an Fc domain of an antibody, e.g., an IgGl antibody.
  • an Fc domain is dimeric.
  • an Fc domain can confer one or more desired properties.
  • an Fc domain can prolong the half-life of a polypeptide.
  • An Fc domain can function as a targeting/delivery domain.
  • the neonatal constant region fragment (Fc) receptor (FcRn) which is responsible for IgG transport across the intestinal epithelium in newborn rodents, is expressed in epithelial cells in adult humans and non-human primates, and FcRn-mediated transport is functional in the lung of non-human primates.
  • This transport system can be used to deliver a polypeptide of interest when it is conjugated to the Fc domain of IgGl . See, e.g., Bitonti AJ, et al., "Pulmonary delivery of an erythropoietin Fc fusion protein in non-human primates through an immunoglobulin transport pathway. Proc Natl Acad Sci U S A 101(26):9763-8, 2004.
  • one of the polypeptides comprises albumin, e.g., human serum albumin.
  • a targeting or delivery domain comprises a ligand for a receptor, wherein the receptor is expressed at the surface of a target cell.
  • a moiety comprises a biocompatible polymer, e.g., a polyalkylene glycol, e.g., a polyethylene glycol (PEG), a polypropylene glycol, or a derivative thereof.
  • a biocompatible polymer e.g., a polyalkylene glycol, e.g., a polyethylene glycol (PEG), a polypropylene glycol, or a derivative thereof.
  • PEG polyethylene glycol
  • the invention offers a number of advantages relative to various other available methods for modifying a polypeptide with a polymer, e.g., other PEGyation methods.
  • PEG is discussed herein for exemplary purposes.
  • inventive methods permit installation of a single PEG chain (or a small number of chains, e.g., 2, 3, 4) at a defined location and avoid PEGylation of residues within the native polypeptide sequence, which could reduce activity, e.g., potency.
  • inventive methods provide means to modify a polypeptide at a defined position without introducing a cysteine residue into the polypeptide or appending a cysteine residue thereto.
  • PEG with an average molecular weight of about 5 kD is used.
  • a PEG with an average molecular weight of 10 kD is used.
  • PEG with an average molecular weight of about 15 kD, 20 kD, 25 kD, 3OkD, 40 kD, 45 kD, 5OkD, 55 kD, or more is used.
  • a linear PEG is used.
  • a branched PEG, forked PEG, or comb structure PEG is used.
  • a polypeptide PEGylated using an inventive method displays increased circulating time without causing a significant reduction in potency. In contrast, standard, random PEGylation approaches often result in considerable reduction in potency. See, e.g., Jevsevar, S, et al., PEGylation of Therapeutic Proteins, Biotechnol. J. 5, 113-128, 2010, and references therein, for discussion of certain PEGylated pharmaceuticals, PEG reagents, etc.
  • a polypeptide to be circularized is one whose N- and C- terminus are located within close proximity to each other in the native structure.
  • the termini are located no more than 15 Angstroms (A) apart.
  • the termini are located no more than 20 A apart.
  • the termini are located no more than 25 A apart.
  • the polypeptide is modified to extend either the N- or C-terminus, or both, with a flexible spacer peptide so that the termini can be in closer proximity to each other.
  • a polypeptide to be circularized and, optionally, labeled as described herein is characterized in that its N- and C-termini are positioned such that they are not required for the activity of the polypeptide and/or for interaction of the polypeptide with a biological target of the polypeptide.
  • the polypeptide of interest comprises or consists of a polypeptide that is at least 80%, or at least 90%, e.g., at least 95%, 86%, 97%, 98%, 99%, 99.5%, or 100% identical to a naturally occurring polypeptide.
  • the polypeptide has no more than 1 , 2, 3, 4, 5, 6, 7, 8, 9, or 10 amino acid differences relative to a naturally occurring sequence.
  • the naturally occurring polypeptide is a mammalian polypeptide, e.g., of human origin.
  • the naturally occurring polypeptide is a cytokine, e.g., a type I cytokine.
  • the polypeptide of interest is a four-helix bundle protein, e.g., a four-helix bundle cytokine.
  • Exemplary four-helix bundle cytokines include, e.g., certain interferons (e.g., a type I intereferon, e.g., IFN- ⁇ ), interleukins (e.g., IL-2, IL -3, IL-4, IL-5, IL-6, IL-7, IL-12), and colony stimulating factors (e.g., G-CSF, GM-CSF, M-CSF).
  • the IFN can be, e.g., interferon alpha 2a or interferon alpha 2b. See, e.g., Mott HR and Campbell ID. "Four-helix bundle growth factors and their receptors: protein-protein interactions.” Curr Opin Struct Biol.
  • the cytokine has a similar structure to one or more of the afore-mentioned cytokines.
  • the cytokine can be an IL-6 class cytokine such as leukemia inhibitory factor (LIF) or oncostatin M.
  • LIF leukemia inhibitory factor
  • the cytokine is one that in nature binds to a receptor that comprises a GP 130 signal transducing subunit.
  • Other four-helix bundle proteins of interest include growth hormone (GH), prolactin (PRL), and placental lactogen.
  • the polypeptide of interest is an erythropoiesis stimulating agent, e.g., erythropoietin (EPO), which is also a four-helix bundle cytokine.
  • EPO erythropoietin
  • an erythropoiesis stimulating agent is an EPO variant, e.g., darbepoetin alfa, also termed novel erythropoiesis stimulating protein (NESP), which is engineered to contain five N-linked carbohydrate chains (two more than recombinant HuEPO).
  • the polypeptide comprises five helices.
  • the polypeptide can be an interferon beta, e.g., interferon beta-la or interferon beta-lb, which (as will be appreciated) is often classified as a four-helix bundle cytokine.
  • a polypeptide of interest is IL-9, IL-IO, IL-1 1, IL- 13, or IL- 15. In some embodiments. See, e.g., Hunter, CA, Nature Reviews Immunology 5, 521- 531, 2005, for discussion of certain cytokines. See also Paul, WE (ed.), Fundamental Immunology, Lippincott Williams & Wilkins; 6th ed., 2008.
  • a polypeptide is one that is approved by the US Food & Drug Administration (or an equivalent regulatory authority such as the European Medicines Evaluation Agency) for use in treating a disease or disorder in humans.
  • Such polypeptide may or may not be one for which a PEGylated version has been tested in clinical trials and/or has been approved for marketing.
  • a polypeptide of interest is a neurotrophic factor, i.e., a factor that promotes survival, development and/or function of neural lineage cells (which term as used herein includes neural progenitor cells, neurons, and glial cells, e.g., astrocytes, oligodendrocytes, microglia).
  • the factor could promote neurite outgrowth.
  • the polypeptide is ciliary neurotrophic factor (CNTF; a four-helix bundle protein) or an analog thereof such as Axokine, which is a modified version of human Ciliary neurotrophic factor with a 15 amino acid truncation of the C terminus and two amino acid substitutions, which is three to five times more potent than CNTF in in vitro and in vivo assays and has improved stability properties.
  • CNTF ciliary neurotrophic factor
  • Axokine an analog thereof
  • Axokine is a modified version of human Ciliary neurotrophic factor with a 15 amino acid truncation of the C terminus and two amino acid substitutions, which is three to five times more potent than CNTF in in vitro and in vivo assays and has improved stability properties.
  • the polypeptide of interest is one that forms homodimers or heterodimers, (or homo- or heterooligomers comprising more than two subunits, such as tetramers).
  • the homodimer, heterodimer, or oligomer structure is such that a terminus of a first subunit is in close proximity to a terminus of a second subunit. For example, an N-terminus of a first subunit is in close proximity to a C-terminus of a second subunit.
  • the homodimer, heterodimer, or oligomer structure is such that a terminus of a first subunit and a terminus of a second subunit are not involved in interaction with a receptor, so that the termini can be joined via a non-genetically encoded peptide element without significantly affecting biological activity.
  • An inventive ligation method is used to join termini of two subunits of a homodimer, heterodimer, or oligomer via a non-genetically encoded peptide element, which optionally comprises a moiety attached to a side chain thereof, thereby producing a dimer (or oligomer) in which at least two subunits are covalently joined.
  • the neurotrophins nerve growth factor NEF
  • brain- derived neurotrophic factor BDNF
  • neurotrophin 3 NT3
  • neurotrophin 4 NT4
  • NGF neurotrophins nerve growth factor
  • BDNF brain- derived neurotrophic factor
  • NT3 neurotrophin 3
  • NT4 neurotrophin 4
  • the dimeric polypeptide is a cytokine, e.g., an interleukin.
  • Other polypeptides of interest are enzymes, e.g., enzymes that are important in metabolism or other physiological processes. As known in the art, deficiencies of enzymes or other proteins can lead to a variety of disease. Such diseases include diseases associated with defects in carbohydrate metabolism, amino acid metabolism, organic acid metabolism, porphyrin metabolism, purine or pyrimidine metabolism, lysosomal storage disorders, blood clotting, etc.
  • a polypeptide is a clotting or coagulation factor,(e.g., factor VII, Vila, VIII or IX).
  • a polypeptide is an enzyme that plays a role in carbohydrate metabolism, amino acid metabolism, organic acid metabolism, porphyrin metabolism, purine or pyrimidine metabolism, and/or lysosomal storage, wherein exogenous administration of the enzyme at least in part alleviates the disease.
  • a polypeptide comprises a receptor or receptor fragment (e.g., extracellular domain).
  • a receptor is a TNF ⁇ receptor.
  • a polypeptide comprises urate oxidase.
  • sequences of polypeptides of interest are found in, e.g., USSN 10/773,530; 11/531,531; USSN 11/707,014; 11/429,276; 1 1/365,008.
  • a polypeptide of interest is listed in Table B.
  • the invention encompasses application of the inventive techniques to any of the polypeptides described.
  • the invention provides modified versions of any of these polypeptides, wherein a modified version comprises (i) one or more nucleophilic residues such as glycine at the N-terminus (e.g., between 1 and 10 residues) and, optionally, a cleavage recognition sequence, e.g., a protease cleavage recognition sequence that masks the nucleophilic residue(s); (ii) a TRS at or near the C-terminus; (iii) both (i) and (ii).
  • Such modified polypeptides are useful, e.g., as substrates for transamidase-mediated ligation as described herein.
  • polypeptides e.g., secreted eukaryotic (e.g., mammalian) polypeptides
  • intracellular processing e.g., cleavage of a secretion signal prior to secretion and/or removal of other portion(s) that are not required for biological activity
  • Such mature, biologically active version is used in certain embodiments of the invention.
  • Hexosaminidase A and B (2gjx) Chain D [00243] It will be appreciated that considerable structure/function information is available regarding many of the afore-mentioned polypeptides, as well as sequences from different mammalian species, that can be used to design variants of the naturally occurring sequence that retain significant biological activity (e.g., at least 25%, 75%, 90% or more of the activity of the naturally occurring polypeptide). For example, crystal structures or NMR structures of a number of these polypeptides, in some instances in a complex with the corresponding receptor, are available.
  • the invention provides pharmaceutical compositions comprising any of the polypeptides described herein, i.e., a polypeptide that has been modified using an inventive ligation composition or method.
  • the polypeptide is circular.
  • the polypeptide is PEGylated in a site-specific manne.
  • the polypeptide is circular and PEGylated, e.g., the polypeptide is circularized via a linker peptide that comprises a PEG moiety attached to at least one side chain.
  • a pharmaceutical composition may comprise a variety of pharmaceutically acceptable carriers.
  • Pharmaceutically acceptable carriers include, for example, aqueous solutions such as water, 5% dextrose, or physiologically buffered saline or other solvents or vehicles such as glycols, glycerol, oils such as olive oil, or injectable organic esters that are suitable for administration to a human or non-human subject. See, e.g., Remington: The Science and Practice of Pharmacy, 21 st edition; Lippincott Williams & Wilkins, 2005.
  • a pharmaceutically acceptable carrier or composition is sterile.
  • a pharmaceutical composition can comprise, in addition to the active agent, physiologically acceptable compounds that act, for example, as bulking agents, fillers, solubilizers, stabilizers, osmotic agents, uptake enhancers, etc.
  • physiologically acceptable compounds include, for example, carbohydrates, such as glucose, sucrose, lactose; dextrans; polyols such as mannitol; antioxidants, such as ascorbic acid or glutathione; preservatives; chelating agents; buffers; or other stabilizers or excipients.
  • a pharmaceutically acceptable carrier(s) and/or physiologically acceptable compound(s) can depend for example, on the nature of the active agent, e.g., solubility, compatibility (meaning that the substances can be present together in the composition without interacting in a manner that would substantially reduce the pharmaceutical efficacy of the pharmaceutical composition under ordinary use situations) and/or route of administration of the composition.
  • the pharmaceutical composition could be in the form of a liquid, gel, lotion, tablet, capsule, ointment, cream, transdermal patch, etc.
  • a pharmaceutical composition can be administered to a subject by various routes including, for example, parenteral administration.
  • Exemplary routes of administration include intravenous administration; respiratory administration (e.g., by inhalation), intramuscular administration, nasal administration, intraperitoneal administration, oral administration, subcutaneous administration and topical administration.
  • the compounds can be formulated with pharmaceutically acceptable carriers as tablets, pills, dragees, capsules, liquids, gels, syrups, slurries, suspensions, etc.
  • a compound may be administered directly to a target tissue. Direct administration could be accomplished, e.g., by injection or by implanting a sustained release implant within the tissue.
  • a sustained release implant could be implanted at any suitable site.
  • a sustained release implant may be particularly suitable for prophylactic treatment of subjects at risk of developing a recurrent cancer.
  • a sustained release implant delivers therapeutic levels of the active agent for at least 30 days, e.g., at least 60 days, e.g., up to 3 months, 6 months, or more.
  • a sustained release implant delivers therapeutic levels of the active agent for at least 30 days, e.g., at least 60 days, e.g., up to 3 months, 6 months, or more.
  • One skilled in the art would select an effective dose and administration regimen taking into consideration factors such as the patient's weight and general health, the particular condition being treated, etc. Exemplary doses may be selected using in vitro studies, tested in animal models, and/or in human clinical trials as standard in the art.
  • the pharmaceutical composition is delivered by means of a microparticle or nanoparticle or a liposome or other delivery vehicle or matrix.
  • a number of biocompatible synthetic or naturally occurring polymeric materials are known in the art to be of use for drug delivery purposes. Examples include polylactide-co-glycolide, polycaprolactone, polyanhydride, cellulose derivatives, and copolymers or blends thereof.
  • Liposomes for example, which consist of phospholipids or other lipids, are nontoxic, physiologically acceptable and metabolizable carriers that are relatively simple to make and administer.
  • a compound e.g., a polypeptide of the invention (e.g., a polypeptide produced at least in part using an inventive ligation method) may be delivered in an effective amount, by which is meant an amount sufficient to achieve a biological response of interest, e.g., reducing one or more symptoms or manifestations of a disease or condition.
  • an effective amount by which is meant an amount sufficient to achieve a biological response of interest, e.g., reducing one or more symptoms or manifestations of a disease or condition.
  • the exact amount required will vary from subject to subject, depending on factors such as the species, age, weight, sex, and general condition of the subject, the severity of the disease or disorder, the particular compound and its activity, its mode of administration, concurrent therapies, and the like.
  • a compound e.g., a polypeptide
  • unit dosage unit form for ease of administration and uniformity of dosage, which term as used herein refers to a physically discrete unit of agent appropriate for the patient to be treated. It will be understood, however, that the total daily dosage will be decided by the attending physician within the scope of sound medical judgment.
  • information available regarding a suitable dose of the unPEGylated version, optionally in conjunction with in vitro activity data can be used as a guideline in selecting an appropriate dose for preclinical testing and/or for clinical use.
  • the pharmaceutical compositions can be used to treat a wide variety of different diseases and disorders.
  • a pharmaceutical composition is used, e.g., to treat any disease or condition for which the unmodified polypeptide is of use.
  • the invention provides methods of treatment comprising administering an inventive polypeptide to a subject in need thereof.
  • the subject is typically a mammalian subject, e.g., a human.
  • the subject is a non-human animal that serves as a model for a disease or disorder that affects humans.
  • the animal model may be used, e.g., in preclinical studies, e.g., to assess efficacy and/or determine a suitable dose.
  • an inventive polypeptide is administered prophylactically, e.g., to a subject who does not exhibit signs or symptoms of the disease or disorder (but may be at increased risk of developing the disorder or is expected to develop the disease or disorder).
  • an inventive polypeptide is administered to a subject who has developed one or more signs or symptoms of the disease or sorder, e.g., the subject has been diagnose as having the disease or disorder.
  • the method comprises diagnosing the subject as having a disease or disorder for which the polypeptide is an appropriate treatment.
  • interferons have a variety of uses, e.g., in the treatment of autoimmune diseases (e.g., multiple sclerosis) and infectious diseases (e.g., viral infections such as those caused by viruses belonging to the Flaviviridae family, e.g., HBV, HCV; bacterial infections, fungal infections, parasites).
  • autoimmune diseases e.g., multiple sclerosis
  • infectious diseases e.g., viral infections such as those caused by viruses belonging to the Flaviviridae family, e.g., HBV, HCV; bacterial infections, fungal infections, parasites.
  • viruses of the Flaviviridae family such as, for example, Hepatitis C Virus, Yellow Fever Virus, West Nile Virus, Japanese Encephalitis Virus, Dengue Virus, and Bovine Viral Diarrhea Virus
  • viruses of the Hepadnaviridae family such as, for example, Hepatitis B Virus
  • viruses of the Picornaviridae family such as, for example, Encephalomyocarditis Virus, Human Rhinovirus, and Hepatitis A Virus
  • viruses of the Retroviridae family such as, for example, Human Immunodeficiency Virus, Simian Immunodeficiency Virus, Human T- Lymphotropic Virus, and Rous Sarcoma Virus
  • viruses of the Coronaviridae family such as, for example, SARS coronavirus
  • viruses of the Rhabdoviridae family such as, for example, Rabies Virus and Vesicular Stomatitis
  • Interferon therapy is used (often in combination with chemotherapy and radiation) as a treatment for many cancers, which term is used herein to encompass solid tumors (carcinomas, sarcomas), and leukemias.
  • the tumor is an adenocarcinoma.
  • the tumor is a sarcoma.
  • the tumor affects an organ or organ system selected from breast, lymph node, prostate, kidney, bladder, lung, liver, gastrointestinal tract, colon, testis, stomach, pancreas, thyroid, skin, ovary, uterus, cervix, skin, nerve, bone, and nervous system (e.g., brain).
  • an interferon is used for treating a hematological malignancy, e.g., a leukemia or a lymphoma, .e.g., hairy cell leukemia, chronic myeloid leukemia, nodular lymphoma, cutaneous T-cell lymphoma.
  • a hematological malignancy e.g., a leukemia or a lymphoma, .e.g., hairy cell leukemia, chronic myeloid leukemia, nodular lymphoma, cutaneous T-cell lymphoma.
  • an IFN e.g., IFN- ⁇ 2b, is used to treat a melanoma.
  • Erythropoiesis stimulating agents such as EPO are of use to treat anemia, which may result from a variety of causes.
  • the anemia may be an anemia of chronic disease, anemia associated with medications (e.g., cancer chemotherapy), radiation, renal disease (e.g., diabetes), infectious diseases, or blood loss.
  • Colony stimulating factors such as G-CSF, GM-CSF, and/or M-CSF may be used to treat leukopenia, e.g., neutropenia and/or lymphopenia, which may result, e.g., from medications (e.g., cancer chemotherapy), radiation, infectious disease, or blood loss.
  • Neurotrophic factor polypeptides may be used, e.g., to treat neurodegenerative diseases (e.g., amyotrophic lateral sclerosis, Huntington disease, Alzheimer disease, Parkinson disease), central or peripheral nervous system injury.
  • neurodegenerative diseases e.g., amyotrophic lateral sclerosis, Huntington disease, Alzheimer disease, Parkinson disease
  • central or peripheral nervous system injury e.g., central or peripheral nervous system injury.
  • Growth hormone may be used, e.g., to treat children's growth disorders and adult growth hormone deficiency.
  • Interleukins are of use to modulate the immune response for a wide variety of purposes, e.g., to stimulate an immune response against an infectious agent or cancer.
  • an interleukin stimulates immune system cells and/or increases the intensity and/or duration of innate and/or adaptive immune responses.
  • certain interleukins help to limit the intensity and/or duration of innate and/or adaptive immune responses.
  • Administration of such interleukins may be of use in treatment of autoimmune diseases, sepsis, or other conditions in which an aberrant or overactivated immune response can be deleterious.
  • Autoimmune disorders include type I diabetes (e.g., juvenile onset diabetes), multiple sclerosis, scleroderma, ankylosing spondylitis, sarcoid, pemphigus vulgaris, myasthenia gravis, systemic lupus erythemotasus, rheumatoid arthritis, juvenile arthritis, Behcet's syndrome, Reiter's disease, Berger's disease, dermatomyositis, Wegener's granulomatosis, autoimmune myocarditis, anti-glomerular basement membrane disease (including Goodpasture's syndrome), dilated cardiomyopathy, thyroiditis (e.g., Hashimoto's thyroiditis, Graves' disease), and Guillane-Barre syndrome.
  • type I diabetes e.g., juvenile onset diabetes
  • multiple sclerosis e.g., multiple sclerosis, scleroderma, ankylosing spondylitis, sarcoid, pe
  • exemplary bacteria and fungi include those falling within the following groups Actinomycetales (e.g., Corynebacterium, Mycobacterium, Norcardia), Aspergillosis, Bacillaceae (e.g., Anthrax, Clostridium), Bacteroidaceae, Blastomycosis, Bordetella, Borrelia, Brucellosis, Candidiasis, Campylobacter, Coccidioidomycosis, Cryptococcosis, Dermatocycoses, Enterobacteriaceae (Klebsiella, Salmonella, Serratia, Yersinia), Erysipelothrix, Helicobacter, Legionella, Leptospires Listeria, Mycoplasmatales, Neisseriacea
  • a modified, e.g., PEGylated and/or circularized polypeptide exhibits increase efficacy relative to an unmodified form and/or requires a lower dose or less frequent administration (greater dosing interval) to achieve equivalent efficacy and/or exhibits reduced toxicity (reduced side effects, greater tolerability, greater safety) and/or can be administered by a more convenient or preferable route of administration.
  • Use ofTransamidasesfor Reporting on Cell-Cell Interactions [00261] There is a dearth of tools that report on cell-cell interactions.
  • the invention provides tools and methods for reporting on (detecting, optionally quantifying) transient cell-cell interactions, where one cell bearing a sortase substrate comes into close proximity to another cell bearing a membrane anchored version of a transamidase, e.g., a SrtA, e.g., either SrtA strep or SrtA sta ph.
  • a transamidase e.g., a SrtA, e.g., either SrtA strep or SrtA sta ph.
  • sortases are embedded in the bacterial membrane through a transmembrane anchor at the N-terminus.
  • We can thus express sortase at the mammalian cell surface by fusing the catalytic domain of sortase to a mammalian type II membrane protein bearing a signal-anchor sequence for ER insertion. This would result in insertion into the plasma membrane and exposure of the sortase catalytic domain to the extracellular space.
  • the label comprises a detectable moiety and/or a tag that can be used for isolating the cells. This approach can be applied in vitro (in cell culture) or in vivo.
  • Immunoglobulins and Transgenic Non-human Animals include, e.g., examining interactions of immune system cells (e.g., lymphocytes, macrophages) with other immune or non-immune system cells, examining cell-cell interactions in the nervous system or during development, cell migration, etc. This approach can be used to report on cell interactions with noncellular materials as well, by attaching a sortase substrate thereto.
  • immune system cells e.g., lymphocytes, macrophages
  • the invention provides a transgenic, non-human animal comprising cells whose genome comprises a DNA segment comprising a portion that encodes a polypeptide of interest and a portion that encodes a sortase recognition motif.
  • Transgenic animal is used consistently with usage in the art and refers to a non-human animal having a non-endogenous (i.e., heterologous) nucleic acid sequence (transgene) stably integrated into its DNA (i.e., in the genomic sequence of most or all of its cells, in many embodiments including somatic cells and cells of the germ line) or, in some embodiments, present as an extrachromosomal element in at least some of its cells.
  • a transgenic animal is a "knockout" animal, in which a gene has been inactivated, e.g., by at least partially deleting the gene or insertion of a heterologous sequence. It will be understood that the term “transgenic” applies both to the original genetically modified animal and to its descendants. [00264]
  • the animal is of a type in which genetic modification, e.g., generating transgenic organisms, has been performed and in which methods for performing genetic modification, e.g., generating transgenic organisms, without undue experimentation are known in the art.
  • the transgenic non-human animal is a mammal.
  • the mammal is ovine, porcine, or bovine.
  • the transgenic non-human mammal is a rodent, e.g., a mouse or rat.
  • the transgenic non-human animal is an avian, e.g., a chicken.
  • the invention further provides offspring of the transgenic animal, wherein the offspring are obtained by crossing the transgenic animal with an animal having a phenotype or genetic modification of interest.
  • the invention further provides a cell derived from the transgenic animal.
  • the cell may be of any cell type.
  • the cell is an immune system cell (e.g., a B or T lineage cell, neutrophil or neutrophil precursor), etc. "Derived from” refers to cells that are obtained from an animal and descendants of such cells.
  • the cells may be subjected to genetic modification or other manipulation.
  • the cells are immortalized.
  • Transgenic animals of the invention have a number of applications. They may be sources of sortase substrates and/or of cells that express sortase substrates comprising a sortase recognition motif. An application of particular interest is the production of antibodies or antibody chains that comprise a sortase recognition motif.
  • Such antibodies may be conveniently labeled or attached to a solid support, e.g., an array, e.g., a glass slide.
  • the animal may be immunized or otherwise contacted with (e.g., exposed to), an antigen of interest (e.g., an allergen, an infectious agent or an extract, portion, or product thereof such as a polypeptide, etc.), may be genetically predisposed to develop an autoimmune disease or immunodeficiency, may be infected with a pathogenic or non-pathogenic infectious agent, etc.
  • Immune system cells e.g., B-lineage cells, may be obtained from the animal.
  • Hybridomas may be generated from the B-lineage cells.
  • the invention provides collections ('panels') of antibodies and hybridomas.
  • the transgenic non-human animal e.g., transgenic mouse
  • the transgenic non-human animal is an animal in which at least one endogenous immunoglobulin locus has been at least in part replaced by a human immunoglobulin gene locus.
  • the transgenic animal is fully reconstituted with human immunoglobulin loci, and, optionally, the endogenous immunoglobulin loci are functionally inactivated, e.g., through targeted deletion, insertion, etc., making it possible to generate fully human antibodies in such animals.
  • Such transgenic mice have been generated by introducing yeast artificial chromosomes (YACs) containing human heavy-chain and K and ⁇ light-chain immunoglobulin genes, into mice whose endogenous heavy-chain and K loci were functionally inactivated by targeted deletion.
  • yeast artificial chromosomes containing human heavy-chain and K and ⁇ light-chain immunoglobulin genes
  • transgenic plants having genetic modifications as described herein for animals (e.g., such plants may have at least part of an immunoglobulin gene inserted into their genome). It will be understood that appropriate modifications may be made to achieve expression in plants.
  • Certain compounds of the present invention may exist in particular geometric or stereoisomeric forms.
  • the present invention contemplates all such compounds, including cis- and tr ⁇ tts-isomers, E- and Z-isomers, R- and 5-enantiomers, diastereomers, (D)-isomers, (L)- isomers, (-)- and (+)-isomers, racemic mixtures thereof, and other mixtures thereof, as falling within the scope of the invention.
  • Additional asymmetric carbon atoms may be present in a substituent such as an alkyl group. All such isomers, as well as mixtures thereof, are intended to be included in this invention.
  • a particular enantiomer of a compound of the present invention may be prepared by asymmetric synthesis, chiral chromatography, or by derivation with a chiral auxiliary, where the resulting diastereomeric mixture is separated and the auxiliary group cleaved to provide the pure desired enantiomers.
  • the molecule contains a basic functional group, such as amino, or an acidic functional group, such as carboxyl, diastereomeric salts are formed with an appropriate optically-active acid or base, followed by resolution of the diastereomers thus formed by fractional crystallization or chromatographic means well known in the art, and subsequent recovery of the pure enantiomers.
  • Isomeric mixtures containing any of a variety of isomer ratios may be utilized in accordance with the present invention. For example, where only two isomers are combined, mixtures containing 50:50, 60:40, 70:30, 80:20, 90:10, 95:5, 96:4, 97:3, 98:2, 99:1, or 100:0 isomer ratios are all contemplated by the present invention. Those of ordinary skill in the art will readily appreciate that analogous ratios are contemplated for more complex isomer mixtures.
  • the compounds, as described herein, may be substituted with any number of substituents or functional moieties.
  • substituted whether preceded by the term “optionally” or not, and substituents contained in formulas of this invention, refer to the replacement of hydrogen radicals in a given structure with the radical of a specified substituent.
  • the substituent may be either the same or different at every position.
  • substituted is contemplated to include all permissible substituents of organic compounds.
  • the permissible substituents include acyclic and cyclic, branched and unbranched, carbocyclic and heterocyclic, aromatic and non-aromatic substituents of organic compounds.
  • heteroatoms such as nitrogen may have hydrogen substituents and/or any permissible substituents of organic compounds described herein which satisfy the valencies of the heteroatoms.
  • this invention is not intended to be limited in any manner by the permissible substituents of organic compounds. Combinations of substituents and variables envisioned by this invention are preferably those that result in the formation of stable compounds.
  • R is alkyl, alkenyl, alkynyl, aryl, carbocylic, heterocyclic, or aromatic heterocyclic.
  • An example of an acyl group is acetyl.
  • aliphatic includes both saturated and unsaturated, straight chain (i.e., unbranched), branched, acyclic, cyclic, or polycyclic aliphatic hydrocarbons, which are optionally substituted with one or more functional groups.
  • aliphatic is intended herein to include, but is not limited to, alkyl, alkenyl, alkynyl, cycloalkyl, cycloalkenyl, and cycloalkynyl moieties.
  • alkyl includes straight, branched and cyclic alkyl groups.
  • alkyl refers to saturated, straight- or branched-chain hydrocarbon radicals derived from a hydrocarbon moiety containing between one and twenty carbon atoms by removal of a single hydrogen atom.
  • the alkyl group employed in the invention contains 1-12 carbon atoms. In another embodiment, the alkyl group employed contains 1-8 carbon atoms. In still other embodiments, the alkyl group contains 1-6 carbon atoms. In yet another embodiment, the alkyl group contains 1-4 carbons.
  • alkyl radicals include, but are not limited to, methyl, ethyl, n-propyl, isopropyl, n-butyl, iso-butyl, sec-butyl, sec-pentyl, iso-pentyl, tert-butyl, n-pentyl, neopentyl, n-hexyl, sec-hexyl, n-heptyl, n-octyl, n-decyl, n-undecyl, dodecyl, and the like, which may bear one or more substituents.
  • aryl and heteroaryl refer to stable mono- or polycyclic, heterocyclic, polycyclic, and polyheterocyclic unsaturated moieties having preferably 3-14 carbon atoms, each of which may be substituted or unsubstituted.
  • Substituents include, but are not limited to, any of the previously mentioned substituents, i.e., the substituents recited for aliphatic moieties, or for other moieties as disclosed herein, resulting in the formation of a stable compound.
  • aryl refers to a mono- or bicyclic carbocyclic ring system having one or two aromatic rings including, but not limited to, phenyl, naphthyl, tetrahydronaphthyl, indanyl, indenyl, and the like.
  • heteroaryl refers to a cyclic aromatic radical having from five to ten ring atoms of which one ring atom is selected from the group consisting of S, O, and N; zero, one, or two ring atoms are additional heteroatoms independently selected from the group consisting of S, O, and N; and the remaining ring atoms are carbon, the radical being joined to the rest of the molecule via any of the ring atoms, such as, for example, pyridyl, pyrazinyl, pyrimidinyl, pyrrolyl, pyrazolyl, imidazolyl, thiazolyl, oxazolyl, isooxazolyl, thiadiazolyl,oxadiazolyl, thiophenyl, furanyl, quinolinyl, isoquinolinyl, and the like.
  • aryl and heteroaryl groups can be unsubstituted or substituted, wherein substitution includes replacement of one, two, three, or more of the hydrogen atoms thereon independently with any one or more of the following moieties including, but not limited to: aliphatic; heteroaliphatic; aryl; heteroaryl; arylalkyl; heteroarylalkyl; alkoxy; aryloxy; heteroalkoxy; heteroaryloxy; alkylthio; arylthio; heteroalkylthio; heteroarylthio; -F; -Cl; -Br; -I; -OH; -NO 2 ; -CN; -CF 3 ; -CH 2 CF 3 ; -CHCl 2 ; - CH 2 OH; -CH 2 CH 2 OH; -CH 2 NH 2 ; -CH 2 SO 2 CH 3 ; -C(O)R x ; -CO 2 (R
  • carboxylic acid refers to a group of formula -CO 2 H.
  • halo and halogen refer to an atom selected from the group consisting of fluorine, chlorine, bromine, and iodine.
  • heteroaliphatic refers to aliphatic moieties that contain one or more oxygen, sulfur, nitrogen, phosphorus, or silicon atoms, e.g., in place of carbon atoms.
  • Heteroaliphatic moieties may be branched, unbranched, cyclic or acyclic and include saturated and unsaturated heterocycles such as morpholino, pyrrolidinyl, etc.
  • heteroaliphatic moieties are substituted by independent replacement of one or more of the hydrogen atoms thereon with one or more moieties including, but not limited to aliphatic; heteroaliphatic; aryl; heteroaryl; arylalkyl; heteroarylalkyl; alkoxy; aryloxy; heteroalkoxy; heteroaryloxy; alkylthio; arylthio; heteroalkylthio; heteroarylthio; -F; -Cl; -Br; -I; -OH; -NO 2 ; -CN; -CF 3 ; -CH 2 CF 3 ; -CHCl 2 ; -CH 2 OH; -CH 2 CH 2 OH; -CH 2 NH 2 ; - CH 2 SO 2 CH 3 ; -C(O)R x ; -CO 2 (R x ); -CON(R X ) 2 ; -OC(O)R x ; -CO 2 (R
  • heterocyclic refers to an aromatic or non-aromatic, partially unsaturated or fully saturated, 3- to 10-membered ring system, which includes single rings of 3 to 8 atoms in size and bi- and tri-cyclic ring systems which may include aromatic five- or six-membered aryl or aromatic heterocyclic groups fused to a non-aromatic ring.
  • heterocyclic rings include those having from one to three heteroatoms independently selected from the group consisting of oxygen, sulfur, and nitrogen, in which the nitrogen and sulfur heteroatoms may optionally be oxidized and the nitrogen heteroatom may optionally be quaternized.
  • heterocyclic refers to a non-aromatic 5-, 6-, or 7-membered ring or a polycyclic group wherein at least one ring atom is a heteroatom selected from the group consisting of O, S, and N (wherein the nitrogen and sulfur heteroatoms may be optionally oxidized), including, but not limited to, a bi- or tri-cyclic group, comprising fused six-membered rings having between one and three heteroatoms independently selected from the group consisting of the oxygen, sulfur, and nitrogen, wherein (i) each 5-membered ring has 0 to 2 double bonds, each 6-membered ring has 0 to 2 double bonds, and each 7-membered ring has 0 to 3 double bonds, (ii) the nitrogen and sulfur heteroatoms may be optionally oxidized, (iii) the nitrogen heteroatom may optionally be quaternized, and (iv) any of the above heterocyclic rings may be fused to an aryl or heteroaryl ring.
  • aromatic heterocyclic refers to a cyclic aromatic radical having from five to ten ring atoms of which one ring atom is selected from the group consisting of sulfur, oxygen, and nitrogen; zero, one, or two ring atoms are additional heteroatoms independently selected from the group consisting of sulfur, oxygen, and nitrogen; and the remaining ring atoms are carbon, the radical being joined to the rest of the molecule via any of the ring atoms, such as, for example, pyridyl, pyrazinyl, pyrimidinyl, pyrrolyl, pyrazolyl, imidazolyl, thiazolyl, oxazolyl, isooxazolyl, thiadiazolyl, oxadiazolyl, thiophenyl, furanyl, quinolinyl, isoquinolinyl, and the like.
  • Aromatic heterocyclic groups can be unsubstituted or substituted with substituents selected from the group consisting of branched and unbranched alkyl, alkenyl, alkynyl, haloalkyl, alkoxy, thioalkoxy, amino, alkylamino, dialkylamino, trialkylamino, acylamino, cyano, hydroxy, halo, mercapto, nitro, carboxyaldehyde, carboxy, alkoxycarbonyl, and carboxamide.
  • heterocyclic and aromatic heterocyclic groups that may be included in the compounds of the invention include: 3 -methyl -4-(3-methylphenyl)piperazine, 3 methylpiperidine, 4-(bis-(4-fluorophenyl)methyl)piperazine, 4-(diphenylmethyl)piperazine, 4-(ethoxycarbonyl)piperazine, 4-(ethoxycarbonylmethyl)piperazine, 4- (phenylmethyl)piperazine, 4-(l-phenylethyl)piperazine, 4-(I 5 I- dimethylethoxycarbonyl)piperazine, 4-(2-(bis-(2-propenyl) amino)ethyl)piperazine, 4-(2- (diethylamino)ethyl)piperazine, 4-(2-chlorophenyl)piperazine, 4-(2-cyanophenyl)piperazine, 4-(2-ethoxyphenyl)piperazine, 4-(2-ethylphenyl)piperazine,
  • arylalkyl refers to alkyl groups in which a hydrogen atom has been replaced with an aryl group.
  • groups include, without limitation, benzyl, cinnamyl, and dihyrocinnamyl.
  • heteroatom means one or more of oxygen, sulfur, nitrogen, phosphorus, or silicon (including, any oxidized form of nitrogen, sulfur, phosphorus, or silicon; the quaternized form of any basic nitrogen or; a substitutable nitrogen of a heterocyclic ring, for example N (as in 3,4-dihydro-2H-pyrrolyl), NH (as in pyrrolidinyl) or NR + (as in N- substituted pyrrolidinyl)).
  • unsaturated means that a moiety has one or more units ofunsaturation.
  • partially unsaturated refers to a ring moiety that includes at least one double or triple bond.
  • partially unsaturated is intended to encompass rings having multiple sites of unsaturation, but is not intended to include aryl or heteroaryl moieties, as herein defined.
  • structures depicted herein are also meant to include compounds that differ only in the presence of one or more isotopically enriched positions of the compound.
  • compounds having the present structures including the replacement of hydrogen by deuterium or tritium, or the replacement of a carbon by a
  • 13 C- or l4 C-enriched carbon are within the scope of this invention. Such compounds are useful, for example, as analytical tools, as probes in biological assays, or as therapeutic agents in accordance with the present invention.
  • protecting group it is meant that a particular functional moiety, e.g., O, S, or N, is masked or blocked, permitting, if desired, a reaction to be carried out selectively at another reactive site in a multifunctional compound.
  • Suitable protecting groups are well known in the art and include those described in detail in Protecting Groups in Organic Synthesis, T. W. Greene and P. G. M. Wuts, 3 rd edition, John Wiley & Sons, 1999, the entirety of which is incorporated herein by reference.
  • a protecting group reacts selectively in good yield to give a protected substrate that is stable to the projected reactions; the protecting group is preferably selectively removable by readily available, preferably nontoxic reagents that do not attack the other functional groups; the protecting group forms a separable derivative (more preferably without the generation of new stereogenic centers); and the protecting group will preferably have a minimum of additional functionality to avoid further sites of reaction.
  • oxygen, sulfur, nitrogen, and carbon protecting groups may be utilized.
  • hydroxyl protecting groups include methyl, methoxylmethyl (MOM), methylthiomethyl (MTM), t-butylthiomethyl, (phenyldimethylsilyl)methoxymethyl (SMOM), benzyloxymethyl (BOM), p- methoxybenzyloxymethyl (PMBM), (4-methoxyphenoxy)methyl (p-AOM), guaiacolmethyl (GUM), t-butoxymethyl, 4-pentenyloxymethyl (POM), siloxymethyl, 2- methoxyethoxymethyl (MEM), 2,2,2-trichloroethoxymethyl, bis(2-chloroethoxy)methyl, 2- (trimethylsilyl)ethoxymethyl (SEMOR), tetrahydropyranyl (THP), 3- bromotetrahydropyranyl, tetrahydrothiopyranyl, 1-methoxycyclohexyl, 4- methoxytetrahydropyranyl (MTHP), 4-
  • the protecting groups include methylene acetal, ethylidene acetal, 1-t-butyl ethylidene ketal, 1-phenylethylidene ketal, (4- methoxyphenyl)ethylidene acetal, 2,2,2-trichloroethylidene acetal, acetonide, cyclopentylidene ketal, cyclohexylidene ketal, cycloheptylidene ketal, benzylidene acetal, p- methoxybenzylidene acetal, 2,4-dimethoxybenzylidene ketal, 3,4-dimethoxybenzylidene acetal, 2-nitrobenzylidene acetal, methoxymethylene acetal, ethoxymethylene acetal, dimethoxymethylene ortho ester, 1-methoxy ethylidene ortho
  • Amino-protecting groups include methyl carbamate, ethyl carbamante, 9-fluorenylmethyl carbamate (Fmoc), 9-(2-sulfo)fluorenylmethyl carbamate, 9-(2,7-dibromo)fluoroenylmethyl carbamate, 2,7-di-t-butyl-[9-( 10, 10-dioxo- 10,10,10,10-tetrahydrothioxanthyl)]methyl carbamate (DBD-Tmoc), 4-methoxyphenacyl carbamate (Phenoc), 2,2,2-trichloroethyl carbamate (Troc), 2-trimethylsilylethyl carbamate (Teoc), 2-phenylethyl carbamate (hZ), 1- (l-adamantyl)-l-methylethyl carbamate (Adpoc), l,l-dimethyl-2-haloethyl carbamate, 1,1-
  • protecting groups are detailed herein, however, it will be appreciated that the present invention is not intended to be limited to these protecting groups; rather, a variety of additional equivalent protecting groups can be readily identified using the above criteria and utilized in the method of the present invention. Additionally, a variety of protecting groups are described by Greene and Wuts (supra).
  • polypeptide comprises a string of at least three amino acids linked together by peptide bonds.
  • the terms “polypeptide”, “peptide”, and “protein”, may be used interchangeably.
  • Peptide may refer to an individual peptide or a collection of peptides.
  • Inventive peptides preferably contain only natural amino acids, although non natural amino acids (i.e., compounds that do not occur in nature but that can be incorporated into a polypeptide chain) and/or amino acid analogs as are known in the art may alternatively be employed.
  • one or more of the amino acids in a peptide may be modified, for example, by the addition of a chemical entity such as a carbohydrate group, a phosphate group, a farnesyl group, an isofarnesyl group, a fatty acid group, a linker for conjugation, functionalization, or other modification, etc.
  • the modifications of the peptide lead to a more stable peptide (e.g., greater half-life in vivo). These modifications may include cyclization of the peptide, the incorporation of D-amino acids, etc. None of the modifications should substantially interfere with the desired biological activity of the peptide.
  • Carbohydrate refers to a sugar or polymer of sugars.
  • saccharide The terms “saccharide”, “polysaccharide”, “carbohydrate”, and “oligosaccharide”, may be used interchangeably.
  • Most carbohydrates are aldehydes or ketones with many hydroxyl groups, usually one on each carbon atom of the molecule.
  • Carbohydrates generally have the molecular formula C n H 2n O n .
  • a carbohydrate may be a monosaccharide, a disaccharide, trisaccharide, oligosaccharide, or polysaccharide.
  • the most basic carbohydrate is a monosaccharide, such as glucose, sucrose, galactose, mannose, ribose, arabinose, xylose, and fructose.
  • Disaccharides are two joined monosaccharides. Exemplary disaccharides include sucrose, maltose, cellobiose, and lactose.
  • an oligosaccharide includes between three and six monosaccharide units (e.g., raffinose, stachyose), and polysaccharides include six or more monosaccharide units.
  • Exemplary polysaccharides include starch, glycogen, and cellulose.
  • Carbohydrates may contain modified saccharide units such as 2'-deoxyribose wherein a hydroxyl group is removed, 2'-fluororibose wherein a hydroxyl group is replace with a fluorine, or N-acetylglucosamine, a nitrogen-containing form of glucose, (e.g., T- fluororibose, deoxyribose, and hexose).
  • Carbohydrates may exist in many different forms, for example, conformers, cyclic forms, acyclic forms, stereoisomers, tautomers, anomers, and isomers.
  • Polysaccharide “carbohydrate” or “oligosaccharide”: The terms “polysaccharide”, “carbohydrate”, or “oligosaccharide” refer to a polymer of sugars. The terms “polysaccharide”, “carbohydrate”, and “oligosaccharide”, may be used interchangeably. Typically, a polysaccharide comprises at least two sugars.
  • the polymer may include natural sugars (e.g., glucose, fructose, galactose, mannose, arabinose, ribose, and xylose) and/or modified sugars (e.g., 2'-fiuororibose, 2 '-deoxyribose, and hexose).
  • natural sugars e.g., glucose, fructose, galactose, mannose, arabinose, ribose, and xylose
  • modified sugars e.g., 2'-fiuororibose, 2 '-deoxyribose, and hexose
  • “Sugar alcohols” include glycerol (glycertil, propane- 1, 2, 3-triol), erythritol, threitol, ribitol (adonitol), arabinitol, xylitol, allitol, altritol, galactitol, glucitol (sorbitol), mannitol, or iditol.
  • glycerol glycertil, propane- 1, 2, 3-triol
  • erythritol threitol
  • ribitol ribitol (adonitol)
  • arabinitol xylitol
  • allitol altritol
  • galactitol galactitol
  • glucitol sorbitol
  • mannitol or iditol.
  • Such natural amino acids include the nonpolar, or hydrophobic amino acids, glycine, alanine, valine, leucine, isoleucine, methionine, phenylalanine, tryptophan, and proline. Cysteine is sometimes classified as nonpolar or hydrophobic and other times as polar. Natural amino acids also include polar, or hydrophilic amino acids, such as tyrosine, serine, threonine, aspartic acid (also known as aspartate, when charged), glutamic acid (also known as glutamate, when charged), asparagine, and glutamine. Certain polar, or hydrophilic, amino acids have charged side-chains. Such charged amino acids include lysine, arginine, and histidine.
  • unnatural amino acid side-chain refers to the side- chain group of amino acids not included in the list of 20 amino acids naturally occuring in proteins, as described above. Such amino acids include the D-isomer of any of the 20 naturally occuring amino acids. Unnatural amino acids also include homoserine, ornithine, norleucine, and thyroxine.
  • unnatural amino acids side-chains are well known to one of ordinary skill in the art and include unnatural aliphatic side chains.
  • Other unnatural amino acids include modified amino acids, including those that are N-alkylated, cyclized, phosphorylated, acetylated, amidated, azidylated, labelled, and the like.
  • an unnatural amino acid is a D-isomer.
  • an unnatural amino acid is a L-isomer.
  • Small molecule As used herein, the term “small molecule” is used to refer to molecules, whether naturally-occurring or artificially created (e.g. , via chemical synthesis) that have a relatively low molecular weight. Typically, a small molecule is an organic compound (i.e., it contains carbon). The small molecule may contain multiple carbon-carbon bonds, stereocenters, and other functional groups (e.g., amines, hydroxyl, carbonyls, heterocyclic rings, etc.). In some embodiments, small molecules are monomeric and have a molecular weight of less than about 1500 g/mol.
  • the molecular weight of the small molecule is less than about 1000 g/mol or less than about 500 g/mol.
  • Preferred small molecules are biologically active in that they produce a biological effect in animals, preferably mammals, more preferably humans.
  • Small molecules include, but are not limited to, radionuclides and imaging agents.
  • the small molecule is a drug.
  • the drug is one that has already been deemed safe and effective for use in humans or animals by the appropriate governmental agency or regulatory body.
  • drugs approved for human use are listed by the FDA under 21 CF. R. ⁇ 330.5, 331 through 361, and 440 through 460, incorporated herein by reference; drugs for veterinary use are listed by the FDA under 21 CF. R. ⁇ 500 through 589, incorporated herein by reference. All listed drugs are considered acceptable for use in accordance with the present invention.
  • Polynucleotide is used herein consistently with usage in the art and is used interchangeably with “nucleic acid” or “oligonucleotide”, with “oligonucleotide” typically being used to refer to short (e.g, 50 residues or less) polynucleotides.
  • the polynucleotide may include natural nucleosides found in RNA and/or DNA, nucleoside analogs (e.g., 2- aminoadenosine, 2-thiothymidine, inosine, pyrrolo-pyrimidine, 3-methyl adenosine, C5- propynylcytidine, C5-propynyluridine, C5-bromouridine, C5-fluorouridine, C5-iodouridine, C5-methylcytidine, 7-deazaadenosine, 7-deazaguanosine, 8-oxoadenosine, 8-oxoguanosine, O(6)-methylguanine, and 2-thiocytidine), and/or nucleosides comprising chemically or biologically modified bases, (e.g., methylated bases) and/or modified sugars (e.g., T- fluororibose, ribose, 2'-deoxyrib
  • Polynucleotides containing modified backbones (relative to those found in RNA or DNA) or non-naturally occurring internucleoside linkages can also be used in the present invention.
  • a polynucleotide may be single-stranded or double-stranded. It should be noted that where the present invention discloses a single-stranded polynucleotide, the perfect complement of the polynucleotide, and a double-stranded polynucleotide comprising both the single-stranded polynucleotide and its perfect complement, are also disclosed. Polynucleotide sequences are listed in a 5' to 3' direction unless otherwise indicated.
  • the term "tag” refers to a moiety appended to another entity that imparts a characteristic or property otherwise not present in the un-tagged entity.
  • the tag is an affinity tag, an epitope tag, a fluorescent tag, etc.
  • fluorescent tags include GFP and other fluorescent proteins mentioned above.
  • Affinity tags can facilitate the purification or solubilization of fusion proteins.
  • affinity tags include maltose binding protein (MBP), glutathione-S-transferase (GST), thioredoxin, polyhistidine (also known as hexa histidine, 6xHis, and by the trademarked name HIS- TAG®), etc.
  • epitope tags which facilitate recognition by antibodies, include c- myc, FLAG (FLAG octapeptides), HA (hemagglutinin), etc.
  • catalyst refers to a substance the presence of which increases the rate and/or extent of a chemical reaction, while not being consumed or undergoing a permanent chemical change itself.
  • label and labeling moiety entity refer to agents that can be visualized, for example following binding to another entity.
  • the detectable agent or moiety may be selected such that it generates a signal which can be measured and whose intensity is related to (e.g., proportional to) the amount of bound entity.
  • a wide variety of systems for labeling and/or detecting proteins and peptides are known in the art. Labeled proteins and peptides can be prepared by incorporation of, or conjugation to, a label that is detectable by spectroscopic, photochemical, biochemical, immunochemical, electrical, optical, chemical or other means.
  • a label or labeling moiety may be directly detectable (i.e., it does not require any further reaction or manipulation to be detectable, e.g. , a fluorophore is directly detectable) or it may be indirectly detectable (i.e., it is made detectable through reaction or binding with another entity that is detectable, e.g., a hapten is detectable by immunostaining after reaction with an appropriate antibody comprising a reporter such as a fluorophore).
  • Suitable detectable agents include, but are not limited to, radionuclides, fluorophores, chemi luminescent agents, microparticles, enzymes, colorimetric labels, magnetic labels, haptens, Molecular Beacons, aptamer beacons, and the like.
  • the term “isolated” often refers to having a specific activity of at least tenfold greater than the sortase-transamidase activity present in a crude extract, lysate, or other state from which proteins have not been removed and also in substantial isolation from proteins found in association with sortase-transamidase in the cell.
  • An "isolated” or “purified” polypeptide or protein is substantially free of cellular material or other contaminating proteins from the cell or tissue source from which the protein is derived, or substantially free from chemical precursors or other chemicals when chemically synthesized.
  • the term "substantially free” refers to preparing a target polypeptide having less than about 30%, 20%, 10% and sometimes 5% (by dry weight), of non-target polypeptide (also referred to herein as a" contaminating protein"), or of chemical precursors or non-target chemicals.
  • the target polypeptide or a biologically active portion thereof is recombinantly produced, it also often is substantially free of culture medium, where culture medium represents less than about 20%, sometimes less than about 10%, and often less than about 5% of the volume of the polypeptide preparation.
  • isolated or purified target polypeptide preparations are 0. 01 milligrams or more.
  • isolated or purified target polypeptide preparations are 0.1 milligrams or more.
  • isolated or purified target polypeptide preparations are 1.0 milligrams or more and 10 milligrams or more in dry weight.
  • the invention encompasses all variations, combinations, and permutations in which one or more limitations, elements, clauses, descriptive terms, etc., from one or more of the claims or from the description (including specific details in the experimental section) is introduced into another claim dependent on the same base claim (or, as relevant, any claim) unless otherwise indicated or unless it would be evident to one of ordinary skill in the art that a contradiction or inconsistency would arise.
  • lists or sets of elements are disclosed herein it is to be understood that each subgroup of the elements and each individual element are also disclosed.
  • a polypepide is not GFP or a derivative thereof.
  • the invention encompasses inventive compositions used in performing the method, and products produced using the method. Where the description or claims recite a composition, the invention encompasses methods of using the composition and methods of making the composition. [00308] Where ranges are mentioned herein, the invention includes embodiments in which the endpoints are included, embodiments in which both endpoints are excluded, and embodiments in which one endpoint is included and the other is excluded. It should be assumed that both endpoints are included unless indicated otherwise.
  • Approximately or “about” generally includes numbers that fall within a range of 1% or in some embodiments 5% or in some embodiments 10% of a number in either direction (greater than or less than the number) unless otherwise stated or otherwise evident from the context (e.g., where such number would impermissibly exceed 100% of a possible value).
  • Protein-lipid conjugates and methods for their construction are valuable tools for studying the role of post-translational lipid modification in controlling protein function and localization. Lipid attachment also provides a means for manipulating the properties of peptides and proteins that normally do not possess these types of modifications. Highlighting the utility of synthetic lipoproteins, Bertozzi and co-workers recently reported the synthesis of GFP-containing GPI-anchor mimetics as a means for probing the role of individual sugar residues in this complex membrane anchor (1, 2). Numerous reports have also shown that the addition of lipids and fatty acids can endow proteins and peptides with cell-penetrating capabilities (3-7), modulate immunogenicity (8, 9), and provide anchors for incorporation into liposomes (10, 11).
  • EPL expressed protein ligation
  • sortase A from Staphylococcus aureus recognizes a five amino acid sequence (LPXTG) near the C-terminus of its natural protein targets (39-41).
  • LPXTG five amino acid sequence
  • the active site cysteine of sortase cleaves between the threonine and glycine residues of the recognition site to produce a thioester intermediate which is then attacked by the amino terminus of an oligoglycine nucleophile, resulting in the formation of a new amide bond.
  • the method is extremely versatile, stemming from the remarkable tolerance of the enzyme for substituents C-terminal to the oligoglycine unit.
  • Synthetic nucleophiles containing 1-5 glycine residues, have been decorated with a range of substituents including fluorophores (33, 34) photoaff ⁇ nity probes (34), peptide nucleic acids (36), polymers (35), solid supports (32, 35, 42) or other polypeptides (33, 38) allowing the site-specific ligation of these moieties to peptide and protein substrates.
  • Mass Spectrometry Electrospray Ionization (ESI) mass spectra were obtained at the MIT Department of Chemistry Instrumentation Facility. Matrix assisted laser desorption- ionization time-of-flight mass spectrometry (MALDI-TOF MS) was performed on a MALDI
  • MS analysis was performed using a Micromass LCT mass spectrometer (Micromass ® MS
  • HPLC/FPLC HPLC purifications were achieved using an Agilent 1100 Series
  • UV- Vis Spectrocopy was performed on a Nanodrop ND-
  • Resin-bound precursor 1 was prepared on Rink amide resin using standard Fmoc chemistry. An orthogonally protected lysine residue was incorporated to allow selective liberation and subsequent acylation of the ⁇ -amino group. Following removal of the 4- methyltrityl (Mtt) group, the lysine side chain was acylated with a range of hydrophobic carboxylic acids, including naturally occurring post-translational modifications such as myristic (1-C14) and palmitic (1-C16) acid, as well as modifications not found in eukaryotic cells (1-ad). The couplings of Cl 8, C20, C22, and C24 acids were performed at 50°C to maintain the solubility of all the reaction components.
  • Mtt 4- methyltrityl
  • Resin-Bound Intermediate 1 A glass solid-phase reaction vessel containing a fritted glass filter and a Teflon stopcock was loaded with Rink amide resin (1.0 g, 0.70 mmol). The resin was first washed/swollen extensively with N-methyl-2-pyrrolidone (NMP) by gentle agitation with a wrist action shaker. The Fmoc protecting group was then removed by treatment with -30 mL of 80:20 NMP/piperidine for 20 min at RT. The resin was washed with -30 mL of NMP (3x, 3-5 min per wash).
  • NMP N-methyl-2-pyrrolidone
  • Amino acid building blocks were then coupled as follows: Fmoc-protected amino acid (1.75 mmol, 2.5 equivalents relative to initial resin loading), benzotriazole- 1 -yl-oxy-tris-pyrrolidino-phosphonium hexafluorophosphate (PyBOP) (911 mg, 1.75 mmol), N-hydroxybenzotriazole (HOBt) (236 mg, 1.75 mmol), and N,N'-diisopropylethylamine (DIPEA) (914 ⁇ L, 5.25 mmol) were dissolved in NMP to a final volume of 8.75 mL (200 mM final concentration of amino acid building block).
  • the resin was then treated with a solution of the appropriate carboxylic acid (Ri-COOH, 0.12 mmol), PyBOP (65 mg, 0.12 mmol), HOBt (16 mg, 0.12 mmol), and DIPEA (65 ⁇ L, 0.38 mmol) in 1.0 mL of NMP.
  • the reaction was incubated at RT for 21 h followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash). Fmoc removal was achieved by treatment with 2.5 mL of 80:20 NMP/piperidine for 20 min at RT followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash) and 2.5 mL of CH2CI2 (3x, 3-5 min per wash).
  • the peptide was cleaved from the resin with 2.5 mL of 95:3:2 TFA/TIPS/H2O (4x, -30 min each) and the combined cleavage solutions were concentrated in vacuo. 1-ad was then precipitated from ether and dried under vacuum. Crude 1-C12 and crude 1-C14 were washed with hexanes (1 mL, 2x) and then dried under vacuum. The identity of all peptides was confirmed by LC- ESI-MS analysis ( Figure 11). Peptides were used without further purification and the yield was not determined.
  • the resin was then treated with a solution of palmitic acid (103 mg, 0.40 mmol), PyBOP (208 mg, 0.40 mmol), HOBt (54 mg, 0.4 mmol), and DIPEA (207 ⁇ L, 1.2 mmol) in 1.6 mL of NMP.
  • the reaction was incubated at RT overnight.
  • the resin was then washed with 2.5 mL of NMP (3x, 3-5 min per wash). Fmoc removal was achieved by treatment with 2.5 mL of 80:20 NMP/piperidine for 20 min at RT followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash) and 2.5 mL of CH2CI2 (3x, 3-5 min per wash).
  • the peptide was cleaved from the resin with 2.5 mL of 95:3:2 TFA/TIPS/H2O (4x, -30 min each) and the combined cleavage solutions were dried under vacuum.
  • the identity of 1-C16 was confirmed by LC-ESI-MS analysis ( Figure 11). This material was used without further purification and yield was not determined.
  • the resin was treated with a solution of the appropriate carboxylic acid (R2-COOH, 0.12 mmol), PyBOP (65 mg, 0.12 mmol), HOBt (16 mg, 0.12 mmol), and DIPEA (65 ⁇ L, 0.38 mmol) in 1.0 mL of NMP.
  • the reaction was incubated at 50 C for 5 h.
  • the reaction was then centrifuged, and 0.5 mL of the supernatant was discarded.
  • An additional 0.5 mL of NMP was then added followed again by centrifugation and removal of 0.5 mL of the supernatant. This process was repeated two additional times.
  • the resin slurry was carefully transferred to a 3.0 mL fritted polypropylene syringe equipped with a capped hypodermic needle and washed with 2.5 mL of NMP (3x, 3-5 min per wash). Fmoc removal was achieved by treatment with 2.5 mL of 80:20 NMP/piperidine for 20 min at RT followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash) and 2.5 mL of CH2CI2 (3x, 3-5 min per wash). The peptide was cleaved from the resin with 2.5 mL of 95:3:2 TFA/TIPS/H2O (3x, -30 min each) and the combined cleavage solutions were concentrated in vacuo.
  • Sortase-Mediated Ligation of Triglycine Nucleophiles to a Protein Substrate [00331] With a series of lipidated nucleophiles in hand, we proceeded to explore their coupling to a protein substrate using sortase.
  • Recombinant sortase A containing an N-terminal His 6 tag was produced as described (40).
  • we decided to incorporate a procedure for removing the sortase enzyme after the reaction similar to a purification scheme proposed by Parthasarathy et al. (35) but with important improvements.
  • eGFP-LPETG-His ⁇ cloning and expression were performed as follows: The gene encoding eGFP was PCR amplified from the commercially available pEGFP-Nl plasmid (Clontech) using forward primer 5'-CGCGCGCC ATGGTG AGC AAGGGCG AGG AG-3 1 and reverse primer 5'
  • the pellet was thawed and resuspended in 60 mL of 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole containing a protease inhibitor cocktail (complete mini tablet, EDTA- free, Roche) and treated with 240 ⁇ L of DNAse I (10 mg/mL in PBS), 480 ⁇ L of lysozyme (50 mg/mL in PBS), and 60 ⁇ L of MgCh (1 M in PBS). The lysis reaction was incubated for 1 h at 4°C. The cells were then sonicated and centrifuged to remove insoluble material.
  • the pellet was then treated with an additional 20 mL of 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole, briefly sonicated, and centrifuged.
  • the combined supernatants were applied to a Ni-NTA column consisting of 7.5 mL of commercial Ni-NTA slurry (Qiagen) equilibrated with 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole.
  • the column was washed with three 45 mL portion of 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole.
  • eGFP-LPETG-His ⁇ was eluted with -10 mL of 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 300 mM imidazole. This material was concentrated and further purified by size exclusion chromatography on a HiLoad 16/60 Superdex 75 column (Amersham), eluting with 20 mM Tris pH 8.0, 150 mM NaCl at a flow rate of 1 mL/min. Fractions containing eGFP-LPETG- His6 were pooled, concentrated, and stored at -80°C.
  • the eGFP-LPETG-His ⁇ stock was thawed and again purified by affinity chromatography over commercial Ni-NTA resin. After binding eGFP-LPETG-His 6 to the resin, the column was washed with three portions of 20 mM Tris pH 8.0, 150 mM NaCl, and 20 mM imidazole. The protein was eluted with 20 mM Tris pH 8.0, 150 mM NaCl, and 300 mM imidazole. This material was
  • Ni-NTA resin containing 1 M NaCl and 40 mM imidazole was then added, and the mixture was incubated for 2 h.
  • removal of His ⁇ -tagged proteins following transpeptidation was achieved with Ni-NTA resin treated in the following way: 500 ⁇ L of commercial Ni-NTA resin (Qiagen) was treated with 1 mL of 40 mM Tris pH 8.0, 1 M NaCl, and 40 mM imidazole. The mixture was then centrifuged and the supernatant was removed. This process was repeated two additional times. The resin was then suspended to a final volume of 500 ⁇ L with 40 mM Tris pH 8.0, 1 M NaCl, and 40 mM imidazole.
  • the eGFP chromophore provided a convenient method for quantifying the yield of the eGFP conjugates.
  • the absorbance at 488 nm of the conjugates relative to the input eGFP-LPETG-HiS ⁇ protein we estimated that the lipid-modified protein conjugates were all obtained in excellent (-60-90%) yield (Table 1 and Figure 14).
  • a reproducible drop in reaction yield for nucleophiles containing fatty acids of intermediate length (1-C16, 1-C18, 1-C20) was observed. Whether this reflects a drop in the efficiency of the actual transpeptidation reaction or limited solubility of the resulting lipoprotein conjugates, which could contribute to losses during the sortase depletion step, is presently unclear.
  • eGFP-LPETG- His6 (12.4 ⁇ L of a 110 ⁇ M solution in 20 mM Tris pH 8.0, 150 mM NaCl) and sortase A (8.35 ⁇ L of a 448 ⁇ M solution in 50 mM Tris pH 8.0, 150 mM NaCl, 10% glycerol (v/v))
  • reaction mixtures were incubated at 37 C for 5 h in the dark and then treated with 50 ⁇ L of the appropriate Ni-NTA slurry described above and incubated for an
  • the cells were washed three times with ⁇ 4 mL of cold PBS containing 1% FBS.
  • the cells were lifted from the culture plate by treatment with 1 mL of 1 mM EDTA in PBS and pelleted at 250 x g for 5 min.
  • the cells were then resuspended in 200 ⁇ L of PBS containing 1% FBS and propidium iodide (0.5 ⁇ M) and analyzed by flow cytometry (Figure 15).
  • lipid-modified eGFP 100Ox stock solutions of lipid-modified eGFP. Solutions of lipid-modified eGFP obtained by transpeptidation and depletion of His6-tagged proteins were used without further purification for cell membrane association studies. Prior to addition to cells, the concentration of eGFP in each sample was measured by UV -Vis (488 nm), and all solutions were adjusted to a final eGFP concentration of 2.5 mg/mL.
  • Dilutions were made with a mock reaction mixture lacking eGFP, sortase A, and lipidated triglycine nucleophile to ensure that all samples contained the same amount of residual components (n-dodecyl maltoside, imidazole, CaCb, etc.) from the sortase labeling procedure.
  • lipid-modified eGFP Cell culture and membrane association of lipid-modified eGFP.
  • HeLa cells were maintained in DME media supplemented with 10% fetal bovine serum (FBS), penicillin (50 units/mL), and streptomycin sulfate (50 ⁇ g/mL). Cells were incubated in a 5% CO2 humidified incubator at 37 C.
  • FBS fetal bovine serum
  • penicillin 50 units/mL
  • streptomycin sulfate 50 ⁇ g/mL
  • Cells were incubated in a 5% CO2 humidified incubator at 37 C.
  • One day prior to treatment with lipid-modified eGFP cells were seeded into 6-well polystyrene cell culture plates at a density of ⁇ 100,000 cells per well and incubated overnight. The media was then removed and replaced with 2 mL of serum-free DME containing 2.5 ⁇ g/mL modified eGFP (lipid modified proteins were delivered as 100Ox stock solutions,
  • Tek II chambered coverglass slides (Nalge Nunc International) and allowed to adhere overnight. The media was then removed and replaced with 200 ⁇ L of serum-free DME containing 2.5 ⁇ g/mL modified eGFP (lipid modified proteins were delivered as 100Ox stock
  • sortase enzyme itself could be perceived as a disadvantage of the transpeptidation strategy
  • the ready availability of sortase and ease of removal following transpeptidation are important features as the enzyme is relatively inefficient and excess sortase is typically employed in the art to drive the labeling reactions to high levels of conversion in a reasonable period of time.
  • the transpeptidation strategy is able to attach extremely hydrophobic modifications, it could provide a new method for interfacing proteins with materials that possess poor water solubility, such as carbon nanotubes.
  • Example 2 Modification of N-Terminal Glycine Residues using Structural Mimetics of the Sortase A Recognition Sequence
  • N-terminal transpeptidation was easily extended to two additional protein substrates (Figure 10).
  • eGFP bearing five glycines and the ubiquitin specific hydrolase UCH- L3 containing a single glycine were labeled efficiently as determined by ESI-MS.
  • eGFP bearing five glycines and the ubiquitin specific hydrolase UCH- L3 containing a single glycine were labeled efficiently as determined by ESI-MS. It should be noted that the utility of this labeling method for recombinant proteins expressed in E. coli is facilitated by natural processing of newly synthesized polypeptides by endogenous methionine aminopeptidase.
  • N-fmet N-formylmethionine
  • the removal of N-fmet is quantitative. Therefore, preparation of substrates for N-terminal transpeptidation requires only basic cloning techniques, and in most cases would only require a single residue substitution.
  • Example 3 Highly Efficient Sortase-Catalyzed Protein Circularization
  • This Example demonstrates that sortase-catalyzed transpeptidation can be used for efficient synthesis of circular and oligomeric proteins.
  • This method has general applicability, as illustrated by successful intramolecular reactions with three structurally unrelated proteins.
  • the multiprotein complex AAA- ATPase p97/VCP/CDC48 with six identical subunits containing the LPATG motif and an N- terminal glycine, was found to preferentially react in daisy chain fashion to yield linear protein fusions.
  • additional methods, and references please see, Antos, JM, et al.
  • Recombinant sortase A (residues 26-206) containing an N-terminal hexahistidine tag was produced in Escherichia coli as described previously (8). Purified sortase A was stored in 10% glycerol, 50 mM Tris, pH 8.0, 150 NaCl at -80 °C until further use.
  • G-Cre-LPETG-His 6 was cloned into the pTriEx-1.1 Neo expression vector (Novagen) using standard molecular biology techniques. The construct contains two point mutations (Ml 17V and E340Q) and a flexible spacer (GGGGSGGGGS) inserted before the LPETG sortase recognition site.
  • G-Cre-LPETG-His 6 was expressed and purified using procedures similar to those reported previously for HTNCre (24).
  • G-Cre-LPETG-His 6 was first transformed into Tuner (DE3) pLacI cells (Novagen), and a starter culture was grown in sterile LB media supplemented with 1% (w/v) glucose, chloramphenicol (34 ⁇ g/ml), and ampicillin (100 ⁇ g/ml). This culture was used to inoculate a large scale culture of sterile LB containing chloramphenicol (34 ⁇ g/ml) and ampicillin (100 ⁇ g/ml).
  • G-Cre-LPETG-His 6 was expressed after a 3-h induction with isopropyl 1-thio- ⁇ -D-galactopyranoside (0.5 ⁇ M) at 37 0 C.
  • Cells were resuspended in 10 mM Tris, 100 mM phosphate, 300 mM NaCl, and 20 HIM imidazole, pH 8.0.
  • the suspension was adjusted to 50 ⁇ g/ml DNase I, 460 ⁇ g/ml lysozyme, and 1 mM MgCl 2 and incubated at 4 °C for 1.5 h. The suspension was then sonicated and centrifuged.
  • the clarified lysate was then treated with Ni-NTA-agarose (Qiagen) for 1 h at 4 °C.
  • the resin was washed with 12 column volumes of 10 mM Tris, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole, pH 8.0, followed by 4 column volumes of 10 mM Tris, 100 mM phosphate, 300 mM NaCl, and 30 mM imidazole, pH 8.0.
  • the protein was then eluted with 10 mM Tris, 100 mM phosphate, 300 mM NaCl, and 300 mM imidazole, pH 8.0.
  • the purified protein was then dialyzed first against 20 mM Tris, pH 7.5, 500 mM NaCl followed by 50% glycerol, 20 mM Tris, pH 7.5, 500 mM NaCl.
  • G-Cre-LPETG-His 6 was then passed through a 0.22- ⁇ m filter to remove minor precipitation and stored at 4 °C.
  • G 5 -eGFP-LPETG-His 6 was prepared from a previously reported eGFP construct lacking the five N-terminal glycine residues using a QuickChange® II site-directed mutagenesis kit (Stratagene) and produced in E . coli using reported procedures (11). Purified G 5 -eGFP-LPETG-His 6 was buffer exchanged into 20 mM Tris, pH 8.0, 150 mM NaCl and stored at 4 °C. UCHL3 with the sortase recognition sequence (LPETG) substituted for amino acids 159-163 was cloned and produced in E . col i as described previously (25).
  • Cells were resuspended in buffer A (50 mM Tris, pH 8.0, 300 mM NaCl, 5% glycerol, 20 mM imidazole, and 7.1 mM ⁇ -mercaptoethanol), adjusted to 15 ⁇ g/ml lysozyme and 10 ⁇ g/ml DNase I, and lysed by two passes through a French pressure cell at 1200 p.s.i. After centrifugation for 30 min at 40,000 x g, the supernatant was bound to nickel-Sepharose resin (GE Healthcare). After washing the resin with 20 column volumes of buffer A, p97 was eluted with buffer A containing 250 ⁇ M imidazole.
  • buffer A 50 mM Tris, pH 8.0, 300 mM NaCl, 5% glycerol, 20 mM imidazole, and 7.1 mM ⁇ -mercaptoethanol
  • Diglycine and triglycine (GGG) peptides were purchased from Sigma. Reactions were halted by the addition of reducing Laemmli sample buffer and analyzed by SDS-PAGE. Gels were visualized by staining with Coomassie Blue. Fluorescence was visualized on a Typhoon 9200 Imager (GE Healthcare). Crude reactions were also diluted into either 0.1% formic acid or water for ESI-MS analysis.
  • ESI-MS was performed on a Micromass LCT mass spectrometer (Micromass® MS Technologies) and a Paradigm MG4 HPLC system equipped with an HTC PAL autosampler (Michrom BioResources) and a Waters symmetry 5- ⁇ m C8 column (2.1 x 50 mm, MeCN:H 2 O (0.1% formic acid) gradient mobile phase, 150 ⁇ l/min).
  • Micromass LCT mass spectrometer Micromass® MS Technologies
  • Paradigm MG4 HPLC system equipped with an HTC PAL autosampler (Michrom BioResources) and a Waters symmetry 5- ⁇ m C8 column (2.1 x 50 mm, MeCN:H 2 O (0.1% formic acid) gradient mobile phase, 150 ⁇ l/min).
  • G 5 -eGFP-LPETG-His 6 (50 ⁇ M) was circularized by treatment with sortase A (50 ⁇ M) in sortase reaction buffer (50 mM Tris, pH 7.5, 150 mM NaCl, 10 mM CaCl 2 ) for 24 h at 37 °C. The reaction was run on a 750- ⁇ l scale. The entire reaction was then diluted into 10 ml of 20 mM Tris, 500 mM NaCl, and 20 mM imidazole, pH 8.0.
  • sortase reaction buffer 50 mM Tris, pH 7.5, 150 mM NaCl, 10 mM CaCl 2
  • Circular and linear eGFP (40 ⁇ l of 18 ⁇ M solutions) was placed in 1.5-ml microcentrifuge tubes and denatured by heating to 90 °C for 5 min. Samples were then incubated at room temperature in the dark for the times indicated. Fluorescent images were acquired using a UV gel documentation system (UVP Laboratory Products).
  • UCHL3 (30 ⁇ M) was incubated with sortase A (150 ⁇ M) in sortase reaction buffer (50 mM Tris, pH 7.5, 150 mM NaCl, 10 mM CaCl 2 ) in the presence or absence of 90 mM GGG peptide (Sigma) on a 25- ⁇ l scale at 37 °C for 3 h. Ten microliters was withdrawn and diluted with 10 ⁇ l of labeling buffer (100 mM Tris, pH 7.5, 150 mM NaCl).
  • Hemagglutinin epitope- tagged ubiquitin vinyl methyl ester (4 ⁇ g) was added as well as 1 mM dithiothreitol and incubated at room temperature for 1 h. Reactions were then separated on an SDS- polyacrylamide gel and visualized by Coomassie staining or ⁇ -HA immunoblot (supplemental Fig . S4). Hemagglutinin epitope-tagged ubiquitin vinyl methyl ester was prepared following published protocols (27).
  • the band corresponding to circular UCHL3 was excised and digested with GIu-C. Crude transpeptidation reactions containing dimeric p97 were separated by SDS-PAGE followed by Coomassie staining. The transpeptidation reaction used for this purpose was incubated for only 2 h and therefore contains less oligomerization than that seen after an overnight incubation (see supplemental Fig . S6). The band corresponding to dimeric p97 was excised and digested with chymotrypsin. For all protein substrates, the peptides generated from proteolytic digestion were extracted and concentrated for analysis by RP-HPLC and tandem mass spectrometry.
  • RP-HPLC was carried out on a Waters NanoAcquity HPLC system with a flow rate of 250 nl/min and mobile phases of 0.1% formic acid in water and 0.1% formic acid in acetonitrile.
  • the gradient used was isocratic 1% acetonitrile for 1 min followed by 2% acetonitrile per min to 40% acetonitrile.
  • the analytical column was 0.075 ⁇ m x 10 cm with the tip pulled to 0.005 ⁇ m and self-packed with 3 ⁇ m Jupiter Cl 8 (Phenomenex).
  • the column was interfaced to a Thermo LTQ linear ion trap mass spectrometer in a nanospray configuration, and data were collected in full scan mode followed by MS/MS analysis in a data-dependent manner.
  • the mass spectral data were data base searched using SEQUEST.
  • eGFP Having verified the cyclization of Cre recombinase, we sought to explore the generality of this technique. To this end we generated a derivative of eGFP containing the LPETG sequence and five N-terminal glycine residues. This construct was of particular interest because inspection of the x-ray crystal structure (3J . ) revealed that the N and C termini were positioned on the same end of the ⁇ -barrel, suggesting that this substrate should be ideal for cyclization (Fig. 28A). Furthermore, in one of the earliest reports on the use of sortase for protein engineering, a similar eGFP substrate was described and reported to cyclize in the presence of sortase Q6).
  • Circularization has been shown to confer unique properties onto proteins when compared with the linear form (35-32)- m the case of GFP circularized using intein-based methods, these properties include a reduced rate of unfolding when exposed to denaturants, as well as an enhanced rate of refolding following denaturation (35_).
  • Fig. 28C Circular eGFP was first separated from residual sortase A using Ni-NTA resin. This material retained fluorescence suggesting that covalent ligation of the N and C termini had minimal impact on the structure of this substrate.
  • Circular and linear eGFP were then subjected to simple thermal denaturation, followed by recovery at room temperature. As shown in Fig. 28C, circular eGFP regained fluorescence more rapidly than linear eGFP.
  • UCHL3 Even an internally positioned LPATG motif was sufficient to effectuate a circularization reaction.
  • UCHL3 We installed a sortase recognition site in the crossover loop of the ubiquitin C-terminal hydrolase UCHL3, and we demonstrated that the continuity of the polypeptide backbone can be disrupted with concomitant installation of a covalent modification that reports on the accuracy of cleavage and transpeptidation (25).
  • This reaction proceeds without complete loss of activity of UCHL3, indicating that even the cleaved form of UCHL3 retains its structural integrity to a significant degree (25).
  • This UCHL3 construct was prepared with an N-terminal glycine residue, and examination of the crystal structure of UCHL3 (30) clearly showed the close apposition of the N terminus and the crossover loop, suggesting that cyclization to yield a circular fragment containing the N-terminal portion of UCHL3 should be readily observable (Fig. 29A).
  • the N-terminal glycine serves as a highly efficient nucleophile to yield a circular fragment that contains the N-terminal portion of UCHL3 (Fig. 29B).
  • the identity of the circular polypeptide was confirmed by MS/MS of the peptide containing the expected fusion of the N-terminal glycine residue with the new C terminus released from the crossover loop (see supplemental Fig. S2). Cyclization was efficiently blocked if a high concentration of triglycine (GGG) was included in the reaction, generating instead the N-terminal fragment of UCHL3 transacylated onto the triglycine nucleophile (Fig. 29B, lane 9, and supplemental Fig.
  • p97 a hexameric AAA-ATPase.
  • G-His 6 -p97-LPSTG-XY a derivative of p97 containing an LPSTG motif near the C terminus, and a hexahistidine tag capped by two serine residues and a single glycine at the N terminus.
  • the structure of a p97 trimer in the presence of ADP has been solved at 3.5 A resolution (28), with several residues from the N and C termini not visible (Fig. 30A).
  • sortase-mediated circularization is efficient despite the potential for competing reaction pathways.
  • these include hydrolysis of the acyl enzyme intermediate, reattachment of the C-terminal protein fragment that is lost upon initial cleavage of the protein substrate by sortase, or, as mentioned above, oligomerization of protein monomers in head-to-tail fashion.
  • millimolar concentrations are necessary to efficiently compete with cyclization.
  • One factor that certainly must contribute to this observed preference for cyclization is the distance between protein termini.
  • sortase fails to cleave LPATG motifs placed in structured loops of class I major histocompatibility complex molecules (14).
  • the sortase-catalyzed approach also provides additional levels of control over the ensuing transpeptidation reaction. This may be particularly useful for oligomeric species, such as the p97 example described here.
  • our modified p97 protein G-His 6 -p97- LPSTG-XX
  • Cross-linking is then induced by the addition of sortase after the individual subunits have been correctly positioned in the hexameric ring.
  • transpeptidation can be further controlled by inclusion of synthetic oligoglycine nucleophiles, either during the transpeptidation reaction or after transpeptidation is complete. The latter scenario even allows cyclization to be completely reversed. Incubating circular protein products with sortase in the presence of an oligoglycine nucleophile restores linearity to the protein product, because in the course of the initial cyclization reaction, the LP XTG motif is restored. An equilibrium between closed and open forms is thus established and can be driven toward the linear state by adding a large excess of the oligoglycine nucleophile.
  • SrtAstrep The expression plasmid for SrtAstrep (residues 82-249) including an
  • N-terminal His6 tag has been described.
  • the construct was transformed into E. coli BL-21. Cells were grown in 2 L of sterile LB containing kanamycin (30 ⁇ g/mL) to an optical density of -0.7 at 600 nm. Cells were induced with IPTG (1 mM) for 3 h at 37 C. Cells were
  • Ni-NTA column consisting of 5.0 mL of commercial Ni-NTA slurry (Qiagen) equilibrated with 50 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole, and 10% glycerol. The column was washed with 80 mL of 50 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole, and 10% glycerol.
  • Protein was eluted with five 5 mL portions of 50 mM Tris pH 8.0, 150 mM NaCl, 300 mM imidazole, and 10% glycerol. Fractions containing SrtAstrep were pooled and further purified by size exclusion chromatography on a HiLoad 16/60 Superdex 75 column (Amersham), eluting with 20 mM Tris pH 8.0, 150 mM NaCl at a flow rate of 1 mL/min. Fractions containing SrtAstrep were pooled and subjected to a second round of Ni-aff ⁇ nity chromatography. Purified SrtAstrep was then dialyzed against 50 mM Tris pH 8.0, 150 mM NaCl, and 10% glycerol. These solutions were stored at -80 C until further use. Protein concentration was estimated by
  • His6 tag was produced in E. coli as previously described. SrtAstaph does not contain an N- terminal glycine residue (retains initiator methionine). Purified SrtAstaph was stored in 10% (w/v) glycerol, 50 mM Tris pH 8.0, 150 NaCl at -80 °C until further use. Protein concentration was estimated by Bradford assay.
  • ⁇ 59-SrtAstaph Recombinant ⁇ 59-SrtAstaph (residues 60-206) containing an N- terminal His6 tag was cloned into p ⁇ T28a+. 59-SrtAstaph does not contain an N-terminal glycine residue (retains initiator methionine). Expression of ⁇ 59-SrtAstaph was achieved following the protocol described above for SrtAstrep. Purification by size exclusion chromatography was not necessary because ⁇ 59-SrtAstaph was sufficiently pure following Ni-affinity chromatography.
  • CtxB The template for construction of Gl-CtxB, G3-CtxB, G5-CtxB, and AG4- CtxB consisted of the B-subunit of cholera toxin fused at its N terminus to the signal peptide
  • E. coli heat labile enterotoxin LTIIb This targets the expressed protein to the periplasm where the signal peptide is removed. Glycine and/or alanine residues were inserted between the signal sequence and CtxB via Quickchange® II Site-Directed Mutagenesis (Stratagene). Plasmids were transformed into E. coli BL21. Cells were grown in 1 L of sterile LB containing chloroamphenicol (34 ⁇ g/mL) to an optical density of -0.5-1.0 at 600 nm.
  • Ni-NTA although it does not possess a His6 tag.
  • the Ni-NTA mixture was incubated at 4 C for 1 h and then poured into a fritted plastic column (Bio-Rad). The resin was washed with 40 mL of 50 mM Tris pH 8.0 and 300 mM NaCl. Protein was eluted with two 10 mL portions of 50 mM Tris pH 8.0, 300 mM NaCl, and 300 mM imidazole. Purified CtxB was buffer exchanged into 20 mM Tris pH 8.0 and 150 mM NaCl. Solutions were stored at 4 C. Protein concentration was estimated by Bradford assay.
  • G5-eGFP and dual labeling eGFP substrate were prepared in pET28a+ (Novagen) using a Quickchange® II Site-Directed Mutagenesis Kit (Stratagene). The template plasmid used for mutagenesis has been described. 6 Plasmids were then transformed into E. coli BL-21. In a typical experiment, cells were grown in sterile LB containing kanamycin (30 ⁇ g/mL) to an optical density of ⁇ 0.6-0.9 at 600 nm. Cells were induced with
  • the pellet was thawed and resuspended in 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40.
  • the cell suspension was then lysed by French press and centrifuged.
  • the clarified lysate was then applied to a Ni-NTA column consisting of 5.0 mL of commercial Ni-NTA slurry (Qiagen) equilibrated with 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40.
  • the column was washed with 40 mL of 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40, followed by 40 mL of 20 mM Tris pH 8.0, 150 mM NaCl, and 20 mM imidazole. Protein was eluted with 20 mM Tris pH 8.0, 150 mM NaCl, and 300 mM imidazole until the characteristic green color was fully removed from the column.
  • This material was concentrated and further purified by size exclusion chromatography on a HiLoad 16/60 Superdex 75 column (Amersham), eluting with 20 mM Tris pH 8.0, 150 mM NaCl at a flow rate of 1 mL/min. Fractions containing eGFP were pooled and subjected to a second round of Ni-affinity chromatography. Purified eGFP was then buffer exchanged into 20 mM Tris pH 8.0, 150 mM NaCl using a PD-10
  • UCHL3 and dual labeling UCHL3 substrate were produced in E. coli as described previously. This construct (in pET28a+, Novagen) was then used to prepare the dual labeling UCHL3 substrate. Synthetic 5'-phosphorylated oligonucleotide duplexes containing appropriate sticky ends were designed to achieve insertion of an N-terminal thrombin site and a C-terminal LPETG sequence separated from UCHL3 by a GGGGSGGGGS spacer in two sequential cloning steps. Duplexes were annealed before ligation into the parent vector.
  • the C-terminal insertion was performed first using the Pstl and Xhol restriction sites.
  • the result of using the Xhol site was the addition of a His6-tag after the LPETG sequence.
  • the N-terminal insertion was then achieved using the Xbal and Ndel restriction sites.
  • This plasmid was then transformed into E. coli BL21. Cells were grown in sterile LB containing kanamycin (30 ⁇ g/mL) to an optical density of -0.6-0.9 at 600 nm.
  • the column was washed with 40 mL of 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40, followed by 40 mL of 20 mM Tris pH 8.0, 150 mM NaCl, and 20 mM imidazole. Protein was eluted with 20 mM Tris pH 8.0, 150 mM NaCl, and 300 mM imidazole.
  • This material was then purified by anion-exchange chromatography on a Mono Q 5/50 GL column (Amersham) [Buffer A (50 mM Tris pH 7.5, 5 mM DTT, 0.5 mM EDTA), Buffer B (50 mM Tris pH 7.5, 5 mM DTT, 0.5 mM EDTA, 500 mM NaCl), 1.5 mL/min, gradient: 100% Buffer A (0-15 mL), 0% Buffer B ⁇ 50% Buffer B (15-45 mL), 50% Buffer B (45-50 mL)].
  • Buffer A 50 mM Tris pH 7.5, 5 mM DTT, 0.5 mM EDTA
  • Buffer B 50 mM Tris pH 7.5, 5 mM DTT, 0.5 mM EDTA, 500 mM NaCl
  • 1.5 mL/min gradient: 100% Buffer A (0-15 mL), 0% Buffer B ⁇ 50% Buffer B (15-45 mL
  • Fractions containing UCHL3 were pooled and further purified by size exclusion chromatography on a HiLoad 16/60 Superdex 75 column (Amersham), eluting with 20 mM Tris pH 8.0, 150 mM NaCl at a flow rate of 1 mL/min.
  • N-terminal labeling N-terminal transpeptidation reactions were performed by combining the necessary proteins/reagents at the specified concentrations in the presence of SrtAstaph or ⁇ 59-SrtAstaph in sortase reaction buffer (50 mM Tris pH 7.5, 150 mM NaCl, 10 mM CaC12) and incubating at 37 °C for the times indicated. Reactions were either diluted with 2x reducing Laemmli sample buffer for SDSPAGE analysis or diluted with water ( ⁇ 50 fold) for ESI-MS analysis. Gels were visualized by staining with coomassie blue. Fluorescence was visualized on a Typhoon 9200 Imager (GE Healthcare).
  • ESI-MS was performed on a Micromass LCT mass spectrometer (Micromass® MS Technologies, USA) and a Paradigm MG4 HPLC system equipped with a HTC PAL autosampler (Michrom BioResources, USA) and a Waters Symmetry 5 m C8 column (2.1 x 50 mm, MeCN:H2O (0.1% formic acid) gradient mobile phase, 150 L/min).
  • reaction was incubated for 7 h at 37 C.
  • ESIMS analysis of the crude reaction mixture revealed excellent conversion to the desired product (Supporting Figure S6a).
  • the reaction was then treated with [2-(trimethylammonium)ethly] methane thiosulfonate bromide (MTSET) (2.5 L of a 500 mM solution in 1 :1 DMSO/H2O) for 10 min at room temperature to quench SrtAstrep.
  • MTSET [2-(trimethylammonium)ethly] methane thiosulfonate bromide
  • the entire reaction was then diluted with 5 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole.
  • TM solution was then concentrated and passed over a PD-10 Sephadex desalting column (equilibrated with 20 mM Tris pH 8.0, 150 mM NaCl) to remove excess 3. This material was concentrated to ⁇ 800 L and subjected to thrombin cleavage.
  • Thrombin CleanCleave Kit Sigma. This mixture was incubated for 1 h at 37 C, and then checked by ESI-MS to ensure quantitative cleavage (Figure 35). The reaction was then filtered to remove the thrombin beads.
  • TM passed over a PD-10 Sephadex desalting column (equilibrated with 20 mM Tris pH 8.0). This material was then purified by anion-exchange chromatography on a Mono Q 5/50 GL column (Amersham) [Buffer A (20 mM Tris pH 8.0), Buffer B (20 mM Tris pH 8.0, 1 M NaCl), 1.5 mL/min, gradient: 100% Buffer A (0-15 mL), 0% Buffer B ⁇ 50% Buffer B (15- 45 mL), 50% Buffer B (45-50 mL)]. Fractions containing dual labeled eGFP were pooled and analyzed by SDS-PAGE and ESI-MS.
  • the resulting modification is disulfide linked, and is easily removed by treatment with DTT following completion of the dual labeling procedure].
  • the diluted reaction solution was then passed over a 1.5 mL column of Ni-NTA that been equilibrated with 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole.
  • the column was then washed with 1.5 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole.
  • UCHL3 solution was then concentrated and passed over a PD-10 Sephadex desalting column (equilibrated with 20 mM Tris pH 8.0, 150 mM NaCl) to remove excess 3. This material was concentrated to 1 mL and subjected to thrombin cleavage. [00451] Thrombin cleavage ofUCHL3. All 1 mL of the solution described above was combined with 100 L of 10x cleavage buffer and 100 L of thrombin agarose beads (from
  • Thrombin CleanCleave Kit Sigma. This mixture was incubated for 1 h at 37 degrees C, and then checked by ESI-MS to ensure quantitative cleavage (Figure 35). The reaction was then filtered to remove the thrombin beads.
  • the column was then washed with 2.0 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole.
  • the eluate was TM then desalted using PD-IO Sephadex columns (equilibrated with 20 mM Tris pH 8.0).
  • This material was then purified by anion-exchange chromatography on a Mono Q 5/50 GL column (Amersham) [Buffer A (20 mM Tris pH 8.0), Buffer B (20 mM Tris pH 8.0, 1 M NaCl), 1.5 mL/min, gradient: 100% Buffer A (0-15 mL), 0% Buffer B ⁇ 50% Buffer B (15-45 mL), 50% Buffer B (45-50 mL)].
  • sortase B from either Staph, aureus or Bacillus anthracis as enzymes with recognition sequences (NPQTN and NPKTG, respectively) orthogonal to that of SrtA staph .(9, 10). Both SrtB enzymes were easily produced in Escherichia coli and purified to homogeneity. We reproduced the reported in vitro enzyme activity using a FRET-based assay to measure cleavage of short peptides substrates (9, 10). However, we did not obtain transpeptidation with either SrtB on protein substrates modified with the appropriate recognition sequences on a time scale or with yields that compare favorably with SrtA sta p h (data not shown).
  • This example describes PEGylation of the four-helix bundle cytokine interferon ⁇ at the C-terminus using sortase and demonstrates that the PEGylated version retains activity and has enhanced in vivo circulating time.
  • pET28a+ vector Novagen
  • SrtA sta p h recognition site separated from the body of the protein by two glycines (Fig 39A).
  • Fig 39A For purification, we added a 6-His tag following the SrtA sta p h cleavage site; this tag is lost upon transpeptidation.
  • Sortase labeling was conducted as described previously (see, e.g., other Examples herein). PEGylated protein was purified by cation exchange chromatography on a Mono-S column (GE) at pH 5.0 or 4.5. Protein concentrations were measured by the Bradford method.
  • sortase reactions are equilibrium reactions and the sortases SrtAstrep and SrtA sta ph are orthogonal in one direction only (SrtA stre p cleaves both LPXTG and LPXTA sites but SrtA st aph attacks only LPXTG), we sought to render the sortase cleavage site on the nucleophile refractory to cleavage during the initial installation of the probe. To that end, we have generated a nucleophile bearing an LPXtG sequence, where t is a phosphorylated threonine residue.
  • the first transpeptidation step can be accomplished without premature cleavage of the SrtA staph site on the PEG nucleophile.
  • the resulting conjugate can then be dephosphorylated and incubated with SrtA st aph (which will not cleave the LPETAA junction between the protein and nucleophile) to join the termini.
  • This site is competent to undergo the second transacylation step; we installed a triglycine nucleophile onto this site by incubating with SrtA staph and GIy 3 peptide (Sigma) (Fig. 44).
  • SrtA staph SrtA staph
  • GIy 3 peptide Sigma
  • Example 8 Sortase-Mediated Installation of a Non-Genetically Encoded Element Between Two Proteins
  • Example 7 The strategy described in Example 7 can be used to install a non-genetically encoded element between two proteins or protein domains as shown, e.g., in Fig. 45.
  • a specific example is the construction of a cytokine variant joined to the Fc region of an antibody, with a non-genetically encoded moiety in the intervening region. Genetic fusions of cytokines to Fc regions can be delivered non-invasively into the bloodstream by Fc receptor bearing epithelial cells in the lungs, after which the half-life of the molecule is prolonged.
  • Implicit in this mechanism is the requirement for an Fc region that is able to bind to its cognate Fc receptor, and thus chemical conjugation of a molecule to the C-terminus or an internal lysine of the Fc portion would likely decrease binding capacity.
  • Using two transacylation steps we will install a PEG moiety onto the C-terminus of the cytokine portion, followed by installation of an unhindered Fc region.
  • Such a conjugate may show even greater gains in half-life relative to the genetic Fc fusion, as kidney filtration of the molecule is predicted to be further reduced.
  • Other applications include installing a detectable label, e.g., for diagnostic purposes or to monitor the distribution or elimination of the molecule in vivo.

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Abstract

The present invention relates to methods for ligation. The invention provides novel reagents and methods for ligating an acyl donor compound with an acyl acceptor compound. Provided acyl donor compounds comprise a transamidase recognition sequence that allows ligation with a nucleophilic acyl acceptor in the presence of transamidase. The invention further provides kits comprising acyl donor compounds and optionally comprising other reagents for ligation.

Description

METHODS FOR LIGATION AND USES THEREOF
GOVERNMENT SUPPORT
[0001] The invention was supported in part by grants from the National Institutes of Health (R01-AI057182, P01-CA100707, R01-AI033456, R21-EB008875. The government has certain rights in the invention.
CROSS-REFERENCE TO RELATED APPLICATION
[0002] This application claims the benefit of U.S. Provisional Application No. 60/361,759, filed January 30, 2009. The entire teachings of the provisional application are incorporated herein by reference.
FIELD OF THE INVENTION
[0003] The present invention relates to compositions and methods for ligation and uses thereof. The invention provides novel reagents and methods for ligating an acyl donor compound with a nucleophilic acyl acceptor compound to form an amide bond using a transamidase. The invention also relates to novel products, e.g., novel polypeptides, that can be produced using transamidate-mediated ligation.
BACKGROUND OF THE INVENTION
[0004] Protein engineering is becoming a widely used tool in many areas of protein biochemistry. One engineering method is controlled protein ligation, and over the past ten years some progress has been made. For instance, synthetic-based chemistry allows the joining of synthetic peptides together through native chemical ligation and a 166 amino-acid polymer-modified erythropoiesis protein has been synthesized using this method. However, native chemical ligation relies on efficient preparation of synthetic peptide esters, which can be technically difficult to prepare for large polypeptides such as proteins. For example, the reaction sometimes is performed in an organic solvent to produce the requisite protein ester for ligation. Other ligation methods not requiring the production of protein esters generate protein thioesters. An intein-based protein ligation system was used to generate a protein by thiolysis of a corresponding protein- intein thioester fusion. A prerequisite for this intein- mediated ligation method is that the target protein is expressed as a correctly folded fusion with the intein, and that sufficient spacing between the target and intein is needed to allow formation of the intein-thioester. In many instances, the intein-fusion proteins can only be obtained from inclusion bodies when expressed in Escherichia coli, which often cannot be refolded. This difficulty significantly limits the application of intein-based protein ligation methods.
[0005] Purification of a tag- free recombinant protein often is challenging and often requires multiple chromatography steps. A tag can be linked to a recombinant protein, and after purification, the tag on the fusion may be cleaved from the target protein by treatment with an exogenously added site-specific protease. Additional chromatographic steps then are required to separate the target protein from the uncleaved fusion, the affinity tag, and the protease. For example, an N-terminal 6x His tag from a recombinant protein may be cleaved by an engineered 6x His-tagged aminoprotease, and a subtractive immobilized metal-ion affinity chromatography (IMAC) step can be used to recover the untagged target. Other methods may require two or more chromatography steps and even special treatment of the exogenous protease, such as biotinylation, to facilitate its removal.
[0006] Methods for the site-specific modification of proteins remain in high demand, and the transpeptidation reaction catalyzed by sortases has emerged as a general method for derivatizing proteins withvarious types of modifications. Target proteins are engineered to contain the sortase A recognition motif (LPXTG) near their C-termini. When incubated with synthetic peptides containing one or more N-terminal glycine residues and a recombinant sortase, these artificial sortase substrates undergo a transacylation reaction resulting in the exchange of residues C-terminal to the threonine residue with the synthetic oligoglycine peptide.
SUMMARY OF THE INVENTION
[0007] The present invention encompasses the recognition that existing methods of transamidase ligation suffer from competition effects and efficiency issues. The inventors sought to extend the practical applications of sortase-mediated ligation to include ligation/labeling at the polypeptide N-terminus using synthetic peptides containing the LPXTG motif and protein substrates with N-terminal glycine residues. In the course of these efforts it was recognized that each successful transfer of an LPXT unit to a target protein releases a stoichiometric amount of a peptide fragment containing an N-terminal glycine. This by-product competes with the protein nucleophile for the same acyl enzyme intermediate, thereby limiting the efficiency of the ligation reaction. In certain aspects, the invention provides compositions and methods that facilitate N-terminal ligation using a transamidase, e.g., a sortase. According to one aspect, the present invention provides methods of ligation utilizing a modified transamidase recognition sequence. In some embodiments, a modified transamidase sequence comprises an ester group in place of a C- terminal amino acid residue.
[0008] According to one aspect, the present invention provides a method of ligation comprising the step of contacting an acyl donor compound of formula:
O
A1- Transamidase recognition sequence iΛ XR1 wherein the transamidase recognition sequence is any peptide motif recognized by a transamidase enzyme; X is -O-, -NR-, or -S-; R is hydrogen, substituted or unsubstituted aliphatic, or substituted or unsubstituted heteroaliphatic; A1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; R1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, or substituted or unsubstituted heteroaryl; and with a nucleophilic compound of formula:
Figure imgf000004_0001
wherein
B1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; and n is an integer from 0 to 100, inclusive; in the presence of a transamidase enzyme under suitable conditions to form a compound of formula:
Figure imgf000005_0001
[0009] In some embodiments, the recognition sequence is LPXT, wherein X is the amino acid D, E, A, N, Q, K, or R.
[0010] In another aspect, the present invention provides a ligation method comprising the step of contacting an acyl donor compound of formula:
Figure imgf000005_0002
wherein
A1, X, and R1 are defined as described above; and R2 is a natural or unnatural amino acid side chain; with a nucleophilic compound of formula:
Figure imgf000005_0003
wherein
B , 1 and n are are defined as described above; in the presence of a transamidase enzyme under suitable conditions to form a compound of formula:
Figure imgf000005_0004
In some embodiments, X is -O-. In some embodiments, R1 is Ci-6 aliphatic. In some embodiments, R is methyl. In some embodiments, R is a natural amino acid side chain. In some embodiments, R2 is the side chain group of arginine. In some embodiments, R2 is the side chain group of glutamic acid. In some embodiments, R2 is the side chain group of lysine. In some embodiments, A and B are each selected from the group consisting of an antibody, an antibody chain, an antibody fragment, an antibody epitope, a recombinant protein, a peptide comprising one or more D-amino acids, a branched peptide, a therapeutic protein, an enzyme, a polypeptide subunit of a multisubunit protein, a transmembrane protein, a cell surface protein, a methylated peptide or protein, an acylated peptide or protein, a lipidated peptide or protein, a phosphorylated peptide or protein, and a glycosylated peptide or protein. In certain embodiments, n is 2. In certain embodiments, n is 4. [0011] In some embodiments, the transamidase is a sortase. In certain embodiments, the sortase is sortase A. In certain embodiments, the sortase is sortase B. [0012] According to one aspect, the present invention provides a compound of formula:
O
.1— Transamidase recognition sequence XR1 wherein the transamidase recognition sequence, A1, X, and R1 are as defined above and described herein. In certain embodiments, X is -O- and R1 is methyl.
[0013] According to one aspect, the present invention provides a compound of formula:
Figure imgf000006_0001
wherein A1, X, R1, and R2 are as defined above and described herein. In certain
embodiments, the compound is of formula:
Figure imgf000006_0002
[0014] According to one aspect, the present invention provides kits comprising an acyl donor compound as described herein. In some embodiments, the kit further comprises a transamidase. In some embodiments, the kit further comprises a sortase. In some embodiments, the kit provides a nucleophilic acyl acceptor as described herein. [0015] One aspect of the instant invention is improved methods for removing sortase from a reaction system in which sortase has been used to perform a transamidation reaction. See Example 1 for exemplary description. It will be appreciated that the methods though described in reference to particular materials, are generalizable to other materials. [0016] Other aspects of the invention are methods and compositions related to use of multiple sortases, recognizing different motifs, for multiple labeling of polypeptides and other applications.
[0017] Other aspects of the invention provide masked transamidase recognition sequences and compounds containing them and methods of use thereof, e.g., for modifying polypeptides. In some aspects, the invention provides methods and compositions relating to use of transamidase-mediated, e.g., sortase-mediated, transpeptidation for the site-specific attachment of a moiety, e.g., a non-polypeptide polymer, e.g., polyethylene glycol or a derivative thereof, to a protein, e.g., a clinically useful protein, to enhance at least one property of the protein, such as extend the circulating half-life, while maintaining high biological activity, as well as covalently joining the N- and C- termini of the protein, e.g. to increase thermal stability. In some aspects, the inventive methods and compositions combine both of these properties by exploiting two distinct transamidase, e.g., sortase, enzymes and engineering a suitable compound (sometimes referred to herein as a "probe") that allows for site-specific modification (e.g., PEGylation) as well as allowing covalent closure in a second transamidase-mediated reaction. The invention provides a circularized version of a polypeptide, wherein the original C- and N-termini of the polypeptide are joined to each other via a linker peptide, wherein the linker peptide comprises a transamidase recognition sequence. In some embodiments of the invention, the polypeptide is a four-helix bundle polypeptide, e.g., a four-helix bundle cytokine. In some embodiments the polypeptide is a secreted polypeptide. In some embodiments the polypeptide binds to a cellular receptor. In some embodiments, the C-terminus, N-terminus, or both, of the polypeptide are not involved in receptor binding.
[0018] The entire contents of all references cited above and herein (including databases and sequences associated with accession numbers) are hereby incorporated by reference. BRIEF DESCRIPTION OF THE DRAWING
[0019] Figure 1. (a) Optimization of a two-step protocol for lipid ligation followed by removal of the sortase enzyme. Conditions: 77 μM eGFP-LPETG-Hisό, 150 μM sortase A, 2 mM nucleophile, 1% (w/v) detergent, 50 mM Tris, pH 7.5, 150 mM NaCl, 10 mM CaC12, 3 h at 37 °C. After transpeptidation, Ni-NTA resin was added as a slurry in 1 M NaCl and 40 mM imidazole and incubated for 2 h at room temperature. Abbreviations: OG = n-octyl glucoside, DM = n-dodecyl maltoside, DOC = deoxycholate. The asterisks indicate samples not treated with Ni-NTA resin, (b) ESI-MS spectrum of eGFP-LPET-l-C22 ligation product. [0020] Figure 2. Lipid attachment through sortase-catalyzed transpeptidation: (a) optimized procedure for lipid coupling followed by removal of His6-tagged proteins with Ni- NTA resin, (b) SDS-PAGE analysis of lipid-modified eGFP following transpeptidation and depletion of His6-tagged proteins ("Input" = eGFP-LPETG-His6 in the absence of sortase and nucleophile; the asterisks indicate samples incubated with Ni-NTA resin and 300 mM imidazole to block binding of Hisό-tagged proteins).
[0021] Figure 3. Association of lipid-modified eGFP with HeLa cells. Cells were incubated with lipid-modified eGFP (2.5 μg/mL) for 1 h in serum-free medium and then analyzed by flow cytometry. Numbers in parentheses represent the fold enhancement in mean cellular fluorescence relative to that of eGFP-GGG. Histograms for eGFP-GGG (black) and eGFP- 1 -ad (gray) are overlapping.
[0022] Figure 4. Subcellular distribution of eGFP-l-C22 and eGFP-2-chol in U373 and HeLa cells. Cells were incubated with lipid-modified eGFP (2.5 μg/mL) at 37 °C in serum- free medium and then imaged live using spinning disk confocal microscopy. Key: (a) U373 cells, 1 h of incubation, (b) U373 cells, 5 h of incubation, (c) HeLa cells, 1.25 h of incubation, (d) HeLa cells, 5 h of incubation.
[0023] Figure 5. eGFP-l-C22 is able to access early endosomal compartments as determined by partial colocalization with transferrin- Alexa 647. U373 cells were incubated with eGFP-l-C22 (2.5 μg/mL) for 5 h in serum-free medium followed by the addition of transferrin- Alexa 647 (100 μg/mL) during the final 15 min. White arrows indicate vesicles with positive staining for both eGFP-l-C22 and transferrin-Alexa 647. Significant colocalization between eGFP-2-chol and transferrin-Alexa 647 was not observed. [0024] Figure 6. Scheme 1. Site-Specific Lipid Attachment through Sortase-Mediated Transpeptidation. [0025] Figure 7. Scheme 2. Synthesis of Lipid-Modified Triglycine Nucleophiles. [0026] Figure 8. Schematic representation of N-terminal labeling method using protein substrates with N-terminal glycine residues and ligating them to synthetic peptides containing the LPXTG motif or structural analogs of this sequence element.
[0027] Figure 9. (a) Fluorescence gel scan showing robust labeling of CtxB polypeptide containing 3 or 5 glycines, (b) ESI-MS showing labeling of CtxB polypeptide containing 5 glycines.
[0028] Figure 10. ESI-MS showing labeling of eGFP and UCH-L3 polypeptides bearing
5 or 1 glycine, respectively.
[0029] Figure 11. Characterization of lipidated triglycine nucleophiles. (a) LC-ESI-MS total ion current chromatogram for lipidated triglycine nucleophiles. (b) RP-HPLC chromatogram (280 nm) for purified 2-chol. (c) ESI-MS data for lipidated triglycine nucleophiles.
[0030] Figure 12. (a) Reconstructed ESI-MS spectra for modified eGFP. (b) MALDI-
TOF MS spectrum of eGFP-2-chol.
[0031] Figure 13. Negative control experiment demonstrating that the formation of the eGFP-LPETG-l-C22 transpeptidation product requires sortase. Conditions: 77 μM eGFP-
LPETG-Hisδ, 150 μM sortase A, 2 mM nucleophile, 1% (w/v) n-dodecyl maltoside, 50 mM
Tris pH 7.5, 150 mM NaCl, 10 mM CaCb, 5 h at 37 °C. Samples analyzed by SDSPAGE.
[0032] Figure 14.(a) Standard curve for estimating the yield of lipid-modified eGFP. (b)
Absorbance of lipid-modified eGFP and estimated yield.
[0033] Figure 15. Control experiment demonstrating minor increases in cellular fluorescence as a result of incubation with eGFP-GGG in combination with free lipidated triglycine nucleophiles.
[0034] Figure 16. (a) Preparation of compounds 1 and 2 (FITC-LPRT-OMe and biotin-
LPRT-OMe); (b) Purification of compound 1. (c) Purification of compound 2.
[0035] Figure 17. ESI-MS showing quantitative labeling of CtxB constructs containing
3 or 5 glycine residues.
[0036] Figure 18. Streptavidin immunoblot showing labeling of biotinylated derivative
GGGGG-CtxB with biotinylated LPRT derivative.
[0037] Figures 19-22 present an overview of biological function of sortase in bacterial cell wall anchoring and examples of C-terminal labeling using sortase.
[0038] Figure 23 shows a schematic overview of N-terminal labeling using sortase. [0039] Figure 24 schematically depicts control of reaction equilibrium using inventive LPXTG mimetics
[0040] Figure 25 schematically shows transpeptidation reactions involving N and C termini.
[0041] Figure 26 illustrates cyclization of Cre recombinase. A, G-Cre-LPETG-His6 (50 μm) was incubated with sortase A (50 μm) in the presence or absence of fluorescent GGG- TMR (10 mm) in sortase reaction buffer (50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12) for 21.5 h at 37 °C. SDS-PAGE revealed the expected C-terminal transpeptidation product when GGG-TMR was included, whereas omission of the triglycine nucleophile resulted in clean conversion to a unique protein species with a lower apparent molecular weight. Schematic representations to the right of the gel indicate the topology of the protein species produced by transpeptidation. B, ESI-MS of linear G-Cre-LPETG-His6 and circular Cre formed by intramolecular transpeptidation. C, MS/MS spectrum of a tryptic fragment of circular Cre showing the ligation of the N-terminal residues (GEFAPK) to the C-terminal LPET motif. Expected masses for y and b ions are listed above and below the peptide sequence. Ions that were positively identified in the MS/MS spectrum are highlighted in blue or red. Only the most prominent daughter ions have been labeled in the MS/MS spectrum. [0042] Figure 27. Cyclization of Cre is reversible. A, G-Cre-LPETG-His6 (50 μm) was circularized by treatment with sortase A (50 μm) in sortase reaction buffer (50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12) for 21.5 h at 37 °C (lane 1). This reaction mixture was then treated with 10 mm GGG-TMR (lane 3) or simply incubated for an additional 24 h at 37 °C (lane 2). All reactions were analyzed by SDS-PAGE with visualization by Coomassie staining or in-gel fluorescence. For comparison, a C-terminal labeling reaction performed using 10 mm GGG-TMR without prior cyclization of the Cre substrate (lane 4) and a sample of linear G-Cre-LPETG-His6 incubated without sortase A or nucleophile (lane 5) are included. B, molecular model of Cre recombinase monomer (generated from PDB code lkbu) (29) showing the proximity relationship between the N and C termini. The N-terminal glycine residue is highlighted in red, and the C-terminal LPET residues are shown in green. [0043] Figure 28. Circularization of eGFP. A, molecular model of eGFP (generated from PDB code lgfl) (31) showing the proximity relationship between the N and C termini. The N-terminal glycine residue is highlighted in red, and the C-terminal LPET residues are shown in green. B, G5-eGFP-LPETG-His6 (50 μm) was circularized by treatment with sortase A (50 μm) in sortase reaction buffer (50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12) for 24 h at 37 0C. Schematic representations to the right of the gel indicate the topology of the protein species produced by transpeptidation. C, circular eGFP (C) recovers fluorescence more rapidly than linear G5-eGFP-LPETG-His6 (L) following thermal denaturation for 5 min at 90 °C. SDS-PAGE analysis confirmed the purity and concentration of the circular eGFP (C) and linear G5-eGFP-LPETG-His6 (L) samples used for refolding. [0044] Figure 29. UCHL3 with an internally positioned LPETG motif is circularized by sortase A. A, molecular model of human UCHL3 (generated from PDB code Ixd3) (30) showing the active site crossover loop bearing an LPETG substitution (LPET residues shown in green and GIy residue shown in red). The N-terminal glycine residue that serves as the nucleophile for intramolecular transpeptidation is highlighted in red. B, UCHL3 (30 μm) bearing an LPETG substitution in the active site crossover loop was incubated with sortase A (150 μm) in the absence or presence of GGG nucleophile (90 mm) in sortase reaction buffer (50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12) for the indicated times at 37 0C and analyzed by SDS-PAGE, followed by Coomassie staining. Schematic representations to the right of the gel indicate the topology of the protein species produced by transpeptidation. [0045] Figure 30. Positions of the N and C termini in the p97 hexamer are suitable for intermolecular cross-linking through sortase-catalyzed transpeptidation.A, molecular model of p97 trimer (generated from PDB code 3cfl) (28) showing the relative position of p97 monomers in the hexameric ring. The visible N and C termini from the published p97 trimer structure are indicated in red and green, respectively. B, molecular model of G-His6-p97- LPSTG-XX showing the proximity relationship between N and C termini in adjacent p97 monomers. N- and C-terminal residues not visible in the published crystal structure have been modeled onto the existing structure. N-terminal glycine residues are shown in red, and the C- terminal LPST residues are shown in green. For clarity, the C-terminal domains of the outer monomers are hidden, as is the N-terminal domain of the central monomer. C, G-His6-p97- LPSTG-XX (1.5 mg/ml) was incubated with sortase A (30 μm) in sortase reaction buffer (50 mm Tris, pH 7.5, 150 mm NaCl, 10 mm CaC12) for the times indicated at 37 °C. After 22 h, diglycine (GG) was added (100 mm final concentration), resulting in disappearance of the covalent oligomers (lane 5). For comparison, a control reaction containing 100 mm diglycine peptide from the outset of the experiment is shown in lane 6.
[0046] Figure 31. Overview of orthogonal labeling strategies using multiple sortases with distinct recognition motifs (recognition motifs described in Pallen, M. J.; Lam, A. C; Antonio, M.; Dunbar, K. Trends in Microbiology 2001, 9(3), 97-101). [0047] Figure 32. N-terminal labeling using SrtAstaph- (a) SrtAstaph catalyzes a transacylation reaction using labeled LPRT methyl esters as substrates. The labeled LPRT fragment is transferred to proteins containing N-terminal glycines in a site-specific fashion, (b) FITC (1) and biotin (2) LPRT methyl esters for N-terminal transacylation. (c) CtxB derivatives (50 μM) were treated with 500 μM 1 and 50 μM SrtAstaph for 2 h at 37 0C in 50 mM Tris (pH 7.5), 150 mM NaCl, and 10 mM CaCl2. Reactions were analyzed by SDS- PAGE with visualization by coomassie staining and fluorescent gel scanning. [0048] Figure 33. Site-specific N- and C-terminal labeling using multiple sortases. (a) Tetramethylrhodamine-labeled dialanine nucleophile (3) for SrtAstrep-mediated transpeptidation. (b) Strategy for the installation of discrete labels at both termini of the same protein using Δ59-SrtAstaph and SrtAstrep. (c, d) SDS-PAGE characterization with fluorescent gel scanning of dual-labeled (c) eGFP and (d) UCHL3. [0049] Figure 34. Scheme for site-specific N- and C-terminal labeling using multiple sortases. Starting materials, intermediates, and products may be analyzed using ESI-MS. [0050] Figure 35. Site-specific labeling at the N and C termini of eGFP and UCHL3. (a) ESI-MS spectra for all intermediates generated during the double labeling procedure. From top to bottom, this includes the eGFP starting material (m/z = 31080 Da), the intermediate formed after C-terminal modification with 3 mediated by SrtAstrep (m/z = 29470 Da), the product of thrombin cleavage (m/z = 28855 Da), crude dual labeled eGFP (m/z = 29726 Da), and dual labeled eGFP after anion exchange chromatography (m/z = 29725 Da). (b) ESI-MS spectra for all intermediates generated during double labeling of UCHL3. From top to bottom, this includes the UCHL3 starting material (m/z = 29252 Da), the intermediate formed after C-terminal modification with 3 mediated by SrtAstrep (m/z = 29050 Da), the product of thrombin cleavage (m/z = 28458 Da), crude dual labeled UCHL3 (m/z = 29412 Da), and dual labeled UCHL3 after anion exchange chromatography (m/z = 29412 Da). The MTSET reagent used to quench SrtAstrep also modifies the active site cysteine of UCHL3 creating an extra +118 Da signal in the mass spectrum. This modification is easily removed from the final product by brief treatment with DTT.
[0051] Figure 36 shows a ribbon structure of a representative four helix bundle cytokine (erythropoietin) and its receptor, showing that the N and C termini are located away from the receptor binding domain and in close proximity to each other. [0052] Figure 37 shows a scheme for C terminal modification or circularization. [0053] Figure 38 shows a nucleotide sequence (SEQ ID NO: 1) encoding an IFN alpha2 variant and corresponding encoded protein (SEQ ID NO: 2). In blue and bold print at the N- terminus of SEQ ID NO: 2 is the initiating methioinine (which gets clipped off when the coding sequence is translated in bacteria), followed by the two glycines used by the transamidase for cyclization. These are not present in the delGG variant described herein. In black (normal text) is the interferon alpha sequence from the normal human interferon alpha 2 protein. This is followed by two glycines in green (underlined), and the SrtAstaph recognition sequence LPETGG in red italics. Finally, the rest of the sequence (GSHHHHHH) in blue (immediately following the LPETGG) includes the 6His tag for purification. It should be noted that the IFN alpha sequence lacks the signal sequence for insertion into the ER and secretion that is found in the naturally occurring version prior to cleavage and secretion. This sequence is dispensable when a secreted eukaryotic, e.g., mammalian, polypeptide is produced in prokaryotes, e.g., in bacteria, or in an in vitro translation system. Sequences in SEQ ID NO: 1 are shown using the same notation as in SEQ ID NO: 2, i.e., blue and bold print denotes start codon (encoding methionine) followed by codons for two glycines; black (normal text) denotes IFN alpha2 coding sequence; followed by green (underlined) codons encoding two glycines; sequence encoding SrtAstaph recognition sequence is in red italics, foolowed by sequence in blue encoding GSHHHHHH. [0054] Figure 39 A shows a Coomassie gel of purified Interferon α (IFNα) variants. The IFNα variant contain two additional G residues at the C terminus that were introduced during cloning and are not depicted in the legend. Cyclization results in removal of GGHisό so that the circularized version contains an additional GGLPETGG relative to native IFNα positioned as follows: -Xaac-GGLPETGG-XaaN-, where Xaac and XaaN represent the C- terminal and N-terminal amino acids, respectively, of native IFNα.
[0055] Figure 39B shows MS/MS identification of the junction peptide for the ciruclar interferon alpha.
[0056] Figure 40 shows results of a Daudi cell proliferation inhibition assay demonstrating that IFNα variants retain biological activity equivalent to the original protein. IFNα variants are as shown in Figure 39. Legend: standard: commercially available IFNα; +GG: GG-IFNα-LPETGG-His6; circular: (see description of Figure 39); delGG: IFNα - LPETGG-His6; PEG: IFNα -LPETGGGK-PEG
[0057] Figure 41 shows serum half life ELISA results for PEGylated vs. linear IFNα demonstrating that PEGylation significantly prolongs the half-life. The linear IFNα variant tested in this experiment is the delGG variant (which comprises an LPETGG-His6 moiety at the C-terminus). [0058] Figure 42 shows Tm's for a thermal denaturation assay performed on IFNα variants with lysozyme as a control and shows that the circular variant exhibits significantly enhanced thermal stability relative to the other variants.
[0059] Figure 43 shows a scheme for scheme for double transpeptidation using two sortases and a probe that contains a masked sortase recognition sequence (masking achieved by using phosphothreonine in the LPXTG motif).
[0060] Figure 44 shows mass spectrometry results showing sequential transpeptidation using a probe containing a masked sortase recognition sequence. Upper panel:
IFNαLPETAAGKGLPEtGG-Hisό; Middle panel: IFNαLPETAAGKGLPETGG-His6;
IFNaLPETAAGKGLPETGGG
[0061] Figure 45 shows a scheme for ligating a first protein or protein domain to a second protein or protein domain using two sortase-mediated reactions.
[0062] Figure 46 shows a scheme for using transamidase-mediated reaction for detecting cell-cell interactions.
[0063] Figure 47 shows (A) exemplary C-terminal probe. (B) exemplary N-terminal probe. (C) exemplary C-terminal masked probe. Representative Rl groups: (I) PEG; (2) biotin; (3) tetramethylrhodamine.
DETAILED DESCRIPTION OF CERTAIN EMBODIMENTS
[0064] In simplest terms, the transpeptidation reaction results in the ligation of species containing a transamidase recognition sequence with those bearing one or more N-terminal glycine residues. In certain embodiments, the recognition sequence is an LPXTG motif. However, a drawback of using such recognition sequences as acyl donors is that the transfer of an LPXT unit to a nucleophilic acyl acceptor releases a stoichiometric amount of a peptide fragment containing an N-terminal glycine. Such by-products compete with the desired acyl acceptor and hinder the progress of the ligation reaction. Moreover, hydrolytic cleavage of an LPXTG peptide, although a relatively slow process, can exacerbate competition with the protein nucleophile as the reaction proceeds. Indeed, initial attempts to perform N-terminal protein labeling with peptides containing all five residues (LPXTG) yielded disappointing results as useful levels of ligation could only be obtained using concentrations > 5mM of the LPXTG-containing peptide.
[0065] Applicants have found that the substitution of the C-terminal residue of the recognition sequence with a moiety exhibiting poor nucleophilicity once released from the transamidase provides for a more efficient ligation. Any moiety exhibiting such poor nucleophilicity can be used in accordance with the present invention. Exemplary embodiments are described herein.
[0066] The present invention provides methods for efficiently linking an acyl donor with a nucleophilic acyl acceptor. The development of these methods is significant as they are widely applicable to many acyl donors and a multitude of different acyl acceptors. In certain embodiments, the processes are useful for ligating proteins and/or peptides to one another, ligating synthetic peptides to recombinant proteins, linking a reporting molecule to a protein or peptide, joining a nucleic acid to a protein or peptide, conjugating a protein or peptide to a solid support or polymer, and linking a protein or peptide to a label. Such products and processes save cost and time associated with ligation product synthesis and are useful for conveniently linking an acyl donor to an acyl acceptor. In certain embodiments, the ligation products and purified products are useful in diagnostic procedures {e.g., an antibody that specifically binds to a cancer cell epitope is joined to a radioisotope and the conjugate is administered to a patient to detect the presence or absence of cancer cells). In certain embodiments, the ligation products and purified products are useful in therapeutic procedures (e.g., an antibody that specifically binds to a cancer cell epitope is joined to a toxin such as ricin A and the conjugate is administered to a patient to selectively treat the cancer). In certain embodiments, the ligation products and purified products are useful in research methods {e.g., a NH2-CH2-derivatized fluorophore and sortase are contacted with fixed cells that express a protein linked to a sortase recognition sequence and the location of the protein is detected by a fluorescence imaging technique).
[0067] Methods for ligation described herein are catalyzed by a transamidase. A transamidase is an enzyme that can form a peptide linkage {i.e., amide linkage) between an acyl donor compound and a nucleophilic acyl acceptor containing a NH2-CH2-moiety. Sortases are enzymes having transamidase activity and have been isolated from Gram- positive bacteria. They have, as part of their cell wall structure, peptidoglycan as well as polysaccharides and/or teichoic acids. Gram- positive bacteria include the following genera: Actinomyces, Bacillus, Bifidobacterium, Cellulomonas, Clostridium, Corynebacterium, Micrococcus, Mycobacterium, Nocardia, Staphylococcus, Streptococcus and Streptomyces. [0068] In certain embodiments, the present invention provides a ligation method comprising the step of contacting an acyl donor compound of formula: O
A1- Transamidase recognition sequence XR1 wherein the transamidase recognition sequence is any peptide motif recognized by a transamidase enzyme; X is -O-, -NR-, or -S-; R is hydrogen, substituted or unsubstituted aliphatic, or substituted or unsubstituted heteroaliphatic; A1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; R1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, or substituted or unsubstituted heteroaryl; and with a nucleophilic compound of formula:
Figure imgf000016_0001
wherein
B1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; and n is an integer from 0 to 100, inclusive; in the presence of a transamidase enzyme under suitable conditions to form a compoundormula:
O
A1- Transamidase recognition sequence
H ffl ^B1 [0069] One of ordinary skill will appreciate that, in certain embodiments, the C-terminal amino acid of the transamidase recognition sequence is omitted. That is, an acyl group O
•T- XR1 replaces the C-terminal amino acid of the transamidase recognition sequence. In
O some embodiments, the acyl group is ^ Α- OR 1 . In some embodiments, the acyl group is
O
"OMe .
[0070] In some embodiments, the transamidase recognition sequence is LPXT, wherein X is a standard or non-standard amino acid. In some embodiments, X is selected from D, E, A, N, Q, K, or R. In some embodiments, the recognition sequence is selected from LPXT, LPXT, SPXT, LAXT, LSXT, NPXT, VPXT, IPXT, and YPXR. In some embodiments X is selected to match a naturally occurring transamidase recognition sequence. In some embodiments, the transamidase recognition sequence is selected from: LPKT, LPIT, LPDT, SPKT, LAET, LAAT, LAET, LAST, LAET, LPLT, LSRT, LPET, VPDT, IPQT, YPRR, LPMT, LPLT, LAFT, LPQT, NSKT, NPQT, NAKT, and NPQS. In some embodiments, e.g., in certain embodiments in which sortase A is used (see below), the transamidase recognition motif comprises the amino acid sequence X1PX2X3, where X1 is leucine, isolucine, valine or methionine; X2 is any amino acid; X3 is threonine, serine or alanine; P is proline and G is glycine. In specific embodiments, as noted above X1, is leucine and X3 is threonine. In certain embodiments, X2 is aspartate, glutamate, alanine, glutamine, lysine or methionine. In certain embodiments, e.g., where sortase B is utilized, the recognition sequence often comprises the amino acid sequence NPX1TX2, where X1 is glutamine or lysine; X2 is asparagine or glycine; N is asparagine; P is proline and T is threonine. The invention encompasses the recognition that selection of X may be based at least in part in order to confer desired properties on the compound containing the recognition motif. In some embodiments, X is selected to modify a property of the compound that contains the recognition motif, such as to increase or decrease solubility in a particular solvent. In some embodiments, X is selected to be compatible with reaction conditions to be used in synthesizing a compound comprising the recognition motif, e.g., to be unreactive towards reactants used in the synthesis.
[0071] In some embodiments, X is -O-. In some embodiments, X is -NR-. In some embodiments, X is -NH-. In some embodiments, X is -S-. [0072] In certain embodiments, R1 is substituted aliphatic. In certain embodiments, R1 is unsubstituted aliphatic. In some embodiments, R1 is substituted CM2 aliphatic. In some embodiments, R1 is unsubstituted CM2 aliphatic. In some embodiments, R1 is substituted Ci- 6 aliphatic. In some embodiments, R1 is unsubstituted Ci-6 aliphatic. In some embodiments, R1 is Ci-3 aliphatic. In some embodiments, R1 is butyl. In some embodiments, R1 is /?-butyl. In some embodiments, R1 is isobutyl. In some embodiments, R1 is propyl. In some embodiments, R1 is w-propyl. In some embodiments, R1 is isopropyl. In some embodiments, R1 is ethyl. In some embodiments, R1 is methyl.
[0073] In certain embodiments, R1 is substituted aryl. In certain embodiments, R1 is unsubstituted aryl. In certain embodiments, R1 is substituted phenyl. In certain embodiments, R1 is unsubstituted phenyl.
[0074] It will be appreciated that a variety of functional groups, motifs, macromolecules, etc., can comprise part of the acyl donor as the A1 moieity. In some embodiments, A1 comprises a protein. In some embodiments, A1 comprises a peptide. In some embodiments, A1 comprises an element selected from the group consisting of an antibody, an antibody chain, an antibody fragment, an antibody epitope, a recombinant protein, a peptide comprising one or more D-amino acids, a branched peptide, a therapeutic protein, an enzyme, a polypeptide subunit of a multisubunit protein, a transmembrane protein, a cell surface protein, a methylated peptide or protein, an acylated peptide or protein, a lipidated peptide or protein, a phosphorylated peptide or protein, and a glycosylated peptide or protein. In some embodiments, A1 is an amino acid. In some embodiments, A1 comprises a protein. In some embodiments, A1 comprises a peptide. In some embodiments, A1 comprises an antibody. In some embodiments, A1 comprises an antibody fragment. In some embodiments, A comprises an antibody epitope. In some embodiments, A1 comprises green fluorescent protein.
[0075] In some embodiments, A1 comprises a lipid. In some embodiments, A1 comprises a saturated hydrocarbon. In some embodiments, A1 comprises a partially unsaturated hydrocarbon. In some embodiments, A1 comprises a Ci-40 hydrocarbon chain. In some embodiments, A1 comprises a Ci-30 hydrocarbon chain. In some embodiments, A1 comprises a Ci-2O hydrocarbon chain. In some embodiments, A1 comprises a Ci2-40 hydrocarbon chain. [0076] In some embodiments, A1 comprises a substituted or unsubstituted Ci-20 aliphatic group. In some embodiments, A1 comprises an adamantyl group.
[0077] In certain embodiments, A1 comprises a small molecule. In certain embodiments, A1 comprises a bioactive small molecule. In certain embodiments, A1 comprises a FDA- approved drug. In certain embodiments, A1 comprises a cytotoxic agent. In certain embodiments, A1 comprises a steroid. In certain embodiments, A1 comprises a steroid analog.
[0078] In certain embodiments, A1 comprises a label. In some embodiments, A1 comprises a fluorescent label. In certain embodiments, A1 comprises a radiolabel. In certain embodiments, A1 comprises a chemiluminescent label. In certain embodiments, A1 comprises a phosphorescent label.
[0079] In certain embodiments, A1 comprises biotin. In certain embodiments, A1 comprises streptavidin. In certain embodiments, A1 comprises fluorescein.
[0080] One of ordinary skill in the art will appreciate that A1 and B1 groups of the present invention are interchangable. That is, a given group A1 on an acyl donor could also be used as a group B1 on a nucleophilic acyl acceptor, and vice versa. Thus, all embodiments and variants of A1 as described herein are also contemplated as B1 groups.
[0081] In certain embodiments, n is an integer from 0 to 50, inclusive. In certain embodiments, n is an integer from 0 to 20, inclusive. In certain embodiments, n is 0. In certain embodiments, n is 1. In certain embodiments, n is 2. In certain embodiments, n is 3.
In certain embodiments, n is 4. In certain embodiments, n is 5. In certain embodiments, n is
6.
[0082] In some embodiments, the present invention provides a ligation method comprising the step of contacting an acyl donor compound of formula:
Figure imgf000019_0001
wherein each of A1, X, R, and R1 is as defined above; and R2 is a natural or unnatural amino acid side chain; with a nucleophilic compound of formula:
Figure imgf000019_0002
wherein B1 and n are as defined above; in the presence of a transamidase enzyme under suitable conditions to form a compound of formula:
Figure imgf000020_0001
[0083] In some embodiments, R2 is a natural amino acid side chain. In some embodiments, R2 is the side chain group of aspartic acid, glutamic acid, alanine, asparagine, glutamine, lysine, or arginine. In some embodiments, R2 is the side chain group of arginine. In some embodiments, R2 is the side chain group of glutamic acid. In some embodiments, R2 is the side chain group of lysine. In some embodiments, R2 is the side chain group of aspartic acid. In some embodiments, R2 is the side chain group of alanine. In some embodiments, R2 is the side chain group of asparagine. In some embodiments, R2 is the side chain group of glutamine.
[[00008844]] In certain embodiments, R2 is an unnatural amino acid side chain.
[0085] In some embodiments, the acyl donor compound is of formula:
Figure imgf000020_0002
[0086] In some embodiments, the acyl donor compound is of formula:
Figure imgf000020_0003
[0087] In some embodiments, the acyl donor compound is of formula:
Figure imgf000020_0004
[0088] In some embodiments, the acyl donor compound is selected from:
Figure imgf000021_0001
[0089] In certain embodiments, the transamidase is a sortase. Enzymes identified as "sortases" from Gram-positive bacteria cleave and translocate proteins to proteoglycan moieties in intact cell walls. Among the sortases that have been isolated from Staphylococcus aureus, are sortase A (Sit A) and sortase B (Srt B). Thus, in certain embodiments, a transamidase used in accordance with the present invention is a sortase A, e.g., from S. aureus. In certain embodiments, a transamidase is a sortase B, e.g., from S. aureus. [0090] Sortases have been classified into 4 classes, designated A , B, C, and D, based on sequence alignment and phylogenetic analysis of 61 sortases from Gram positive bacterial genomes (Dramsi S, Trieu-Cuot P, Bierne H, Sorting sortases: a nomenclature proposal for the various sortases of Gram-positive bacteria. Res Microbiol.156(3):289-97, 2005. These classes correspond to the following subfamilies, into which sortases have also been classified by Comfort and Clubb (Comfort D, Clubb RT. A comparative genome analysis identifies distinct sorting pathways in gram-positive bacteria. Infect Immun., 72(5):2710-22, 2004): Class A (Subfamily 1), Class B (Subfamily 2), Class C (Subfamily 3), Class D (Subfamilies 4 and 5). The aforementioned references disclose numerous sortases and recognition motifs. See also Pallen, M. J.; Lam, A. C; Antonio, M.; Dunbar, K. TRENDS in Microbiology, 2001, 9(3), 97-101. Those skilled in the art will readily be able to assign a sortase to the correct class based on its sequence and/or other characteristics such as those described in Drami, et al., supra. The term "sortase A" is used herein to refer to a class A sortase, usually named SrtA in any particular bacterial species, e.g., SrtA from S. aureus. Likewise "sortase B" is used herein to refer to a class B sortase, usually named SrtB in any particular bacterial species, e.g., SrtB from S. aureus. The invention encompasses embodiments relating to a sortase A from any bacterial species or strain. The invention encompasses embodiments relating to a sortase B from any bacterial species or strain. The invention encompasses embodiments relating to a class C sortase from any bacterial species or strain. The invention encompasses embodiments relating to a class D sortase from any bacterial species or strain. [0091] Amino acid sequences of Srt A and Srt B and the nucleotide sequences that encode them are disclosed in a number of references cited herein and which are incorporated herein by reference. The amino acid sequences of S. aureus SrtA and SrtB are homologous, sharing, for example, 22% sequence identity and 37% sequence similarity. The amino acid sequence of a sortase-transamidase from Staphylococcus aureus also has substantial homology with sequences of enzymes from other Gram-positive bacteria, and such transamidases can be utilized in the ligation processes described herein. For example, for SrtA there is about a 31 % sequence identity (and about 44% sequence similarity) with best alignment over the entire sequenced region of the S. pyogenes open reading frame. There is about a 28% sequence identity with best alignment over the entire sequenced region of the A. naeslundii open reading frame. It will be appreciated that different bacterial strains may exhibit differerences in sequence of a particular polypeptide, and the sequences herein are exemplary.
[0092] In certain embodiments a transamidase bearing 18% or more sequence identity, 20% or more sequence identity, or 30% or more sequence identity with the S. pyogenes, A. naeslundii, S. mutans, E. faecalis or B. subtilis open reading frame encoding a sortase can be screened, and enzymes having transamidase activity comparable to Srt A or Srt B from S. aureas can be utilized (e. g. , comparable activity sometimes is 10% of Srt A or Srt B activity or more).
[0093] Thus in some embodiments of the invention the sortase is a sortase A (SrtA). SrtA recognizes the motif LPXTG, with common recognition motifs being, e.g., LPKTG, LPATG, LPNTG. In some embodiments LPETG is used. However, motifs falling outside this concensus may also be recognized. For example, in some embodiments the motif comprises an 'A' rather than a 'T' at position 4, e.g., LPXAG, e.g., LPNAG. In some embodiments the motif comprises an 'A' rather than a 'G' at position 5, e.g., LPXTA, e.g., LPNTA. In some embodiments the motif comprises a 'G' rather than 'P' at position 2, e.g., LGXTG, e.g., LGATG. In some embodiments the motif comprises an T rather than 'L' at position 1, e.g., IPXTG, e.g., IPNTG or IPETG. [0094] It will be appreciated that the terms "recognition motif and "recognition sequence", with respect to sequences recognized by a transamidase, are used interchangably. The term "transamidase recognition sequence" is sometimes abbreviated "TRS" herein. [0095] In some embodiments of the invention the sortase is a sortase B (SrtB), e.g., a sortase B of S. aureus, B. anthracis, or L. monocytogenes. Motifs recognized by sortases of the B class (SrtB) often fall within the consensus sequences NPXTX, e.g., NP[Q/K]-[T/s]- [N/G/s], such as NPQTN or NPKTG. For example, sortase B of S. aureus or B. anthracis cleaves the NPQTN or NPKTG motif of IsdC in the respective bacteria (see, e.g., Marraffini, L. and Schneewind, O., Journal of Bacteriology, 189(17), p. 6425-6436, 2007). Other recognition motifs found in putative substrates of class B sortases are NSKTA, NPQTG, NAKTN, and NPQSS. For example, SrtB from L. monocytogenes recognizes certain motifs lacking P at position 2 and/or lacking Q or K at position 3, such as NAKTN and NPQSS (Mariscotti JF, Garcia-Del Portillo F, Pucciarelli MG. The listeria monocytogenes sortase-B recognizes varied amino acids at position two of the sorting motif. J Biol Chem. 2009 Jan 7. [Epub ahead of print])
[0096] In some embodiments, the sortase is a class C sortase. Class C sortases may utilize LPXTG as a recognition motif.
[0097] In some embodiments, the sortase is a class D sortase. Sortases in this class are predicted to recognize motifs with a consensus sequence NA-[E/A/S/H]-TG (Comfort D, supra). Class D sortases have been found, e.g., in Streptomyces spp., Corynebacterium spp., Tropheryma whipplei, Thermobifida fusca, and Bifidobacterium longhum. LPXTA or LAXTG may serve as a recognition sequence for class D sortases, e.g., of subfamilies 4 and 5, respectively subfamily-4 and subfamily-5 enzymes process the motifs LPXTA and LAXTG, respectively). For example, B. anthracis Sortase C, which is a class D sortase, has been shown to specifically cleave the LPNTA motif in B. anthracis Basl and BasH (Marrafini, supra).
[0098] See Barnett and Scott for description of a sortase from that recognizes QVPTGV motif (Barnett, TC and Scott, JR, Differential Recognition of Surface Proteins in Streptococcus pyogenes by Two Sortase Gene Homologs. Journal of Bacteriology, Vol. 184, No. 8, p. 2181-2191, 2002).
[0099] The invention contemplates use of sortases found in any gram positive organism, such as those mentioned herein and/or in the references (including databases) cited herein. The invention also contemplates use of sortases found in gram negative bacteria, e.g., Colwellia psychrerythraea, Microbulbifer degradans, Bradyrhizobium japonicum, Shewanella oneidensis, and Shewanella putrefaciens. They recognize sequence motifs LP[Q/K]T[A/S]T. In keeping with the variation tolerated at position 3 in sortases from gram positive organisms, a sequence motif LPXT[A/S], e.g., LPXTA or LPSTS may be used. [00100] The invention contemplates use of sortase recognition motifs from any of the experimentally verified or putative sortase substrates listed at http://bamics3.cmbi.kun.nl/jos/sortase substrates/help.html, the contents of which are incorporated herein by reference, and/or in any of the above-mentioned references. In some embodiments the sortase recognition motif is selected from: LPKTG, LPITG, LPDTA, SPKTG, LAETG, LAATG, LAHTG, LASTG, LAETG, LPLTG, LSRTG, LPETG, VPDTG, IPQTG, YPRRG, LPMTG, LPLTG, LAFTG, LPQTS, it being understood that in various embodiments of the invention the 5 residue is replaced, as described elsewhere herein. For example, the sequence used may be LPXT, LAXT, LPXA, LGXT, IPXT, NPXT, NPQS, LPST, NSKT, NPQT, NAKT, LPIT, LAET, or NPQS. The invention comprises embodiments in which 'X' in any sortase recognition motif disclosed herein or known in the art is any standard or non-standard amino acid. Each variation is disclosed. In some embodiments, X is selected from the 20 standard amino acids found most commonly in proteins found in living organisms. In some embodiments, e.g., where the recognition motif is LPXTG or LPXT, X is D, E, A, N, Q, K, or R. In some embodiments, X in a particular recognition motif is selected from those amino acids that occur naturally at position 3 in a naturally occurring sortase substrate. For example, in some embodiments X is selected from K, E, N, Q, A in an LPXTG or LPXT motif where the sortase is a sortase A. In some embodiments X is selected from K, S, E, L, A, N in an LPXTG or LPXT motif and a class C sortase is used.
[00101] In some embodiments, a recognition sequence further comprises one or more additional amino acids, e.g., at the N or C terminus. For example, one or more amino acids (e.g., up to 5 amino acids) having the identity of amino acids found immediately N-terminal to, or C-terminal to, a 5 amino acid recognition sequence in a naturally occurring sortase substrate may be incorporated. Such additional amino acids may provide context that improves the recognition of the recognition motif.
[00102] The term "transamidase recognition sequence" may refer to a masked or unmasked transamidase recognition sequence. A unmasked transamidase recognition sequence can be recognized by a transamidase. An unmasked transamidase recognition sequence may have been previously masked, e.g., as described herein. In some embodiments, a "masked transamidase recognition sequence" is a sequence that is not recognized by a transamidase but that can be readily modified ("unmasked") such that the resulting sequence is recognized by a transamidase. For example, in some embodiments at least one amino acid of a masked transamidase recognition sequence has a side chain that comprises a moiety that inhibits, e.g., substantially prevents, recognition of the sequence by a transamidase of interest, wherein removal of the moiety allows the transamidase to recognize the sequence. Masking may, for example, reduce recognition by at least 80%, 90%, 95%, or more (e.g., to undetectable levels) in certain embodiments. By way of example, in certain embodiments a threonine residue in a transamidase recognition sequence such as LPXTG is phosphorylated, thereby rendering it refractory to recognition and cleavage by SrtA. The masked recognition sequence can be unmasked by treatment with a phosphatase, thus allowing it to be used in a SrtA-catalyzed transamidation reaction. The invention provides novel masked transamidase recognition sequences, and compounds comprising them. In certain embodiments, the transamidase recognition sequence comprises the formula:
Figure imgf000025_0001
wherein
R2 is the side chain of any natural or unnatural amino acid, optionally modified or substituted; and
RB is hydrogen; phosphate; sulfate; an oxygen-protecting group; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl; or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00103] In certain embodiments, the transamidase recognition sequence comprises the formula: [00104]
Figure imgf000026_0001
.In certain embodiments, the transamidase recognition sequence is of the formula:
Figure imgf000026_0002
wherein
R2 is the side chain of any natural or unnatural amino acid, optionally modified or substituted; and
RB is hydrogen; phosphate; sulfate; an oxygen-protecting group; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00105] In certain embodiments, the transamidase recognition sequence is of the formula:
Figure imgf000026_0003
wherein
R ,2 is the side chain of any natural or unnatural amino acid, optionally modified or substituted; and RB is hydrogen; phosphate; sulfate; an oxygen-protecting group; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
In certain embodiments, R2 is the side chain of a natural amino acid. In certain embodiments, R2 is the side chain group of aspartic acid, glutamic acid, alanine, asparagine, glutamine, lysine, or arginine. In certain embodiments, R2 is the side chain group of arginine. In certain embodiments, R2 is the side chain group of glutamic acid. In certain embodiments, R2 is the side chain group of lysine. In certain embodiments, R2 is the side chain group of aspartic acid. In certain embodiments, R is the side chain group of alanine. In certain embodiments, R2 is the side chain group of asparagine. In certain embodiments, R2 is the side chain group of glutamine. In certain embodiments, the side chain of aspartic acid, glutamic acid, alanine, asparagine, glutamine, lysine, arginine, or other amino acid of R2 is modified so as to mask the recognition sequence of the transamidase. For example, a lysine side chain may be acylated or the terminal amino group may be protected with a nitrogen- protecting group. An aspartic acid or glutamic acid may be esterified or amidated. A threonine, serine, or asparagine may be glycosylated. A threonine, serine, or tyrosine may be phosphorylated or sulfated. An amino acid side chain may also be modified using a photocleavable moiety such as o-nitrobenzyl or dimethoxynitrobenzyl or derivatives thereof. In other embodiments, a chemical cleavage method is employed. For example, periodate cleavage can be used to cleave a vicinal diol. See, e.g,. Rodenko B J, lass I major histocompatibility complexes loaded by a periodate trigger. J. Am Chem Soc.;131(34):12305-13, 2009.
[00106] A masked transamidase recognition sequence may be unmasked by a chemical or biological process that does not adversely affect other moieties of the protein or the protein itself. In certain embodiments, a phosphatase is used to remove a phosphate group masking a recognition sequence. In certain embodiments, a sulfatase is used to remove a sulfate group. In certain embodiments, an esterase or amidase is used to remove an acyl group. In certain embodiments, a glycosidase, e.g., an N-glycosidase, is used to remove a carbohydrate moiety. In certain embodiments, a photocleavable moiety is removed by exposing the protein or peptide to light. In some embodiments, mild alkaline hydrolysis is used to remove a masking moiety. In certain embodiments, a protecting group is removed using reagents and/or conditions typically used to remove the protecting group. See, e.g., Wuts et al, Greene 's Protective Groups in Organic Synthesis (Wiley-Interscience; 4 edition; October 30, 2006). [00107] In certain embodiments, the unmasked transamidase recognition sequence is of the formula:
Figure imgf000028_0001
[00108] In certain embodiments, the masked transamidase recognition sequence is of the formula:
Figure imgf000028_0002
[00109] In certain embodiments, the unmasked transamidase recognition sequence is of the formula:
Figure imgf000028_0003
[00110] In certain embodiments, the masked transamidase recognition sequence is of the formula:
Figure imgf000029_0001
[00111] The invention provides compounds, sometimes referred to herein as "probes" that comprise a novel masked transamidase recognition sequence and are of use in a transamidase-mediated reaction. Optionally, the probe further comprises one or more additional amino acids either N- or C-terminal to the masked transamidase recognition sequence. Such additional amino acid(s) may be modified with, e.g., carbohydrates, lipids, phosphate groups, labels, tags, other polymers (for example, a non-polypeptide polymer such as polyethylene glycol), and acetyl groups. The invention further provides methods of ligation using an inventive probe. In some aspects, inventive methods comprise N-terminal and/or C-terminal modification of a polypeptide using an inventive probe. In some embodiments, both N- and C-termini are modified (dual modification). In some aspects, the invention provides methods of circularizing a polypeptide using an inventive probe. The invention further provides methods of joining two or more polypeptides using an inventive probe, thereby resulting in insertion of a non-genetically encoded peptide element between the two polypeptides. The non-genetically encoded peptide element in some embodiments comprises a modifying moiety, e.g., an acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a particle, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer (e.g,. a polyethylene glycol), a recognition element, a small molecule, a lipid, or a label.
[00112] The invention provides methods of using inventive transamidase recognition sequences, and probes containing them, for a variety of purposes. In some embodiments, a probe comprising a masked transamidase recognition sequence is used for C-terminal labeling, which in some embodiments is followed by unmasking and cyclization (see, e.g., Figure 43 and discussion below). In some embodiments, a probe comprising a masked transamidase recognition sequence is used for transamidase-mediated C-terminal labeling, followed by unmasking, followed by a second transamidase-mediated reaction. The second transamidase-mediated reaction may append a second polypeptide at the C-terminus of the oligopeptide probe. (See, e.g., Figure 44, wherein the second transamidase-mediated reaction appends a GGG sequence to an IFNalpha variant that has undergone a first transamidase- mediated reaction.) Optionally, the first transamidase-mediated reaction installs a modifying group near the C-terminus, as shown in Figure 33, wherein the modifying group is denoted as "Label". The first and second polypeptides are often each produced by translation of an RNA, e.g., recombinantly produced. The resulting product comprises two polypeptides joined by a non-genetically encoded element. Products produced using an inventive ligation method and/or probe are aspects of the invention.
[00113] For C-terminal labeling, e.g., as shown in Figure 43 (upper reaction) or Figure 44 (step 1), in certain embodiments the inventive method uses an oligopeptide with a nucleophilic amino N-terminus to attack the acyl enzyme and form an amide bond between the protein to be labeled and the oligopeptide. The oligopeptide may have any sequence of natural and/or unnatural amino acids and one or more of the amino acids may be modified or labeled in various embodiments. To give a few examples, the label may include a fluorescent tag, a phosphorescent tag, biotin, poly (histi dine) tag, or a radioactive label. The oligopeptide may also be modified with carbohydrates, lipids, phosphate groups, labels, tags, other polymers (for example, a non-polypeptide polymer such as polyethylene glycol), and acetyl groups. Any biological or chemical modification of an amino acid or protein may be incorporated into the oligopeptide to be ligated using a transamidase. In certain embodiments, the oligopeptide includes a second transamidase recognition sequence or a masked transamidase recognition sequence. In certain embodiments, the oligopeptide is of the formula:
Figure imgf000031_0001
wherein j is an integer between 0 and 10, inclusive; k is an integer between 0 and 10, inclusive;
X is -O-, -NR-, or -S-;
R is hydrogen; substituted or unsubstituted aliphatic; or substituted or unsubstituted heteroaliphatic;
R1 is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl; each occurrence of R3 is independently the side chain of a natural or unnatural amino acid; R4 is the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; and each occurrence of R5 is independently the side chain of a natural or unnatural amino acid.
In certain embodiments, the oligopeptide is of the formula:
Figure imgf000032_0001
wherein transamidase recognition sequence is a sequence recognized by a transamidase; j is an integer between 0 and 10, inclusive; k is an integer between 0 and 10, inclusive; m is an integer between 0 and 10, inclusive; p is 1 or 2;
X is -O-, -NR-, or -S-;
R is hydrogen; substituted or unsubstituted aliphatic; or substituted or unsubstituted heteroaliphatic; each occurrence of R1 is independently hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl; each occurrence of R3 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl;
R4 is the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; each occurrence of R is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; and each occurrence of R6 is independently the side chain of a natural or unnatural amino acid.
[00114] In certain embodiments, the transamidase recognition sequence is LPXT, wherein X is a natural or unnatural amino acid. In certain embodiments, X is selected from D, E, A, N, Q, K, or R. In certain embodiments, the recognition sequence is selected from LPXT, LPXT, SPXT, LAXT, LSXT, NPXT, VPXT, IPXT, and YPXR. In certain embodiments, X is selected to match a naturally occurring transamidase recognition sequence. In certain embodiments, the transamidase recognition sequence is selected from: LPKT, LPIT, LPDT, SPKT, LAET, LAAT, LAET, LAST, LAET, LPLT, LSRT, LPET, VPDT, IPQT, YPRR, LPMT, LPLT, LAFT, LPQT, NSKT, NPQT, NAKT, and NPQS. In certain embodiments, e.g., in which sortase A is used, the transamidase recognition motif comprises the amino acid sequence XiPX2X3, where Xi is leucine, isolucine, valine or methionine; X2 is any amino acid; X3 is threonine, serine, or alanine; P is proline; and G is glycine. In specific embodiments, as noted above Xi is leucine, and X3 is threonine. In certain embodiments, X2 is aspartate, glutamate, alanine, glutamine, lysine, or methionine. In certain embodiments, e.g., where sortase B is utilized, the recognition sequence often comprises the amino acid sequence NPXiTX2, where Xj is glutamine or lysine; X2 is asparagine or glycine; N is asparagine; P is proline and T is threonine. In certain embodiments, e.g., where sortase A from Staphylcoccus aureus (SrtAstaph) is utilized, the recognition sequence comprises the amino acid sequence LPXiTX2, where Xi is selected from D, E, A, N, Q, K, or R; X2 is alanine or glycine; L is leucine; P is proline and T is threonine. In certain embodiments, for recognition sequence of SrtAstaph is LPXiTA. In other embodiments, for recognition sequence of SrtAstaph is LPX)TG. The invention encompasses the recognition that selection of X may be based at least in part in order to confer desired properties on the compound containing the recognition motif. In some embodiments, X is selected to modify a property of the compound that contains the recognition motif, such as to increase or decrease solubility in a particular solvent. In some embodiments, X is selected to be compatible with reaction conditions to be used in synthesizing a compound comprising the recognition motif, e.g., to be unreactive towards reactants used in the synthesis.
[00115] In certain embodiments, j is 0. In certain embodiments, j is 1. In certain embodiments, j is 2. In certain embodiments, j is 3. In certain embodiments, j is 4. In certain embodiments, j is 5.
[00116] In certain embodiments, k is 0. In certain embodiments, k is 1. In certain embodiments, k is 2. In certain embodiments, k is 3. In certain embodiments, k is 4. In certain embodiments, k is 5.
[00117] In certain embodiments, m is 0. In certain embodiments, m is 1. In certain embodiments, m is 2. In certain embodiments, m is 3. In certain embodiments, m is 4. In certain embodiments, m is 5.
[00118] In certain embodiments, X is -O-. In certain embodiments, X is -NH-.
[00119] In certain embodiments, R1 is substituted hydrogen. In certain embodiments, R1 is substituted aliphatic. In certain embodiments, R1 is unsubstituted aliphatic. In some embodiments, R1 is substituted Ci-12 aliphatic. In some embodiments, R1 is unsubstituted Ci-
12 aliphatic. In some embodiments, R1 is substituted Ci-6 aliphatic. In some embodiments, R1 is unsubstituted Ci-6 aliphatic. In some embodiments, R1 is Ci-3 aliphatic. In certain embodiments, R1 is Ci-6 alkyl. In some embodiments, R1 is butyl. In some embodiments, R1 is H-butyl. In some embodiments, R1 is isobutyl. In some embodiments, R1 is propyl. In some embodiments, R1 is H-propyl. In some embodiments, R1 is isopropyl. In some embodiments, R1 is ethyl. In some embodiments, R1 is methyl. In certain embodiments, R1 is substituted aryl. In certain embodiments, R1 is unsubstituted aryl. In certain embodiments,
R1 is substituted phenyl. In certain embodiments, R1 is unsubstituted phenyl.
[00120] In certain embodiments, -XR1 is -OCH3. In certain embodiments, -XR1 is -OH.
In certain embodiments, -XR1 is -NH2.
[00121] In certain embodiments, R3 is the side chain of a natural amino acid. In certain embodiments, R3 is hydrogen. In certain embodiments, R3 is methyl.
[00122] In certain embodiments, R4 is a modified side chain of a natural amino acid. In certain embodiments, R4 is a modified side chain of serine, threonine, lysine, aspartate, glutamate, arginine, asparagine, glutamine, or tyrosine.
[00123] In certain embodiments, R4 is of the formula:
Figure imgf000034_0001
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00124] In certain embodiments, R4 is of the formula:
Figure imgf000035_0001
wherein RD is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00125] In certain embodiments, R4 is of the formula:
Figure imgf000035_0002
wherein R is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
[00126] In certain embodiments, R4 is of the formula:
Figure imgf000035_0003
wherein RD is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00127] In certain embodiments, R4 is of the formula:
Figure imgf000036_0001
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
[00128] In certain embodiments, R4 is of the formula:
Figure imgf000036_0002
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00129] In certain embodiments, R4 is of the formula:
Figure imgf000036_0003
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00130] In certain embodiments, R4 is of the formula:
Figure imgf000036_0004
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
[00131] In certain embodiments, RD is of the formula:
Figure imgf000037_0001
wherein i is an integer between 1 and 100, inclusive.
[00132] In certain embodiments, R5 is the side chain of a natural amino acid. In certain embodiments, R5 is hydrogen. In certain embodiments, R5 is methyl.
[00133] In certain embodiments, R6 is the side chain of a natural amino acid. In certain embodiments, R6 is hydrogen. In certain embodiments, R6 is methyl.
[00134] In certain embodiments, m is 0, and -XR1 is -OCH3. In certain embodiments, m is
1 , R6 is methyl, and -XR1 is -OH. In certain embodiments, m is 1 , R6 is hydrogen, and -XR1 is -OH.
[00135] In certain embodiments, the oligopeptide for c-terminal labeling is of the formula:
Figure imgf000037_0002
wherein
RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. In certain embodiments, RD is of the formula:
Figure imgf000037_0003
wherein i is an integer between 1 and 100, inclusive. In certain embodiments, RD is of the formula:
Figure imgf000038_0001
In certain embodiments, RD is of the formula:
Figure imgf000038_0002
[00136] For N-terminal labeling, e.g., as shown in Figure 24, inventive methods use an oligopeptide with a transamidase recognition sequence that forms an acyl enzyme. The oligopeptide may have any sequence of natural and/or unnatural amino acids and one or more of the amino acids may be modified or labeled in various embodiments. To give a few examples, the label may include a fluorescent tag, a phosphorescent tag, biotin, poly(histidine) tag, or a radioactive label. The oligopeptide may also be modified with carbohydrates, lipids, phosphate groups, labels, tags, other polymers (for example, a non- polypeptide polymer such as polyethylene glycol), and acetyl groups. Any biological or chemical modification of an amino acid or protein may be incorporated into the oligopeptide to be ligated using a transamidase. In certain embodiments, the oligopeptide includes a second transamidase recognition sequence or a masked transamidase recognition sequence. In certain embodiments, the oligopeptide is of the formula:
Figure imgf000038_0003
wherein transamidase recognition sequence is a sequence recognized by a transamidase; j is an integer between 0 and 10, inclusive; k is an integer between 0 and 10, inclusive; m is an integer between 0 and 10, inclusive; p is 1 or 2;
X is -O-, -NR-, or -S-; R is hydrogen; substituted or unsubstituted aliphatic; or substituted or unsubstituted heteroaliphatic; each occurrence of R1 is independently hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl; each occurrence of R3 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl;
R4 is the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; each occurrence of R5 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; and each occurrence of R6 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl.
[00137] In certain embodiments, the transamidase recognition sequence is LPXT, wherein X is a natural or unnatural amino acid. In certain embodiments, X is selected from D, E, A, N, Q, K, or R. In certain embodiments, the recognition sequence is selected from LPXT, LPXT, SPXT, LAXT, LSXT, NPXT, VPXT, IPXT, and YPXR. In certain embodiments, X is selected to match a naturally occurring transamidase recognition sequence. In certain embodiments, the transamidase recognition sequence is selected from: LPKT, LPIT, LPDT, SPKT, LAET, LAAT, LAET, LAST, LAET, LPLT, LSRT, LPET, VPDT, IPQT, YPRR, LPMT, LPLT, LAFT, LPQT5 NSKT, NPQT, NAKT, and NPQS. In certain embodiments, e.g., in which sortase A is used, the transamidase recognition motif comprises the amino acid sequence XiPX2X3, where Xi is leucine, isolucine, valine or methionine; X2 is any amino acid; X3 is threonine, serine, or alanine; P is proline; and G is glycine. In specific embodiments, as noted above Xj is leucine, and X3 is threonine. In certain embodiments, X2 is aspartate, glutamate, alanine, glutamine, lysine, or methionine. In certain embodiments, e.g., where sortase B is utilized, the recognition sequence often comprises the amino acid sequence NPXiTX2, where Xi is glutamine or lysine; X2 is asparagine or glycine; N is asparagine; P is proline and T is threonine. In certain embodiments, e.g., where sortase A from Streptococcus pyogenes (SrtAstrep) is utilized, the recognition sequence comprises the amino acid sequence LPXiTX2, where Xi is selected from D, E, A, N, Q, K, or R; X2 is alanine or glycine; L is leucine; P is proline and T is threonine. In certain embodiments, a recognition sequence for SrtAstrep is LPXiTG. In certain embodiments, a recognition sequence for SrtAstrep is LPXi TA. In certain embodiments, a recognition sequence for SrtAstrep is LPETA or LPETG. In certain embodiments, e.g., where sortase A from Staphylcoccus aureus (SrtAstaph) is utilized, the recognition sequence comprises the amino acid sequence LPX]TG, where Xi is selected from D, E, A, N, Q, K, or R; X2 is glycine; L is leucine; P is proline and T is threonine. In certain embodiments, a recognition sequence for SrtAstaph is LPETG. In certain embodiments, a recognition sequence for SrtAstrep is LPXiTA. The invention encompasses the recognition that selection of X may be based at least in part in order to confer desired properties on the compound containing the recognition motif. In some embodiments, X is selected to modify a property of the compound that contains the recognition motif, such as to increase or decrease solubility in a particular solvent. In some embodiments, X is selected to be compatible with reaction conditions to be used in synthesizing a compound comprising the recognition motif, e.g., to be unreactive towards reactants used in the synthesis. In some embodiments, X, e.g., Xi, is selected such that the transamidase recognition sequence is masked. [00138] In certain embodiments, j is 0. In certain embodiments, j is 1. In certain embodiments, j is 2. In certain embodiments, j is 3. In certain embodiments, j is 4. In certain embodiments, j is 5.
[00139] In certain embodiments, k is 0. In certain embodiments, k is 1. In certain embodiments, k is 2. In certain embodiments, k is 3. In certain embodiments, k is 4. In certain embodiments, k is 5. [00140] In certain embodiments, m is 0. In certain embodiments, m is 1. In certain embodiments, m is 2. In certain embodiments, m is 3. In certain embodiments, m is 4. In certain embodiments, m is 5.
[00141] In certain embodiments, p is 1. In certain embodiments, p is 2.
[00142] In certain embodiments, X is -O-. In certain embodiments, X is -NH-.
[00143] In certain embodiments, R1 is hydrogen. In certain embodiments, R1 is substituted aliphatic. In certain embodiments, R1 is unsubstituted aliphatic. In some embodiments, R1 is substituted CM2 aliphatic. In some embodiments, R1 is unsubstituted Ci- i2 aliphatic. In some embodiments, R1 is substituted Cj-6 aliphatic. In some embodiments, R1 is unsubstituted Ci-6 aliphatic. In some embodiments, R1 is Ci-3 aliphatic. In certain embodiments, R1 is Ci-6 alkyl. In some embodiments, R1 is butyl. In some embodiments, R1 is M-butyl. In some embodiments, R1 is isobutyl. In some embodiments, R1 is propyl. In some embodiments, R1 is n-propyl. In some embodiments, R1 is isopropyl. In some embodiments, R1 is ethyl. In some embodiments, R1 is methyl. In certain embodiments, R1 is substituted aryl. In certain embodiments, R1 is unsubstituted aryl. In certain embodiments,
R1 is substituted phenyl. In certain embodiments, R1 is unsubstituted phenyl.
[00144] In certain embodiments, -XR1 is -OCH3. In certain embodiments, -XR1 is -OH.
In certain embodiments, -XR1 is -NH2.
[00145] In certain embodiments, R3 is the side chain of a natural amino acid. In certain embodiments, R is hydrogen. In certain embodiments, R3 is methyl.
[00146] In certain embodiments, R4 is a modified side chain of a natural amino acid. In certain embodiments, R4 is a modified side chain of serine, threonine, lysine, aspartate, glutamate, arginine, asparagine, glutamine, or tyrosine.
[00147] In certain embodiments, R4 is of the formula:
Figure imgf000041_0001
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00148] In certain embodiments, R4 is of the formula:
Figure imgf000042_0001
wherein RD is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00149] In certain embodiments, R4 is of the formula:
Figure imgf000042_0002
wherein RD is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
[00150] In certain embodiments, R4 is of the formula:
Figure imgf000042_0003
wherein RD is substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
[00151] In certain embodiments, R4 is of the formula:
Figure imgf000042_0004
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00152] In certain embodiments, R4 is of the formula:
Figure imgf000043_0001
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00153] In certain embodiments, R4 is of the formula:
Figure imgf000043_0002
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00154] In certain embodiments, R4 is of the formula:
Figure imgf000043_0003
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl. [00155] In certain embodiments, RD is of the formula:
Figure imgf000043_0004
wherein i is an integer between 1 and 100, inclusive.
[00156] In certain embodiments, R5 is the side chain of a natural amino acid. In certain embodiments, R5 is hydrogen. In certain embodiments, R5 is methyl. [00157] In certain embodiments, R6 is the side chain of a natural amino acid. In certain embodiments, R6 is hydrogen. In certain embodiments, R6 is methyl.
[00158] In certain embodiments, m is 0, and -XR1 is -OCH3. In certain embodiments, m is
1, R6 is methyl, and -XR1 is -OH. In certain embodiments, m is 1, R6 is hydrogen, and -XR1 is -OH.
[00159] In certain embodiments, the oligopeptide for c-terminal labeling is of the formula:
Figure imgf000044_0001
wherein j, k, p, m, X, R1, R3, R4, R5, and R6 are as defined herein.
In some embodiments, a probe for use in N-terminal labeling comprises a modified transamidase sequence that comprises an ester group in place of a C-terminal amino acid residue. In some embodiments, a probe for use in n-terminal labeling comprises an amino acid residue at the C-terminus, e.g., G, GG, GGG, etc. In some embodiments, a nucleophile located at the N-terminus of a polypeptide to be labeled comprises at least 2 G residues, e.g., 2, 3, 4, 5, or more G residues.
[00160] Transamidase fragments having transamidation activity can be utilized in the methods described herein. Such fragments can be identified by producing transamidase fragments by known recombinant techniques or proteolytic techniques, for example, and determining the rate of protein or peptide ligation. The fragment sometimes consists of about 80% of the full-length transamidase amino acid sequence, and sometimes about 70%, about 60%, about 50%, about 40% or about 30% of the full- length transamidase amino acid sequence such as that of S. aureus Sortase A (GenBank Accession number AAD48437). In some embodiments, the fragment lacks an N-terminal portion of the full-length sequence, e.g., the fragment lacks the N-terminal portion extending to the end of the membrane anchor sequence. In some embodiments the fragment comprises the C-terminus of a full-length transamidase amino acid sequence. In some embodiments, a catalytic core region from a sortase is utilized, e.g., a region is from about position 60 to about position 206 of SrtA, e.g., S. aureus SrtA, or about from position 82 to about position 249 of SrtAstrep. [00161] Transamidases from other organisms also can be utilized in the processes described herein. Such transamidases often are encoded by nucleotide sequences substantially identical or similar to the nucleotide sequences that encode Srt A and Srt B. A similar or substantially identical nucleotide sequence may include modifications to the native sequence, such as substitutions, deletions, or insertions of one or more nucleotides. Included are nucleotide sequences that sometimes are 55%, 60%, 65%, 70%, 75%, 80%, or 85% or more identical to a native nucleotide sequence, and often are 90% or 95% or more identical to the native nucleotide sequence (each identity percentage can include a 1%, 2%, 3% or 4% variance). One test for determining whether two nucleic acids are substantially identical is to determine the percentage of identical nucleotide sequences shared between the nucleic acids. [00162] Calculations of sequence identity can be performed as follows. Sequences are aligned for optimal comparison purposes and gaps can be introduced in one or both of a first and a second nucleic acid sequence for optimal alignment. Also, non-homologous sequences can be disregarded for comparison purposes. The length of a reference sequence aligned for comparison purposes sometimes is 30% or more, 40% or more, 50% or more, often 60% or more, and more often 70%, 80%, 90%, 100% of the length of the reference sequence. The nucleotides at corresponding nucleotide positions then are compared among the two sequences. When a position in the first sequence is occupied by the same nucleotide as the corresponding position in the second sequence, the nucleotides are deemed to be identical at that position. The percent identity between the two sequences is a function of the number of identical positions shared by the sequences, taking into account the number of gaps, and the length of each gap, introduced for optimal alignment of the two sequences. [00163] Comparison of sequences and determination of percent identity between two sequences can be accomplished using a mathematical algorithm. Percent identity between two nucleotide sequences can be determined using the algorithm of Meyers & Miller, CABIOS 4: 11 17 (1989), which has been incorporated into the ALIGN program (version 2.0), using a PAM 120 weight residue table, a gap length penalty of 12 and a gap penalty of 4. Percent identity between two nucleotide sequences can be determined using the GAP program in the GCG software package (available at www.gcg.com), using a NWSgapdna. CMP matrix and a gap weight of 40, 50, 60, 70, or 80 and a length weight of 1, 2, 3, 4, 5, or 6. A set of parameters often used is a Blossum 62 scoring matrix with a gap open penalty of 12, a gap extend penalty of 4, and a frame shift gap penalty of 5.
[00164] Another manner for determining if two nucleic acids are substantially identical is to assess whether a polynucleotide homologous to one nucleic acid will hybridize to the other nucleic acid under stringent conditions. As use herein, the term" stringent conditions"refers to conditions for hybridization and washing. Stringent conditions are known to those skilled in the art and can be found in Ausubel et al. Current Protocols in Molecular Biology (John Wiley & Sons, Inc., New York, 1999). Aqueous and non-aqueous methods are described in that reference and either can be used. An example of stringent conditions is hybridization in 6X sodium chloride/sodium citrate (SSC) at about 450C, followed by one or more washes in 0.2X SSC, 0.1% SDS at 50°C. Another example of stringent conditions are hybridization in 6X sodium chloride/sodium citrate (SSC) at about 45°C, followed by one or more washes in 0.2X SSC, 0.1% SDS at 55°C. A further example of stringent conditions is hybridization in 6X sodium chloride/sodium citrate (SSC) at about 45°C, followed by one or more washes in 0.2X SSC, 0. 1% SDS at 600C. Often, stringent conditions are hybridization in 6X sodium chloride/sodium citrate (SSC) at about 45°C, followed by one or more washes in 0.2X SSC, 0.1% SDS at 650C. Also, stringency conditions include hybridization in 0. 5M sodium phosphate, 7% SDS at 65°C, followed by one or more washes at 0.2X SSC, 1% SDS at 65°C. [00165] A variant sequence can depart from a native amino acid sequence in different manners. Amino acid substitutions may be made on the basis of similarity in polarity, charge, solubility, hydrophobicity, hydrophilicity, helix-forming properties and/or amphipathic properties and the resulting variants are screened for antimicrobial activity. For example, negatively charged amino acids include aspartic acid and glutamic acid; positively charged amino acids include lysine and arginine; and amino acids with uncharged polar head groups having similar hydrophilicity values include leucine, isoleucine, valine, glycine, alanine, asparagine, glutamine, serine, threonine, phenylalanine, and tyrosine. In certain embodiments, conservative substitutions may be made, according to Table A. Amino acids in the same block in the second column and in the same line in the third column may be substituted for one another other in a conservative substitution. Certain conservative substitutions are substituting an amino acid in one row of the third column corresponding to a block in the second column with an amino acid from another row of the third column within the same block in the second column.
Table A
Figure imgf000046_0001
Figure imgf000047_0001
[00166] In certain embodiments homologous substitution may occur, which is a substitution or replacement of like amino acids, such as basic for basic, acidic for acidic, polar for polar amino acids, and hydrophobic for hydrophobic, for example. Non-homologous substitutions can be introduced to a native sequence, such as from one class of residue to another (e. g. , a non-hydrophobic to a hydrophobic amino acid), or substituting a naturally occurring amino acid with an unnatural amino acids or non- classical amino acid replacements.
[00167] Srt A and Srt B nucleotide sequences may be used as "query sequences" to perform a search against public databases to identify related sequences. Such searches can- be performed using the NBLAST and XBLAST programs (version 2.0) of Altschul, et ah, J. MoI. Biol. 215: 403 410 (1990). BLAST nucleotide searches can be performed with the NBLAST program, score = 100, wordlength = 12 to obtain homologous nucleotide sequences. To obtain gapped alignments for comparison purposes, gapped BLAST can be utilized as described in Altschul, et al, Nucleic Acids Res. 25 (17): 3389-3402 (1997). When utilizing BLAST and Gapped BLAST programs, default parameters of the respective programs {e.g., XBLAST and NBLAST) can be used (see www.ncbi.nlm.nih.gov). [00168] Different transamidases may specifically recognize different recognition sequences. In some embodiments, acyl donors utilized in the ligation processes described herein include or are modified with an appropriate sortase recognition motif. One or more appropriate sortase recognition sequences can be added to an acyl donor not having one by known synthetic and recombinant techniques. In certain embodiments, 2, 3, 4, 5, 6, 7, 8, 9, or 10 or more sortase or transamidase recognition sequences are incorporated in an acyl donor. [00169] In certain embodiments where Srt A is utilized as a transamidase enzyme, the acyl donor comprises the amino acid sequence XiPX2X3G, where Xi is leucine, isolucine, valine or methionine; X2 is any amino acid; X3 is threonine, serine or alanine; P is proline and G is glycine. In some embodiments, Xi is leucine and X3 is threonine. In certain embodiments, X2 is aspartate, glutamate, alanine, glutamine, lysine or methionine. In certain embodiments, the G is omitted and replaced with a acyl group as described herein. In some embodiments, the
O acyl donor comprises the sequence LPXT OR1 5 wherein X is any amino acid and R1 is as described herein.
[00170] In certain embodiments where Srt B is utilized as a transamidase enzyme, the acyl donor comprises the amino acid sequence NPXiTX2, where Xi is glutamine or lysine; X2 is asparagine or glycine; N is asparagine; P is proline and T is threonine. [00171] Transamidases utilized in the inventive ligation methods described herein sometimes are isolated and incorporated into a kit. Any convenient method known can be utilized to isolate the sortase or transamidase. In certain embodiments, the transamidase is produced with a N-terminal or C- terminal amino acid sequence that facilitates purification. For example, the transamidase sometimes is produced with a C-terminal or N-terminal polyhistidine sequence, often six histidines, which have affinity and bind to nickel-derivitized solid supports. In some embodiments, a transamidase used in accordance with the present invention further comprises an affinity tag. Examples of affinity tags include , e.g., His-tag (His6), FLAG, Streptag, HA tag, Myc tag, maltose binding protein, SNUT tag, NusA, T7, thioredoxin, GST, etc. (See, e.g., Arnau J, Lauritzen C, Petersen GE, Pedersen J., "Current strategies for the use of affinity tags and tag removal for the purification of recombinant proteins." Protein Expr Purif, 48(1):1-13, 2006).
[00172] In some embodiments, a kit includes a plasmid having a transamidase-encoding nucleotide sequence that the user uses to produce the sortase or transamidase in a cell culture or cell free translation system, and often, then purifies the sortase or transamidase according to instructions provided with the kit.
[00173] In the ligation methods described herein, the transamidase, acyl donor, and nucleophilic acyl acceptor are contacted with one another under suitable conditions to effect ligation of the acyl donor to the acyl acceptor. As used herein, the term "contacting" refers to placing the components of the process in close proximity to one another and allowing the molecules to collide by diffusion. Contacting these components with one another can be accomplished by adding them to one body of fluid and/or in one reaction vessel, for example. The components in the system may be mixed in a variety of manners, such as by oscillating a vessel, subjecting a vessel to a vortex generating apparatus, repeated mixing with a pipette or pipettes, or by passing fluid containing one assay component over a surface having another assay component immobilized thereon, for example. The components may be added in any order to the system. [00174] The ligation may be performed in any convenient vessel (e.g., tubes such as microfuge tubes, flask, dish), microtiter plates (e.g., 96-well or 384-well plates), glass slides, silicon chips, filters, or any solid or semisolid support having surface (optionally coated) having molecules immobilized thereon and optionally oriented in an array (see, e.g., U. S. Patent No. 6,261,776 and Fodor, Nature 364: 555-556 (1993)), and microfluidic devices (see, e.g., U. S. Patent Nos. 6,440,722; 6,429,025; 6,379,974; and 6,316,781). The system can include attendant equipment such as signal detectors, robotic platforms, and pipette dispensers.
[00175] The reaction mixture often is cell free and often does not include bacterial cell wall components or intact bacterial cell walls. In some embodiments, the system includes one or more cells or cell wall components, often non-bacterial cells or non-Gram-positive bacterial cells. In such embodiments, one or more components often are expressed by one or more recombinant nucleotide sequences in a cell, which nucleotide sequences are integrated into the cell genome or non-integrated (e.g., in a plasmid). Cells in such systems often are maintained in vivo, sometimes ex vivo, and sometimes in vitro.
[00176] The reaction mixture is maintained at any convenient temperature at which the ligation reaction can be performed. In some embodiments, the ligation is performed at a temperature ranging from about 15 0C to about 50 0C. In some embodiments, the ligation is performed at a temperature ranging from about 23 0C to about 37 0C. In certain embodiments, the temperature is room temperature (e.g., about 25°C). The temperature can be optimized by repetitively performing the same ligation procedure at different temperatures and determining ligation rates. Any convenient assay volume and component ratio is utilized. In certain embodiments, a component ratio of 1 : 1000 or greater transamidase enzyme to acyl donor is utilized, or a ratio of 1 : 1000 or greater transamidase enzyme to acyl acceptor is utilized. In specific embodiments, ratios of enzyme to acyl donor or enzyme to acyl acceptor is about 1 :1, including 1 :2 or greater, 1 :3 or greater, 1 :4 or greater, 1 :5 or greater, 1 :6 or greater, 1 :7 or greater, 1 :8 or greater, and 1 :9 or greater.
[00177] In some embodiments, the acyl donor is present at a concentration ranging from about 10 μM to about 10 mM. In some embodiments, the acyl donor is present at a concentration ranging from about 100 μM to about 1 mM. In some embodiments, the acyl donor is present at a concentration ranging from about 100 μM to about 5 mM. In some embodiments, the acyl donor is present at a concentration ranging from about 200 μM to about 1 mM. In some embodiments, the acyl donor is present at a concentration ranging from about 200 μM to about 800 μM. In some embodiments, the acyl donor is present at a concentration ranging from about 400 μM to about 600 μM. [00178] In certain embodiments, the nucleophilic acyl acceptor is present at a concentration ranging from about 1 μM to about 500 μM. In certain embodiments, the nucleophilic acyl acceptor is present at a concentration ranging from about 15 μM to about 150 μM. In certain embodiments, the nucleophilic acyl acceptor is present at a concentration ranging from about 25 μM to about 100 μM. In certain embodiments, the nucleophilic acyl acceptor is present at a concentration ranging from about 40 μM to about 60 μM. [00179] In certain embodiments, the transamidase is present at a concentration ranging from about 1 μM to about 500 μM. In certain embodiments, the transamidase is present at a concentration ranging from about 15 μM to about 150 μM. In certain embodiments, the transamidase is present at a concentration ranging from about 25 μM to about 100 μM. In certain embodiments, the transamidase is present at a concentration ranging from about 40 μM to about 60 μM.
[00180] In certain embodiments, the ligation method is performed in a reaction mixture comprising an aqueous environment. Water with an appropriate buffer and/or salt content often may be utilized. An alcohol or organic solvent may be included in certain embodiments. The amount of an organic solvent often does not appreciably esterify a protein or peptide in the ligation process (e.g., esterified protein or peptide often increase only by 5% or less upon addition of an alcohol or organic solvent). Alcohol and/or organic solvent contents sometimes are 20% or less, 15% or less, 10% or less or 5% or less, and in embodiments where a greater amount of an alcohol or organic solvent is utilized, 30% or less, 40% or less, 50% or less, 60% or less, 70% or less, or 80% or less alcohol or organic solvent is present. In certain embodiments, the system includes only an alcohol or an organic solvent, with only limited amounts of water if it is present.
[00181] In some embodiments, suitable ligation conditions comprise a buffer. One of ordinary skill in the art will be familiar with a variety of buffers that could be used in accordance with the present invention. In some embodiments, the buffer solution comprises calcium ions. In certain embodiments, the buffer solution does not contain substances that precipitate calcium ions. In some embodiments, the buffer solution does not include phosphate ions. In some embodiments, the buffer solution does not contain chelating agents. [00182] In some embodiments, suitable ligation conditions comprise pH in the range of 6 to 8.5. In some embodiments, suitable ligation conditions comprise pH in the range of 6 to 8. In some embodiments, suitable ligation conditions comprise pH in the range of 6 to 7.5. In some embodiments, suitable ligation conditions comprise pH in the range of 6.5 to 8.5. In some embodiments, suitable ligation conditions comprise pH in the range of 7 to 8.5. In some embodiments, suitable ligation conditions comprise pH in the range of 7.5 to 8.5. In some embodiments, suitable ligation conditions comprise pH in the range of 7.0 to 8.5. In some embodiments, suitable ligation conditions comprise pH in the range of 7.3 to 7.8. [00183] One or more components for ligation or a ligation product may be immobilized to a solid support. The attachment between an assay component and the solid support may be covalent or non-covalent (e.g., U. S. Patent No. 6,022,688 for non-covalent attachments). The solid support may be one or more surfaces of the system, such as one or more surfaces in each well of a microtiter plate, a surface of a glass slide or silicon wafer, Biacore chip, a surface of a particle, e.g., a bead (e.g., Lam, Nature 354: 82-84 (1991)) that is optionally linked to another solid support, or a channel in a microfluidic device, for example. Types of solid supports, linker molecules for covalent and non-covalent attachments to solid supports, and methods for immobilizing nucleic acids and other molecules to solid supports are known (e.g., U. S. Patent Nos. 6,261,776; 5,900,481; 6,133,436; and 6,022, 688; and WIPO publication WO 01/18234). Any material may be used, e.g., plastic (e.g., polystyrene), metal, glass, cellulose, gels (e.g., formed at least in part from organic polymers such as PDMS), etc. In some embodiments the solid support is semi-solid and/or gel-like, deformable, flexible, or the like.
[00184] Any protein or peptide may be utilized as an acyl donor or nucleophilic acyl acceptor in the ligation process described herein. The protein or peptide often is isolated when utilized in a cell-free system. The protein or peptide sometimes is a subregion of a protein, such as in the N-terminus, C-terminus, extracellular region, intracellular region, transmembrane region, active site (e.g., nucleotide binding region or a substrate binding region), a domain (e.g., an SH2 or SH3 domain) or a post-translationally modified region (e.g., phosphorylated, glycosylated or ubiquinated region), for example. Peptides often are 50 amino acids or fewer in length (e.g., 45, 40, 35, 30, 25, 20, or 15 amino acids or fewer in length) and proteins sometimes are 100 or fewer amino acids in length, or 200, 300, 400, 500, 600, 700, or 900 or fewer amino acids in length. The protein or peptide sometimes includes the modification moiety or a portion thereof (e. g. , the glycosyl group or a portion thereof). In certain embodiments, the protein is a signal transduction factor, cell proliferation factor, apoptosis factor, angiogenesis factor, or cell interaction factor. Examples of cell interaction factors include but are not limited to cadherins (e.g., cadherins E, N, BR, P, R, and M; desmocollins; desmogleins; and protocadherins); connexins; integrins; proteoglycans ; immunoglobulins (e.g., ALCAM, NCAM-I (CD56), CD44, intercellular adhesion molecules (e.g., ICAM-I and ICAM-2), LFA-I, LFA-2, LFA-3, LECAM-I, VLA-4, ELAM and N- <BR> CAM); selectins (e.g., L-selectin (CD62L), E-selectin (CD62e), and P-selectin (CD62P)) ; agrin; CD34; and a cell surface protein that is cyclically internalized or internalized in response to ligand binding.
[00185] Examples of signal transduction factors include but are not limited to protein kinases (e.g., mitogen activated protein (MAP) kinase and protein kinases that directly or indirectly phosphorylate it, Janus kinase (JAKl), cyclin dependent kinases, epidermal growth factor (EGF) receptor, platelet-derived growth factor (PDGF) receptor, fibroblast-derived growth factor receptor (FGF), insulin receptor and insulin-like growth factor (IGF) receptor); protein phosphatases (e.g., PTPlB, PP2A and PP2C); GDP/GTP binding proteins (e.g., Ras, Raf, ARF, Ran and Rho); GTPase activating proteins (GAFs); guanine nucleotide exchange factors (GEFs); proteases (e.g., caspase 3, 8 and 9), ubiquitin ligases (e.g., MDM2, an E3 ubiquitin ligase), acetylation and methylation proteins (e.g., p300/CBP, a histone acetyl transferase) and tumor suppressors (e.g., p53, which is activated by factors such as oxygen tension, oncogene signaling, DNA damage and metabolite depletion). The protein sometimes is a nucleic acid- associated protein (e.g., histone, transcription factor, activator, repressor, co-regulator, polymerase or origin recognition (ORC) protein), which directly binds to a nucleic acid or binds to another protein bound to a nucleic acid. The protein sometimes is useful as a detectable label, such as a green or blue fluorescent protein. In some embodiments a protein is a therapeutically useful protein. Certain proteins of interest are described further in the section entitled "Polypeptides" below.
[00186] In certain embodiments, the acyl donor comprises an antibody or antibody chain (heavy or light chain) or a portion thereof comprising an immunoglobulin domain (e.g., constant domain or variable domain). In some embodiments, antibodies are IgG, IgM, IgA, or IgE. The antibody may be of any class, subclass, or isotype in various embodiments of the invention. In some embodiments the antibody is of a class or isotype that is secreted. See, e.g., Murphy, K., et al., Janeway's Immunobiology, Garland Science; 7th edition (November 27, 2007). In some embodiments, antibodies are polyclonal or monoclonal, and may be chimeric, humanized or bispecific. Polyclonal and monoclonal antibodies that bind specific antigens are commercially available, and methods for generating such antibodies are known. In general, polyclonal antibodies are produced by injecting an isolated antigen into a suitable animal (e.g., a goat or rabbit); collecting blood and/or other tissues from the animal containing antibodies specific for the antigen and purifying the antibody. Methods for generating monoclonal antibodies, in general, include injecting an animal with an isolated antigen (e.g., often a mouse or a rat); isolating splenocytes from the animal; fusing the splenocytes with myeloma cells to form hybridomas; isolating the hybridomas and selecting hybridomas that produce monoclonal antibodies which specifically bind the antigen (e.g., Kohler & Milstein, Nature 256: 495 497 (1975) and StGroth & Scheidegger, J Immunol Methods 5: 1 21 (1980)). Examples of monoclonal antibodies are anti MDM 2 antibodies, anti-p53 antibodies (pAB421, DO 1, and an antibody that binds phosphoryl-serl5), anti- dsDNA antibodies and anti-BrdU antibodies, described hereafter.
[00187] Methods for generating chimeric and humanized antibodies also are known (see, e.g., U. S. patent No. 5,530,101 (Queen, et al), U. S. patent No. 5,707,622 (Fung, et al. ) and U. S. Patent Nos. 5,994,524 and 6,245,894 (Matsushima, et al.)), which generally involve transplanting an antibody variable region from one species (e.g., mouse) into an antibody constant domain of another species (e.g., human). Antigen-binding regions of antibodies (e.g., Fab regions) include a light chain and a heavy chain, and the variable region is composed of regions from the light chain and the heavy chain.
[00188] Given that the variable region of an antibody is formed from six complementarity- determining regions (CDRs) in the heavy and light chain variable regions, one or more CDRs from one antibody can be substituted (e.g., grafted) with a CDR of another antibody to generate chimeric antibodies. Also, humanized antibodies are generated by introducing amino acid substitutions that render the resulting antibody less immunogenic when administered to humans.
[00189] In some embodiments, the acyl donor comprises an antibody fragment, such as a Fab, Fab', F(ab)'2, Dab, Fv or single-chain Fv (ScFv) fragment, and recombinant methods for generating antibody fragments are known (e.g., U. S. Patent Nos. 6,099,842 and 5,990,296 and PCT/GBOO/04317). In general, single-chain antibody fragments are constructed by joining a heavy chain variable region with a light chain variable region by a polypeptide linker (e.g., the linker is attached at the C-terminus or N- terminus of each chain), and such fragments often exhibit specificities and affinities for an antigen similar to the original monoclonal antibodies. Bifunctional antibodies sometimes are constructed by engineering two different binding specificities into a single antibody chain and sometimes are constructed by joining two Fab'regions together, where each Fab'region is from a different antibody (e.g., U.S. Patent No. 6,342,221). Antibody fragments often comprise engineered regions such as CDR-grafted or humanized fragments. In certain embodiments the binding partner is an intact immunoglobulin, and in other embodiments the binding partner is a Fab monomer or a Fab dimer.
[00190] Acyl donors comprising proteins and peptides may chemically synthesized using known techniques (e.g., Creighton, 1983 Proteins. New York, N. Y.: W. H. Freeman and Company; and Hunkapiller et al, (1984) Nature July 12-18; 310 (5973): 105-11). For example, a peptide can be synthesized by a peptide synthesizer. If desired, non-classical amino acids or chemical amino acid analogs can be introduced as a substitution or addition into the fragment sequence. Non-classical amino acids include but are not limited to D- isomers of the common amino acids, 2, 4-diaminobutyric acid, a-amino isobutyric acid, 4- aminobutyric acid, Abu, 2-amino butyric acid, g-Abu, e-Ahx, 6-amino hexanoic acid, Aib, 2- amino isobutyric acid, 3 -amino propionic acid, ornithine, norleucine, norvaline, hydroxyproline, sarcosine, citrulline, homocitrulline, cysteic acid, t-butylglycine, t- butylalanine, phenylglycine, cyclohexylalanine, b-alanine, fluoroamino acids, designer amino acids such as b-methyl amino acids, Ca-methyl amino acids, Na-methyl amino acids, and amino acid analogs in general. Each amino acid in the peptide often is L (levorotary) and sometimes is D (dextrorotary). Proteins often are produced by known recombinant methods, or sometimes are purified from natural sources.
[00191] Native protein and peptide sequences sometimes are modified. For example, conservative amino acid modifications may be introduced at one or more positions in the amino acid sequences of target polypeptides. A "conservative amino acid substitution" is one in which the amino acid is replaced by another amino acid having a similar structure and/or chemical function. Families of amino acid residues having similar structures and functions are well known. These families include amino acids with basic side chains (e.g., lysine, arginine, histidine), acidic side chains (e.g., aspartic acid, glutamic acid), uncharged polar side chains (e.g., glycine, asparagine, glutamine, serine, threonine, tyrosine, cysteine), nonpolar side chains (e.g., alanine, valine, leucine, isoleucine, proline, phenylalanine, methionine, tryptophan), beta-branched side chains (e.g., threonine, valine, isoleucine) and aromatic side chains (e.g., tyrosine, phenylalanine, tryptophan, histidine). Also, essential and non- essential amino acids may be replaced. A "non-essential" amino acid is one that can be altered without abolishing or substantially altering the biological function of a target polypeptide, whereas altering an "essential" amino acid abolishes or substantially alters the biological function of a target polypeptide. Amino acids that are conserved among target polypeptides typically are essential amino acids. [00192] Proteins or peptides of an acyl donor may exist as chimeric or fusion polypeptides. As used herein, a "chimeric polypeptide" or "fusion polypeptide" includes a protein or peptide linked to a different polypeptide. The different polypeptide can be fused to the N- terminus or C-terminus of the target polypeptide. Fusion polypeptides can include a moiety having high affinity for a ligand. For example, the fusion polypeptide can be a GST-target fusion polypeptide in which the protein or peptide sequences are fused to the C-terminus of the GST sequences, or a polyhistidine-target fusion polypeptide in which the protein or peptide is fused at the N-or C-terminus to a string of histidine residues (e.g., sometimes three to six histidines). Such fusion polypeptides can facilitate purification of recombinant protein or peptide. Expression vectors are commercially available that already encode a fusion moiety, and a nucleotide sequence encoding the peptide or polypeptide can be cloned into an expression vector such that the fusion moiety is linked in-frame to the target polypeptide. Further, the fusion polypeptide can be a protein or peptide containing a heterologous signal sequence at its N- terminus. In certain host cells (e.g., mammalian host cells), expression, secretion, cellular internalization, and cellular localization of a target polypeptide can be increased through use of a heterologous signal sequence. Fusion polypeptides sometimes include all or a part of a serum polypeptide (e.g., an IgG constant region or human serum albumin).
[00193] Suitable systems for producing polypeptides in prokaryotic and eukaryotic systems are well known in the art and are of use in the invention. One of skill in the art will select an appropriate system (e.g., appropriate cell type and appropriate vector for inserting a nucleic acid encoding the protein). In some embodiments, a host cell is transformed to contain a vector that encodes a polypeptide whereby the polypeptide is produced in the cell. A host cell can be prokaryotic or eukaryotic cell, e.g., bacterial, fungal, plant, or animal (e.g., insect or mammalian). Exemplary host cells include bacterial cells (e.g., Gram-negative bacteria such as E. coli or Gram-positive bacteria such as B. subtilis or Lactococcus lactis), insect cells (e.g., Sf9), mammalian cells (e.g., CHO cells, COS cells, SP2/0 and NS/0 myeloma cells, human embryonic kidney (e.g., HEK 293) cells, baby hamster kidney (BHK) cell, human B cells, seed plant cells, and Ascomycete cells (e.g., Neurospora, Aspergillus and yeast cells; e.g., yeast of the genera Saccharomyces, Pichia, Hansenula, Schizosaccharomyces, Kluyveromyces, Yarrowia, and Candida). Exemplary yeast species include S. cerevisiae, Hansenula polymorpha, Kluyveromyces lactis, Pichia pastoris, Schizosaccharomyces pombe, and Yarrowia lipolytica. [00194] For a glycosylated protein, a cell type capable of performing such glycosylation can be selected. For production in eukaryotic cells, e.g., mammalian cells, yeast cells, insect cells (e.g., baculovirus-based), plant cells, or transgenic non-human animals or plants, a suitable signal sequence may be included at the N-terminus. In such instances, the nucleophilic residue(s), e.g., G or GG, and optional masking residues (e.g., a sequence comprising a protease cleavage site), are located C-terminal to the signal sequence, so that they are located at the N-terminus of the mature, secreted polypeptide. In some embodiments, a secretion signal sequence whose cleavage generates an N-terminal nucleophilic residue (e.g., an A or G) is used if a polypeptide is produced in eukaryotic, e.g., mammalian, cells. For example, cleavage of the H-2kb secretion sequence generates an N- terminal glycine. The protein sequence of the H-2kb secretion signal sequence is MVPCTLLLLLAAALAPTQTRA-GG (SEQ ID NO: 3). It gets cleaved at the dash to leave the GG at the N-terminus). An exemplary nucleotide sequence encoding this sequence is: atggtaccgt gcacgctgct cctgctgttg g cggccgccc tggctccgac tcagacccgc gcg (SEQ ID NO: 4). In some embodiments, a secretion signal sequence is selected such that, when cleaved, it leaves a masked nucleophilic residue near the N-terminus.
[00195] In certain embodiments, the acyl donor or acyl acceptor is modified by a process or with a moiety not typically incorporated into a protein during translation. In specific embodiments, the acyl donor or acyl acceptor comprises one or more moieties selected from an alkyl moiety (e.g., methyl moiety), an alkanoyl moiety (e.g., an acetyl group (e.g., an acetylated histone)), an alkanoic acid or alkanoate moiety (e.g., a fatty acid), a glyceryl moiety (e.g., a lipid), a phosphoryl moiety, a glycosyl moiety (e.g., N-linked or O-linked carbohydrate chains) or an ubiquitin moiety. Further, any of numerous chemical modifications may be carried out by known techniques, including but not limited to specific chemical cleavage by cyanogen bromide, trypsin, chymotrypsin, papain, V8 protease, NaBH4; acetylation, formylation, oxidation, reduction; metabolic synthesis in the presence of tunicamycin; and the like. The N-terminal and/or C-terminal ends may be processed (e.g., the N-terminal methionine may not be present due to prokaryotic expression of the protein or peptide) and chemical moieties may be attached to the amino acid backbone. Proteins and peptides sometimes are modified with a detectable label, such as an enzymatic, fluorescent, isotopic or affinity label to allow for detection and isolation of the polypeptide. [00196] When no transamidase or sortase recognition sequence is present in a acyl donor or acyl acceptor to be ligated, the acyl donor or acyl acceptor is modified to include an appropriate recognition sequence. When a recognition sequence is present in a native protein or peptide amino acid sequence, the recognition sequence often is removed unless it is located near the N-terminus or C-terminus. A recognition sequence can be removed in a native amino acid sequence by synthesizing it without the recognition sequence or by modifying some and/or all amino acids in the nucleotide sequence encoding the amino acid recognition sequence by known recombinant techniques. In some embodiments, when a recognition sequence and non-native sequence useful for purification are introduced to the native protein or peptide amino acid sequence, the recognition sequence is incorporated closer such that the non-native sequence useful for purification is cleaved from the acyl donor during ligation. In such embodiments, the transamidase also is modified with the non-native sequence and the ligated product is purified away from the reactants when contacted with a solid support that binds the non-native sequence. In embodiments where the acyl donor is modified with a detectable label or homing sequence for a detectable label, such sequences often are incorporated closer to the N-terminus than the recognition sequence so they are not cleaved from the protein or peptide in the ligation process.
[00197] In certain embodiments, the present invention provides an acyl donor compound of formula:
O vi— Transamidase recognition sequence XR1 wherein the transamidase recognition sequence, X, R1, and A1 are as defined above. [00198] In certain embodiments, the present invention provides an acyl donor compound of formula:
Figure imgf000057_0001
wherein X, R1, R2, and A1 are as defined above.
[00199] It will be appreciated that any acyl donor compound described herein for use in methods of ligation is similarly provided by the present invention. [00200] As described above, the transamidase catalyzes formation of an amide linkage between a NH2-CH2-moiety, which is joined to and/or is in the acyl acceptor, and an acyl moiety in the acyl donor. Suitable NH2-CH2-moieties are known and can be determined by performing the linkage processes described herein in a routine manner. Where an acyl acceptor does not include a suitable NH2-CH2-moiety, one or more NF^-CF^-moieties are joined to the molecule. Methods for joining one or more NH2-CH2-moieties to a molecule of interest are known and can be developed using techniques known in the art. In some embodiments, NH2-CH2-moieties utilized in the methods described herein are present as one or more glycine amino acids in attached to a B1 group. In certain embodiments, between one and seven glycines are present in or are incorporated into/onto a B1 group, and in specific embodiments, a B1 group is derivitized with three glycines.
[00201] The nucleophilic acyl acceptor can be any molecule that leads to a useful ligated conjugate. In certain embodiments, the nucleophilic acyl acceptor comprises a protein or peptide. In some embodiments, the nucleophilic acyl acceptor comprises an antibody epitope, an antibody, a recombinant protein, a synthetic peptide or polypeptide, a peptide comprising one or more D-amino acids, a peptide comprising all D-amino acids, a peptide comprising one or more unnatural or non-classical amino acids (e. g. , ornithine), a peptide mimetic, or a branched peptide. In some embodiments, the nucleophilic acyl acceptor comprises a peptide that confers enhanced cell penetrance to the acyl donor (e.g., a greater amount of the acyl donor compound conjugated to the acyl acceptor is translocated across a cell membrane in a certain time frame as compared to the acyl donor not conjugated to the acyl acceptor), which is referred to herein as a "protein transduction domain (PTD)" peptide or "transduction peptide." Any PTD can be conjugated to a protein or peptide using the methods described herein. PTD peptides are known, and include amino acid subsequences from HIV-tat (e.g., U. S. Patent No. 6,316,003), sequences from a phage display library (e.g., U. S. 20030104622) and sequences rich in amino acids having positively charged side chains (e.g., guanidino-, amidino-and amino-containing side chains; e.g., U. S. Patent No. 6,593,292). The PTD peptide sometimes is branched. The appended peptides promote cellular uptake and in some cases, cell-type specificity. Organelle-specific PTDs have also been generated, providing a means to target specific subcellular sites. See, e.g., Stewart KM, Horton KL, Kelley SO. Cell-penetrating peptides as delivery vehicles for biology and medicine. Org Biomol Chem. 6(13):2242-55, 2008. Also of interest are moieties that enhance stability of a second moiety such as a polypeptide, when conjugated thereto. For example, such moieties may increase the half-life of a compound in vivo. Examples include non-polypeptide polymers such as polyethylene glycol and derivatives thereof. In some embodiments a polymer is biocompatible. In some embodiments a polymer is biodegradable. [00202] In some embodiments, the nucleophilic acyl acceptor comprises a detectable moiety. Any known and convenient detectable moiety can be utilized. In certain embodiments, avidin, streptavidin, a fluorescent molecule, or a radioisotope is linked to the acyl donor. In some embodiments, biotin or another vitamin, such as thiamine or folate, is linked to the acyl donor. Examples of detectable moieties include various enzymes, prosthetic groups, fluorescent materials, luminescent materials, bioluminescent materials, and radioisotopes. Examples of suitable enzymes include horseradish peroxidase, alkaline phosphatase, p-galactosidase, or acetylcholinesterase; examples of suitable prosthetic group complexes include streptavidin/biotin and avidin/biotin; examples of suitable fluorescent materials include umbelliferone, fluorescein, fluorescein isothiocyanate, rhodamine, dichlorotriazinylamine fluorescein, dansyl chloride or phycoerythrin; an example of a luminescent material includes luminol; examples of bioluminescent materials include luciferase, luciferin, and aequorin, and examples of suitable radioisotopes include 1251, 131 I, 35S or 3H. The radioisotope sometimes is selected based upon its appropriate use in a nuclear medicinal procedure, such as Be-7, Mg-28, Co-57, Zn-65, Cu-67, Ge-68, Sr-82, Rb-83, Tc- 95m, Tc-96, Pd- 103, Cd- 109, and Xe- 127, to name but a few.
[00203] Conjugates between an acyl donor and a detectable label are useful in diagnostic procedures. Diagnostic procedures include, for example, nuclear medicinal procedures for locating diseased locations of a subject, and procedures for detecting specific components or pathogens in a biological sample from a subject. The conjugates also are useful as research tools. For example, the conjugates are useful in flow cytometry techniques and for detecting a cellular location of a specific protein or peptide in a cell. Thus, in certain embodiments, a NH2-CH2-derivitized fluorophore and a transamidase are contacted with cells that express a protein linked to a sortase recognition sequence. The transamidase, often a sortase, joins the fluorophore to the protein and allows detection of the cell, protein in the cell, or protein on the cell surface. In certain embodiments, the transamidase is expressed by a nucleotide sequence that encodes it in the cell (e.g., the nucleotide sequence sometimes is in a plasmid), and in other embodiments useful for detecting a protein on a cell surface or in a fixed cell, exogenous transamidase protein, often isolated protein, is contacted with the cell. [00204] The location of a protein in a cell sometimes is detected by a fluorescence imaging technique in cells fixed to a solid support. Imaging techniques include, for example, using a standard light microscope or a confocal microscope (e.g., U. S. Patent Nos. 5,283,433 and 5,296,703 (Tsien)). Appropriate light microscopes are commercially available and are useful for probing cells in two dimensions (/. e., the height of a cell often is not resolved), and confocal microscopy is useful for probing cells in three-dimensions. Many microscopy techniques are useful for determining the location of a protein in a cell (e.g., in the nucleus, cytoplasm, plasma cell membrane, nucleolus, mitochondria, vacuoles, endoplasmic reticulum or Golgi apparatus). Some microscopic techniques are useful for determining the location of molecular antigens in groups of cells, tissue samples, and organs. Cellular locations often are visualized by counter-staining for subcellular organelles.
[00205] In some embodiments, cells expressing the protein are subjected to a known flow cytometry procedure, such as flow microfluorimetry (FMF) and fluorescence activated cell sorting (FACS); U. S. Patent Nos. 6,090,919 (Cormack, et al.) ; 6,461,813 (Lorens); and 6,455,263 (Payan)). For use in these procedures, the protein often is expressed on the cell surface.
[00206] In certain embodiments, the nucleophilic acyl acceptor comprises a polymer or a small molecule. Polymers can be useful for enhancing protein or peptide solubility, stability and circulating time, and/or for decreasing immunogenicity when the protein or peptide is administered to a subject. In some embodiments, the polymer is a water soluble polymer such as polyethylene glycol, ethylene glycol/propylene glycol copolymers, carboxymethylcellulose, dextran, polyvinyl alcohol and the like, for example. The acyl donor may include one, two, three or more attached polymer moieties after ligation. The polymer may be of any molecular weight, and may be branched or unbranched. For polyethylene glycol, the molecular weight often is between about 1 kDa and about 100 kDa (the term "about" indicating that in preparations of polyethylene glycol, some molecules will weigh more, some less, than the stated molecular weight). Other sizes may be used, depending on a desired therapeutic profile {e.g., the duration of sustained release desired, the effects if any on biological activity, the ease in handling, the degree or lack of antigenicity and other known effects of the polyethylene glycol to a therapeutic protein or analog). [00207] Any small molecule derivatized with or having a NH2-CH2-moiety can be linked to an acyl donor having a transamidase recognition site. In certain embodiments, the small molecule is known to be bioactive. Such small molecules can be obtained using any of the numerous approaches in combinatorial library methods known in the art, including: biological libraries; peptoid libraries (libraries of molecules having the functionalities of peptides, but with a novel, non-peptide backbone which are resistant to enzymatic degradation but which nevertheless remain bioactive (see, e.g., Zuckermann et al. , J. Med. Chem. 37 : 2678-85 (1994)); spatially addressable parallel solid phase or solution phase libraries; synthetic library methods requiring deconvolution; "one-bead one-compound" library methods; and synthetic library methods using affinity chromatography selection. Biological library and peptoid library approaches are typically limited to peptide libraries, while the other approaches are applicable to peptide, non-peptide oligomer or small molecule libraries of compounds (Lam, Anticancer Drug Des. 12: 145, (1997)). Examples of methods for synthesizing molecular libraries are described, for example, in De Witt et al. , Proc. Natl. Acad. Sci. U. S. A. 90: 6909 (1993); Erb et al, Proc. Natl. Acad. Sci. USA 91 : 1 1422 (1994); Zuckermann et al, J. Med. Chem. 37: 2678 (1994); Cho et al, Science 261 : 1303 (1993); Carrell et al, Angew. Chem. Int. Ed. Engl. 33: 2059 (1994); Carell et al, Angew. Chem. Int. Ed. Engl. 33: 2061 (1994); and in Gallop et al, J. Med. Chem. 37: 1233 (1994). Libraries of compounds may be presented in solution {e.g., Houghten, Biotechniques 13: 412-421 (1992)), or on beads (Lam, Nature 354: 82-84 (1991)), chips (Fodor, Nature 364: 555-556 (1993)), bacteria or spores (Ladner, United States Patent No. 5,223,409), plasmids (Cull et al, Proc. Natl. Acad. Sci. USA 89: 1865-1869 (1992)). Small molecules include, but are not limited to, peptides, peptidomimetics (e. g. , peptoids), amino acids, amino acid analogs, polynucleotides, polynucleotide analogs, nucleotides, nucleotide analogs, organic or inorganic compounds (i. e. , including heteroorganic and organometallic compounds) having a molecular weight less than about 10,000 grams per mole, organic or inorganic compounds having a molecular weight less than about 5,000 grams per mole, organic or inorganic compounds having a molecular weight less than about 1 ,000 grams per mole, organic or inorganic compounds having a molecular weight less than about 500 grams per mole, and salts, esters, and other pharmaceutically acceptable forms of such compounds. In certain embodiments, the small molecule folate, spermine or puromycin is a component of an acyl donor. In other embodiments, the small molecule is a modification moiety described above, such as a phosphoryl moiety, ubiquitin moiety or a glycosyl moiety, for example. [00208] In some embodiments, the acyl acceptor comprises is a nucleic acid, such as a deoxyribonucleic acid, a ribonucleic acid, nucleic acid derivatives, and a modified nucleic acid. The nucleic acid may comprise or consist of DNA nucleotide sequences (e.g., genomic DNA (gDNA) and complementary DNA (cDNA)) or RNA nucleotide sequences (e.g., mRNA, tRNA, and rRNA). The nucleic acid sometimes is about 8 to about 50 nucleotides in length, about 8 to about 35 nucleotides in length, and sometimes from about 10 to about 25 nucleotides in length. Nucleic acids often are 40 or fewer nucleotides in length, and sometimes are 35 or fewer, 30 or fewer, 25 or fewer, 20 or fewer, and 15 or fewer nucleotides in length. Synthetic oligonucleotides can be synthesized using standard methods and equipment, such as by using an ABI3900 High Throughput DNA Synthesizer, which is available from Applied Biosystems (Foster City, CA). [00209] A nucleic acid sometimes is an analog or derivative nucleic acid, which can include backbone/linkage modifications (e.g., peptide nucleic acid (PNA) or phosphothioate linkages) and/or nucleobase modifications. Examples of such modifications are set forth in U. S. Patent No. 6,455,308 (Freier et al.) ; in U. S. Patent Nos. 4,469,863; 5,536,821 ; 5,541,306; 5,637,683; 5,637,684; 5,700,922; 5,717,083; 5,719,262; 5,739,308; 5,773,601; 5,886,165; 5,929, 226; 5,977,296; 6,140,482; and in WIPO publications WO 00/56746 and WO 01/14398. Methods for synthesizing oligonucleotides comprising such analogs or derivatives are disclosed, for example, in the patent publications cited above, and in U. S. Patent Nos. 6,455,308; 5,614, 622; 5,739,314; 5,955,599; 5,962,674; 6,117,992; and in WO 00/75372. Nucleic acids may be modified by chemical linkages, moieties, or conjugates that enhance activity, cellular distribution, or cellular uptake of nucleic acid, and examples of modifications in modified nucleic acids are in U. S. Patent Nos. 6,455,308 (Freier), 6,455,307 (McKay et al. ), 6,451,602 (Popoff et al.), and 6,451,538 (Cowsert). [00210] In some embodiements, the acyl acceptor comprises a toxin. Any toxin may be selected, and often is selected for high cytotoxic activity. Proteins or peptides ligated to a toxin often are useful as therapeutics. For example, a protein or peptide antibody or receptor that specifically binds to a cancer cell when linked to a toxin such as ricin is useful for treating cancer in subjects. In certain embodiments, the toxin is selected from the group consisting of abrin, ricin A, pseudomonas exotoxin and diphtheria toxin. [00211] In some embodiments, the acyl acceptor comprises a solid support. The solid support often is derivitized with multiple NH2-CH2-moieties, such as triglycine moieties. The solid support may be any described herein. In certain embodiments, the solid support is a glass slide, a glass bead, an agarose bead, a magnetic bead, a silicon wafer or a resin. In specific embodiments, a resin such as EAH Sepharose is derivitized with triglycine moieties using a FMOC/EDC derivitization procedure. In certain embodiments the solid support is a particle, e.g., a microparticle (e.g. a particle having an average diameter or smallest cross- sectional length greater than about 1 micron) or nanoparticle (average diameter or smallest cross-sectional length equal to or less than about 1 micron), liposome, etc. [00212] In some embodiments, the acyl acceptor comprises a phage that expresses a NH2- CH2-moiety on the surface. In some embodiments, the phage expresses a protein or peptide comprising one or more N- terminal glycines, sometimes three or five glycines at the N- terminus, and the phage expressing such a protein is contacted with a protein or peptide containing a transamidase recognition motif and a transamidase, thereby producing a phage/protein or phage/peptide conjugate. In some embodiments, a protein or peptide expressed at the phage surface comprises the transamidase recognition motif, and the phage is contacted with an acyl acceptor comprising a NH2-CH2-moiety and a transamidase, thereby producing a conjugate between the phage and the acyl acceptor. Methods for displaying a wide variety of peptides or proteins at the surface of a phage are known. The protein or peptide often is expressed as a fusion with a bacteriophage coat protein (Scott & Smith, Science 249: 386-390 (1990); Devlin, Science 249: 404-406 (1990); Cwirla et al, Proc. Natl. Acad. Sci. 87: 6378-6382 (1990); Felici, J. MoI. Biol. 222: 301-310 (1991)). Methods also are available for linking the test polypeptide to the N-terminus or the C-terminus of the phage coat protein. The original phage display system was disclosed, for example, in U. S. Patent Nos. 5,096,815 and 5,198,346. This system used the filamentous phage M13, which required that the cloned protein be generated in E. coli and required translocation of the cloned protein across the E. coli inner membrane. Lytic bacteriophage vectors, such as lambda, T4 and T7 are more practical since they are independent of E. coli secretion. T7 is commercially available and described in U. S. Patent Nos. 5,223,409; 5,403,484; 5,571,698 ; and 5,766,905. A protein or peptide comprising a NH2-CH2-moiety or a transamidase recognition sequence can be expressed on the surface of any other phage or virus, including but not limited to, murine leukemia virus (MLV), mouse mammary tumor virus (MMTV), Rous sarcoma virus (RSV), Fujinami sarcoma virus (FuSV), Moloney murine leukemia virus (Mo-MLV), FBR murine osteosarcoma virus (FBR MSV), Moloney murine sarcoma virus (Mo-MSV), Abelson murine leukemia virus (A-MLV), Avian myelocytomatosis virus- 29 (MC29), and Avian erythroblastosis virus (AEV), human immunodeficiency virus (HIV), simian immunodeficiency virus (SIV), visna/maedi virus (VMV), caprine arthritis-encephalitis virus (CAEV), equine infectious anemia virus (EIAV), feline immunodeficiency virus (FIV), bovine immunodeficiency virus (BIV), a hepatitis virus {e.g., hepatitis B or C), rhinovirus, herpes-zoster virus (VZV), herpes simplex virus {e.g., HSV-I or HSV-2), cytomegalovirus (CMV), vaccinia virus, influenza virus, encephalitis virus, hantavirus, arbovirus, West Nile virus, human papilloma virus (HPV), Epstein-Barr virus, and respiratory syncytial virus. [00213] In some embodiments, the acyl donor or acyl acceptor comprises a cleavable moiety, e.g., Ai or B1 comprises a cleavable moiety. In some embodiments the acyl donor or acyl acceptor comprises a cleavage site for a protease (e.g., a polypeptide sequence that is recognized by a protease and cleaved). In such embodiments, a cleavage reagent, e.g., a protease, may be used to cleave the product of a transamidation reaction. The cleavable moiety may be positioned at any desired location, e.g., between a sortase recognition sequence and a moiety of interest such as a tag, label, etc. A number of proteases that cleave polypeptides at particular sequences are known in the art. Examples of sequences having peptidase activity are known (e. g., cysteine-type endopeptidases, aspartic-type endopeptidases, elastases, metalloendopeptidases, mitochondrial inner membrane peptidases, serine-type endopeptidases, threonine endopeptidases, thrombin and other proteases involved in the coagulation and/or clotting cascade or other biological cascades. In some embodiments the cleavable moiety is photocleavable. In some embodiments the cleavage site is located at a position 1,2, 3,4, 5,6, 7, 8,9 or 10 amino acids away from an end of the recognition sequence, and sometimes at a position 15 or fewer, 20 or fewer, 50 or fewer or 100 or fewer amino acids away from the an end of the recognition sequence or, in some embodiments, from an N- or C-terminal end of a polypeptide comprising a recognition sequence or that acts as a nuclephile in a method described herein. In some embodiments, the acyl donor or acyl acceptor comprises a linker sequence, also referred to as a "spacer". A linker sequencemay be, e.g., 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 25 or fewer, 30 or fewer, 40 or fewer, 50 or fewer, 60 or fewer, 70 or fewer, 80 or fewer, 90 or fewer or 100 or fewer amino acids in length. The linker may be positioned at any desired location, e.g., between a sortase recognition sequence and a moiety of interest such as a tag, label, etc. [00214] The invention provides kits comprising one or more acyl donor compounds as described above. In certain embodiments, a kit comprises a compound of formula:
O
A1- Transamidase recognition sequence XR1 wherein the transamidase recognition sequence, X, R1, and A1 are as defined above. In certain embodiments, a kit comprises a compound of formula:
Figure imgf000064_0001
wherein X, R1, R2, and A1 are as defined above. In some embodiments, a kit comprises a compound comprising a masked transamidase recognition sequence, e.g., any of the inventive probes described herein. In some embodiments, the kit further comprises a transamidase. In some embodiments, the kit further comprises a sortase. In some embodiments, the kit further comprises sortase A, e.g., SrtAstaph, SrtAstrep, or both. In certain embodiments a kit comprises an enzyme or other reagent for unmasking a masked transamidase recognition sequence. In certain embodiments, the kit further comprises instructions for ligation with a nucleophilic compound.
[00215] In some embodiments, a kit provides a nucleophilic compound of formula:
Figure imgf000065_0001
wherein B1 and n are as defined above.
[00216] Other techniques, ligands, antibodies, and enzymes are known in the art and may be used in accordance with the present invention, including those described by Hornbeck, P., Curr Protoc Immunol., Enzyme-Linked Immunosorbent Assays, 2001 May; Chapter 2, Unit 2.1; Ausubel et al. Current Protocols in Molecular Biology (John Wiley & Sons, Inc., New York, 1999); Molecular Cloning: A Laboratory Manual, 2nd Ed., ed. by Sambrook, Fritsch, and Maniatis (Cold Spring Harbor Laboratory Press: 1989); Antibodies: A Laboratory Manual, E. Harlow and D. Lane, ed., Cold Spring Harbor Laboratory (Cold Spring Harbor, NY, 1988), each of which is herein incorporated by reference. [00217] Transamidase-Mediated Protein Circular ization
[00218] The invention encompasses the recognition that transamidases can be used to circularize polypeptides with high efficiency. In one aspect, the invention provides a method of circularizing a polypeptide comprising contacting the polypeptide with a transamidase, e.g., sortase, wherein the polypeptide comprises one or more nucleophilic residue(s) at its N- terminus and a transamidase recognition sequence (e.g., LPXTG) at or near its C-terminus, under suitable conditions such that circularization occurs. The nucleophilic residue at the N- terminus is one that can be used by the transamidase and the transamidase recognition sequence is one that can be recognized by the transamidase. For example, if the transamidase is S. aureus SrtA, the N-terminus can comprise one or more G residues (e.g., 1, 2, 3, 4, 5, etc.), and the transamidase recognition sequence can comprise LPXTG. The resulting circular polypeptide comprises a transamidase recognition sequence positioned between the original C- and N- termini of the polypeptide. Remarkably, it has been discovered that circularization can proceed with high efficiency, thus making the transamidase-mediated circularization reaction a feasible means of producing circular proteins with yield and purity compatible with the needs of large-scale and/or commercially feasible production. In certain embodiments of the invention at least 30%, 40%, 50%, 60%, 70%, 80%, 90%, or more of the starting polypeptide is converted to circular form. [00219] In certain embodiments, the invention provides a circular variant of a polypeptide of interest, wherein the original N- and C-terminal amino acids of the polypeptide of interest are joined together via a linker oligopeptide that comprises or consists of a transamidase recognition sequence. For example, in some embodiments the circular polypeptide comprises the sequence Xaac-(Xaa)k-| transamidase recognition sequence|-(Xaa)m -XaaN, where"Xaac" and "XaaN" represent the amino acids present at the C- and N-termini of the original linear polypeptide, "Xaa" is any amino acid (wherein each Xaa may be a natural or unnatural amino acid and optionally comprises a modified or substituted side chain in certain embodiments, e.g., as defined elsewhere herein), and k and m are independently integers between 0 and 15. In some embodiments, k and m are each independently between 0 and 5 (e.g., 0, 1, or 2), or between 0 and 10. In some embodiments, k+m is between 0 and 5, between 0 and 10, or between 0 and 20. In some embodiments the transamidase recognition sequence is LPXTG, e.g., LPETG. In some embodiments the circular polypeptide comprises Xaac-LPXTG-XaaN; Xaac-LPXTGG-XaaN; Xaac-GLPXTGG-XaaN; Xaac-GGLPXTGG-XaaN. In some embodiments X is E.
[00220] The invention provides means for purifying a circularized polypeptide away from a starting linear polypeptide. In one aspect, the method comprises (i) providing a polypeptide of interest that comprises one or more nucleophilic residue(s) at its N-terminus and a sequence comprising a transamidase recognition sequence (e.g., LPXTG) and a peptide that serves as an affinity tag at or near its C-terminus; and (ii) contacting the polypeptide of interest with a transamidase under conditions suitable for transamidation reaction to occur. For example, the sequence at or near the C-terminus of the polypeptide of interest can comprise His6, e.g., LPXTGG-His6. The transamidase in some embodiments also comprisesa tag, which may be the same or different from the tag present in the polypeptide of interest. In accordance with the inventive method, transamidase-mediated circularization removes a portion of the C-terminal sequence comprising the tag. The reaction mixture can then be contacted with a moiety that binds to the tag(s). The circular polypeptide will not be bound and can be conveniently separated from the starting linear polypeptide and/or transamidase. For example, the reaction mixture can be contacted with a resin that binds to the tag (e.g., by passing the material through a column containing the resin). The circular polypeptide does not bind to the resin, flows through the column, and can thus be easily purified. [00221] The invention provides purified preparations of a circularized polypeptide as described above, wherein the circularized polypeptide is at least 50%, 60%, 70%, 80%, 90%, 95%, 96%, 97%, 98%, 99%, or more of the polypeptide material in the preparation by dry weight. In some embodiments, the circularized polypeptide is at least 50%, 60%, 70%, 80%, 90%, 95%, 96%, 97%, 98%, 99%, or more of the material in the preparation by dry weight (optionally excluding counterions that may be present). In some embodiments, a polypeptide preparation comprises at least 10 mg, at least 100 mg, or at least 1 g of polypeptide by dry weight.
[00222] In some embodiments, a circularized polypeptide of the invention displays at least one enhanced property relative to a non-circular form. In some embodiments, the polypeptide displays increased stability, e.g., increased resistance to exoprotease(s), increased thermal stability, increased circulating time in vivo, increased biological half-life, less propensity to aggregate, and/or increased rate of refolding. [00223] Dual Modification Using Different Sortases
[00224] The invention provides methods for modifying a polypeptide at both the N- and C-termini. In some embodiments, the inventive methods make use of two transamidases, e.g., sortases, that recognize distinct transamidase recognition sequences. In some embodiments a first transamidase is able to recognize a first TRS but is not able to significantly recognize a second TRS, while the second transamidase is able to recognize the second TRS but is not able to significantly recognize the first TRS. In such embodiments the transamidase reactions can be carried out sequentially (in either order) or simultaneously in various embodiments. In some embodiments the inventive methods make use of two transamidases, e.g., sortases, wherein the first transamidase is able to recognize a first TRS but is not able to recognize a second TRS, and the second transmidase is able to recognize both the first TRS and a second TRS. For example, Streptococcus pyogenes Sortase A (SrtAstrep) will accept di-alanine based nucleophiles. This sortase will efficiently cleave LPXTA between theronine and alanine and install modified alanine-based nucleophiles. SrtAstrep will also recognize and cleave LPXTG motifs, albeit with reduced efficiency. SrtAstaph will not significantly cleave LPXTA motifs or accept alanine based nucleophiles. In one embodiment, a polypeptide is contacted with SrtAstrep and an alanine-containing nucleophile comprising the desired modifying moiety. The polypeptide comprises a TRS that can recognized by SrtA strep at or near its C-terminus and one or more amino acids capable of serving as a nucleophile for a SrtAstaph-mediated reaction at or near its N-terminus (e.g., (G)n, where n is between 1 and 10, e.g., between 1 and 5). This leads to the formation of an LPXTA sequence at the site of ligation, a motif refractory to cleavage by SrtAstaph- This allows SrtAstaph to act on the N terminus without affecting the C-terminal modification installed with SrtAstrep. In certain embodiments the nucleophilic amino acid(s) are masked, so that they are not recognized by SrtAstrep . For example, a sequence that can be cleaved by a protease can be positioned so that cleavage exposes the nucleophilic amino acid(s). In the absence of such cleavage, the nucleophilic residue cannot participate in a sortase-mediated reaction. A sequence that contains two amino acids in suitable context for cleavage by a protease is referred to as a "protease recognition site" herein. The protease recognition sequence serves to mask the nucleophilic amino acid. Additional amino acids may be present N-terminal of the protease recognition site. In some embodiments, the protease recognition site is a thrombin recognition site. In some embodiments the thrombin recognition site comprises the sequence LVPRG, LVPRGG or LVPRGS, wherein thrombin cleaves between R and G. In another embodiment, PreScission Protease, a genetically engineered fusion protein consisting of human rhino virus 3 C protease and GST, is used. LEVLF Q/GP is the standard recognition site. Alternative sites can be cleaved. LE-P4-LFQ/GP (where P4=VaI Ala or Thr) can be used. Other proteases that cleave between a first amino acid and a second amino acid, wherein the second amino acid can serve as a nucleophile for a transamidase, can be used. One of skill in the art will be able to select an appropriate protease to cleave C- terminal to a nucleophilic amino acid of interest. The protease and/or cleavage conditions can be selected such that minimal or no undesired cleavage within the polypeptide occurs. The cleaving conditions and agent (e.g., protease) may be selected consistent with maintaining stability of the engineered protein except with respect to the desired cleavage. After cleavage, the protease may be removed or the protein isolated from the reaction mixture in which cleavage was performed. The protease can comprise a tag for convenient removal after cleavage. In some embodiments the protease is immobilized, e.g., on a solid or semisolid support, e.g., particles. Following a transamidase-mediated ligation at the C-terminus, the polypeptide is contacted with the protease to expose the N-terminal nucleophilic amino acid. The polypeptide is contacted with a second transamidase and an appropriate probe for N-terminal modification. An exemplary strategy for dual-terminus labeling is outlined in Figures 33b and 34. The invention also encompasses use of chemical agents for cleavage to expose a nucleophilic amino acid. Polypeptides comprising a masked nucleophilic amino acid usable by a transamidase and appropriate cleavable masking sequence (often positioned near the N-terminus of the polypeptide) and a transamidase recognition sequence at or near the C-terminus are an aspect of the invention and have a variety of uses. [00225] Site-Specific Modification and Circular ization of Polypeptides [00226] The invention provides methods for both circularizing and site-specifically modifying a polypeptide. In some embodiments, modification is performed using an oligonucleotide probe comprising a TRS, which in some embodiments is a masked TRS. The TRS comprises a side chain comprising a modifying moiety of interest. Figure 43 shows a schematic diagram of an inventive approach according to this aspect of the invention. A polypeptide is equipped with a nucleophilic residue at or near the N-terminus and a first TRS at or near its C-terminus. The nucleophilic residue may be masked, e.g., with a protease recognition sequence that, when cleaved, exposes a nucleophilic residue. The polypeptide is contacted with a transamidase and an inventive oligonucleotide probe comprising a second TRS (which is masked in some embodiments and/or is different in sequence to the first TRS in some embodiments) and an amino acid having a modifying moiety (e.g., a label) attached thereto. The transamidase appends the oligonucleotide probe at the C-terminus of the polypeptide. In embodiments in which the second TRS (in the probe) is a masked TRS, the polypeptide is contacted with an agent or condition (phosphatase, light, etc.) that unmasks the TRS. In embodiments in which the nucleophilic residue at the N terminus is masked, the polypeptide is also contacted with an agent that unmasks it (e.g., a protease). The polypeptide is contacted with a second transamidase, which catalyzes a second transamidase reaction, which circularizes the polypeptide. The sequence of the polypeptide between the original N- and C-terminal amino acids can be unchanged relative to the original sequence. The N- and C-termini of the polypeptide are joined in the circularized version by a short linker peptide that comprises at least one TRS. In some embodiments the linker peptide comprises two TRSs. It should be noted that the probe depicted in Fig. 43 is exemplary. In some embodiments, the G residues in the GKG sequence are omitted, or other amino acids are used. In some embodiments, a probe comprises two or more lysine residues (or other residues having a readily modifiable side chain), wherein at least two moieties are attached to the side chains. In some embodiments, the probe comprises two or more different modifying moieties, which are optionally attached to different amino acids. [00227] In some embodiments, a polypeptide circularized using an inventive probe comprises the following sequence: — lpetAAGKGLPETgg — wherein lpet in lower case is from the C-terminus of the polypeptide. The AAGKGLPET is from the probe. The gg in lower case is from the N-terminus of the polypeptide. It will be understood that the lpet and gg are often not present in an original naturally occurring polypeptide but are present in a modified polypeptide for purposes of serving as a TRS and nucleophile, respectively, in transamidase-mediated reactions. Thus, in certain embodiments a circularized polypeptide comprises the sequence (Xaa)c — TRS1-SP-TRS2 — (Xaa)N , wherein TRSl is a first TRS, TRS2 is a second TRS, SP is a spacer peptide comprising sequences from the probe (e.g.,GKG), and each — represents one or more optionally present amino acid residues. In some embodiments, a circularized version of an original (e.g., naturally occurring) polypeptide comprises the sequence (Xaa)clpetAAGKGLPETgg(Xaa)N, wherein (Xaa)c is from the C-terminus of the original polypeptide, and (Xaa)N is from the N-terminus of the original polypeptide. A moiety, e.g., a PEG, is attached to the lysine side chain in some embodiments. In some embodiments, one or more of the G residues in the probe (and thus the circularized polypeptide) is omitted.
[00228] Joining Two or More Polypeptides or Polypeptide Domains [00229] The invention provides methods of covalently linking two or more polypeptides using an inventive olignucleotide probe, which in some embodiments comprises a TRS, e.g., a masked TRS. Figure 45 is a schematic diagram showing certain embodiments of the inventive approach. In some embodiments, the probe comprises a moiety of interest such as PEG, a detectable label, etc. In some embodiments, at least one of the polypeptides comprises a targeting or delivery domain. A delivery domain facilitates delivery of a compound, e.g,. a polypeptide, to a site of interest, e.g., a site in the body. A targeting domain (which can function as a delivery domain in some embodiments) specifically binds to a molecule of interest, such as a receptor. For example, a targeting domain can be an an antibody, antibody chain, antibody fragment, e.g., a single-chain antibody or an antigen-binding portion thereof. In some embodiments, one of the polypeptides comprises an Fc domain of an antibody, e.g., an IgGl antibody. In some embodiments an Fc domain is dimeric. Without limitation, an Fc domain can confer one or more desired properties. For example, an Fc domain can prolong the half-life of a polypeptide. An Fc domain can function as a targeting/delivery domain. For example, the neonatal constant region fragment (Fc) receptor (FcRn), which is responsible for IgG transport across the intestinal epithelium in newborn rodents, is expressed in epithelial cells in adult humans and non-human primates, and FcRn-mediated transport is functional in the lung of non-human primates. This transport system can be used to deliver a polypeptide of interest when it is conjugated to the Fc domain of IgGl . See, e.g., Bitonti AJ, et al., "Pulmonary delivery of an erythropoietin Fc fusion protein in non-human primates through an immunoglobulin transport pathway. Proc Natl Acad Sci U S A 101(26):9763-8, 2004. See also U.S. Pat. Pub. No. 2007/0178112. In some embodiments, one of the polypeptides comprises albumin, e.g., human serum albumin. In some embodiments, a targeting or delivery domain comprises a ligand for a receptor, wherein the receptor is expressed at the surface of a target cell. [00230] Selected Moieties of Interest
[00231] Without limiting the invention in any way, in some embodiments of interest, a moiety comprises a biocompatible polymer, e.g., a polyalkylene glycol, e.g., a polyethylene glycol (PEG), a polypropylene glycol, or a derivative thereof. In some aspects, the invention offers a number of advantages relative to various other available methods for modifying a polypeptide with a polymer, e.g., other PEGyation methods. PEG is discussed herein for exemplary purposes. Without limitation, the inventive methods permit installation of a single PEG chain (or a small number of chains, e.g., 2, 3, 4) at a defined location and avoid PEGylation of residues within the native polypeptide sequence, which could reduce activity, e.g., potency. Inventive methods provide means to modify a polypeptide at a defined position without introducing a cysteine residue into the polypeptide or appending a cysteine residue thereto. In some embodiments, PEG with an average molecular weight of about 5 kD is used. In some embodiments a PEG with an average molecular weight of 10 kD is used. In some embodiments, PEG with an average molecular weight of about 15 kD, 20 kD, 25 kD, 3OkD, 40 kD, 45 kD, 5OkD, 55 kD, or more is used. In some embodiments, a linear PEG is used. In some embodiments a branched PEG, forked PEG, or comb structure PEG is used. In some embodiments, a polypeptide PEGylated using an inventive method displays increased circulating time without causing a significant reduction in potency. In contrast, standard, random PEGylation approaches often result in considerable reduction in potency. See, e.g., Jevsevar, S, et al., PEGylation of Therapeutic Proteins, Biotechnol. J. 5, 113-128, 2010, and references therein, for discussion of certain PEGylated pharmaceuticals, PEG reagents, etc. [00232] Selected Polypeptides of Interest
[00233] Without limiting the invention in any way, this section discusses certain polypeptides of interest. Certain aspects of the present invention relate to the recognition that certain polypeptides are particularly amenable to the circularization approaches described herein. In certain embodiments, a polypeptide to be circularized is one whose N- and C- terminus are located within close proximity to each other in the native structure. For example, in certain embodiments the termini are located no more than 15 Angstroms (A) apart. In certain embodiments the termini are located no more than 20 A apart. In certain embodiments the termini are located no more than 25 A apart. In certain embodiments, where the termini are located more than, e.g., about 15A apart in the native structure, the polypeptide is modified to extend either the N- or C-terminus, or both, with a flexible spacer peptide so that the termini can be in closer proximity to each other. In certain embodiments, a polypeptide to be circularized and, optionally, labeled as described herein (e.g., PEGylated) is characterized in that its N- and C-termini are positioned such that they are not required for the activity of the polypeptide and/or for interaction of the polypeptide with a biological target of the polypeptide. For example, if the polyptide is one that naturally interacts with a receptor, the N- and C-termini are positioned such that they are not required for such interaction, e.g., they are positioned away from the receptor binding domain.In some embodiments the polypeptide of interest comprises or consists of a polypeptide that is at least 80%, or at least 90%, e.g., at least 95%, 86%, 97%, 98%, 99%, 99.5%, or 100% identical to a naturally occurring polypeptide. In some embodiments, the polypeptide has no more than 1 , 2, 3, 4, 5, 6, 7, 8, 9, or 10 amino acid differences relative to a naturally occurring sequence. In some embodiments the naturally occurring polypeptide is a mammalian polypeptide, e.g., of human origin. In some embodiments the naturally occurring polypeptide is a cytokine, e.g., a type I cytokine. In some embodiments of particular interest, the polypeptide of interest is a four-helix bundle protein, e.g., a four-helix bundle cytokine. Exemplary four-helix bundle cytokines include, e.g., certain interferons (e.g., a type I intereferon, e.g., IFN-α), interleukins (e.g., IL-2, IL -3, IL-4, IL-5, IL-6, IL-7, IL-12), and colony stimulating factors (e.g., G-CSF, GM-CSF, M-CSF). The IFN can be, e.g., interferon alpha 2a or interferon alpha 2b. See, e.g., Mott HR and Campbell ID. "Four-helix bundle growth factors and their receptors: protein-protein interactions." Curr Opin Struct Biol. 1995 Feb;5(l): 114-21; Chaiken IM, Williams WV. "Identifying structure-function relationships in four-helix bundle cytokines: towards de novo mimetics design." Trends Biotechnol. 1996 Oct;14(10):369-75; Klaus W, et al., "The three-dimensional high resolution structure of human interferon alpha- 2a determined by heteronuclear NMR spectroscopy in solution". J MoI Biol., 274(4):661-75, 1997, for further discussion of certain of these cytokines.
[00234] In some embodiments, the cytokine has a similar structure to one or more of the afore-mentioned cytokines. For example, the cytokine can be an IL-6 class cytokine such as leukemia inhibitory factor (LIF) or oncostatin M. In some embodiments, the cytokine is one that in nature binds to a receptor that comprises a GP 130 signal transducing subunit. Other four-helix bundle proteins of interest include growth hormone (GH), prolactin (PRL), and placental lactogen. In some embodiments, the polypeptide of interest is an erythropoiesis stimulating agent, e.g., erythropoietin (EPO), which is also a four-helix bundle cytokine. In some embodiments, an erythropoiesis stimulating agent is an EPO variant, e.g., darbepoetin alfa, also termed novel erythropoiesis stimulating protein (NESP), which is engineered to contain five N-linked carbohydrate chains (two more than recombinant HuEPO). In some embodiments, the polypeptide comprises five helices. For example, the polypeptide can be an interferon beta, e.g., interferon beta-la or interferon beta-lb, which (as will be appreciated) is often classified as a four-helix bundle cytokine.
[00235] In some embodiments, a polypeptide of interest is IL-9, IL-IO, IL-1 1, IL- 13, or IL- 15. In some embodiments. See, e.g., Hunter, CA, Nature Reviews Immunology 5, 521- 531, 2005, for discussion of certain cytokines. See also Paul, WE (ed.), Fundamental Immunology, Lippincott Williams & Wilkins; 6th ed., 2008.
[00236] In some embodiments, a polypeptide is one that is approved by the US Food & Drug Administration (or an equivalent regulatory authority such as the European Medicines Evaluation Agency) for use in treating a disease or disorder in humans. Such polypeptide may or may not be one for which a PEGylated version has been tested in clinical trials and/or has been approved for marketing.
[00237] In some embodiments, a polypeptide of interest is a neurotrophic factor, i.e., a factor that promotes survival, development and/or function of neural lineage cells (which term as used herein includes neural progenitor cells, neurons, and glial cells, e.g., astrocytes, oligodendrocytes, microglia). For example, the factor could promote neurite outgrowth. In some embodiments, the polypeptide is ciliary neurotrophic factor (CNTF; a four-helix bundle protein) or an analog thereof such as Axokine, which is a modified version of human Ciliary neurotrophic factor with a 15 amino acid truncation of the C terminus and two amino acid substitutions, which is three to five times more potent than CNTF in in vitro and in vivo assays and has improved stability properties.
[00238] In some embodiments, the polypeptide of interest is one that forms homodimers or heterodimers, (or homo- or heterooligomers comprising more than two subunits, such as tetramers). In certain embodiments the homodimer, heterodimer, or oligomer structure is such that a terminus of a first subunit is in close proximity to a terminus of a second subunit. For example, an N-terminus of a first subunit is in close proximity to a C-terminus of a second subunit. In certain embodiments the homodimer, heterodimer, or oligomer structure is such that a terminus of a first subunit and a terminus of a second subunit are not involved in interaction with a receptor, so that the termini can be joined via a non-genetically encoded peptide element without significantly affecting biological activity. An inventive ligation method is used to join termini of two subunits of a homodimer, heterodimer, or oligomer via a non-genetically encoded peptide element, which optionally comprises a moiety attached to a side chain thereof, thereby producing a dimer (or oligomer) in which at least two subunits are covalently joined. For example, the neurotrophins nerve growth factor (NGF); brain- derived neurotrophic factor (BDNF); neurotrophin 3 (NT3); and neurotrophin 4 (NT4) are dimeric molecules which share approximately 50% sequence identity and exist in dimeric forms. See, e.g., Robinson RC, et al., "Structure of the brain-derived neurotrophic factor/neurotrophin 3 heterodimer.", Biochemistry. 34(13):4139-46, 1995; Robinson RC, et al., "The structures of the neurotrophin 4 homodimer and the brain-derived neurotrophic factor/neurotrophin 4 heterodimer reveal a common Trk-binding site." Protein Sci. 8(12):2589-97, 1999, and references therein. In some embodiments, the dimeric polypeptide is a cytokine, e.g., an interleukin. Other polypeptides of interest are enzymes, e.g., enzymes that are important in metabolism or other physiological processes. As known in the art, deficiencies of enzymes or other proteins can lead to a variety of disease. Such diseases include diseases associated with defects in carbohydrate metabolism, amino acid metabolism, organic acid metabolism, porphyrin metabolism, purine or pyrimidine metabolism, lysosomal storage disorders, blood clotting, etc. Examples include Fabry disease, Gaucher disease, Pompe disease, adenosine deaminase deficiency, asparaginase deficiency, porphyria, hemophilia, and hereditary angioedema. In some embodiments, a polypeptide is a clotting or coagulation factor,(e.g., factor VII, Vila, VIII or IX). In other embodiments a polypeptide is an enzyme that plays a role in carbohydrate metabolism, amino acid metabolism, organic acid metabolism, porphyrin metabolism, purine or pyrimidine metabolism, and/or lysosomal storage, wherein exogenous administration of the enzyme at least in part alleviates the disease.
[00239] In some embodiments, a polypeptide comprises a receptor or receptor fragment (e.g., extracellular domain). In some embodiments a receptor is a TNFα receptor. [00240] In certain embodiments, a polypeptide comprises urate oxidase. [00241] One of skill in the art will be aware of the sequences of polypeptides. Without limitation, sequences of certain polypeptides of interest are found in, e.g., USSN 10/773,530; 11/531,531; USSN 11/707,014; 11/429,276; 1 1/365,008. In some embodiments, a polypeptide of interest is listed in Table B. The invention encompasses application of the inventive techniques to any of the polypeptides described. The invention provides modified versions of any of these polypeptides, wherein a modified version comprises (i) one or more nucleophilic residues such as glycine at the N-terminus (e.g., between 1 and 10 residues) and, optionally, a cleavage recognition sequence, e.g., a protease cleavage recognition sequence that masks the nucleophilic residue(s); (ii) a TRS at or near the C-terminus; (iii) both (i) and (ii). Such modified polypeptides are useful, e.g., as substrates for transamidase-mediated ligation as described herein.
[00242] One of skill in the art will be aware that certain polypeptides, e.g., secreted eukaryotic (e.g., mammalian) polypeptides, often undergo intracellular processing (e.g., cleavage of a secretion signal prior to secretion and/or removal of other portion(s) that are not required for biological activity), to generate a mature form. Such mature, biologically active version, is used in certain embodiments of the invention.
Table B: Protein Sequences
Figure imgf000076_0001
4-sulfatase) (lfsu) YTQPLTPSRSQLLTGRYQIRTGLQHQHWPCQPSCVPLDEKLLPQL
LKEAGYTTHMVGKWHLGMYRKECLPTRRGFDTYFGYLLGSEDY
YSHERCTLIDALNVTRCALDFRDGEEVATGYKNMYSTNIFTKRAI
ALITNHPPEKPLFLYLALQSVHEPLQVPEEYLKPYDFIQDKNRHH
YAGMVSLMDEAVGNVTAALKSSGLWNNTVFIFSTDNGGQTLAG
GNNWPLRGRKWSLWEGGVRGVGFVASPLLKQKGVKNRELIHIS DWLPTLVKLARGHTNGTKPLDGFDVWKTISEGSPSPRIELLHNID PNFVDSSPCSAFNTSVHAAIRHGNWKLLTGYPGCGYWFPPPSQY NVSEIPSSDPPTKTLWLFDIDRDPEERHDLSREYPHIVTKLLSRLQF YHKHSVPVYFPAQDPRCDPKATGVWGPWM (SEQ ID NO: 1 1)
LWPWPQNFQTSDQRYVLYPNNFQFQYDVSSAAQPGCSVLDEAF
QRYRDLLFGTLEKNVL vvsvvTPGCNQLPTLESVEN YTLTΓNDDQ
CLLLSETVWGALRGLETFSQLVWKSAEGTFFINKTEIEDFPRFPHR
GLLLDTSRHYLPLSSILDTLDVMAYNKLNVFHWHLVDDPSFPYES
FTFPELMRKGSYNPVTHIYTAQDVKEVIEYARLRGIRVLAEFDTP
GHTLSWGPGIPGLLTPCYSGSEPSGTFGPVNPSLNNTYEFMSTFFL
EVSSVFPDFYLHLGGDEVDFTCWKSNPEIQDFMRKKGFGEDFKQ
LESFYIQTLLDIVSSYGKGYVVWQEVFDNKVKIQPDTIIQVWREDI
PVNYMKELELVTKAGFRALLSAPWYLNRISYGPDWKDFYVVEPL
AFEGTPEQKALVIGGEACMWGEYVDNTNLVPRLWPRAGAVAER
LWSNKLTSDLTFAYERLSHFRCELLRRGVQAQPLNVGFCEQEFEQ beta-hexosaminidase A (2gjx) (SEQ ID NO: 12)
CHAIN A:
LWPWPQNFQTSDQRYVLYPNNFQFQYDVSSAAQPGCSVLDEAF
QRYRDLLFGTLEKNVLVVSVVTPGCNQLPTLESVENYTLTINDDQ
CLLLSETVWGALRGLETFSQLVWKSAEGTFFINKTEIEDFPRFPHR
GLLLDTSRHYLPLSSILDTLDVMAYNKLNVFHWHLVDDPSFPYES
FTFPELMRKGSYNPVTHIYTAQDVKEVIEYARLRGIRVLAEFDTP
GHTLSWGPGIPGLLTPCYSGSEPSGTFGPVNPSLNNTYEFMSTFFL
EVSSVFPDFYLHLGGDEVDFTCWKSNPEIQDFMRKKGFGEDFKQ
LESFYIQTLLDIVSSYGKGYVVWQEVFDNKVKIQPDTIIQVWREDI
PVNYMKELELVTKAGFRALLSAPWYLNRISYGPDWKDFYVVEPL
AFEGTPEQKALVIGGEACMWGEYVDNTNLVPRLWPRAGAVAER
LWSNKLTSDLTFAYERLSHFRCELLRRGVQAQPLNVGFCEQEFEQ
(SEQ ID NO: 13)
Chain B:
PALWPLPLSVKMTPNLLHLAPENFYISHSPNSTAGPSCTLLEEAFR
RYHGYIFGTQVQQLLVSITLQSECDAFPNISSDESYTLLVKEPVAV
LKANRVWGALRGLETFSQLVYQDSYGTFTINESTIIDSPRFSHRGI
LIDTSRHYLPVKIILKTLDAMAFNKFNVLHWHIVDDQSFPYQSITF
PELSNKGSYSLSHVYTPNDVRMVIEYARLRGIRVLPEFDTPGHTLS
WGKGQKDLLTPCYSDSFGPINPTLNTTYSFLTTFFKEISEVFPDQFI
HLGGDEVEFKCWESNPKIQDFMRQKGFGTDFKKLESFYIQKVLDI
IATINKGSIVWQEVFDDKAKLAPGTIVEVWKDSA YPEELSRVTAS
GFPVILSAPWYLDLISYGQDWRKYYKVEPLDFGGTQKQKQLFIG
GEACLWGEYVDATNLTPRLWPRASAVGERLWSSKDVRDMDDA
YDRLTRHRCRMVERGIAAQPLYAGYCN (SEQ ID NO: 14)
Chain C:
PALWPLPLSVKMTPNLLHLAPENFYISHSPNSTAGPSCTLLEEAFR
RYHGYIFGTQVQQLLVSITLQSECDAFPNISSDESYTLLVKEPVAV
LKANRVWGALRGLETFSQLVYQDSYGTFTINESTIIDSPRFSHRGI
LIDTSRHYLPVKΠLKTLDAMAFNKFNVLHWHIVDDQSFPYQSITF
PELSNKGSYSLSHVYTPNDVRMVIEYARLRGIRVLPEFDTPGHTLS
WGKGQKDLLTPCYSLDSFGPINPTLNTTYSFLTTFFKEISEVFPDQ
FIHLGGDEVEFKCWESNPKIQDFMRQKGFGTDFKKLESFYIQKVL
DIIATINKGSIVWQEVFDDKAKLAPGTIVEVWKDSAYPEELSRVT
ASGFPVILSAPWYLDLISYGQDWRKYYKVEPLDFGGTQKQKQLFI
GGEACLWGEYVDATNLTPRLWPRASAVGERLWSSKDVRDMDD
AYDRLTRHRCRMVERGIAAQPLYAGYCN (SEQ ID NO: 15)
Hexosaminidase A and B (2gjx) Chain D:
Figure imgf000078_0001
Figure imgf000079_0001
Figure imgf000080_0001
[00243] It will be appreciated that considerable structure/function information is available regarding many of the afore-mentioned polypeptides, as well as sequences from different mammalian species, that can be used to design variants of the naturally occurring sequence that retain significant biological activity (e.g., at least 25%, 75%, 90% or more of the activity of the naturally occurring polypeptide). For example, crystal structures or NMR structures of a number of these polypeptides, in some instances in a complex with the corresponding receptor, are available. In addition, it will be understood that, if the naturally occurring N- and C-termini are not located in close proximity to each other in the native structure, a naturally occurring sequence can be extended at the N- and/or C-termini, e.g., with a flexible peptide spacer so that the termini can come into close proximity. [00244] Pharmaceutical Compositions
[00245] The invention provides pharmaceutical compositions comprising any of the polypeptides described herein, i.e., a polypeptide that has been modified using an inventive ligation composition or method. In some embodiments the polypeptide is circular. In some embodiments the polypeptide is PEGylated in a site-specific manne. In some embodiments the polypeptide is circular and PEGylated, e.g., the polypeptide is circularized via a linker peptide that comprises a PEG moiety attached to at least one side chain. [00246] A pharmaceutical composition may comprise a variety of pharmaceutically acceptable carriers. Pharmaceutically acceptable carriers are well known in the art and include, for example, aqueous solutions such as water, 5% dextrose, or physiologically buffered saline or other solvents or vehicles such as glycols, glycerol, oils such as olive oil, or injectable organic esters that are suitable for administration to a human or non-human subject. See, e.g., Remington: The Science and Practice of Pharmacy, 21st edition; Lippincott Williams & Wilkins, 2005. In some embodiments, a pharmaceutically acceptable carrier or composition is sterile. A pharmaceutical composition can comprise, in addition to the active agent, physiologically acceptable compounds that act, for example, as bulking agents, fillers, solubilizers, stabilizers, osmotic agents, uptake enhancers, etc. Physiologically acceptable compounds include, for example, carbohydrates, such as glucose, sucrose, lactose; dextrans; polyols such as mannitol; antioxidants, such as ascorbic acid or glutathione; preservatives; chelating agents; buffers; or other stabilizers or excipients. The choice of a pharmaceutically acceptable carrier(s) and/or physiologically acceptable compound(s) can depend for example, on the nature of the active agent, e.g., solubility, compatibility (meaning that the substances can be present together in the composition without interacting in a manner that would substantially reduce the pharmaceutical efficacy of the pharmaceutical composition under ordinary use situations) and/or route of administration of the composition. The pharmaceutical composition could be in the form of a liquid, gel, lotion, tablet, capsule, ointment, cream, transdermal patch, etc. A pharmaceutical composition can be administered to a subject by various routes including, for example, parenteral administration. Exemplary routes of administration include intravenous administration; respiratory administration (e.g., by inhalation), intramuscular administration, nasal administration, intraperitoneal administration, oral administration, subcutaneous administration and topical administration. For oral administration, the compounds can be formulated with pharmaceutically acceptable carriers as tablets, pills, dragees, capsules, liquids, gels, syrups, slurries, suspensions, etc. In some embodiments a compound may be administered directly to a target tissue. Direct administration could be accomplished, e.g., by injection or by implanting a sustained release implant within the tissue. Of course a sustained release implant could be implanted at any suitable site. In some embodiments, a sustained release implant may be particularly suitable for prophylactic treatment of subjects at risk of developing a recurrent cancer. In some embodiments, a sustained release implant delivers therapeutic levels of the active agent for at least 30 days, e.g., at least 60 days, e.g., up to 3 months, 6 months, or more. One skilled in the art would select an effective dose and administration regimen taking into consideration factors such as the patient's weight and general health, the particular condition being treated, etc. Exemplary doses may be selected using in vitro studies, tested in animal models, and/or in human clinical trials as standard in the art.
[00247] In some embodiments, the pharmaceutical composition is delivered by means of a microparticle or nanoparticle or a liposome or other delivery vehicle or matrix. A number of biocompatible synthetic or naturally occurring polymeric materials are known in the art to be of use for drug delivery purposes. Examples include polylactide-co-glycolide, polycaprolactone, polyanhydride, cellulose derivatives, and copolymers or blends thereof. Liposomes, for example, which consist of phospholipids or other lipids, are nontoxic, physiologically acceptable and metabolizable carriers that are relatively simple to make and administer.
[00248] A compound, e.g., a polypeptide of the invention (e.g., a polypeptide produced at least in part using an inventive ligation method) may be delivered in an effective amount, by which is meant an amount sufficient to achieve a biological response of interest, e.g., reducing one or more symptoms or manifestations of a disease or condition. The exact amount required will vary from subject to subject, depending on factors such as the species, age, weight, sex, and general condition of the subject, the severity of the disease or disorder, the particular compound and its activity, its mode of administration, concurrent therapies, and the like. In some embodiments, a compound, e.g., a polypeptide, is formulated in unit dosage unit form for ease of administration and uniformity of dosage, which term as used herein refers to a physically discrete unit of agent appropriate for the patient to be treated. It will be understood, however, that the total daily dosage will be decided by the attending physician within the scope of sound medical judgment. In some embodiments, e.g., when administering a PEGylated polypeptide, information available regarding a suitable dose of the unPEGylated version, optionally in conjunction with in vitro activity data, can be used as a guideline in selecting an appropriate dose for preclinical testing and/or for clinical use. [00249]
[00250] The pharmaceutical compositions can be used to treat a wide variety of different diseases and disorders. In some embodiments, a pharmaceutical composition is used, e.g., to treat any disease or condition for which the unmodified polypeptide is of use. Thus the invention provides methods of treatment comprising administering an inventive polypeptide to a subject in need thereof. The subject is typically a mammalian subject, e.g., a human. In some embodiments the subject is a non-human animal that serves as a model for a disease or disorder that affects humans. The animal model may be used, e.g., in preclinical studies, e.g., to assess efficacy and/or determine a suitable dose.
[00251] In some embodiments, an inventive polypeptide is administered prophylactically, e.g., to a subject who does not exhibit signs or symptoms of the disease or disorder (but may be at increased risk of developing the disorder or is expected to develop the disease or disorder). In some embodiments an inventive polypeptide is administered to a subject who has developed one or more signs or symptoms of the disease or sorder, e.g., the subject has been diagnose as having the disease or disorder. Optionally, the method comprises diagnosing the subject as having a disease or disorder for which the polypeptide is an appropriate treatment. For example, interferons have a variety of uses, e.g., in the treatment of autoimmune diseases (e.g., multiple sclerosis) and infectious diseases (e.g., viral infections such as those caused by viruses belonging to the Flaviviridae family, e.g., HBV, HCV; bacterial infections, fungal infections, parasites). Exemplary viruses include, but are not limited to, viruses of the Flaviviridae family, such as, for example, Hepatitis C Virus, Yellow Fever Virus, West Nile Virus, Japanese Encephalitis Virus, Dengue Virus, and Bovine Viral Diarrhea Virus; viruses of the Hepadnaviridae family, such as, for example, Hepatitis B Virus; viruses of the Picornaviridae family, such as, for example, Encephalomyocarditis Virus, Human Rhinovirus, and Hepatitis A Virus; viruses of the Retroviridae family, such as, for example, Human Immunodeficiency Virus, Simian Immunodeficiency Virus, Human T- Lymphotropic Virus, and Rous Sarcoma Virus; viruses of the Coronaviridae family, such as, for example, SARS coronavirus; viruses of the Rhabdoviridae family, such as, for example, Rabies Virus and Vesicular Stomatitis Virus, viruses of the Paramyxoviridae family, such as, for example, Respiratory Syncytial Virus and Parainfluenza Virus, viruses of the Papillomaviridae family, such as, for example, Human Papillomavirus, and viruses of the Herpesviridae family, such as, for example, Herpes Simplex Virus.
[00252] Interferon therapy is used (often in combination with chemotherapy and radiation) as a treatment for many cancers, which term is used herein to encompass solid tumors (carcinomas, sarcomas), and leukemias. In some embodiments the tumor is an adenocarcinoma. In some embodiments the tumor is a sarcoma. In some embodiments the tumor affects an organ or organ system selected from breast, lymph node, prostate, kidney, bladder, lung, liver, gastrointestinal tract, colon, testis, stomach, pancreas, thyroid, skin, ovary, uterus, cervix, skin, nerve, bone, and nervous system (e.g., brain). In some embodiments, an interferon is used for treating a hematological malignancy, e.g., a leukemia or a lymphoma, .e.g., hairy cell leukemia, chronic myeloid leukemia, nodular lymphoma, cutaneous T-cell lymphoma. In some embodiments an IFN, e.g., IFN-α2b, is used to treat a melanoma.
[00253] Erythropoiesis stimulating agents such as EPO are of use to treat anemia, which may result from a variety of causes. For example, the anemia may be an anemia of chronic disease, anemia associated with medications (e.g., cancer chemotherapy), radiation, renal disease (e.g., diabetes), infectious diseases, or blood loss. Colony stimulating factors such as G-CSF, GM-CSF, and/or M-CSF may be used to treat leukopenia, e.g., neutropenia and/or lymphopenia, which may result, e.g., from medications (e.g., cancer chemotherapy), radiation, infectious disease, or blood loss.
[00254] Neurotrophic factor polypeptides may be used, e.g., to treat neurodegenerative diseases (e.g., amyotrophic lateral sclerosis, Huntington disease, Alzheimer disease, Parkinson disease), central or peripheral nervous system injury.
[00255] Growth hormone may be used, e.g., to treat children's growth disorders and adult growth hormone deficiency.
[00256] Interleukins are of use to modulate the immune response for a wide variety of purposes, e.g., to stimulate an immune response against an infectious agent or cancer. In some embodiments, an interleukin stimulates immune system cells and/or increases the intensity and/or duration of innate and/or adaptive immune responses. As known in the art, certain interleukins help to limit the intensity and/or duration of innate and/or adaptive immune responses. Administration of such interleukins may be of use in treatment of autoimmune diseases, sepsis, or other conditions in which an aberrant or overactivated immune response can be deleterious.
[00257] Autoimmune disorders include type I diabetes (e.g., juvenile onset diabetes), multiple sclerosis, scleroderma, ankylosing spondylitis, sarcoid, pemphigus vulgaris, myasthenia gravis, systemic lupus erythemotasus, rheumatoid arthritis, juvenile arthritis, Behcet's syndrome, Reiter's disease, Berger's disease, dermatomyositis, Wegener's granulomatosis, autoimmune myocarditis, anti-glomerular basement membrane disease (including Goodpasture's syndrome), dilated cardiomyopathy, thyroiditis (e.g., Hashimoto's thyroiditis, Graves' disease), and Guillane-Barre syndrome.
[00258] Diseases caused by gram- positive or gram-negative bacteria, mycobacteria, fungi such as Candida or Aspergillus, helminths, etc., are of interest in certain embodiments. Exemplary bacteria and fungi include those falling within the following groups Actinomycetales (e.g., Corynebacterium, Mycobacterium, Norcardia), Aspergillosis, Bacillaceae (e.g., Anthrax, Clostridium), Bacteroidaceae, Blastomycosis, Bordetella, Borrelia, Brucellosis, Candidiasis, Campylobacter, Coccidioidomycosis, Cryptococcosis, Dermatocycoses, Enterobacteriaceae (Klebsiella, Salmonella, Serratia, Yersinia), Erysipelothrix, Helicobacter, Legionella, Leptospires Listeria, Mycoplasmatales, Neisseriaceae (e.g., Acinetobacter, Menigococci), Pasteurellacea (e.g., Actinobacillus, Heamophilus, Pasteurella), Pseudomonas, Rickettsiaceae, Chlamydiaceae, Treponema, and Staphylococci.
[00259] In some embodiments a modified, e.g., PEGylated and/or circularized polypeptide exhibits increase efficacy relative to an unmodified form and/or requires a lower dose or less frequent administration (greater dosing interval) to achieve equivalent efficacy and/or exhibits reduced toxicity (reduced side effects, greater tolerability, greater safety) and/or can be administered by a more convenient or preferable route of administration. [00260] Use ofTransamidasesfor Reporting on Cell-Cell Interactions [00261] There is a dearth of tools that report on cell-cell interactions. Currently available split-GFP reporters only detect long-lasting interactions (GFP Reconstitution Across Synaptic Partners (GRASP) defines cell contacts and synapses in living nervous systems. Feinberg EH, Vanhoven MK, Bendesky A, Wang G, Fetter RD, Shen K, Bargmann CI. Neuron. 2008 Feb 7;57(3):353-63.). We have previously shown that type II membrane proteins bearing the requisite sortase cleavage site at their C-terminus and expressed at the living cell surface are susceptible to sortase-mediated labeling when incubated with a soluble recombinant sortase and a suitable probe (Popp et al. Nature Chemical Biology, 2007). In one aspect, the invention provides tools and methods for reporting on (detecting, optionally quantifying) transient cell-cell interactions, where one cell bearing a sortase substrate comes into close proximity to another cell bearing a membrane anchored version of a transamidase, e.g., a SrtA, e.g., either SrtAstrep or SrtAstaph. This would allow for acyl-enzyme formation between the sortase and substrate on opposite cells and when incubated with a functionalized probe (either based on an AA nucleophile or a GG nucleophile for SrtAstreP and SrtAstaph, respectively) will ultimately result in labeling of the cell bearing the sortase substrate. In this way a long-lived, e.g., indelible, mark for a possibly transient cell-cell interaction is imparted on the cell bearing the sortase substrate, given that the interaction is long-lived enough for the transacylation reaction to occur (Fig. 46). In its natural context, sortases are embedded in the bacterial membrane through a transmembrane anchor at the N-terminus. We can thus express sortase at the mammalian cell surface by fusing the catalytic domain of sortase to a mammalian type II membrane protein bearing a signal-anchor sequence for ER insertion. This would result in insertion into the plasma membrane and exposure of the sortase catalytic domain to the extracellular space. In some embodiments, the label comprises a detectable moiety and/or a tag that can be used for isolating the cells. This approach can be applied in vitro (in cell culture) or in vivo. Potential applications include, e.g., examining interactions of immune system cells (e.g., lymphocytes, macrophages) with other immune or non-immune system cells, examining cell-cell interactions in the nervous system or during development, cell migration, etc. This approach can be used to report on cell interactions with noncellular materials as well, by attaching a sortase substrate thereto. [00262] Immunoglobulins and Transgenic Non-human Animals
[00263] The invention provides a transgenic, non-human animal comprising cells whose genome comprises a DNA segment comprising a portion that encodes a polypeptide of interest and a portion that encodes a sortase recognition motif. "Transgenic animal" is used consistently with usage in the art and refers to a non-human animal having a non-endogenous (i.e., heterologous) nucleic acid sequence (transgene) stably integrated into its DNA (i.e., in the genomic sequence of most or all of its cells, in many embodiments including somatic cells and cells of the germ line) or, in some embodiments, present as an extrachromosomal element in at least some of its cells. In some embodiments a transgenic animal is a "knockout" animal, in which a gene has been inactivated, e.g., by at least partially deleting the gene or insertion of a heterologous sequence. It will be understood that the term "transgenic" applies both to the original genetically modified animal and to its descendants. [00264] In certain embodiments the animal is of a type in which genetic modification, e.g., generating transgenic organisms, has been performed and in which methods for performing genetic modification, e.g., generating transgenic organisms, without undue experimentation are known in the art. In some embodiments of the invention, the transgenic non-human animal is a mammal. In some embodiments of the invention, the mammal is ovine, porcine, or bovine. In some embodiments of the invention, the transgenic non-human mammal is a rodent, e.g., a mouse or rat. In some embodiments, the transgenic non-human animal is an avian, e.g., a chicken. The invention further provides offspring of the transgenic animal, wherein the offspring are obtained by crossing the transgenic animal with an animal having a phenotype or genetic modification of interest.
[00265] The invention further provides a cell derived from the transgenic animal. The cell may be of any cell type. In some embodiments the cell is an immune system cell (e.g., a B or T lineage cell, neutrophil or neutrophil precursor), etc. "Derived from" refers to cells that are obtained from an animal and descendants of such cells. The cells may be subjected to genetic modification or other manipulation. In some embodiments the cells are immortalized. [00266] Transgenic animals of the invention have a number of applications. They may be sources of sortase substrates and/or of cells that express sortase substrates comprising a sortase recognition motif. An application of particular interest is the production of antibodies or antibody chains that comprise a sortase recognition motif. Such antibodies may be conveniently labeled or attached to a solid support, e.g., an array, e.g., a glass slide. The animal may be immunized or otherwise contacted with (e.g., exposed to), an antigen of interest (e.g., an allergen, an infectious agent or an extract, portion, or product thereof such as a polypeptide, etc.), may be genetically predisposed to develop an autoimmune disease or immunodeficiency, may be infected with a pathogenic or non-pathogenic infectious agent, etc. Immune system cells, e.g., B-lineage cells, may be obtained from the animal. Hybridomas may be generated from the B-lineage cells. The invention provides collections ('panels') of antibodies and hybridomas. See, e.g., USSN 10/ 324,1 14 (US Pub. No. 20030224490) for information regarding production of monoclonal antibodies, hybridomas, and various other methods that may be employed in the present invention. [00267] In some embodiments, the transgenic non-human animal, e.g., transgenic mouse, is an animal in which at least one endogenous immunoglobulin locus has been at least in part replaced by a human immunoglobulin gene locus. In some embodiments, the transgenic animal is fully reconstituted with human immunoglobulin loci, and, optionally, the endogenous immunoglobulin loci are functionally inactivated, e.g., through targeted deletion, insertion, etc., making it possible to generate fully human antibodies in such animals. Such transgenic mice have been generated by introducing yeast artificial chromosomes (YACs) containing human heavy-chain and K and λ light-chain immunoglobulin genes, into mice whose endogenous heavy-chain and K loci were functionally inactivated by targeted deletion. See, e.g., Jakobovits, A., et al., "From XenoMouse technology to panitumumab, the first fully human antibody product from transgenic mice." Nature Biotechnology 25, 1134 - 1143 (2007), and references therein for further details. It will be appreciated that a variety of other approaches could have been used to generate such mice or mice having similar properties. [00268] The invention also contemplates transgenic plants having genetic modifications as described herein for animals (e.g., such plants may have at least part of an immunoglobulin gene inserted into their genome). It will be understood that appropriate modifications may be made to achieve expression in plants.
Definitions
[00269] Definitions of specific functional groups and chemical terms are described in more detail below. For purposes of this invention, the chemical elements are identified in accordance with the Periodic Table of the Elements, CAS version, Handbook of Chemistry and Physics, 75th Ed., inside cover, and specific functional groups are generally defined as described therein. Additionally, general principles of organic chemistry, as well as specific functional moieties and reactivity, are described in Organic Chemistry, Thomas Sorrell, University Science Books, Sausalito: 1999, the entire contents of which are incorporated herein by reference.
[00270] Certain compounds of the present invention may exist in particular geometric or stereoisomeric forms. The present invention contemplates all such compounds, including cis- and trαtts-isomers, E- and Z-isomers, R- and 5-enantiomers, diastereomers, (D)-isomers, (L)- isomers, (-)- and (+)-isomers, racemic mixtures thereof, and other mixtures thereof, as falling within the scope of the invention. Additional asymmetric carbon atoms may be present in a substituent such as an alkyl group. All such isomers, as well as mixtures thereof, are intended to be included in this invention.
[00271] If, for instance, a particular enantiomer of a compound of the present invention is desired, it may be prepared by asymmetric synthesis, chiral chromatography, or by derivation with a chiral auxiliary, where the resulting diastereomeric mixture is separated and the auxiliary group cleaved to provide the pure desired enantiomers. Alternatively, where the molecule contains a basic functional group, such as amino, or an acidic functional group, such as carboxyl, diastereomeric salts are formed with an appropriate optically-active acid or base, followed by resolution of the diastereomers thus formed by fractional crystallization or chromatographic means well known in the art, and subsequent recovery of the pure enantiomers.
[00272] Isomeric mixtures containing any of a variety of isomer ratios may be utilized in accordance with the present invention. For example, where only two isomers are combined, mixtures containing 50:50, 60:40, 70:30, 80:20, 90:10, 95:5, 96:4, 97:3, 98:2, 99:1, or 100:0 isomer ratios are all contemplated by the present invention. Those of ordinary skill in the art will readily appreciate that analogous ratios are contemplated for more complex isomer mixtures.
[00273] It will be appreciated that the compounds, as described herein, may be substituted with any number of substituents or functional moieties. In general, the term "substituted" whether preceded by the term "optionally" or not, and substituents contained in formulas of this invention, refer to the replacement of hydrogen radicals in a given structure with the radical of a specified substituent. When more than one position in any given structure may be substituted with more than one substituent selected from a specified group, the substituent may be either the same or different at every position. As used herein, the term "substituted" is contemplated to include all permissible substituents of organic compounds. In a broad aspect, the permissible substituents include acyclic and cyclic, branched and unbranched, carbocyclic and heterocyclic, aromatic and non-aromatic substituents of organic compounds. For purposes of this invention, heteroatoms such as nitrogen may have hydrogen substituents and/or any permissible substituents of organic compounds described herein which satisfy the valencies of the heteroatoms. Furthermore, this invention is not intended to be limited in any manner by the permissible substituents of organic compounds. Combinations of substituents and variables envisioned by this invention are preferably those that result in the formation of stable compounds. The term "stable", as used herein, preferably refers to compounds which possess stability sufficient to allow manufacture and which maintain the integrity of the compound for a sufficient period of time to be detected and preferably for a sufficient period of time to be useful for the purposes detailed herein. [00274] The term acyl as used herein refers to a moiety that includes a carbonyl group oro a group having the general formula -C(=O)R, where R is alkyl, alkenyl, alkynyl, aryl, carbocylic, heterocyclic, or aromatic heterocyclic. An example of an acyl group is acetyl. [00275] The term aliphatic, as used herein, includes both saturated and unsaturated, straight chain (i.e., unbranched), branched, acyclic, cyclic, or polycyclic aliphatic hydrocarbons, which are optionally substituted with one or more functional groups. As will be appreciated by one of ordinary skill in the art, "aliphatic" is intended herein to include, but is not limited to, alkyl, alkenyl, alkynyl, cycloalkyl, cycloalkenyl, and cycloalkynyl moieties. Thus, as used herein, the term "alkyl" includes straight, branched and cyclic alkyl groups. An analogous convention applies to other generic terms such as "alkenyl", "alkynyl", and the like. Furthermore, as used herein, the terms "alkyl", "alkenyl", "alkynyl", and the like encompass both substituted and unsubstituted groups. In certain embodiments, as used herein, "lower alkyl" is used to indicate those alkyl groups (cyclic, acyclic, substituted, unsubstituted, branched or unbranched) having 1-6 carbon atoms. [00276] The term alkyl as used herein refers to saturated, straight- or branched-chain hydrocarbon radicals derived from a hydrocarbon moiety containing between one and twenty carbon atoms by removal of a single hydrogen atom. In some embodiments, the alkyl group employed in the invention contains 1-12 carbon atoms. In another embodiment, the alkyl group employed contains 1-8 carbon atoms. In still other embodiments, the alkyl group contains 1-6 carbon atoms. In yet another embodiment, the alkyl group contains 1-4 carbons. Examples of alkyl radicals include, but are not limited to, methyl, ethyl, n-propyl, isopropyl, n-butyl, iso-butyl, sec-butyl, sec-pentyl, iso-pentyl, tert-butyl, n-pentyl, neopentyl, n-hexyl, sec-hexyl, n-heptyl, n-octyl, n-decyl, n-undecyl, dodecyl, and the like, which may bear one or more substituents.
[00277] In general, the terms aryl and heteroaryl, as used herein, refer to stable mono- or polycyclic, heterocyclic, polycyclic, and polyheterocyclic unsaturated moieties having preferably 3-14 carbon atoms, each of which may be substituted or unsubstituted. Substituents include, but are not limited to, any of the previously mentioned substituents, i.e., the substituents recited for aliphatic moieties, or for other moieties as disclosed herein, resulting in the formation of a stable compound. In certain embodiments of the present invention, aryl refers to a mono- or bicyclic carbocyclic ring system having one or two aromatic rings including, but not limited to, phenyl, naphthyl, tetrahydronaphthyl, indanyl, indenyl, and the like. In certain embodiments of the present invention, the term heteroaryl, as used herein, refers to a cyclic aromatic radical having from five to ten ring atoms of which one ring atom is selected from the group consisting of S, O, and N; zero, one, or two ring atoms are additional heteroatoms independently selected from the group consisting of S, O, and N; and the remaining ring atoms are carbon, the radical being joined to the rest of the molecule via any of the ring atoms, such as, for example, pyridyl, pyrazinyl, pyrimidinyl, pyrrolyl, pyrazolyl, imidazolyl, thiazolyl, oxazolyl, isooxazolyl, thiadiazolyl,oxadiazolyl, thiophenyl, furanyl, quinolinyl, isoquinolinyl, and the like.
[00278] It will be appreciated that aryl and heteroaryl groups can be unsubstituted or substituted, wherein substitution includes replacement of one, two, three, or more of the hydrogen atoms thereon independently with any one or more of the following moieties including, but not limited to: aliphatic; heteroaliphatic; aryl; heteroaryl; arylalkyl; heteroarylalkyl; alkoxy; aryloxy; heteroalkoxy; heteroaryloxy; alkylthio; arylthio; heteroalkylthio; heteroarylthio; -F; -Cl; -Br; -I; -OH; -NO2; -CN; -CF3; -CH2CF3; -CHCl2; - CH2OH; -CH2CH2OH; -CH2NH2; -CH2SO2CH3; -C(O)Rx; -CO2(Rx); -CON(RX)2; -OC(O)Rx; -OCO2Rx; -0C0N(Rx)2; -N(RX)2; -S(O)2Rx; -NRx(CO)Rx, wherein each occurrence of Rx independently includes, but is not limited to, aliphatic, heteroaliphatic, aryl, heteroaryl, arylalkyl, or heteroarylalkyl, wherein any of the aliphatic, heteroaliphatic, arylalkyl, or heteroarylalkyl substituents described above and herein may be substituted or unsubstituted, branched or unbranched, cyclic or acyclic, and wherein any of the aryl or heteroaryl substituents described above and herein may be substituted or unsubstituted. Additional examples of generally applicable substituents are illustrated by the specific embodiments shown in the Examples that are described herein.
[00279] The term carboxylic acid as used herein refers to a group of formula -CO2H. [00280] The terms halo and halogen as used herein refer to an atom selected from the group consisting of fluorine, chlorine, bromine, and iodine.
[00281] The term heteroaliphatic, as used herein, refers to aliphatic moieties that contain one or more oxygen, sulfur, nitrogen, phosphorus, or silicon atoms, e.g., in place of carbon atoms. Heteroaliphatic moieties may be branched, unbranched, cyclic or acyclic and include saturated and unsaturated heterocycles such as morpholino, pyrrolidinyl, etc. In certain embodiments, heteroaliphatic moieties are substituted by independent replacement of one or more of the hydrogen atoms thereon with one or more moieties including, but not limited to aliphatic; heteroaliphatic; aryl; heteroaryl; arylalkyl; heteroarylalkyl; alkoxy; aryloxy; heteroalkoxy; heteroaryloxy; alkylthio; arylthio; heteroalkylthio; heteroarylthio; -F; -Cl; -Br; -I; -OH; -NO2; -CN; -CF3; -CH2CF3; -CHCl2; -CH2OH; -CH2CH2OH; -CH2NH2; - CH2SO2CH3; -C(O)Rx; -CO2(Rx); -CON(RX)2; -OC(O)Rx; -OCO2Rx; -OCON(RX)2; -N(RX)2; - S(O)2Rx; -NRx(CO)Rx, wherein each occurrence of Rx independently includes, but is not limited to, aliphatic, heteroaliphatic, aryl, heteroaryl, arylalkyl, or heteroarylalkyl, wherein any of the aliphatic, heteroaliphatic, arylalkyl, or heteroarylalkyl substituents described above and herein may be substituted or unsubstituted, branched or unbranched, cyclic or acyclic, and wherein any of the aryl or heteroaryl substituents described above and herein may be substituted or unsubstituted.
[00282] The term heterocyclic, as used herein, refers to an aromatic or non-aromatic, partially unsaturated or fully saturated, 3- to 10-membered ring system, which includes single rings of 3 to 8 atoms in size and bi- and tri-cyclic ring systems which may include aromatic five- or six-membered aryl or aromatic heterocyclic groups fused to a non-aromatic ring. These heterocyclic rings include those having from one to three heteroatoms independently selected from the group consisting of oxygen, sulfur, and nitrogen, in which the nitrogen and sulfur heteroatoms may optionally be oxidized and the nitrogen heteroatom may optionally be quaternized. In certain embodiments, the term heterocyclic refers to a non-aromatic 5-, 6-, or 7-membered ring or a polycyclic group wherein at least one ring atom is a heteroatom selected from the group consisting of O, S, and N (wherein the nitrogen and sulfur heteroatoms may be optionally oxidized), including, but not limited to, a bi- or tri-cyclic group, comprising fused six-membered rings having between one and three heteroatoms independently selected from the group consisting of the oxygen, sulfur, and nitrogen, wherein (i) each 5-membered ring has 0 to 2 double bonds, each 6-membered ring has 0 to 2 double bonds, and each 7-membered ring has 0 to 3 double bonds, (ii) the nitrogen and sulfur heteroatoms may be optionally oxidized, (iii) the nitrogen heteroatom may optionally be quaternized, and (iv) any of the above heterocyclic rings may be fused to an aryl or heteroaryl ring.
[00283] The term aromatic heterocyclic, as used herein, refers to a cyclic aromatic radical having from five to ten ring atoms of which one ring atom is selected from the group consisting of sulfur, oxygen, and nitrogen; zero, one, or two ring atoms are additional heteroatoms independently selected from the group consisting of sulfur, oxygen, and nitrogen; and the remaining ring atoms are carbon, the radical being joined to the rest of the molecule via any of the ring atoms, such as, for example, pyridyl, pyrazinyl, pyrimidinyl, pyrrolyl, pyrazolyl, imidazolyl, thiazolyl, oxazolyl, isooxazolyl, thiadiazolyl, oxadiazolyl, thiophenyl, furanyl, quinolinyl, isoquinolinyl, and the like. Aromatic heterocyclic groups can be unsubstituted or substituted with substituents selected from the group consisting of branched and unbranched alkyl, alkenyl, alkynyl, haloalkyl, alkoxy, thioalkoxy, amino, alkylamino, dialkylamino, trialkylamino, acylamino, cyano, hydroxy, halo, mercapto, nitro, carboxyaldehyde, carboxy, alkoxycarbonyl, and carboxamide.
[00284] Specific heterocyclic and aromatic heterocyclic groups that may be included in the compounds of the invention include: 3 -methyl -4-(3-methylphenyl)piperazine, 3 methylpiperidine, 4-(bis-(4-fluorophenyl)methyl)piperazine, 4-(diphenylmethyl)piperazine, 4-(ethoxycarbonyl)piperazine, 4-(ethoxycarbonylmethyl)piperazine, 4- (phenylmethyl)piperazine, 4-(l-phenylethyl)piperazine, 4-(I5I- dimethylethoxycarbonyl)piperazine, 4-(2-(bis-(2-propenyl) amino)ethyl)piperazine, 4-(2- (diethylamino)ethyl)piperazine, 4-(2-chlorophenyl)piperazine, 4-(2-cyanophenyl)piperazine, 4-(2-ethoxyphenyl)piperazine, 4-(2-ethylphenyl)piperazine, 4-(2-fluorophenyl)piperazine, 4- (2-hydroxyethyl)piperazine, 4-(2-methoxyethyl)piperazine, 4-(2-methoxyphenyl)piperazine, 4-(2-methylphenyl)piperazine, 4-(2-methylthiophenyl) piperazine, 4-(2- nitrophenyl)piperazine, 4-(2-nitrophenyl)piperazine, 4-(2-phenylethyl)piperazine, 4-(2- pyridyl)piperazine, 4-(2-pyrimidinyl)piperazine, 4-(2,3-dimethylphenyl)piperazine, 4-(2,4- difluorophenyl) piperazine, 4-(2,4-dimethoxyphenyl)piperazine, 4-(2,4- dimethylphenyl)piperazine, 4-(2,5-dimethylphenyl)piperazine, 4-(2,6- dimethylphenyl)piperazine, 4-(3-chlorophenyl)piperazine, 4-(3-methylphenyl)piperazine, 4- (3 -trifluoromethylphenyl)piperazine, 4-(3 ,4-dichlorophenyl)piperazine, 4-3 ,4- dimethoxyphenyl)piperazine, 4-(3 ,4-dimethylphenyl)piperazine, 4-(3 ,4- methylenedioxyphenyl)piperazine, 4-(3,4,5-trimethoxyphenyl)piperazine, 4-(3,5- dichlorophenyl)piperazine, 4-(3,5-dimethoxyphenyl)piperazine, 4-(4- (phenylmethoxy)phenyl)piperazine, 4-(4-(3 , 1 -dimethylethyl)phenylmethyl)piperazine, 4-(4- chloro-3 -trifluoromethylphenyl)piperazine, 4-(4-chlorophenyl)-3 -methylpiperazine, 4-(4- chlorophenyl)piperazine, 4-(4-chlorophenyl)piperazine, 4-(4-chlorophenylmethyl)piperazine, 4-(4-fluorophenyl)piperazine, 4-(4-methoxyphenyl)piperazine, 4-(4- methylphenyl)piperazine, 4-(4-nitrophenyl)piperazine, 4-(4- trifluoromethylphenyl)piperazine, 4-cyclohexylpiperazine, 4-ethylpiperazine, 4-hydroxy-4- (4-chlorophenyl)methylpiperidine, 4-hydroxy-4-phenylpiperidine, 4-hydroxypyrrolidine, 4- methylpiperazine, 4-phenylpiperazine, 4-piperidinylpiperazine, 4-(2- furanyl)carbonyl)piperazine, 4-((l ,3-dioxolan-5-yl)methyl)piperazine, 6-fluoro-l ,2,3,4- tetrahydro-2-methylquinoline, 1 ,4-diazacylcloheptane, 2,3-dihydroindolyl, 3,3- dimethylpiperidine, 4,4-ethylenedioxypiperidine, 1,2,3,4-tetrahydroisoquinoline, 1,2,3,4- tetrahydroquinoline, azacyclooctane, decahydroquinoline, piperazine, piperidine, pyrrolidine, thiomorpholine, and triazole. [00285] The terms substituted, whether preceded by the term "optionally" or not, and substituent, as used herein, refer to the ability, as appreciated by one skilled in this art, to change one functional group for another functional group provided that the valency of all atoms is maintained. When more than one position in any given structure may be substituted with more than one substituent selected from a specified group, the substituent may be either the same or different at every position. The substituents may also be further substituted {e.g., an aryl group substituent may have another substituent off it, such as another aryl group, which is further substituted with fluorine at one or more positions).
[00286] The term arylalkyl refers to alkyl groups in which a hydrogen atom has been replaced with an aryl group. Such groups include, without limitation, benzyl, cinnamyl, and dihyrocinnamyl.
[00287] The term heteroatom means one or more of oxygen, sulfur, nitrogen, phosphorus, or silicon (including, any oxidized form of nitrogen, sulfur, phosphorus, or silicon; the quaternized form of any basic nitrogen or; a substitutable nitrogen of a heterocyclic ring, for example N (as in 3,4-dihydro-2H-pyrrolyl), NH (as in pyrrolidinyl) or NR+ (as in N- substituted pyrrolidinyl)).
[00288] The term unsaturated, as used herein, means that a moiety has one or more units ofunsaturation.
[00289] As used herein, the term partially unsaturated refers to a ring moiety that includes at least one double or triple bond. The term "partially unsaturated" is intended to encompass rings having multiple sites of unsaturation, but is not intended to include aryl or heteroaryl moieties, as herein defined.
[00290] Additionally, unless otherwise stated, structures depicted herein are also meant to include compounds that differ only in the presence of one or more isotopically enriched positions of the compound. For example, compounds having the present structures including the replacement of hydrogen by deuterium or tritium, or the replacement of a carbon by a
13C- or l4C-enriched carbon are within the scope of this invention. Such compounds are useful, for example, as analytical tools, as probes in biological assays, or as therapeutic agents in accordance with the present invention.
[00291] One of ordinary skill in the art will appreciate that the synthetic methods, as described herein, utilize a variety of protecting groups. By the term "protecting group," as used herein, it is meant that a particular functional moiety, e.g., O, S, or N, is masked or blocked, permitting, if desired, a reaction to be carried out selectively at another reactive site in a multifunctional compound. Suitable protecting groups are well known in the art and include those described in detail in Protecting Groups in Organic Synthesis, T. W. Greene and P. G. M. Wuts, 3rd edition, John Wiley & Sons, 1999, the entirety of which is incorporated herein by reference. In certain embodiments, a protecting group reacts selectively in good yield to give a protected substrate that is stable to the projected reactions; the protecting group is preferably selectively removable by readily available, preferably nontoxic reagents that do not attack the other functional groups; the protecting group forms a separable derivative (more preferably without the generation of new stereogenic centers); and the protecting group will preferably have a minimum of additional functionality to avoid further sites of reaction. As detailed herein, oxygen, sulfur, nitrogen, and carbon protecting groups may be utilized. By way of non-limiting example, hydroxyl protecting groups include methyl, methoxylmethyl (MOM), methylthiomethyl (MTM), t-butylthiomethyl, (phenyldimethylsilyl)methoxymethyl (SMOM), benzyloxymethyl (BOM), p- methoxybenzyloxymethyl (PMBM), (4-methoxyphenoxy)methyl (p-AOM), guaiacolmethyl (GUM), t-butoxymethyl, 4-pentenyloxymethyl (POM), siloxymethyl, 2- methoxyethoxymethyl (MEM), 2,2,2-trichloroethoxymethyl, bis(2-chloroethoxy)methyl, 2- (trimethylsilyl)ethoxymethyl (SEMOR), tetrahydropyranyl (THP), 3- bromotetrahydropyranyl, tetrahydrothiopyranyl, 1-methoxycyclohexyl, 4- methoxytetrahydropyranyl (MTHP), 4-methoxytetrahydrothiopyranyl, 4- methoxytetrahydrothiopyranyl S,S-dioxide, 1 -[(2-chloro-4-methyl)phenyl]-4- methoxypiperidin-4-yl (CTMP), 1 ,4-dioxan-2-yl, tetrahydrofuranyl, tetrahydrothiofuranyl, 2,3,3a,4,5,6,7,7a-octahydro-7,8,8-trimethyl-4,7-methanobenzofuran-2-yl, 1 -ethoxyethyl, 1- (2-chloroethoxy)ethyl, 1 -methyl- 1-methoxyethyl, 1 -methyl- 1 -benzyloxyethyl, 1 -methyl- 1- benzyloxy-2-fluoroethyl, 2,2,2-trichloroethyl, 2-trimethylsilylethyl, 2-(phenylselenyl)ethyl, t- butyl, allylj/j-chlorophenyl^-methoxyphenyl, 2,4-dinitrophenyl, benzyl, />-methoxy benzyl, 3 ,4-dimethoxybenzyl, o-nitrobenzy 1, /7-nitrobenzyl, p-halobenzyl, 2,6-dichlorobenzyl, p- cyanobenzyl,p-phenylbenzyl, 2-picolyl, 4-picolyl, 3-methyl-2-picolyl N-oxido, diphenylmethyl, p,p '-dinitrobenzhydryl, 5-dibenzosuberyl, triphenylmethyl, α- naphthyldiphenylmethyl, /7-methoxyphenyldiphenylmethyl, di(p- methoxyphenyl)phenylmethyl, tri(p-methoxyphenyl)methyl, 4-(4'- bromophenacyloxyphenyl)diphenylmethyl, 4,4',4"-tris(4,5- dichlorophthalimidophenyl)methyl, 4,4',4"-tris(levulinoyloxyphenyl)methyl, 4,4',4"- tris(benzoyloxyphenyl)methyl, 3-(imidazol-l -yl)bis(4',4"-dimethoxyphenyl)methyl, 1,1- bis(4-methoxyphenyl)-l '-pyrenylmethyl, 9-anthryl, 9-(9-phenyl)xanthenyl, 9-(9-phenyl-10- oxo)anthryl, l,3-benzodithiolan-2-yl, benzisothiazolyl S,S-dioxido, trimethylsilyl (TMS), triethylsilyl (TES), triisopropylsilyl (TIPS), dimethylisopropylsilyl (IPDMS), diethylisopropylsilyl (DEIPS), dimethylthexylsilyl, t-butyldimethylsilyl (TBDMS), t- butyldiphenylsilyl (TBDPS), tribenzylsilyl, tri-p-xylylsilyl, triphenylsilyl, diphenylmethylsilyl (DPMS), /-butylmethoxyphenylsilyl (TBMPS), formate, benzoylformate, acetate, chloroacetate, dichloroacetate, trichloroacetate, trifluoroacetate, methoxyacetate, triphenylmethoxyacetate, phenoxyacetate^-chlorophenoxyacetate, 3-phenylpropionate, 4- oxopentanoate (levulinate), 4,4-(ethylenedithio)pentanoate (levulinoyldithioacetal), pivaloate, adamantoate, crotonate, 4-methoxycrotonate, benzoate, /?-phenylbenzoate, 2,4,6- trimethylbenzoate (mesitoate), alkyl methyl carbonate, 9-fluorenylmethyl carbonate (Fmoc), alkyl ethyl carbonate, alkyl 2,2,2-trichloroethyl carbonate (Troc), 2-(trimethylsilyl)ethyl carbonate (TMSEC), 2-(phenylsulfonyl) ethyl carbonate (Psec), 2-(triphenylphosphonio) ethyl carbonate (Peoc), alkyl isobutyl carbonate, alkyl vinyl carbonate alkyl allyl carbonate, alkyl /?-nitrophenyl carbonate, alkyl benzyl carbonate, alkyl /?-methoxybenzyl carbonate, alkyl 3,4-dimethoxybenzyl carbonate, alkyl o-nitrobenzyl carbonate, alkyl p-nitrobenzyl carbonate, alkyl 5-benzyl thiocarbonate, 4-ethoxy-l-napththyl carbonate, methyl dithiocarbonate, 2-iodobenzoate, 4-azidobutyrate, 4-nitro-4-methylpentanoate, o- (dibromomethyl)benzoate, 2-formylbenzenesulfonate, 2-(methylthiomethoxy)ethyl, 4- (methylthiomethoxy)butyrate, 2-(methylthiomethoxymethyl)benzoate, 2,6-dichloro-4- methylphenoxyacetate, 2,6-dichloro-4-(l ,1 ,3,3-tetramethylbutyl)phenoxyacetate, 2,4-bis(l , 1 - dimethylpropyl)phenoxyacetate, chlorodiphenylacetate, isobutyrate, monosuccinoate, (E)-2- methyl-2-butenoate, o-(methoxycarbonyl)benzoate, α-naphthoate, nitrate, alkyl N,N,N',N'- tetramethylphosphorodiamidate, alkyl iV-phenylcarbamate, borate, dimethylphosphinothioyl, alkyl 2,4-dinitrophenylsulfenate, sulfate, methanesulfonate (mesylate), benzylsulfonate, and tosylate (Ts). For protecting 1,2- or 1,3-diols, the protecting groups include methylene acetal, ethylidene acetal, 1-t-butyl ethylidene ketal, 1-phenylethylidene ketal, (4- methoxyphenyl)ethylidene acetal, 2,2,2-trichloroethylidene acetal, acetonide, cyclopentylidene ketal, cyclohexylidene ketal, cycloheptylidene ketal, benzylidene acetal, p- methoxybenzylidene acetal, 2,4-dimethoxybenzylidene ketal, 3,4-dimethoxybenzylidene acetal, 2-nitrobenzylidene acetal, methoxymethylene acetal, ethoxymethylene acetal, dimethoxymethylene ortho ester, 1-methoxy ethylidene ortho ester, 1 -ethoxyethylidine ortho ester, 1 ,2-dimethoxyethylidene ortho ester, α-methoxybenzylidene ortho ester, \-(N,N- dimethylamino)ethylidene derivative, α-(N,N'-dimethylamino)benzylidene derivative, 2- oxacyclopentylidene ortho ester, di-/-butylsilylene group (DTBS), 1, 3-(l, 1,3,3- tetraisopropyldisiloxanylidene) derivative (TIPDS), tetra-t-butoxydisiloxane-l,3-diylidene derivative (TBDS), cyclic carbonates, cyclic boronates, ethyl boronate, and phenyl boronate. Amino-protecting groups include methyl carbamate, ethyl carbamante, 9-fluorenylmethyl carbamate (Fmoc), 9-(2-sulfo)fluorenylmethyl carbamate, 9-(2,7-dibromo)fluoroenylmethyl carbamate, 2,7-di-t-butyl-[9-( 10, 10-dioxo- 10,10,10,10-tetrahydrothioxanthyl)]methyl carbamate (DBD-Tmoc), 4-methoxyphenacyl carbamate (Phenoc), 2,2,2-trichloroethyl carbamate (Troc), 2-trimethylsilylethyl carbamate (Teoc), 2-phenylethyl carbamate (hZ), 1- (l-adamantyl)-l-methylethyl carbamate (Adpoc), l,l-dimethyl-2-haloethyl carbamate, 1,1- dimethyl-2,2-dibromoethyl carbamate (DB-/-BOC), l,l-dimethyl-2,2,2-trichloroethyl carbamate (TCBOC), 1 -methyl- l-(4-biphenylyl)ethyl carbamate (Bpoc), l-(3,5-di-t- butylphenyl)-l-methylethyl carbamate (t-Bumeoc), 2-(2'- and 4'-pyridyl)ethyl carbamate (Pyoc), 2-(N,N-dicyclohexylcarboxamido)ethyl carbamate, t-butyl carbamate (BOC), 1- adamantyl carbamate (Adoc), vinyl carbamate (Voc), allyl carbamate (Alloc), 1 - isopropylallyl carbamate (Ipaoc), cinnamyl carbamate (Coc), 4-nitrocinnamyl carbamate (Noc), 8-quinolyl carbamate, iV-hydroxypiperidinyl carbamate, alkyldithio carbamate, benzyl carbamate (Cbz), /7-methoxybenzyl carbamate (Moz), /?-nitobenzyl carbamate, p- bromobenzyl carbamate, /?-chlorobenzyl carbamate, 2,4-dichlorobenzyl carbamate, 4- methylsulfinylbenzyl carbamate (Msz), 9-anthrylmethyl carbamate, diphenylmethyl carbamate, 2-methylthioethyl carbamate, 2-methylsulfonylethyl carbamate, 2-(p- toluenesulfonyl)ethyl carbamate, [2-(l,3-dithianyl)]methyl carbamate (Dmoc), 4- methylthiophenyl carbamate (Mtpc), 2,4-dimethylthiophenyl carbamate (Bmpc), 2- phosphonioethyl carbamate (Peoc), 2-triphenylphosphonioisopropyl carbamate (Ppoc), 1,1- dimethyl-2-cyanoethyl carbamate, /w-chloro-p-acyloxybenzyl carbamate, p- (dihydroxyboryl)benzyl carbamate, 5-benzisoxazolylmethyl carbamate, 2-(trifluoromethyl)- 6-chromonylmethyl carbamate (Tcroc), /n-nitrophenyl carbamate, 3,5-dimethoxybenzyl carbamate, o-nitrobenzyl carbamate, 3,4-dimethoxy-6-nitrobenzyl carbamate, phenyl(o- nitrophenyl)methyl carbamate, phenothiazinyl-(10)-carbonyl derivative, N'-p- toluenesulfonylaminocarbonyl derivative, N'-phenylaminothiocarbonyl derivative, t-amyl carbamate, S-benzyl thiocarbamate, /7-cyanobenzyl carbamate, cyclobutyl carbamate, cyclohexyl carbamate, cyclopentyl carbamate, cyclopropylmethyl carbamate, p- decyloxybenzyl carbamate, 2,2-dimethoxycarbonylvinyl carbamate, o-(N,N- dimethylcarboxamido)benzyl carbamate, 1 , 1 -dimethyl-3-(ΛζiV-dimethylcarboxamido)propyl carbamate, 1,1-dimethylpropynyl carbamate, di(2-pyridyl)methyl carbamate, 2-furanylmethyl carbamate, 2-iodoethyl carbamate, isoborynl carbamate, isobutyl carbamate, isonicotinyl carbamate, p-(p '-methoxyphenylazo)benzyl carbamate, 1-methylcyclobutyl carbamate, 1- methylcyclohexyl carbamate, 1 -methyl- 1-cyclopropylmethyl carbamate, l-methyl-l-(3,5- dimethoxyphenyl)ethyl carbamate, 1 -methyl- l-(/?-phenylazophenyl)ethyl carbamate, 1- methyl-1-phenylethyl carbamate, 1 -methyl- l-(4-pyridyl)ethyl carbamate, phenyl carbamate, /?-(phenylazo)benzyl carbamate, 2,4,6-tri-t-butylphenyl carbamate, 4- (trimethylammonium)benzyl carbamate, 2,4,6-trimethylbenzyl carbamate, formamide, acetamide, chloroacetamide, trichloroacetamide, trifluoroacetamide, phenylacetamide, 3- phenylpropanamide, picolinamide, 3-pyridylcarboxamide, N-benzoylphenylalanyl derivative, benzamide, /?-phenylbenzamide, o-nitophenylacetamide, o-nitrophenoxyacetamide, acetoacetamide, (iV'-dithiobenzyloxycarbonylamino)acetamide, 3-(p- hydroxypheny l)propanamide, 3 -(o-nitrophenyl)propanamide, 2-methyl-2-(o- nitrophenoxy)propanamide, 2-methyl-2-(o-phenylazophenoxy)propanamide, 4- chlorobutanamide, 3-methyl-3-nitrobutanamide, o-nitrocinnamide, N-acetylmethionine derivative, o-nitrobenzamide, o-(benzoyloxymethyl)benzamide, 4,5-diphenyl-3-oxazolin-2- one, N-phthalimide, iV-dithiasuccinimide (Dts), iV-2,3-diphenylmaleimide, N-2,5- dimethylpyrrole, N-l,l,4,4-tetramethyldisilylazacyclopentane adduct (STABASE), 5- substituted l,3-dimethyl-l,3,5-triazacyclohexan-2-one, 5-substituted l,3-dibenzyl-l,3,5- triazacyclohexan-2-one, 1 -substituted 3,5-dinitro-4-pyridone, iV-methylamine, N-allylamine, N-[2-(trimethylsilyl)ethoxy]methylamine (SEM), N-3-acetoxypropylamine, N-(l-isopropyl-4- nitro-2-oxo-3-pyroolin-3-yl)amine, quaternary ammonium salts, N-benzylamine, N-di(4- methoxyphenyl)methylamine, N-5-dibenzosuberylamine, iV-triphenylmethylamine (Tr), N- [(4-methoxyphenyl)diphenylmethyl]amine (MMTr), N-9-phenylfluorenylamine (PhF), N-2,7- dichloro-9-fluorenylmethyleneamine, N-ferrocenylmethylamino (Fcm), N-2-picolylamino N'- oxide, N-l,l-dimethylthiomethyleneamine, N-benzylideneamine, N-p- methoxybenzylideneamine, N-diphenylmethyleneamine, N- [(2- pyridyl)mesityl]methyleneamine, N-(N',N'-dimethylaminomethylene)amine, NN'- isopropylidenediamine, N-j9-nitrobenzylideneamine, N-salicylideneamine, N-5- chlorosalicylideneamine, N-(5-chloro-2-hydroxyphenyl)phenylmethyleneamine, N- cyclohexylideneamine, N-(5,5-dimethyl-3-oxo-l-cyclohexenyl)amine, N-borane derivative, N-diphenylborinic acid derivative, N-[phenyl(pentacarbonylchromium- or tungsten)carbonyl]amine, N-copper chelate, N-zinc chelate, N-nitroamine, N-nitrosoamine, amine N-oxide, diphenylphosphinamide (Dpp), dimethylthiophosphinamide (Mpt), diphenylthiophosphinamide (Ppt), dialkyl phosphoramidates, dibenzyl phosphoramidate, diphenyl phosphoramidate, benzenesulfenamide, o-nitrobenzenesulfenamide (Νps), 2,4- dinitrobenzenesulfenamide, pentachlorobenzenesulfenamide, 2-nitro-4- methoxybenzenesulfenamide, triphenylmethylsulfenamide, 3 -nitropyridinesulfenamide (Npys), /?-toluenesulfonamide (Ts), benzenesulfonamide, 2,3,6,-trimethyl-4- methoxybenzenesulfonamide (Mtr), 2,4,6-trimethoxybenzenesulfonamide (Mtb), 2,6- dimethyl-4-methoxybenzenesulfonamide (Pme), 2,3,5,6-tetramethyl-4- methoxybenzenesulfonamide (Mte), 4-methoxybenzenesulfonamide (Mbs), 2,4,6- trimethylbenzenesulfonamide (Mts), 2,6-dimethoxy-4-methylbenzenesulfonamide (iMds), 2,2,5,7,8-pentamethylchroman-6-sulfonamide (Pmc), methanesulfonamide (Ms), β- trimethylsilylethanesulfonamide (SES), 9-anthracenesulfonamide, 4-(4',8'- dimethoxynaphthylmethyl)benzenesulfonamide (DNMBS), benzylsulfonamide, trifluoromethylsulfonamide, and phenacylsulfonamide. Exemplary protecting groups are detailed herein, however, it will be appreciated that the present invention is not intended to be limited to these protecting groups; rather, a variety of additional equivalent protecting groups can be readily identified using the above criteria and utilized in the method of the present invention. Additionally, a variety of protecting groups are described by Greene and Wuts (supra).
[00292] "Polypeptide", "peptide", or "protein": According to the present invention, a "polypeptide", "peptide", or "protein" comprises a string of at least three amino acids linked together by peptide bonds. The terms "polypeptide", "peptide", and "protein", may be used interchangeably. Peptide may refer to an individual peptide or a collection of peptides. Inventive peptides preferably contain only natural amino acids, although non natural amino acids (i.e., compounds that do not occur in nature but that can be incorporated into a polypeptide chain) and/or amino acid analogs as are known in the art may alternatively be employed. Also, one or more of the amino acids in a peptide may be modified, for example, by the addition of a chemical entity such as a carbohydrate group, a phosphate group, a farnesyl group, an isofarnesyl group, a fatty acid group, a linker for conjugation, functionalization, or other modification, etc. In one embodiment, the modifications of the peptide lead to a more stable peptide (e.g., greater half-life in vivo). These modifications may include cyclization of the peptide, the incorporation of D-amino acids, etc. None of the modifications should substantially interfere with the desired biological activity of the peptide. [00293] "Carbohydrate": The term "carbohydrate" refers to a sugar or polymer of sugars. The terms "saccharide", "polysaccharide", "carbohydrate", and "oligosaccharide", may be used interchangeably. Most carbohydrates are aldehydes or ketones with many hydroxyl groups, usually one on each carbon atom of the molecule. Carbohydrates generally have the molecular formula CnH2nOn. A carbohydrate may be a monosaccharide, a disaccharide, trisaccharide, oligosaccharide, or polysaccharide. The most basic carbohydrate is a monosaccharide, such as glucose, sucrose, galactose, mannose, ribose, arabinose, xylose, and fructose. Disaccharides are two joined monosaccharides. Exemplary disaccharides include sucrose, maltose, cellobiose, and lactose. Typically, an oligosaccharide includes between three and six monosaccharide units (e.g., raffinose, stachyose), and polysaccharides include six or more monosaccharide units. Exemplary polysaccharides include starch, glycogen, and cellulose. Carbohydrates may contain modified saccharide units such as 2'-deoxyribose wherein a hydroxyl group is removed, 2'-fluororibose wherein a hydroxyl group is replace with a fluorine, or N-acetylglucosamine, a nitrogen-containing form of glucose, (e.g., T- fluororibose, deoxyribose, and hexose). Carbohydrates may exist in many different forms, for example, conformers, cyclic forms, acyclic forms, stereoisomers, tautomers, anomers, and isomers.
[00294] "Polysaccharide", "carbohydrate" or "oligosaccharide": The terms "polysaccharide", "carbohydrate", or "oligosaccharide" refer to a polymer of sugars. The terms "polysaccharide", "carbohydrate", and "oligosaccharide", may be used interchangeably. Typically, a polysaccharide comprises at least two sugars. The polymer may include natural sugars (e.g., glucose, fructose, galactose, mannose, arabinose, ribose, and xylose) and/or modified sugars (e.g., 2'-fiuororibose, 2 '-deoxyribose, and hexose). "Sugar alcohols" include glycerol (glycertil, propane- 1, 2, 3-triol), erythritol, threitol, ribitol (adonitol), arabinitol, xylitol, allitol, altritol, galactitol, glucitol (sorbitol), mannitol, or iditol. [00295] As used herein, the phrase "natural amino acid side-chain" refers to the side-chain group of any of the 20 amino acids naturally occuring in proteins. Such natural amino acids include the nonpolar, or hydrophobic amino acids, glycine, alanine, valine, leucine, isoleucine, methionine, phenylalanine, tryptophan, and proline. Cysteine is sometimes classified as nonpolar or hydrophobic and other times as polar. Natural amino acids also include polar, or hydrophilic amino acids, such as tyrosine, serine, threonine, aspartic acid (also known as aspartate, when charged), glutamic acid (also known as glutamate, when charged), asparagine, and glutamine. Certain polar, or hydrophilic, amino acids have charged side-chains. Such charged amino acids include lysine, arginine, and histidine. One of ordinary skill in the art would recognize that protection of a polar or hydrophilic amino acid side-chain can render that amino acid nonpolar. For example, a suitably protected tyrosine hydroxyl group can render that tyroine nonpolar and hydrophobic by virtue of protecting the hydroxyl group. [00296] As used herein, the phrase "unnatural amino acid side-chain" refers to the side- chain group of amino acids not included in the list of 20 amino acids naturally occuring in proteins, as described above. Such amino acids include the D-isomer of any of the 20 naturally occuring amino acids. Unnatural amino acids also include homoserine, ornithine, norleucine, and thyroxine. Other unnatural amino acids side-chains are well known to one of ordinary skill in the art and include unnatural aliphatic side chains. Other unnatural amino acids include modified amino acids, including those that are N-alkylated, cyclized, phosphorylated, acetylated, amidated, azidylated, labelled, and the like. In some embodiments, an unnatural amino acid is a D-isomer. In some embodiments, an unnatural amino acid is a L-isomer.
[00297] "Small molecule": As used herein, the term "small molecule" is used to refer to molecules, whether naturally-occurring or artificially created (e.g. , via chemical synthesis) that have a relatively low molecular weight. Typically, a small molecule is an organic compound (i.e., it contains carbon). The small molecule may contain multiple carbon-carbon bonds, stereocenters, and other functional groups (e.g., amines, hydroxyl, carbonyls, heterocyclic rings, etc.). In some embodiments, small molecules are monomeric and have a molecular weight of less than about 1500 g/mol. In certain embodiments, the molecular weight of the small molecule is less than about 1000 g/mol or less than about 500 g/mol. Preferred small molecules are biologically active in that they produce a biological effect in animals, preferably mammals, more preferably humans. Small molecules include, but are not limited to, radionuclides and imaging agents. In certain embodiments, the small molecule is a drug. Preferably, though not necessarily, the drug is one that has already been deemed safe and effective for use in humans or animals by the appropriate governmental agency or regulatory body. For example, drugs approved for human use are listed by the FDA under 21 CF. R. §§ 330.5, 331 through 361, and 440 through 460, incorporated herein by reference; drugs for veterinary use are listed by the FDA under 21 CF. R. §§ 500 through 589, incorporated herein by reference. All listed drugs are considered acceptable for use in accordance with the present invention.
[00298] "Polynucleotide" is used herein consistently with usage in the art and is used interchangeably with "nucleic acid" or "oligonucleotide", with "oligonucleotide" typically being used to refer to short (e.g, 50 residues or less) polynucleotides. The polynucleotide may include natural nucleosides found in RNA and/or DNA, nucleoside analogs (e.g., 2- aminoadenosine, 2-thiothymidine, inosine, pyrrolo-pyrimidine, 3-methyl adenosine, C5- propynylcytidine, C5-propynyluridine, C5-bromouridine, C5-fluorouridine, C5-iodouridine, C5-methylcytidine, 7-deazaadenosine, 7-deazaguanosine, 8-oxoadenosine, 8-oxoguanosine, O(6)-methylguanine, and 2-thiocytidine), and/or nucleosides comprising chemically or biologically modified bases, (e.g., methylated bases) and/or modified sugars (e.g., T- fluororibose, ribose, 2'-deoxyribose, arabinose, and hexose). Polynucleotides containing modified backbones (relative to those found in RNA or DNA) or non-naturally occurring internucleoside linkages can also be used in the present invention. A polynucleotide may be single-stranded or double-stranded. It should be noted that where the present invention discloses a single-stranded polynucleotide, the perfect complement of the polynucleotide, and a double-stranded polynucleotide comprising both the single-stranded polynucleotide and its perfect complement, are also disclosed. Polynucleotide sequences are listed in a 5' to 3' direction unless otherwise indicated.
[00299] As used herein, the term "tag" refers to a moiety appended to another entity that imparts a characteristic or property otherwise not present in the un-tagged entity. In some embodiments, the tag is an affinity tag, an epitope tag, a fluorescent tag, etc. Examples of fluorescent tags include GFP and other fluorescent proteins mentioned above. Affinity tags can facilitate the purification or solubilization of fusion proteins. Examples of affinity tags include maltose binding protein (MBP), glutathione-S-transferase (GST), thioredoxin, polyhistidine (also known as hexa histidine, 6xHis, and by the trademarked name HIS- TAG®), etc. Examples of epitope tags, which facilitate recognition by antibodies, include c- myc, FLAG (FLAG octapeptides), HA (hemagglutinin), etc.
[00300] As used herein, the term "catalyst" refers to a substance the presence of which increases the rate and/or extent of a chemical reaction, while not being consumed or undergoing a permanent chemical change itself.
[00301] The terms "label" and "labeling moiety" entity refer to agents that can be visualized, for example following binding to another entity. The detectable agent or moiety may be selected such that it generates a signal which can be measured and whose intensity is related to (e.g., proportional to) the amount of bound entity. A wide variety of systems for labeling and/or detecting proteins and peptides are known in the art. Labeled proteins and peptides can be prepared by incorporation of, or conjugation to, a label that is detectable by spectroscopic, photochemical, biochemical, immunochemical, electrical, optical, chemical or other means. A label or labeling moiety may be directly detectable (i.e., it does not require any further reaction or manipulation to be detectable, e.g. , a fluorophore is directly detectable) or it may be indirectly detectable (i.e., it is made detectable through reaction or binding with another entity that is detectable, e.g., a hapten is detectable by immunostaining after reaction with an appropriate antibody comprising a reporter such as a fluorophore). Suitable detectable agents include, but are not limited to, radionuclides, fluorophores, chemi luminescent agents, microparticles, enzymes, colorimetric labels, magnetic labels, haptens, Molecular Beacons, aptamer beacons, and the like.
[00302] As used herein and in the claims, the singular forms "a", "an", and "the" include the plural reference unless the context clearly indicates otherwise. Thus, for example, a reference to "a compound" includes a plurality of such compounds.
[00303] It will be understood that wherein the claims or description use the word "is" (e.g., as in "A1 is xxx" or "recognition motif is xxx"), the invention encompasses embodiments where A1 (or recognition motif) "comprises xxx" and embodiments in which A1 (or recognition motif) "consists of xxx".
[00304] As used herein, the term "isolated" often refers to having a specific activity of at least tenfold greater than the sortase-transamidase activity present in a crude extract, lysate, or other state from which proteins have not been removed and also in substantial isolation from proteins found in association with sortase-transamidase in the cell. An "isolated" or "purified" polypeptide or protein is substantially free of cellular material or other contaminating proteins from the cell or tissue source from which the protein is derived, or substantially free from chemical precursors or other chemicals when chemically synthesized. In one embodiment, the term "substantially free" refers to preparing a target polypeptide having less than about 30%, 20%, 10% and sometimes 5% (by dry weight), of non-target polypeptide (also referred to herein as a" contaminating protein"), or of chemical precursors or non-target chemicals. When the target polypeptide or a biologically active portion thereof is recombinantly produced, it also often is substantially free of culture medium, where culture medium represents less than about 20%, sometimes less than about 10%, and often less than about 5% of the volume of the polypeptide preparation. In certain embodiments, isolated or purified target polypeptide preparations are 0. 01 milligrams or more. In certain embodiments, isolated or purified target polypeptide preparations are 0.1 milligrams or more. In certain embodiments, isolated or purified target polypeptide preparations are 1.0 milligrams or more and 10 milligrams or more in dry weight.
[00305] Those skilled in the art will recognize, or be able to ascertain using no more than routine experimentation, many equivalents to the specific embodiments of the invention described herein. The scope of the present invention is not intended to be limited to the description or examples herein. Claims or descriptions that include "or" between one or more members of a group are considered satisfied if one, more than one, or all of the group members are present in, employed in, or otherwise relevant to a given product or process unless indicated to the contrary or otherwise evident from the context. The invention includes embodiments in which exactly one member of the group is present in, employed in, or otherwise relevant to a given product or process. The invention also includes embodiments in which more than one, or all of the group members are present in, employed in, or otherwise relevant to a given product or process.
[00306] The invention encompasses all variations, combinations, and permutations in which one or more limitations, elements, clauses, descriptive terms, etc., from one or more of the claims or from the description (including specific details in the experimental section) is introduced into another claim dependent on the same base claim (or, as relevant, any claim) unless otherwise indicated or unless it would be evident to one of ordinary skill in the art that a contradiction or inconsistency would arise. Where lists or sets of elements are disclosed herein it is to be understood that each subgroup of the elements and each individual element are also disclosed. In general, where the invention, or aspects of the invention, is/are referred to as comprising particular elements, features, etc., certain embodiments of the invention or aspects of the invention consist, or consist essentially of, such elements, features, etc. It should also be understood that any embodiment of the invention can be explicitly excluded from the claims. For example, in some embodiments, a polypepide is not GFP or a derivative thereof.
[00307] Where the description or claims recite a method, the invention encompasses inventive compositions used in performing the method, and products produced using the method. Where the description or claims recite a composition, the invention encompasses methods of using the composition and methods of making the composition. [00308] Where ranges are mentioned herein, the invention includes embodiments in which the endpoints are included, embodiments in which both endpoints are excluded, and embodiments in which one endpoint is included and the other is excluded. It should be assumed that both endpoints are included unless indicated otherwise. Furthermore, it is to be understood that unless otherwise indicated or otherwise evident from the context and understanding of one of ordinary skill in the art, values that are expressed as ranges can assume any specific value or subrange within the stated ranges in different embodiments of the invention, to the tenth of the unit of the lower limit of the range, unless the context clearly dictates otherwise. It is also understood that where a list of numerical values is stated herein (whether or not prefaced by "at least"), the invention includes embodiments that relate analogously to any intervening value or range defined by any two values in the list, and that the lowest value may be taken as a minimum and the greatest value may be taken as a maximum. Furthermore, where a list of numbers, e.g., percentages, is prefaced by "at least", the term applies to each number in the list. For any embodiment of the invention in which a numerical value is prefaced by "about" or "approximately", the invention includes an embodiment in which the exact value is recited. For any embodiment of the invention in which a numerical value is not prefaced by "about" or "approximately", the invention includes an embodiment in which the value is prefaced by "about" or "approximately". "Approximately" or "about" generally includes numbers that fall within a range of 1% or in some embodiments 5% or in some embodiments 10% of a number in either direction (greater than or less than the number) unless otherwise stated or otherwise evident from the context (e.g., where such number would impermissibly exceed 100% of a possible value).
Exemplification
Example 1: Lipid Modification using Sortase [00309] Overview
[00310] Protein-lipid conjugates and methods for their construction are valuable tools for studying the role of post-translational lipid modification in controlling protein function and localization. Lipid attachment also provides a means for manipulating the properties of peptides and proteins that normally do not possess these types of modifications. Highlighting the utility of synthetic lipoproteins, Bertozzi and co-workers recently reported the synthesis of GFP-containing GPI-anchor mimetics as a means for probing the role of individual sugar residues in this complex membrane anchor (1, 2). Numerous reports have also shown that the addition of lipids and fatty acids can endow proteins and peptides with cell-penetrating capabilities (3-7), modulate immunogenicity (8, 9), and provide anchors for incorporation into liposomes (10, 11).
[00311] With respect to full-size protein substrates, the attachment of lipids in site-specific fashion remains a significant bioconjugation challenge. Only a relatively limited set of chemical and chemoenzymatic strategies are available for this purpose. These include the use of enzymes such as myristoyl (12, 13) and prenyl (14-16) transferases, wherein the user is limited to the natural substrates of these enzymes or closely related analogoues. In the case of chemical labeling, a common strategy is cysteine derivatization through alkylation (17, 18) or disulfide formation (19, 20), an approach that requires site-directed mutagenesis to ensure that protein substrates contain only a single reactive cysteine residue. Among the available strategies for lipid attachment, expressed protein ligation (EPL) (1, 2, 21-25) has proven to be the most versatile. For example, this method has been used to prepare GFP bearing a range of lipid modifications (1, 2, 24) and to generate lipidated Ras (25) and Rab (22) proteins. However, EPL mandates the expression of protein substrates as fusions with large intein domains, a necessity that can reduce protein expression yields and may require careful selection of the intein domain to prevent premature intein cleavage and a corresponding drop in the yield of ligation products (26-29).
[00312] With the goal of complementing existing strategies for lipoprotein synthesis, we have developed a general method for the site-specific installation of lipids and fatty acids using sortase-catalyzed transpeptidation (Scheme 1). As mentioned above, sortase A from Staphylococcus aureus recognizes a five amino acid sequence (LPXTG) near the C-terminus of its natural protein targets (39-41). The active site cysteine of sortase cleaves between the threonine and glycine residues of the recognition site to produce a thioester intermediate which is then attacked by the amino terminus of an oligoglycine nucleophile, resulting in the formation of a new amide bond. The method is extremely versatile, stemming from the remarkable tolerance of the enzyme for substituents C-terminal to the oligoglycine unit. Synthetic nucleophiles, containing 1-5 glycine residues, have been decorated with a range of substituents including fluorophores (33, 34) photoaffϊnity probes (34), peptide nucleic acids (36), polymers (35), solid supports (32, 35, 42) or other polypeptides (33, 38) allowing the site-specific ligation of these moieties to peptide and protein substrates. Here we describe the synthesis of lipid-modified oligoglycine nucleophiles compatible with the sortase-mediated transpeptidation reaction and demonstrate their high-yielding ligation to a protein substrate. Lipoproteins prepared using this procedure were shown to strongly associate with mammalian cells in a lipid tail-dependent fashion and were found to localize to the plasma membrane and endosomes. Materials and Instrumentation
[00313] Chemicals. Unless otherwise noted, all chemicals were obtained from commercial sources and used without further purification. Rink amide resin (100-200 mesh, 0.7 mmol/g) was obtained from Advanced Chemtech. Fmoc-Gly-OH, Fmoc-Lys(Mtt)-OH, and Fmoc-Trp(Boc)-OH were obtained from EMD Biosciences/Novabiochem. Triglycine peptide was purchased from Sigma (Gl 377). Water used in biological procedures or as a reaction solvent was purified using a MiIIiQ purification system (Millipore). DriSolv
® anhydrous CH2CI2 and DriSolv anhydrous MeCN were purchased from EMD Chemicals. Redistilled, anhydrous N,N'-diisopropylethylamine (DIPEA) was obtained from Sigma- Aldrich.
1 13
[00314] NMR. H and C spectra were measured with a Bruker AV ANCE-400 (400 MHz) spectrometer at the MIT Department of Chemistry Instrumentation Facility. H NMR chemical shifts are reported as δ in units of parts per million (ppm) relative to chloroform-d (δ 7.24, singlet). Multiplicities are reported as follows: s (singlet), d (doublet), or m (multiplet). Coupling constants are reported as a J value in Hertz (Hz). The number of protons (n) for a given resonance is indicated as nH, and is based on spectral integration
13 values. C NMR chemical shifts are reported as δ in units of parts per million (ppm) relative to chloroform-d (δ 77.23, triplet).
[00315] Mass Spectrometry. Electrospray Ionization (ESI) mass spectra were obtained at the MIT Department of Chemistry Instrumentation Facility. Matrix assisted laser desorption- ionization time-of-flight mass spectrometry (MALDI-TOF MS) was performed on a MALDI
TM micro MX system (Micromass MS Technologies, USA). Samples were co-crystallized using a sinapinic acid solution (10 mg/mL in 70:30 MeCN:H2θ with 0.1% TFA). LC-ESI-
MS analysis was performed using a Micromass LCT mass spectrometer (Micromass® MS
Technologies, USA) and a Paradigm MG4 HPLC system equipped with a HTC PAL autosampler (Michrom BioResources, USA) and a Waters Symmetry 5 μm C8 column (2.1 x
50 mm, MeCN:H2θ (0.1% formic acid) gradient mobile phase, 150 μL/min).
[00316] HPLC/FPLC. HPLC purifications were achieved using an Agilent 1100 Series
HPLC system equipped with a Waters Delta Pak 5 μm, 100 A C4 column (3.9 x 150 mm,
MeCN:H2θ gradient mobile phase containing 0.1% trifluoroacetic acid, 1 mL/min), a Waters
Delta Pak 15 μm, 100 A Cl 8 column (7.8 x 300 mm, 2-propanol:H2θ gradient mobile phase,
2 mL/min), or a Waters Cosmosil 5PE column (8 x 250 mm, 2propanol:H2θ gradient mobile phase, 1 mL/min) as indicated below. Size exclusion chromatography was performed on a
Pharmacia AKTA Purifier system equipped with a HiLoad 16/60 Superdex 75 column
(Amersham).
[00317] UV- Vis Spectrocopy. UV-Vis spectroscopy was performed on a Nanodrop ND-
1000 spectrophotometer (Thermo Scientific, USA).
[00318] Flow Cytometry. Flow cytometry was performed on a LSR-II system (BD
Biosciences).
[00319] Spinning Disc Confocal Microscopy. Fluorescence microscopy was performed on a Nikon spinning disc confocal microscope with MetaMorph 7 software. Multidimensional acquisition was used to collect images in the 488, 647, and phase contrast channels from the same focal plane.
Design, Synthesis, and Characterization of Lipid-Modified Triglycine Nucleophiles [00320] Most nucleophiles compatible with sortase-mediated transpeptidation that have been identified to date have the simple structural requirement of a stretch of glycine residues with a free amino terminus. While successful transpeptidation has been reported with nucleophiles containing anywhere from one to five glycines, maximum reaction rates are obtained when two or more glycines are present.(32, 38). It should be noted that primary alkylamines have been shown to participate in the transpeptidation reaction, (31 , 35) though in general these appeared to be less efficient than oligoglycine derivatives. With these considerations in mind, we synthesized a panel of lipid-modified triglycine nucleophiles using solid-phase synthesis (Scheme 2).
[00321] Resin-bound precursor 1 was prepared on Rink amide resin using standard Fmoc chemistry. An orthogonally protected lysine residue was incorporated to allow selective liberation and subsequent acylation of the ε-amino group. Following removal of the 4- methyltrityl (Mtt) group, the lysine side chain was acylated with a range of hydrophobic carboxylic acids, including naturally occurring post-translational modifications such as myristic (1-C14) and palmitic (1-C16) acid, as well as modifications not found in eukaryotic cells (1-ad). The couplings of Cl 8, C20, C22, and C24 acids were performed at 50°C to maintain the solubility of all the reaction components. Following Fmoc deprotection and resin cleavage, the identity of nucleophiles derived from 1 was confirmed by LC-ESI-MS (Figure 11, and see below). All peptides were obtained with good purity and did not require extensive purification prior to transpeptidation.
[00322] In addition to purely aliphatic substituents, we also prepared a cholesterol- modified triglycine nucleophile (2-chol, Scheme 2). Peptide 2 was prepared on Rink amide resin and then cleaved from the solid support, leaving the N-terminal Fmoc group intact. A tryptophan residue was included in this peptide as a UV-active chromophore to aid in purification by HPLC. Peptide 2 was then reacted with cholesterol NHS-carbonate 3, followed by the addition of piperidine to remove the Fmoc group. The crude material was then purified by RP-HPLC to yield 2-chol in 22% yield.
[00323] Further details regarding synthesis and characterization of the lipidated triglycine nucleophiles are as follows:
[00324] Resin-Bound Intermediate 1. A glass solid-phase reaction vessel containing a fritted glass filter and a Teflon stopcock was loaded with Rink amide resin (1.0 g, 0.70 mmol). The resin was first washed/swollen extensively with N-methyl-2-pyrrolidone (NMP) by gentle agitation with a wrist action shaker. The Fmoc protecting group was then removed by treatment with -30 mL of 80:20 NMP/piperidine for 20 min at RT. The resin was washed with -30 mL of NMP (3x, 3-5 min per wash). Amino acid building blocks were then coupled as follows: Fmoc-protected amino acid (1.75 mmol, 2.5 equivalents relative to initial resin loading), benzotriazole- 1 -yl-oxy-tris-pyrrolidino-phosphonium hexafluorophosphate (PyBOP) (911 mg, 1.75 mmol), N-hydroxybenzotriazole (HOBt) (236 mg, 1.75 mmol), and N,N'-diisopropylethylamine (DIPEA) (914 μL, 5.25 mmol) were dissolved in NMP to a final volume of 8.75 mL (200 mM final concentration of amino acid building block). This solution was mixed until all reagents had dissolved, and then added to the deprotected Rink amide resin. Couplings were incubated for 16-48 h at RT. The resin was then washed with ~30 mL of NMP (3x, 3-5 min per wash). The extent of coupling was assessed by Kaiser test. In the event that the coupling was incomplete, the above procedure was repeated. Fmoc removal was then achieved by exposing the resin to ~30 mL of 80:20 NMP/piperidine for 20 min at RT, followed by additional washing with -30 mL of NMP (3x, 3-5 min per wash). Cycles of amino acid coupling and Fmoc deprotection were then repeated to complete the synthesis of 1. The resin was then washed with ~ 30 mL of CH2CI2 (5x, 3-5 min per wash) and dried.
[00325] 1-ad, 1-C12, and 1-C14 (General Procedure). A 3.0 mL fritted polypropylene syringe equipped with a capped hypodermic needle was loaded with dry resin 1 (50 mg). The resin was washed with 2.5 mL of CH2CI2 (3x, 3-5 min per wash). Next, the 4methyltrityl (Mtt) protecting group was removed by treatment with 2.5 mL of 94:5:1 CH2CI2/TIPS/TFA at RT (5x, 5 min each) followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash). The resin was then treated with a solution of the appropriate carboxylic acid (Ri-COOH, 0.12 mmol), PyBOP (65 mg, 0.12 mmol), HOBt (16 mg, 0.12 mmol), and DIPEA (65 μL, 0.38 mmol) in 1.0 mL of NMP. The reaction was incubated at RT for 21 h followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash). Fmoc removal was achieved by treatment with 2.5 mL of 80:20 NMP/piperidine for 20 min at RT followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash) and 2.5 mL of CH2CI2 (3x, 3-5 min per wash). The peptide was cleaved from the resin with 2.5 mL of 95:3:2 TFA/TIPS/H2O (4x, -30 min each) and the combined cleavage solutions were concentrated in vacuo. 1-ad was then precipitated from ether and dried under vacuum. Crude 1-C12 and crude 1-C14 were washed with hexanes (1 mL, 2x) and then dried under vacuum. The identity of all peptides was confirmed by LC- ESI-MS analysis (Figure 11). Peptides were used without further purification and the yield was not determined.
[00326] 1-C16. A 3.0 mL fritted polypropylene syringe equipped with a capped hypodermic needle was loaded with dry resin 1 (200 mg). The resin was washed with 2.5 mL of CH2CI2 (3x, 3-5 min per wash). Next, the 4-methyltrityl (Mtt) protecting group was removed by treatment with 2.5 mL of 94:5:1 CH2CI2/TIPS/TFA at RT (5x, 5 min each). The resin was then washed with 2.5 mL of NMP (3x, 3-5 min per wash). The resin was then treated with a solution of palmitic acid (103 mg, 0.40 mmol), PyBOP (208 mg, 0.40 mmol), HOBt (54 mg, 0.4 mmol), and DIPEA (207 μL, 1.2 mmol) in 1.6 mL of NMP. The reaction was incubated at RT overnight. The resin was then washed with 2.5 mL of NMP (3x, 3-5 min per wash). Fmoc removal was achieved by treatment with 2.5 mL of 80:20 NMP/piperidine for 20 min at RT followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash) and 2.5 mL of CH2CI2 (3x, 3-5 min per wash). The peptide was cleaved from the resin with 2.5 mL of 95:3:2 TFA/TIPS/H2O (4x, -30 min each) and the combined cleavage solutions were dried under vacuum. The identity of 1-C16 was confirmed by LC-ESI-MS analysis (Figure 11). This material was used without further purification and yield was not determined.
[00327] 1-C18, 1-C20, 1-C22, and 1-C24 (General Procedure). A 3.0 mL fritted polypropylene syringe equipped with a capped hypodermic needle was loaded with dry resin 1 (50 mg). The resin was washed with 2.5 mL of CH2CI2 (3x, 3-5 min per wash). Next, the 4- methyltrityl (Mtt) protecting group was removed by treatment with 2.5 mL of 94:5:1 CH2CI2/TIPS/TFA at RT (5x, 5 min each) followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash). The resin was then carefully transferred to a 1.5 mL microcentrifuge tube. The resin was treated with a solution of the appropriate carboxylic acid (R2-COOH, 0.12 mmol), PyBOP (65 mg, 0.12 mmol), HOBt (16 mg, 0.12 mmol), and DIPEA (65 μL, 0.38 mmol) in 1.0 mL of NMP. The reaction was incubated at 50 C for 5 h. The reaction was then centrifuged, and 0.5 mL of the supernatant was discarded. An additional 0.5 mL of NMP was then added followed again by centrifugation and removal of 0.5 mL of the supernatant. This process was repeated two additional times. The resin slurry was carefully transferred to a 3.0 mL fritted polypropylene syringe equipped with a capped hypodermic needle and washed with 2.5 mL of NMP (3x, 3-5 min per wash). Fmoc removal was achieved by treatment with 2.5 mL of 80:20 NMP/piperidine for 20 min at RT followed by washing with 2.5 mL of NMP (3x, 3-5 min per wash) and 2.5 mL of CH2CI2 (3x, 3-5 min per wash). The peptide was cleaved from the resin with 2.5 mL of 95:3:2 TFA/TIPS/H2O (3x, -30 min each) and the combined cleavage solutions were concentrated in vacuo. 1-C18, 1-C20, 1- C22, and 1-C24 were precipitated from cold ether and dried under vacuum. The identity of all peptides was confirmed by LC-ESIMS analysis (Figure 11). Peptides were used without further purification and yield was not determined.
[00328] Cholesterol NHS-carbonate (3). An oven dried round bottom flask equipped with an argon inlet was charged with cholesterol (500 mg, 1.29 mmol) and N5N'- disuccinimidyl carbonate (DSC) (665 mg, 2.59 mmol) in 15 mL of 1 : 1 : 1 CtaCb/MeCN/DIPEA (all anhydrous). The reaction was stirred at RT for 24 h. The reaction mixture was then partitioned between brine and CH2CI2. The aqueous layer was extracted two additional times with CH2CI2. The combined organic layers were then dried over MgSCU, filtered, and concentrated. The remaining residue was then purified by flash chromatography (95:5 CH2Cb/EtOAc) to yield 3 as a white solid (274 mg, 40%). Η NMR (400 MHz, CDCb): δ, 5.39 (d, IH, J = 4.4 Hz), 4.57 (m, IH), 2.81 (s, 4H), 2.46 (m, 2H), 2.05-0.80 (m, 26H), 1.00 (s, 3H), 0.89 (d, 3H, J = 6.4 Hz), 0.84 (d, 3H, J = 6.4 Hz), 0.83 (d,
3H, J = 6.8 Hz), 0.65 (s, 3H) . C NMR (100 MHz, CDCb): δ, 169.0, 151.0, 138.7, 123.9, 82.4, 56.8, 56.3, 50.1, 42.5, 39.9, 39.7, 37.8, 36.9, 36.7, 36.4, 36.0, 32.1, 32.0, 28.4, 28.2, 27.6, 25.7, 24.5, 24.0, 23.0, 22.8, 21.2, 19.4, 18.9, 12.0. HRMS (ESI+) calculated for C32H49NOsNa ([M+Naf) 550.3503, found 550.3383.
[00329] Fmoc-Gly-Gly-Gly-Trp-Lys-CONH2 (2). Intermediate 2 was synthesized on Rink amide resin following the procedure described above for the preparation of 1. Peptide 2 was cleaved from the resin with 95:3:2 TFA/TIPS/H2O (3x, ~30 min each). The combined cleavage solutions were concentrated and 2 was precipitated from ether and dried. The identity of 2 was confirmed by LC-ESI-MS. Yield not determined. LRMS (ESI+) calculated for C38H45N8θ7 ([M+H]+) 725.3, found 725.4.
[00330] 2-chol. To a 1.5 mL microcentrifuge tube was added 3 (10.5 mg dissolved in 50 μL of CHCb, 19.9 μmol), 2 (7.2 mg dissolved in 50 μL of NMP, 9.9 μmol), and anhydrous DIPEA (5.00 μL, 28.7 μmol). After overnight incubation at RT, piperidine (25 μL) was added and the reaction was incubated for an additional 2 h at RT. The reaction was then diluted with 0.5 mL of 2-propanol and fractionated by RP-HPLC [semi-preparative Cl 8 column, 2-propanol:H2θ gradient mobile phase, 2 mL/min, 50% 2-propanol → 90% 2- propanol (0-20 min)]. Fractions containing 2-chol were pooled, concentrated, and further purified by RP-HPLC [semi-preparative PE column, 2-propanol:H2θ gradient mobile phase, 1 mL/min, 50% 2-propanol → 90% 2-propanol (0-20 min)] to yield 2-chol (2 mg, 22%). The identity of 2-chol was confirmed by LC-ESI-MS (Figure 1 1). Sortase-Mediated Ligation of Triglycine Nucleophiles to a Protein Substrate [00331] With a series of lipidated nucleophiles in hand, we proceeded to explore their coupling to a protein substrate using sortase. A model protein consisting of eGFP equipped with a C-terminal LPETG sequence followed by a His6 affinity handle was expressed and purified from Escherichia coli. Recombinant sortase A containing an N-terminal His6 tag was produced as described (40). At the outset of these studies, we decided to incorporate a procedure for removing the sortase enzyme after the reaction, similar to a purification scheme proposed by Parthasarathy et al. (35) but with important improvements. The configuration of His6 tags on both sortase and the eGFP substrate provided a simple means for doing so, where Ni-NTA resin was added following transpeptidation to retrieve the sortase enzyme as well as any unreacted eGFP-LPETG-His6. In this scenario, the transpeptidation product should no longer be His6-tagged because residues C-terminal to the LPETG motif are lost in the course of transpeptidation, and thus, this material will not be bound by Ni-NTA. [00332] eGFP-LPETG-Hisδ cloning and expression were performed as follows: The gene encoding eGFP was PCR amplified from the commercially available pEGFP-Nl plasmid (Clontech) using forward primer 5'-CGCGCGCC ATGGTG AGC AAGGGCG AGG AG-31 and reverse primer 5'
CGCGCGGATCCCGACCAGTTTCAGGAAGCTTGTACAGCTCGTCCATGCCG-S'. The PCR product was digested with Ncol and BamHI and ligated into pET28a+ (Novagen). This plasmid was then transformed into E. coli BL-21. In a typical experiment, cells were grown in two 2 L batches of sterile LB containing kanamycin (30 μg/mL) to an optical density of -0.6-0.9 at 600 nm. Cells were induced with IPTG (1 mM) for 3 h at 37°C. Cells were harvested by centrifugation and the pellet was stored overnight at -20°C. The pellet was thawed and resuspended in 60 mL of 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole containing a protease inhibitor cocktail (complete mini tablet, EDTA- free, Roche) and treated with 240 μL of DNAse I (10 mg/mL in PBS), 480 μL of lysozyme (50 mg/mL in PBS), and 60 μL of MgCh (1 M in PBS). The lysis reaction was incubated for 1 h at 4°C. The cells were then sonicated and centrifuged to remove insoluble material. The pellet was then treated with an additional 20 mL of 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole, briefly sonicated, and centrifuged. The combined supernatants were applied to a Ni-NTA column consisting of 7.5 mL of commercial Ni-NTA slurry (Qiagen) equilibrated with 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole. The column was washed with three 45 mL portion of 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole. eGFP-LPETG-Hisό was eluted with -10 mL of 10 mM Tris pH 8.0, 100 mM phosphate, 300 mM NaCl, and 300 mM imidazole. This material was concentrated and further purified by size exclusion chromatography on a HiLoad 16/60 Superdex 75 column (Amersham), eluting with 20 mM Tris pH 8.0, 150 mM NaCl at a flow rate of 1 mL/min. Fractions containing eGFP-LPETG- His6 were pooled, concentrated, and stored at -80°C.
[00333] Immediately prior to sortase-catalyzed transpeptidation, the eGFP-LPETG-Hisό stock was thawed and again purified by affinity chromatography over commercial Ni-NTA resin. After binding eGFP-LPETG-His6 to the resin, the column was washed with three portions of 20 mM Tris pH 8.0, 150 mM NaCl, and 20 mM imidazole. The protein was eluted with 20 mM Tris pH 8.0, 150 mM NaCl, and 300 mM imidazole. This material was
TM TM buffer exchanged into 20 mM Tris pH 8.0, 150 mM NaCl using a NAP 5 Sephadex column (GE Healthcare) and concentrated. The concentration was estimated by UV-Vis
-1 spectroscopy using the absorbance of eGFP at 488 nm (extinction coefficient 55,900 M cm
') (43).
[00334] As shown in Figure Ia, exposing eGFP-LPETG-His6 to 150 μM sortase and 2 mM triglycine (GGG) in Tris buffer (pH 7.5) containing 10 mM CaCl2 resulted in the appearance of a lower molecular weight species just below the band corresponding to sortase (lane 2). Excess sortase was used to drive the reaction to completion in a reasonable time frame. Near- quantitative conversion of the input eGFP-LPETG-His6 protein (lane 1) was observed over the course of a 3 h incubation at 37 0C. A slurry of Ni-NTA resin containing 1 M NaCl and 40 mM imidazole was then added, and the mixture was incubated for 2 h. In further detail, removal of Hisό-tagged proteins following transpeptidation was achieved with Ni-NTA resin treated in the following way: 500 μL of commercial Ni-NTA resin (Qiagen) was treated with 1 mL of 40 mM Tris pH 8.0, 1 M NaCl, and 40 mM imidazole. The mixture was then centrifuged and the supernatant was removed. This process was repeated two additional times. The resin was then suspended to a final volume of 500 μL with 40 mM Tris pH 8.0, 1 M NaCl, and 40 mM imidazole. This slurry was used to treat samples depicted in Figure Ia lanes 3-11 and Figure 2b lanes 3-13. For control experiments (Figure 2b, lanes 1-2), the above procedure was performed on a separate batch of commercial Ni-NTA resin using 40 mM Tris pH 8.0, 1 M NaCl, and 600 mM imidazole to block binding of Hisβ-tagged proteins. [00335] The addition of imidazole and NaCl at the specified concentrations contributed importantly to preventing nonspecific binding of the transpeptidation products. After filtration to remove Ni-NTA, the filtrate was analyzed by SDS-PAGE. A single polypeptide was observed with no evidence for the presence of residual sortase (lane 3). Characterization by ESI-MS confirmed that the protein observed in lane 3 was indeed the desired ligation product (Figure 12, see below). Also, judging from the intensity of the band in lane 3 as compared to the corresponding eGFP bands in lanes 1 and 2, we were confident that very little material was lost over the course of the two-step transpeptidation/sortase-depletion protocol.
[00336] Initial attempts to ligate one of the lipid-modified nucleophiles (1-C22) using the conditions described above yielded only small amounts of the putative transpeptidation product as well as an unidentified higher molecular weight species (Figure Ia, lane 4). The high molecular weight byproduct may correspond to the acyl enyme intermediate formed between sortase A and the eGFP substrate. This assignment implies that the affinity of the His6 tag on the N-terminus of sortase is impaired in the acyl enzyme intermediate because this species is not removed during depletion of His6-tagged proteins using Ni-NTA resin. Further characterization of this byproduct was not performed.
[00337] Not surprisingly, the solubility of 1-C22 in aqueous buffer was extremely poor, and we suspected that this may limit the amount of nucleophile available in solution. To improve solubility, we examined the effect of adding mild detergents to the reaction mixture. As shown in Figure 1_a (lane 8), the addition of 1% (w/v) «-dodecyl maltoside afforded a significant increase in the level of transpeptidation product relative to that of the other detergents tested. This material was further characterized by ESI-MS and found to consist exclusively of the desired lipid-modified eGFP derivative (Figure 1b). [00338] Using 1% (w/v) rø-dodecyl maltoside to maintain nucleophile solubility, we were able to successfully ligate the entire panel of lipid-modified triglycine nucleophiles to our eGFP model substrate (Figure 2). In all cases, a single major protein that migrated at a lower apparent molecular weight than unreacted eGFP-LPETG-His6 (lane 1) was observed in the filtrate of reactions using lipidated nucleophiles (lanes 5-13). As expected, these samples also showed complete removal of the sortase enzyme. Coupling reactions using only triglycine (lanes 2 and 3) served as positive controls for transpeptidation. A reaction lacking an oligoglycine nucleophile resulted in slow hydrolysis of the acyl enzyme intermediate and the formation of a higher molecular weight byproduct (43) (lane 4). As an additional negative control, we confirmed that the formation of transpeptidation products was dependent on the presence of sortase (Figure 13). The identity of all eGFP conjugates was ultimately established by mass spectrometry (Table 1 and Figure 12).
Table 1. Mass Spectral Characterization and Yield (%) of eGFP-Lipid Conjugates
Figure imgf000115_0001
[00339] The eGFP chromophore provided a convenient method for quantifying the yield of the eGFP conjugates. By comparing the absorbance at 488 nm of the conjugates relative to the input eGFP-LPETG-HiSδ protein, we estimated that the lipid-modified protein conjugates were all obtained in excellent (-60-90%) yield (Table 1 and Figure 14). A reproducible drop in reaction yield for nucleophiles containing fatty acids of intermediate length (1-C16, 1-C18, 1-C20) was observed. Whether this reflects a drop in the efficiency of the actual transpeptidation reaction or limited solubility of the resulting lipoprotein conjugates, which could contribute to losses during the sortase depletion step, is presently unclear. It should be noted, however, that the purity of these eGFP conjugates, as determined by both SDS-PAGE (Figure 2) and ESI-MS (Figure 12), was not compromised. [00340] Further details regarding lipid modification of GFP-LPETG-His6, removal of His6- tagged proteins, acetone precipitation of eGFP conjugates and characterization by ESI-MS, and MALDI-TOF MS Characterization of eGFP-2-chol., and estimation of % yield of eGFP conjugates are as follows:
[00341] Lipid modification of GFP-LPETG-His6 and removal of His6-tagged proteins (General Procedure). Lipidated triglycine nucleophile (0.5 μL of a 100 mM solution in DMSO) was combined with 2.5 μL of 10x sortase reaction buffer (500 mM Tris pH 7.5, 100 mM CaC12, 1.5 M NaCl) and 1.25 μL of 20% (w/v) n-dodecyl maltoside. This mixture was
O repeatedly heated in a 90 C heat block and incubated in a sonicating water bath to disperse and solubilize the lipidated nucleophile. After cooling to room temperature, eGFP-LPETG- His6 (12.4 μL of a 110 μM solution in 20 mM Tris pH 8.0, 150 mM NaCl) and sortase A (8.35 μL of a 448 μM solution in 50 mM Tris pH 8.0, 150 mM NaCl, 10% glycerol (v/v))
O were added. The reaction mixtures were incubated at 37 C for 5 h in the dark and then treated with 50 μL of the appropriate Ni-NTA slurry described above and incubated for an
® additional 2 h at room temperature. The mixtures were then filtered (Spin-X Centrifugal
Tube Filters 0.22 μm, Corning) to yield solutions containing lipid-modified eGFP. Samples were analyzed by SDS-PAGE with visualization by Coomassie blue staining. [00342] Acetone Precipitation of eGFP conjugates and Characterization by ESI-MS. 20 μL of lipid-modified eGFP solution was treated with 1 mL of acetone and centrifuged at maximum speed for 3 minutes. The supernatant was removed and the pellet was washed with 1 mL of acetone. The sample was again centrifuged and the pellet was dissolved in 100 μL of 0.1% formic acid. Samples were then analyzed by LC-ESI-MS (Figure 12a). [00343] MALDI-TOF MS Characterization of eGFP-2-chol. eGFP-2-chol was desalted by RP-HPLC [C4 column, MeCN:H2θ gradient mobile phase with 0.1% TFA, 1 mL/min, 5% MeCN → 50% MeCN (0-15 min), 50% MeCN → 80% MeCN (15-18 min)]. The fraction containing eGFP-2-chol was analyzed by MALDI-TOF-MS (Figure 12b). [00344] Estimation of % Yield of eGFP Conjugates. The yield of lipid modified eGFP was estimated using the absorbance of eGFP at 488 nm. As a standard, a sample of unmodified eGFP-LPETG-Hisό was incubated in the absence of sortase A and lipidated nucleophile (Figure 2b, lane 1) and treated with Ni-NTA resin containing excess imidazole to prevent protein binding. After filtration to remove Ni-NTA, the absorbance of this sample at 488 nm was measured and assumed to represent 100% recovery. Serial dilutions of this sample were measured in triplicate and used to construct a standard curve (Figure 14). [00345] Interaction of Lipid-Modified eGFP with Mammalian Cells [00346] The presence of a hydrophobic tail on eGFP should render it capable of spontaneous association with biological membranes (1, 2, 24, 44). As an initial investigation into the effect of the identity of the lipid tail on the ability of these lipoproteins to associate with cells, we incubated HeLa cells with lipid-modified eGFP (2.5 μg/mL) in serum-free medium for 1 h at 37 °C. After washing, the cells were analyzed by flow cytometry (Figure 3). In general, we observed a steady increase in cellular fluorescence with increasing length of the lipid tail. In the case of eGFP-l-C22, we recorded a 500-fold enhancement in mean cellular fluorescence relative to that of eGFP-GGG. Interestingly, eGFP-l-C24 consistently yielded lower association than eGFP-l-C22. For all samples cell viability was >94% as determined by exclusion of propidium iodide, indicative of a lack of cytotoxicity of the lipidated eGFP derivatives. Also, because the eGFP preparations contained low levels of free lipidated nucleophile (~1 μM in culture medium), we verified that this contaminant did not contribute to the observed increase in cellular fluorescence. eGFP-GGG in combination with 1 μM 1-C22, 1-C24, or 2-chol produced only modest increases in fluorescence, <5% of the magnitude observed for the corresponding covalently modified eGFP conjugates (Figure 15). In this control experiment, cells were seeded into 6-well polystyrene cell culture plates at a density of -100,000 cells per well and incubated overnight. The media was then removed and replaced with 2 mL of serum-free DME containing 2.5 μg/mL eGFP-GGG and 1 μM lipidated triglycine nucleophile (1-C22, 1-C24, or 2-chol). Cells were incubated for 1 h at 37
C. Next, the cells were washed three times with ~4 mL of cold PBS containing 1% FBS. The cells were lifted from the culture plate by treatment with 1 mL of 1 mM EDTA in PBS and pelleted at 250 x g for 5 min. The cells were then resuspended in 200 μL of PBS containing 1% FBS and propidium iodide (0.5 μM) and analyzed by flow cytometry (Figure 15).
[00347] A preliminary evaluation of the subcellular localization of eGFP-l-C22 and eGFP-2-chol was performed using spinning disk confocal microscopy. HeLa cells and U373 cells were incubated with 2.5 μg/mL lipoprotein in serum-free medium, followed by washing and live cell imaging. For both cell types we observed staining of the cell surface as well as the appearance of internal fluorescent structures (Figure 4). For all cells, filamentous membrane extensions, presumably filopodia, were evident in the fluorescent micrographs, indicating the presence of the eGFP lipoproteins on the plasma membrane. In U373 cells, distinct vesicular structures were observed at early (1 h) and later (5 h) time points, with a more pronounced presence of vesicles observed for eGFP-l-C22 than for eGFP-2-chol. In general, less internalization was observed for HeLa cells, though punctate internal staining could be observed with eGFP-l-C22 after a 5 h incubation in these cells. In the case of U373, we were also able to verify that eGFP-l-C22 had access to early/recycling endosomal compartments as determined by partial colocalization with transferrin (Figure 5) (6, 45). Colocalization between eGFP— 2-chol and transferrin was not observed (Figure 5) for this cell line. Taken together, these results demonstrate that synthetic lipoproteins prepared using sortase-mediated transpeptidation can interact strongly with the plasma membrane and access endosomal compartments. The range of staining observed for our eGFP conjugates suggests that interactions with cells could be fine-tuned, and studies are under way to characterize the differences in the behavior of protein conjugates bearing different lipid anchors, specifically looking for differences in subcellular distribution and routes of endocytosis. [00348] Further details regarding materials and methods used in the experiments described in this section are as follows:
[00349] 100Ox stock solutions of lipid-modified eGFP. Solutions of lipid-modified eGFP obtained by transpeptidation and depletion of His6-tagged proteins were used without further purification for cell membrane association studies. Prior to addition to cells, the concentration of eGFP in each sample was measured by UV -Vis (488 nm), and all solutions were adjusted to a final eGFP concentration of 2.5 mg/mL. Dilutions were made with a mock reaction mixture lacking eGFP, sortase A, and lipidated triglycine nucleophile to ensure that all samples contained the same amount of residual components (n-dodecyl maltoside, imidazole, CaCb, etc.) from the sortase labeling procedure.
[00350] Cell culture and membrane association of lipid-modified eGFP. HeLa cells were maintained in DME media supplemented with 10% fetal bovine serum (FBS), penicillin (50 units/mL), and streptomycin sulfate (50 μg/mL). Cells were incubated in a 5% CO2 humidified incubator at 37 C. One day prior to treatment with lipid-modified eGFP, cells were seeded into 6-well polystyrene cell culture plates at a density of ~ 100,000 cells per well and incubated overnight. The media was then removed and replaced with 2 mL of serum-free DME containing 2.5 μg/mL modified eGFP (lipid modified proteins were delivered as 100Ox stock solutions, see above). Cells were then incubated for 1 h at 37°C. Next, the cells were washed three times with ~4 mL of cold PBS containing 1% FBS. The cells were lifted from the culture plate by treatment with 1 mL of 1 mM EDTA in PBS and pelleted at 250 x g for 5 min. The cells were then resuspended in 200 μL of PBS containing 1% FBS and propidium iodide (0.5 μM) and analyzed by flow cytometry.
[00351] Spinning Disc Confocal Microscopy. HeLa and U373 cells were maintained in DME media supplemented with 10% fetal bovine serum (FBS), penicillin (50 units/mL), and streptomycin sulfate (50 μg/mL). Cells were incubated in a 5% CO2 humidified incubator at
37 C. One day prior to treatment with lipid-modified eGFP, cells were seeded into Lab-
TM
Tek II chambered coverglass slides (Nalge Nunc International) and allowed to adhere overnight. The media was then removed and replaced with 200 μL of serum-free DME containing 2.5 μg/mL modified eGFP (lipid modified proteins were delivered as 100Ox stock
O solutions, see above). Cells were then incubated for 1-5 h at 37 C. Next, the cells were washed three times with -0.5 mL of cold PBS containing 1% FBS. Cells were then covered with 200 uL of PBS containing 1% FBS and imaged. For transferrin colocalization, U373 were incubated with 200 μL of serum-free DME containing 2.5 μg/mL modified eGFP for 5 h at 37 C. Transferrin- Alexa 647 (Invitrogen, 100 μg/mL final concentration) was added during the final 15 minutes of this incubation. Cells were then washed as described above and imaged.
Discussion of Example 1
[00352] In summary, we have developed a general strategy using sortase-mediated transpeptidation as a means to install hydrophobic lipid modifications onto protein substrates in site-specific fashion. The ease of use of this method stands out as a significant asset. Protein substrates require, e.g., only a five amino acid extension (such as LPETG) to serve as sortase substrates, a modest insertion that is not expected to impede the function of most proteins and should also have minimal impact on the expression yield of these polypeptides. Recombinant proteins containing the LPETG motif are also stable and unreactive until activated by the sortase enzyme. This affords a distinct advantage over the expressed protein ligation approach where premature cleavage of intein fusion proteins has been documented, leading to a reduction in the yield of final ligation products. The requisite lipid-modified nucleophiles compatible with sortase-mediated transpeptidation also have a very straightforward structural requirement of a short stretch of glycine residues and are prepared by standard solid-phase synthesis. Therefore, both natural and non-natural hydrophobic modifications can be easily incorporated using this system. [00353] While the requirement for the sortase enzyme itself could be perceived as a disadvantage of the transpeptidation strategy, it should be noted that we routinely express batches with yields of >50 mg/L, and stock solutions of the enzyme can be stored for several months with no apparent degradation in enzymatic activity. Moreover, in this work we provided a convenient method for removing sortase following transpeptidation. The ready availability of sortase and ease of removal following transpeptidation are important features as the enzyme is relatively inefficient and excess sortase is typically employed in the art to drive the labeling reactions to high levels of conversion in a reasonable period of time.
[00354] In this initial work, we used eGFP as our model protein substrate due to its natural fluorescence and verified that eGFP proteins lipidated through sortase-mediated transpeptidation strongly associate with mammalian cells. We envision further applications of this chemical modification strategy to include anchorage of proteins to cellular membranes that do not normally occur on the cell surface to create artificial cell surface receptors.
Additionally, because the transpeptidation strategy is able to attach extremely hydrophobic modifications, it could provide a new method for interfacing proteins with materials that possess poor water solubility, such as carbon nanotubes.
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[00400] Please note that methods and references described in Exampes herein are applicable to other Eexamples and aspects of the invention. Example 2: Modification of N-Terminal Glycine Residues using Structural Mimetics of the Sortase A Recognition Sequence
[00401] The transpeptidation reaction catalyzed by sortase A has emerged as a general method for derivatizing proteins with a variety of modifications. Yet, in its present incarnation, it appears that the practical application of this approach has been limited to the protein C-terminus. Target proteins are engineered to contain the sortase A recognition motif (LPXTG) near their C-termini. When incubated with synthetic peptides containing one or more N-terminal glycine residues and recombinant sortase A, these artificial sortase substrates undergo a transacylation reaction resulting in the exchange of residues C-terminal to the threonine residue with the synthetic oligoglycine peptide. The use of excess oligoglycine drives this equilibrium process, and in most cases quantitative protein labeling can be achieved.
[00402] In simple terms, the transpeptidation reaction results in the ligation of species containing an LPXTG motif with those bearing one or more N-terminal glycine residues. We therefore became interested in whether a similar method for N-terminal labeling could be achieved by preparing protein substrates with N-terminal glycine residues and ligating them to synthetic peptides containing the LPXTG motif or structural analogs of this recognition element (Figure 8). We herein describe the successful development of a general strategy for site-specific labeling of proteins with one or more N-terminal glycine residues. This technique allows for the installation of modifications suitable for a range of proteomic and biological applications.
[00403] As noted above, synthetic peptides containing the LPXTG motif have been shown to function as substrates for sortase A, generating the acyl enzyme intermediate necessary for transpeptidation. However, at the outset of our studies we were concerned that peptides containing the entire LPXTG sequence could create a potential complication for N-terminal protein labeling. As outlined in Figure 8a, each successful transfer of an LPXT unit to the target protein would release a stoichiometric amount of a peptide fragment containing an N- terminal glycine. This by-product would compete with the protein nucleophile for the same acyl enzyme intermediate, thereby limiting the efficiency of the labeling reaction. Moreover, hydrolytic cleavage of an LPXTG peptide, although a relatively slow process, would exacerbate competition with the protein nucleophile as the reaction proceeded. Indeed, preliminary attempts in our laboratory to perform N-terminal protein labeling with peptides containing all five residues (LPXTG) yielded disappointing results and useful levels of protein modification could only be obtained using high concentrations (>5 mM) of the LPXTG-containing peptide (data not shown). We reasoned that a simple solution to this problem could be to substitute the glycine in the LPXTG motif with a moiety that would exhibit poor nucleophilicity once released by sortase (Figure 8b). With this design principle in mind, we synthesized fluorescein (1) and biotin (2) derivatives of an LPRT peptide where the glycine residue was replaced by a simple methyl ester. Compounds 1 and 2 were prepared through a combination of solid-phase and solution-phase transformations and purified to homogeneity by reversed phase-HPLC (see Figure 16). Arginine was placed in the X position to enhance water solubility and because a side chain that would be unreactive toward reagents used to modify the N-terminus of the LPRT peptide.
[00404] With 1 and 2 in hand we expressed a series of model protein substrates containing N-terminal glycine residues. It should be noted that recombinant protein bearing N-terminal glycine residues have been shown to function as nucleophiles for sortase-mediated transpeptidation, though only in the context of ligation to other proteins bearing the LPXTG motif. For our studies, three variants of the cholera toxin B-subunit (CtxB) were prepared containing 1, 3, or 5 N-terminal glycine residues. To investigate selectivity for glycine, a final construct containing an N-terminal alanine residue was also prepared. Following some brief optimization, we were able to arrive at conditions that yielded quantitative labeling of constructs containing 3 or 5 glycines using 500 μM 1 with only trace labeling of the alanine- containing control. As shown in Figure 9a, a fluorescence gel scan revealed robust labeling of CtxB if 3 or 5 glycines were present. No background labeling was observed in the absence of sortase A. For CtxB constructs containing 3 or 5 glycines residues, quantitative labeling was evident after 2 h at 37 0C as determined by ESI-MS (Figure 9b, and Figure 17). Similar labeling experiments with biotinylated derivative 2 GGGGG-CtxB yielded identical results and the resulting conjugates could be detected by streptavidin immunoblot (Figure 18) and conjugates were characterized using ESI-MS. Conditions used for experiment shown in Fig. 18 were: 33 μM G5-QxB, 50 mM SrtAstaph, 500 μM 2, 50 mM Tris pH 7.5, 150 mM NaCl, 10 mM CaC12, 2h at 37 degrees C. In all cases, residual labeling of the sortase enzyme itself could be detected. This was expected because the transpeptidation reaction proceeds through a covalent acyl enzyme intermediate.
[00405] N-terminal transpeptidation was easily extended to two additional protein substrates (Figure 10). eGFP bearing five glycines and the ubiquitin specific hydrolase UCH- L3 containing a single glycine were labeled efficiently as determined by ESI-MS. It should be noted that the utility of this labeling method for recombinant proteins expressed in E. coli is facilitated by natural processing of newly synthesized polypeptides by endogenous methionine aminopeptidase. When the initiator N-formylmethionine (N-fmet) is followed by small residues such as glycine, the removal of N-fmet is quantitative. Therefore, preparation of substrates for N-terminal transpeptidation requires only basic cloning techniques, and in most cases would only require a single residue substitution.
Example 3: Highly Efficient Sortase-Catalyzed Protein Circularization [00406] This Example demonstrates that sortase-catalyzed transpeptidation can be used for efficient synthesis of circular and oligomeric proteins. This method has general applicability, as illustrated by successful intramolecular reactions with three structurally unrelated proteins. In addition to circularization of individual protein units, the multiprotein complex AAA- ATPase p97/VCP/CDC48, with six identical subunits containing the LPATG motif and an N- terminal glycine, was found to preferentially react in daisy chain fashion to yield linear protein fusions. For supplemental figures, additional methods, and references, please see, Antos, JM, et al. "A straight path to circular proteins" J Biol Chem. ;284(23): 16028-36, 2009. [00407] Synthesis of Triglycine Tetramethylrhodamine Peptide. The structure of GGG- TMR5 and a detailed synthetic protocol are provided in the supplemental material and supplemental Fig. S7. [00408] Materials and Methods [00409] Cloning and Protein Expression
[00410] Full amino acid sequences for all proteins used in this study are given in supplemental Fig. S8.
[00411] Recombinant sortase A (residues 26-206) containing an N-terminal hexahistidine tag was produced in Escherichia coli as described previously (8). Purified sortase A was stored in 10% glycerol, 50 mM Tris, pH 8.0, 150 NaCl at -80 °C until further use. [00412] G-Cre-LPETG-His6 was cloned into the pTriEx-1.1 Neo expression vector (Novagen) using standard molecular biology techniques. The construct contains two point mutations (Ml 17V and E340Q) and a flexible spacer (GGGGSGGGGS) inserted before the LPETG sortase recognition site. G-Cre-LPETG-His6 was expressed and purified using procedures similar to those reported previously for HTNCre (24). G-Cre-LPETG-His6 was first transformed into Tuner (DE3) pLacI cells (Novagen), and a starter culture was grown in sterile LB media supplemented with 1% (w/v) glucose, chloramphenicol (34 μg/ml), and ampicillin (100 μg/ml). This culture was used to inoculate a large scale culture of sterile LB containing chloramphenicol (34 μg/ml) and ampicillin (100 μg/ml). G-Cre-LPETG-His6 was expressed after a 3-h induction with isopropyl 1-thio-β-D-galactopyranoside (0.5 ΓΠM) at 37 0C. Cells were resuspended in 10 mM Tris, 100 mM phosphate, 300 mM NaCl, and 20 HIM imidazole, pH 8.0. The suspension was adjusted to 50 μg/ml DNase I, 460 μg/ml lysozyme, and 1 mM MgCl2 and incubated at 4 °C for 1.5 h. The suspension was then sonicated and centrifuged. The clarified lysate was then treated with Ni-NTA-agarose (Qiagen) for 1 h at 4 °C. The resin was washed with 12 column volumes of 10 mM Tris, 100 mM phosphate, 300 mM NaCl, and 20 mM imidazole, pH 8.0, followed by 4 column volumes of 10 mM Tris, 100 mM phosphate, 300 mM NaCl, and 30 mM imidazole, pH 8.0. The protein was then eluted with 10 mM Tris, 100 mM phosphate, 300 mM NaCl, and 300 mM imidazole, pH 8.0. The purified protein was then dialyzed first against 20 mM Tris, pH 7.5, 500 mM NaCl followed by 50% glycerol, 20 mM Tris, pH 7.5, 500 mM NaCl. G-Cre-LPETG-His6 was then passed through a 0.22-μm filter to remove minor precipitation and stored at 4 °C.
[00413] G5-eGFP-LPETG-His6 was prepared from a previously reported eGFP construct lacking the five N-terminal glycine residues using a QuickChange® II site-directed mutagenesis kit (Stratagene) and produced in E . coli using reported procedures (11). Purified G5-eGFP-LPETG-His6 was buffer exchanged into 20 mM Tris, pH 8.0, 150 mM NaCl and stored at 4 °C. UCHL3 with the sortase recognition sequence (LPETG) substituted for amino acids 159-163 was cloned and produced in E . col i as described previously (25). [00414] Human p97 (806 amino acids) was PCR-amplified and cloned via the Ndel and HindIII restriction sites into a pET28a+ expression vector (Novagen) to yield the G-His6-p97 construct. G-His6-p97-LPSTG-XX was generated by introducing two point mutations (G782L and Q785T) and a stop codon at position 791 using QuickChange® mutagenesis (Stratagene). Recombinant p97 was expressed at 30 °C in E . col i after induction for 3 h with 0.5 mM isopropyl 1-thio-β-D-galactopyranoside. Cells were resuspended in buffer A (50 mM Tris, pH 8.0, 300 mM NaCl, 5% glycerol, 20 mM imidazole, and 7.1 mM β-mercaptoethanol), adjusted to 15 μg/ml lysozyme and 10 μg/ml DNase I, and lysed by two passes through a French pressure cell at 1200 p.s.i. After centrifugation for 30 min at 40,000 x g, the supernatant was bound to nickel-Sepharose resin (GE Healthcare). After washing the resin with 20 column volumes of buffer A, p97 was eluted with buffer A containing 250 ΓΠM imidazole. Hexameric rings of p97 were further purified on a Superdex 200 HR 16/60 column (GE Healthcare) using 25 mM Tris, pH 8.0, 150 mM KCl, 2.5 mM MgCl2, 5% glycerol as the mobile phase. The purified protein was snap-frozen and stored at -80 °C. [00415] Circularization and Intermolecular Transpeptidation [00416] Transpeptidation reactions were performed by combining the necessary proteins/reagents at the specified concentrations in the presence of sortase reaction buffer (50 ΓΓLM Tris, pH 7.5, 150 mM NaCl, 10 ΓΠM CaCl2) and incubating at 37 °C for the times indicated. Diglycine and triglycine (GGG) peptides were purchased from Sigma. Reactions were halted by the addition of reducing Laemmli sample buffer and analyzed by SDS-PAGE. Gels were visualized by staining with Coomassie Blue. Fluorescence was visualized on a Typhoon 9200 Imager (GE Healthcare). Crude reactions were also diluted into either 0.1% formic acid or water for ESI-MS analysis. ESI-MS was performed on a Micromass LCT mass spectrometer (Micromass® MS Technologies) and a Paradigm MG4 HPLC system equipped with an HTC PAL autosampler (Michrom BioResources) and a Waters symmetry 5-μm C8 column (2.1 x 50 mm, MeCN:H2O (0.1% formic acid) gradient mobile phase, 150 μl/min). [00417] Purification and Refolding of eGFP
[00418] G5-eGFP-LPETG-His6 (50 μM) was circularized by treatment with sortase A (50 μM) in sortase reaction buffer (50 mM Tris, pH 7.5, 150 mM NaCl, 10 mM CaCl2) for 24 h at 37 °C. The reaction was run on a 750-μl scale. The entire reaction was then diluted into 10 ml of 20 mM Tris, 500 mM NaCl, and 20 mM imidazole, pH 8.0. This solution was then applied to a column consisting of 2 ml of Ni-NT A-agarose (Qiagen) pre-equilibrated with 20 mM Tris, 500 mM NaCl, and 20 mM imidazole, pH 8.0. The flow-through was then concentrated and buffer exchanged in 20 mM Tris, 150 mM NaCl, pH 8.0, using a NAP™ 5 Sephadex™ column (GE Healthcare). The concentrations of circular eGFP and linear G5-eGFP-LPETG-His6 were estimated by UV-visible spectroscopy using the absorbance of eGFP at 488 nm (extinction coefficient 55,900 M~' cm"1) (^6). Circular and linear eGFP (40 μl of 18 μM solutions) was placed in 1.5-ml microcentrifuge tubes and denatured by heating to 90 °C for 5 min. Samples were then incubated at room temperature in the dark for the times indicated. Fluorescent images were acquired using a UV gel documentation system (UVP Laboratory Products). [00419] Reaction of Cyclic UCHL3 with Activity-based Ubiquitin Probe [00420] UCHL3 (30 μM) was incubated with sortase A (150 μM) in sortase reaction buffer (50 mM Tris, pH 7.5, 150 mM NaCl, 10 mM CaCl2) in the presence or absence of 90 mM GGG peptide (Sigma) on a 25-μl scale at 37 °C for 3 h. Ten microliters was withdrawn and diluted with 10 μl of labeling buffer (100 mM Tris, pH 7.5, 150 mM NaCl). Hemagglutinin epitope- tagged ubiquitin vinyl methyl ester (4 μg) was added as well as 1 mM dithiothreitol and incubated at room temperature for 1 h. Reactions were then separated on an SDS- polyacrylamide gel and visualized by Coomassie staining or α-HA immunoblot (supplemental Fig . S4). Hemagglutinin epitope-tagged ubiquitin vinyl methyl ester was prepared following published protocols (27).
[00421] MS/MS Sequencing of Proteolytic Fragments from Circular Proteins [00422] Prior to MS/MS analysis, circular eGFP and Cre were separated from sortase A by RP-HPLC using an Agilent 1100 Series HPLC system equipped with a Waters Delta Pak 5 μm, 100 A Cl 8 column (3.9 x 150 mm, MeCN:H2O gradient mobile phase containing 0.1% trifluoroacetic acid, 1 ml/min). Fractions containing the circular proteins were pooled and subjected to trypsin digestion. Crude transpeptidation reactions containing circular UCHL3 were separated by SDS-PAGE followed by Coomassie staining. The band corresponding to circular UCHL3 was excised and digested with GIu-C. Crude transpeptidation reactions containing dimeric p97 were separated by SDS-PAGE followed by Coomassie staining. The transpeptidation reaction used for this purpose was incubated for only 2 h and therefore contains less oligomerization than that seen after an overnight incubation (see supplemental Fig . S6). The band corresponding to dimeric p97 was excised and digested with chymotrypsin. For all protein substrates, the peptides generated from proteolytic digestion were extracted and concentrated for analysis by RP-HPLC and tandem mass spectrometry. RP-HPLC was carried out on a Waters NanoAcquity HPLC system with a flow rate of 250 nl/min and mobile phases of 0.1% formic acid in water and 0.1% formic acid in acetonitrile. The gradient used was isocratic 1% acetonitrile for 1 min followed by 2% acetonitrile per min to 40% acetonitrile. The analytical column was 0.075 μm x 10 cm with the tip pulled to 0.005 μm and self-packed with 3 μm Jupiter Cl 8 (Phenomenex). The column was interfaced to a Thermo LTQ linear ion trap mass spectrometer in a nanospray configuration, and data were collected in full scan mode followed by MS/MS analysis in a data-dependent manner. The mass spectral data were data base searched using SEQUEST. [00423] Construction of Molecular Models
[00424] Molecular models were generated from published crystal structures (PDB codes lkbu, lgf 1, Ixd3, and 3cf 1) (^8-3J1). N- and C-terminal residues were added using Coot 0.5 (3_2). Protein termini were repositioned using the Auto Sculpting function in MacPyMOL (DeLano Scientific LLC). Residues visible in the published crystal structures were not moved during positioning of the extended N and C termini. All protein images in this study were generated using MacPyMOL. [00425] Results [00426] Cre Recombinase. We first noticed the presence of a circular protein product when installing a C-terminal modification onto a nonfunctional mutant of Cre recombinase containing a single N-terminal glycine residue and an LPETG sequence near the C terminus. The LPETG motif was separated from the native protein by a flexible amino acid linker (GGGGSGGGGS). Whereas installation of the label at the Cre C terminus proceeded efficiently when a triglycine nucleophile containing tetramethylrhodamine (GGG-TMR) was included, we observed a product that migrated more rapidly on SDS-PAGE when nucleophile was omitted from the reaction mixture (Fig. 26). Hydrolysis of the sortase acyl enzyme is known to proceed slowly in the absence of glycine nucleophiles (3^9, 3_3> 3_4). However, when reaction mixtures were analyzed by ESI-MS, we consistently observed a protein species that differed from the mass expected for hydrolysis by approximately -18 Da (Fig . 2^B). This mass was consistent with intramolecular nucleophilic attack, suggesting that the single N-terminal glycine residue was serving as the nucleophile in this transformation. Ultimately, MS/MS on tryptic digests of this species showed unequivocally that it consisted of a covalently closed circular product of Cre, with the N-terminal glycine fused exactly at the LPETG cleavage site in the expected position (Fig. 26C). Recognizing that the LPETG motif is maintained in the cyclized Cre product, we suspected that sortase should be capable of cleaving the circular protein at this site, thus producing an equilibrium between circular and linear forms of Cre. To demonstrate this point, Cre was first incubated with sortase in the presence or absence of triglycine nucleophile (Fig. 27A). A portion of the cyclized reaction mixture (Fig. 21A, lane 1) was then treated with a large molar excess of triglycine nucleophile or left alone for a further 24 h (Fig. 27A, lanes 2 and 3). Remarkably, upon treatment with exogenous nucleophile, the pre-cyclized material yielded a reaction mixture that was nearly identical to the result obtained when nucleophile was included from the very beginning of the experiment (Fig. 27A, compare lanes 3 and 4). This result provided further evidence that cyclized Cre indeed contains the expected LPETG motif at the site of covalent closure. In addition, it suggested that hydrolysis of the acyl enzyme intermediate does not effectively compete during cyclization, because the hydrolyzed material should be unable to participate in the transpeptidation reaction. The circularization reaction observed for Cre proceeded with remarkable efficiency. Conversion was estimated to be >90% by SDS-PAGE. By taking an existing crystal structure (29) of the Cre protein and modeling in those residues not visible in the structure, it was clear that the N and C termini were located in sufficiently close proximity to permit closure without significant perturbation of the native structure (Fig. 27B). We assume that these regions possess considerable flexibility because they are not resolved in the crystal structure.
[00427] eGFP. Having verified the cyclization of Cre recombinase, we sought to explore the generality of this technique. To this end we generated a derivative of eGFP containing the LPETG sequence and five N-terminal glycine residues. This construct was of particular interest because inspection of the x-ray crystal structure (3J.) revealed that the N and C termini were positioned on the same end of the β-barrel, suggesting that this substrate should be ideal for cyclization (Fig. 28A). Furthermore, in one of the earliest reports on the use of sortase for protein engineering, a similar eGFP substrate was described and reported to cyclize in the presence of sortase Q6). In this instance, cyclization only proceeded in modest yield, and the putative cyclized product was produced as a mixture with higher molecular weight species assigned as oligomers of eGFP formed by intermolecular transpeptidation. Thus, to explore potential complications caused by intermolecular reactions, we studied the reaction of our eGFP construct in the presence of sortase.
[00428] In our hands, we observed clean conversion to a lower molecular weight species (>90% estimated conversion) with little to no evidence for oligomerization (Fig. 28B). A higher molecular weight polypeptide was observed at early time points and may represent a covalent eGFP dimer that is generated transiently over the course of the reaction. Higher molecular species, however, were only observed in trace quantities in the final reaction mixture. As in the case of Cre, evidence for circularization was provided by mass spectral characterization of the intact circular protein and MS/MS sequencing of tryptic peptides (supplemental Fig. SlV As an additional control to demonstrate that the N-terminal glycine residue was the only nucleophile participating in intramolecular transpeptidation, we analyzed the behavior of an eGFP derivative that lacked an N-terminal glycine. In this case, ESI-MS revealed products consistent with hydrolysis of the acyl enzyme intermediate, rather than intramolecular nucleophilic attack (supplemental Fig. Sl).
[00429] Circularization has been shown to confer unique properties onto proteins when compared with the linear form (35-32)- m the case of GFP circularized using intein-based methods, these properties include a reduced rate of unfolding when exposed to denaturants, as well as an enhanced rate of refolding following denaturation (35_). We observed a similar phenomenon for eGFP circularized using sortase (Fig. 28C). Circular eGFP was first separated from residual sortase A using Ni-NTA resin. This material retained fluorescence suggesting that covalent ligation of the N and C termini had minimal impact on the structure of this substrate. Circular and linear eGFP were then subjected to simple thermal denaturation, followed by recovery at room temperature. As shown in Fig. 28C, circular eGFP regained fluorescence more rapidly than linear eGFP.
[00430] UCHL3. Even an internally positioned LPATG motif was sufficient to effectuate a circularization reaction. We installed a sortase recognition site in the crossover loop of the ubiquitin C-terminal hydrolase UCHL3, and we demonstrated that the continuity of the polypeptide backbone can be disrupted with concomitant installation of a covalent modification that reports on the accuracy of cleavage and transpeptidation (25). This reaction proceeds without complete loss of activity of UCHL3, indicating that even the cleaved form of UCHL3 retains its structural integrity to a significant degree (25). This UCHL3 construct was prepared with an N-terminal glycine residue, and examination of the crystal structure of UCHL3 (30) clearly showed the close apposition of the N terminus and the crossover loop, suggesting that cyclization to yield a circular fragment containing the N-terminal portion of UCHL3 should be readily observable (Fig. 29A).
[00431] As expected, in the absence of added nucleophile, the N-terminal glycine serves as a highly efficient nucleophile to yield a circular fragment that contains the N-terminal portion of UCHL3 (Fig. 29B). The identity of the circular polypeptide was confirmed by MS/MS of the peptide containing the expected fusion of the N-terminal glycine residue with the new C terminus released from the crossover loop (see supplemental Fig. S2). Cyclization was efficiently blocked if a high concentration of triglycine (GGG) was included in the reaction, generating instead the N-terminal fragment of UCHL3 transacylated onto the triglycine nucleophile (Fig. 29B, lane 9, and supplemental Fig. S3). Cyclization could also be reversed by adding an excess of triglycine to reaction mixtures preincubated with sortase to allow cyclization. This reopening reaction was observed by both SDS-PAGE and ESI-MS (supplemental Fig. S3).
[00432] To test the functional properties of cyclic UCHL3, we incubated reaction mixtures with an activity-based probe consisting of ubiquitin equipped with an electrophilic vinyl methyl ester moiety at the C terminus (supplemental Fig. S4). Probes of this nature are able to specifically alkylate active site cysteine residues in ubiquitin-specific hydrolases such as UCHL3 (25, 27, 38). Following circularization, the active site cysteine (Cys-95) of UCHL3 is located in the circular N-terminal fragment, and indeed we observed covalent labeling of this fragment with a corresponding shift in apparent molecular weight consistent with the attachment of ubiquitin. This result suggests that despite cleavage of the polypeptide backbone, the circular N-terminal fragment of UCHL3 and the C-terminal portion released during transpeptidation remain associated and preserve the affinity of UCHL3 for ubiquitin. This result is consistent with previous observations from our laboratory demonstrating that covalent closure of the UCHL3 crossover loop is dispensable for enzyme activity (25). [00433] p97. The examples described above in this Example concern single chain proteins whose termini are sufficiently close to allow covalent closure by means of the sortase- mediated transacylation reaction. Similar proximity relationships between protein termini should also be present on separate polypeptides that assemble into defined oligomeric structures. As an example, we examined p97, a hexameric AAA-ATPase. We generated a derivative of p97 (G-His6-p97-LPSTG-XY) containing an LPSTG motif near the C terminus, and a hexahistidine tag capped by two serine residues and a single glycine at the N terminus. The structure of a p97 trimer in the presence of ADP has been solved at 3.5 A resolution (28), with several residues from the N and C termini not visible (Fig. 30A). When all the residues present in our modified version of p97 were modeled onto the published trimer of p97, it was evident that the N and C termini of adjacent p97 units were sufficiently close to permit covalent cross-linking (Fig. 30B). G-His6-p97-LPSTG-JOfwas expressed in E. coli and yielded the hexameric p97 ring, as assessed by gel filtration. As expected, this derivative of p97 was an excellent substrate for transpeptidation at its C terminus, allowing efficient installation of a label when incubated in the presence of sortase and GGG-TMR (supplemental Fig. S5). In contrast, a variant of p97 lacking the LPSTG sequence showed no labeling (supplemental Fig. S5). When G-His6-p97-LPSTG-ΛXwas treated with sortase A in the absence of added nucleophile, we observed formation of an SDS-resistant ladder of polypeptides, as would be expected for intermolecular cross-linking of p97 monomers (Fig. 30C). We were confident that these species arise from head-to-tail ligation of p97 because introduction of excess diglycine peptide after oligomerization caused collapse of the higher molecular weight structures back to monomeric p97 (Fig. 3OC, lane 5). This suggested that the higher order aggregates are held together by newly formed LPSTG units formed from the C-terminal LPST residues of one p97 monomer and the N-terminal glycine residue of a neighboring monomer. The banding pattern observed for reopening was also nearly identical to that seen when diglycine was included from the very beginning of the experiment, a scenario where installation of diglycine at the C terminus of each p97 subunit is presumed to be the major reaction pathway (Fig. 3OC, lane 6). We have also been able to identify peptides consistent with intermolecular cross-linking of p97 subunits by MS/MS (supplemental Fig.
S6).
[00434] In this Example we have explored transpeptidation reactions using four structurally diverse protein substrates. Cyclization has been confirmed for three proteins, including an example (UCHL3) utilizing an LPXTG sequence positioned in a flexible internal loop rather than near the C terminus of the protein. Cyclization and oligomerization via sortase-mediated transpeptidation have been previously suggested to occur for an eGFP construct modified in a manner similar to that used here (16), and for a by-product from a protein purification system where the substrate circularized appears to be sortase A itself (20). In both cases, the identity of the circular products was not rigorously confirmed. Our data identify the circular or oligomeric products unambiguously by MS/MS for all substrates studied. We also find that our eGFP derivative strongly favors cyclization over oligomerization, showing little evidence for the formation of higher order structures that might be expected by the head-to-tail ligation of termini from separate eGFP monomers. Subtle differences in the structure of the eGFP constructs cannot be overlooked as a potential cause for the observed results. For example, our eGFP is extended at the N terminus by only five glycine residues, whereas the construct studied by Parthasarathy et al. Q6) contains an additional 17 residues, including 3 N-terminal glycines. Future work will be required to thoroughly characterize the effect of distance relationships between protein termini on favoring intra- versus intermolecular transpeptidation.
With respect to protein cyclization, sortase-mediated circularization is efficient despite the potential for competing reaction pathways. In the absence of added oligoglycine nucleophile, these include hydrolysis of the acyl enzyme intermediate, reattachment of the C-terminal protein fragment that is lost upon initial cleavage of the protein substrate by sortase, or, as mentioned above, oligomerization of protein monomers in head-to-tail fashion. Even when oligoglycine nucleophile is added with the intent of blocking the cyclization pathway, millimolar concentrations are necessary to efficiently compete with cyclization. One factor that certainly must contribute to this observed preference for cyclization is the distance between protein termini. Inspection of the data base of PDB shows that nearly one-third of proteins with known structures have their termini in rather close apposition (within 20 A) (40). The LPATG sequence itself spans roughly 15 A in an extended conformation, suggesting that circularization via sortase-catalyzed transpeptidation might be amenable to a significant fraction of proteins using the LPXTG sequence alone to bridge the gap between N and C termini. Larger distances could simply be covered by inserting flexible amino acid spacers at either termini. We also consider it likely that the circularized version of a protein will show more restricted mobility in the segment that corresponds to the newly established LPATG connection between its termini. This fact alone may render the circular product a comparatively worse substrate for sortase and therefore assist in driving the transpeptidation reaction toward cyclization. As evidence for this point, we have observed previously that sortase fails to cleave LPATG motifs placed in structured loops of class I major histocompatibility complex molecules (14).
[00435] The sortase-catalyzed approach also provides additional levels of control over the ensuing transpeptidation reaction. This may be particularly useful for oligomeric species, such as the p97 example described here. Specifically, our modified p97 protein (G-His6-p97- LPSTG-XX) is produced in a form that is by itself unreactive. This allows protein expression and the subsequent assembly and purification of the hexamer to be completed first, without complications caused by premature covalent oligomerization. Cross-linking is then induced by the addition of sortase after the individual subunits have been correctly positioned in the hexameric ring. The extent of transpeptidation can be further controlled by inclusion of synthetic oligoglycine nucleophiles, either during the transpeptidation reaction or after transpeptidation is complete. The latter scenario even allows cyclization to be completely reversed. Incubating circular protein products with sortase in the presence of an oligoglycine nucleophile restores linearity to the protein product, because in the course of the initial cyclization reaction, the LP XTG motif is restored. An equilibrium between closed and open forms is thus established and can be driven toward the linear state by adding a large excess of the oligoglycine nucleophile.
Example 4: Dual Modification Using Distinct Sortases
[00436] Materials and Methods.
[00437] SrtAstrep. The expression plasmid for SrtAstrep (residues 82-249) including an
3
N-terminal His6 tag has been described. The construct was transformed into E. coli BL-21. Cells were grown in 2 L of sterile LB containing kanamycin (30 μg/mL) to an optical density of -0.7 at 600 nm. Cells were induced with IPTG (1 mM) for 3 h at 37 C. Cells were
O harvested by centrifugation and the pellet was stored overnight at -20 C. The pellet was thawed and resuspended in 70 mL of 50 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 10% glycerol. Cells were then treated with 300 L of DNAse I (10 mg/mL in PBS), 500 L of lysozyme (50 mg/mL in PBS), and 10 L of MgC12 (1 M in PBS). The lysis reaction was
O incubated for 1 h at 4 C. The cells were then sonicated and centrifuged to remove insoluble material. The clarified lysate was then applied to a Ni-NTA column consisting of 5.0 mL of commercial Ni-NTA slurry (Qiagen) equilibrated with 50 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole, and 10% glycerol. The column was washed with 80 mL of 50 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole, and 10% glycerol. Protein was eluted with five 5 mL portions of 50 mM Tris pH 8.0, 150 mM NaCl, 300 mM imidazole, and 10% glycerol. Fractions containing SrtAstrep were pooled and further purified by size exclusion chromatography on a HiLoad 16/60 Superdex 75 column (Amersham), eluting with 20 mM Tris pH 8.0, 150 mM NaCl at a flow rate of 1 mL/min. Fractions containing SrtAstrep were pooled and subjected to a second round of Ni-affϊnity chromatography. Purified SrtAstrep was then dialyzed against 50 mM Tris pH 8.0, 150 mM NaCl, and 10% glycerol. These solutions were stored at -80 C until further use. Protein concentration was estimated by
Bradford assay.
[00438] SrtAstaph. Recombinant SrtAstaph (residues 26-206) containing an N-terminal
4
His6 tag was produced in E. coli as previously described. SrtAstaph does not contain an N- terminal glycine residue (retains initiator methionine). Purified SrtAstaph was stored in 10% (w/v) glycerol, 50 mM Tris pH 8.0, 150 NaCl at -80 °C until further use. Protein concentration was estimated by Bradford assay.
[00439] Δ59-SrtAstaph. Recombinant Δ59-SrtAstaph (residues 60-206) containing an N- terminal His6 tag was cloned into pΕT28a+. 59-SrtAstaph does not contain an N-terminal glycine residue (retains initiator methionine). Expression of Δ59-SrtAstaph was achieved following the protocol described above for SrtAstrep. Purification by size exclusion chromatography was not necessary because Δ59-SrtAstaph was sufficiently pure following Ni-affinity chromatography.
[00440] CtxB. The template for construction of Gl-CtxB, G3-CtxB, G5-CtxB, and AG4- CtxB consisted of the B-subunit of cholera toxin fused at its N terminus to the signal peptide
5 sequence of E. coli heat labile enterotoxin LTIIb. This targets the expressed protein to the periplasm where the signal peptide is removed. Glycine and/or alanine residues were inserted between the signal sequence and CtxB via Quickchange® II Site-Directed Mutagenesis (Stratagene). Plasmids were transformed into E. coli BL21. Cells were grown in 1 L of sterile LB containing chloroamphenicol (34 μg/mL) to an optical density of -0.5-1.0 at 600 nm.
Cells were induced with arabinose (0.25% w/v) for 3 h at 37 C. Cells were harvested by centrifugation and the pellet was stored overnight at -20 C. The pellet was thawed and resuspended in 30 mL of 50 mM Tris pH 8.0 and 300 mM NaCl. This suspension was then treated with 3 mL of polymixin B solution (5 mg/mL freshly made in water). This was mixture was gently stirred at room temperature for 1 h and then centrifuged. The clarified lysate was treated with 2.5 mL of Ni-NTA slurry (Qiagen). CtxB has a naturally affinity for
Ni-NTA although it does not possess a His6 tag. The Ni-NTA mixture was incubated at 4 C for 1 h and then poured into a fritted plastic column (Bio-Rad). The resin was washed with 40 mL of 50 mM Tris pH 8.0 and 300 mM NaCl. Protein was eluted with two 10 mL portions of 50 mM Tris pH 8.0, 300 mM NaCl, and 300 mM imidazole. Purified CtxB was buffer exchanged into 20 mM Tris pH 8.0 and 150 mM NaCl. Solutions were stored at 4 C. Protein concentration was estimated by Bradford assay.
[00441] G5-eGFP and dual labeling eGFP substrate. G5-eGFP (containing a C-terminal His6 tag) and the eGFP dual labeling substrate (containing an N-terminal thrombin cleavage site and a C-terminal LPETG motif followed by a His6 tag) and were prepared in pET28a+ (Novagen) using a Quickchange® II Site-Directed Mutagenesis Kit (Stratagene). The template plasmid used for mutagenesis has been described.6 Plasmids were then transformed into E. coli BL-21. In a typical experiment, cells were grown in sterile LB containing kanamycin (30 μg/mL) to an optical density of ~0.6-0.9 at 600 nm. Cells were induced with
IPTG (1 mM) for 3 h at 37 C. Cells were harvested by centrifugation and the pellet was
O stored overnight at -20 C. The pellet was thawed and resuspended in 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40. The cell suspension was then lysed by French press and centrifuged. The clarified lysate was then applied to a Ni-NTA column consisting of 5.0 mL of commercial Ni-NTA slurry (Qiagen) equilibrated with 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40. The column was washed with 40 mL of 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40, followed by 40 mL of 20 mM Tris pH 8.0, 150 mM NaCl, and 20 mM imidazole. Protein was eluted with 20 mM Tris pH 8.0, 150 mM NaCl, and 300 mM imidazole until the characteristic green color was fully removed from the column. This material was concentrated and further purified by size exclusion chromatography on a HiLoad 16/60 Superdex 75 column (Amersham), eluting with 20 mM Tris pH 8.0, 150 mM NaCl at a flow rate of 1 mL/min. Fractions containing eGFP were pooled and subjected to a second round of Ni-affinity chromatography. Purified eGFP was then buffer exchanged into 20 mM Tris pH 8.0, 150 mM NaCl using a PD-10
TM
Sephadex column (GE Healthcare), concentrated, and treated with glycerol (10% v/v final
O concentration). These solutions were stored at -80 C until further use. Protein concentration was estimated by UV -vis spectroscopy using the absorbance of eGFP at 488 nm (extinction
-1 -! 7 coefficient 55,900 M cm ).
[00442] UCHL3 and dual labeling UCHL3 substrate. UCHL3 containing a single N- g terminal glycine residue was produced in E. coli as described previously. This construct (in pET28a+, Novagen) was then used to prepare the dual labeling UCHL3 substrate. Synthetic 5'-phosphorylated oligonucleotide duplexes containing appropriate sticky ends were designed to achieve insertion of an N-terminal thrombin site and a C-terminal LPETG sequence separated from UCHL3 by a GGGGSGGGGS spacer in two sequential cloning steps. Duplexes were annealed before ligation into the parent vector. The C-terminal insertion was performed first using the Pstl and Xhol restriction sites. The result of using the Xhol site was the addition of a His6-tag after the LPETG sequence. The N-terminal insertion was then achieved using the Xbal and Ndel restriction sites. This plasmid was then transformed into E. coli BL21. Cells were grown in sterile LB containing kanamycin (30 μg/mL) to an optical density of -0.6-0.9 at 600 nm.
[00443] Cells were induced with IPTG (1 mM) for 3 h at 37 C. Bacteria were then
O harvested by centrifugation and the pellet was stored overnight at -20 C. The pellet was thawed and resuspended in 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40. The cell suspension was then lysed by French press and centrifuged. The clarified lysate was then applied to a Ni-NTA column consisting of 5.0 mL of commercial Ni-NTA slurry (Qiagen) equilibrated with 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40. The column was washed with 40 mL of 20 mM Tris pH 8.0, 150 mM NaCl, 20 mM imidazole and 1% NP-40, followed by 40 mL of 20 mM Tris pH 8.0, 150 mM NaCl, and 20 mM imidazole. Protein was eluted with 20 mM Tris pH 8.0, 150 mM NaCl, and 300 mM imidazole. This material was then purified by anion-exchange chromatography on a Mono Q 5/50 GL column (Amersham) [Buffer A (50 mM Tris pH 7.5, 5 mM DTT, 0.5 mM EDTA), Buffer B (50 mM Tris pH 7.5, 5 mM DTT, 0.5 mM EDTA, 500 mM NaCl), 1.5 mL/min, gradient: 100% Buffer A (0-15 mL), 0% Buffer B → 50% Buffer B (15-45 mL), 50% Buffer B (45-50 mL)]. Fractions containing UCHL3 were pooled and further purified by size exclusion chromatography on a HiLoad 16/60 Superdex 75 column (Amersham), eluting with 20 mM Tris pH 8.0, 150 mM NaCl at a flow rate of 1 mL/min. Fractions containing UCHL3 were pooled and subjected to a final purification step by anion-exchange chromatography on a Mono Q 5/50 GL column (Amersham) [Buffer A (50 mM phosphate pH 6.0), Buffer B (50 mM phosphate pH 6.0, 500 mM NaCl), 1.5 mL/min, gradient: 100% Buffer A (0-15 mL), 0% Buffer B → 50% Buffer B (15-45 mL), 50% Buffer B (45-50 mL)]. The dual labeling UCHL3 substrate was buffer exchanged into 20 mM Tris pH 8.0, 150 NaCl and protein concentration was estimated by Bradford assay.
[00444] N-terminal labeling. N-terminal transpeptidation reactions were performed by combining the necessary proteins/reagents at the specified concentrations in the presence of SrtAstaph or Δ59-SrtAstaph in sortase reaction buffer (50 mM Tris pH 7.5, 150 mM NaCl, 10 mM CaC12) and incubating at 37 °C for the times indicated. Reactions were either diluted with 2x reducing Laemmli sample buffer for SDSPAGE analysis or diluted with water (~50 fold) for ESI-MS analysis. Gels were visualized by staining with coomassie blue. Fluorescence was visualized on a Typhoon 9200 Imager (GE Healthcare). For detection of biotinylation, proteins were separated by SDS-PAGE and transferred to a nitrocellulose membrane. The membrane was then probed with a streptavidin-horseradish peroxidase conjugate (GE Healthcare) and visualized by chemiluminescence. ESI-MS was performed on a Micromass LCT mass spectrometer (Micromass® MS Technologies, USA) and a Paradigm MG4 HPLC system equipped with a HTC PAL autosampler (Michrom BioResources, USA) and a Waters Symmetry 5 m C8 column (2.1 x 50 mm, MeCN:H2O (0.1% formic acid) gradient mobile phase, 150 L/min).
[00445] Dual labeling ofeGFP . Immediately prior to starting the dual labeling sequence, the eGFP stock was thawed and again purified by affinity chromatography over commercial Ni-NTA resin. After binding eGFP to the resin, the column was washed with 20 mM Tris pH 8.0, 150 mM NaCl, and 20 mM imidazole. The protein was eluted with 20 mM Tris pH 8.0, 150 mM NaCl, and 300 mM imidazole. This material was buffer exchanged into 20 mM Tris
TM TM pH 8.0, 150 mM NaCl using a NAP 5 Sephadex column (GE Healthcare) and concentrated. The concentration was estimated to be 84 M by UV-vis spectroscopy using
-1 -1 7 eGFP absorbance at 488 nm (extinction coefficient 55,900 M cm ).
[00446] C-terminal modification ofeGFP with 3 and SrtAstrep. 400 L of the freshly purified eGFP solution was then treated with SrtAstrep (87 L of a 140 M stock solution) and
2+ 3
3 (4.9 L of a 100 mM stock solution) [Note: SrtAstrep does not require Ca for activity].
O
The reaction was incubated for 7 h at 37 C. ESIMS analysis of the crude reaction mixture revealed excellent conversion to the desired product (Supporting Figure S6a). The reaction was then treated with [2-(trimethylammonium)ethly] methane thiosulfonate bromide (MTSET) (2.5 L of a 500 mM solution in 1 :1 DMSO/H2O) for 10 min at room temperature to quench SrtAstrep. The entire reaction was then diluted with 5 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole. This solution was then passed over a 1.5 mL column of Ni-NTA that been equilibrated with 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole. The column was then washed with 1.5 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole. His6-tagged SrtAstrep was bound by Ni-NTA while the eGFP product (which lost its His6 tag during the course of transpeptidation) was not retained. The eGFP
TM solution was then concentrated and passed over a PD-10 Sephadex desalting column (equilibrated with 20 mM Tris pH 8.0, 150 mM NaCl) to remove excess 3. This material was concentrated to ~800 L and subjected to thrombin cleavage.
[00447] Thrombin cleavage of eGFP. All 800 uL of the solution described above was combined with 100 L of 10x cleavage buffer and 100 L of thrombin agarose beads (from
TM o
Thrombin CleanCleave Kit, Sigma). This mixture was incubated for 1 h at 37 C, and then checked by ESI-MS to ensure quantitative cleavage (Figure 35). The reaction was then filtered to remove the thrombin beads.
[00448] Η -terminal labeling of eGFP with 1 and 59-SrtAstaph. 389 L of the thrombin cleaved material was combined with 1 (25 L of a 10 mM DMSO solution), 59-SrtAstaph (36 L of a 700 M stock solution), and 10x sortase reaction buffer (50 L of 500 mM Tris pH 8.0,
1.5 M NaCl, 100 mM CaC12). The reaction was incubated for 75 min at 37 C. ESI-MS of the crude reaction mixture showed clean formation of the dual labeled product as the major reaction product (Supporting Figure S6a). The reaction was then diluted with 5 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole. This solution was passed over a 1.5 mL column of Ni-NTA that been equilibrated with 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole in order to remove His6-tagged 59-SrtAstaph. 2.5 mL of this eluate was then
TM passed over a PD-10 Sephadex desalting column (equilibrated with 20 mM Tris pH 8.0). This material was then purified by anion-exchange chromatography on a Mono Q 5/50 GL column (Amersham) [Buffer A (20 mM Tris pH 8.0), Buffer B (20 mM Tris pH 8.0, 1 M NaCl), 1.5 mL/min, gradient: 100% Buffer A (0-15 mL), 0% Buffer B → 50% Buffer B (15- 45 mL), 50% Buffer B (45-50 mL)]. Fractions containing dual labeled eGFP were pooled and analyzed by SDS-PAGE and ESI-MS. Coomassie stained gels were imaged using a CanoScan 8600F scanner. Protein purity was estimated from these images using ImageJ 1.42q densitometry software. [00449] Dual labeling of UCHL3 [00450] C-terminal modification of UCHL3 with 3 and SrtAstrep. UCHL3 (350 L of a 65 M stock solution) was treated with SrtAstrep (76 L of a 140 M stock solution) and 3 (4.3 L of
2+ 3 a 100 mM stock solution) [Note: SrtAstrep does not require Ca for activity]. The reaction
O was incubated for 15 h at 37 C. ESIMS analysis of the crude reaction mixture revealed excellent conversion to the desired product (Supporting Figure S6b). The entire reaction was then diluted with 5 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole. This solution was then treated with [2-(trimethylammonium)ethly] methane thiosulfonate bromide (MTSET) (5.0 L of a 500 mM solution in 1:1 DMSO/H2O) for 10 min at room temperature to quench SrtAstrep. [Note: UCHL3 contains an active site cysteine residue and is therefore modified by MTSET. The resulting modification is disulfide linked, and is easily removed by treatment with DTT following completion of the dual labeling procedure]. The diluted reaction solution was then passed over a 1.5 mL column of Ni-NTA that been equilibrated with 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole. The column was then washed with 1.5 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole. The
TM
UCHL3 solution was then concentrated and passed over a PD-10 Sephadex desalting column (equilibrated with 20 mM Tris pH 8.0, 150 mM NaCl) to remove excess 3. This material was concentrated to 1 mL and subjected to thrombin cleavage. [00451] Thrombin cleavage ofUCHL3. All 1 mL of the solution described above was combined with 100 L of 10x cleavage buffer and 100 L of thrombin agarose beads (from
TM
Thrombin CleanCleave Kit, Sigma). This mixture was incubated for 1 h at 37 degrees C, and then checked by ESI-MS to ensure quantitative cleavage (Figure 35). The reaction was then filtered to remove the thrombin beads.
[00452] N-terminal labeling of UCHL3 with 1 and 59-SrtAstaph. 778 L of the thrombin cleaved material was combined with 1 (50 L of a 10 mM DMSO solution), 59-SrtAstaph (72 L of a 700 M stock solution), and 10x sortase reaction buffer (100 L of 500 mM Tris pH 8.0,
1.5 M NaCl, 100 mM CaC12). The reaction was incubated for 60 min at 37 C. ESI-MS of the crude reaction mixture showed clean formation of the dual labeled product as the major reaction product (Supporting Figure S6b). The reaction was then diluted with 5 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole. This solution was passed over a 1.5 mL column of Ni-NTA that been equilibrated with 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole in order to remove His6-tagged 59-SrtAstaph. The column was then washed with 2.0 mL of 20 mM Tris pH 8.0, 500 mM NaCl, and 20 mM imidazole. The eluate was TM then desalted using PD-IO Sephadex columns (equilibrated with 20 mM Tris pH 8.0). This material was then purified by anion-exchange chromatography on a Mono Q 5/50 GL column (Amersham) [Buffer A (20 mM Tris pH 8.0), Buffer B (20 mM Tris pH 8.0, 1 M NaCl), 1.5 mL/min, gradient: 100% Buffer A (0-15 mL), 0% Buffer B → 50% Buffer B (15-45 mL), 50% Buffer B (45-50 mL)]. Fractions containing dual labeled UCHL3 were pooled and analyzed by SDS-PAGE and ESI-MS. Prior to ESIMS, dual labeled UCHL3 was treated with 10 mM DTT for 10 min at RT to remove the MTSET modification on the active site cysteine residue. Coomassie stained gels were imaged using a CanoScan 8600F scanner. Protein purity was estimated from these images using ImageJ 1.42q densitometry software. [00453] Results
[00454] We synthesized FITC (1) and biotin (2) derivatives of an LPRT peptide in which the glycine of the normal LPXTG motif was replaced by a methyl ester (Figure 32; see also Example 2). With the ability of SrtAstaph to append labels at either terminus, as described herein (see, e.g., Example 2), we pursued the possibility of installing two modifications within the same protein. Attempts to execute this type of transformation using SrtAstaph alone failed to yield desired levels of product, due to intramolecular transpeptidation between N- terminal glycines and the C-terminal LPXTG motif that occurred in most cases. Therefore, we considered the possibility of using a second, distinct sortase. We initially sought to use sortase B (SrtB) from either Staph, aureus or Bacillus anthracis as enzymes with recognition sequences (NPQTN and NPKTG, respectively) orthogonal to that of SrtAstaph.(9, 10). Both SrtB enzymes were easily produced in Escherichia coli and purified to homogeneity. We reproduced the reported in vitro enzyme activity using a FRET-based assay to measure cleavage of short peptides substrates (9, 10). However, we did not obtain transpeptidation with either SrtB on protein substrates modified with the appropriate recognition sequences on a time scale or with yields that compare favorably with SrtAstaph (data not shown). [00455] We ultimately arrived at a more successful orthogonal strategy using SrtAstrep, which recognizes the same LPXTG sequence used by SrtAstaph but can accept alanine-based nucleophiles (11) This leads to the formation of an LPXTA sequence at the site of ligation, a motif refractory to cleavage by SrtAςlaph.(12) This allows SrtAstaph to act on the N terminus without affecting the C-terminal modification installed with SrtAstrep- An exemplary strategy for dual-terminus labeling is outlined in Figures 33b and 34. We first synthesized a tetramethylrhodamine-labeled peptide (3) containing two N-terminal alanine residues to serve as the nucleophile for SrtAstrep-mediated protein ligation (Figure 33a). We prepared two model substrates (eGFP and UCHL3) containing masked N-terminal glycines that are exposed only upon thrombin cleavage. Masking was required because SrtAstrep was observed to ligate both glycine and alanine nucleophiles (data not shown). Substrates also contained an LPXTG motif at the C terminus to allow a first round of labeling with SrtAstrep. For both eGFP and UCHL3, C-terminal labeling using 3 and SrtAstrep resulted in >90% conversion to the desired adduct, as revealed by ESI-MS (Figure 35). SrtAstrep was quenched by the addition of MTSET followed by removal of His6-tagged SrtAstrep using Ni-NTA. Residual 3 was then removed using a disposable desalting column. Thrombin cleavage proceeded in quantitative fashion using commercial thrombin agarose resin (Figure 35). The exposed N-terminal glycines were then labeled by treatment with 500 μM 1 and 50 μM Δ59-SrtAstaph£i3) for -1 h at 37 °C. ESI-MS of crude reaction mixtures showed the dual-labeled material as the major component, with only minor amounts of byproduct (Figure 35). A final separation by anion- exchange chromatography yielded dual-labeled eGFP and UCHL3 with excellent purity, as determined by both SDS-PAGE and ESI-MS (Figure 34 and Figure 35). In the case of UCHL3, we observed some additional low- intensity bands in the fluorescent gel scan (Figure 33). However, quantitative densitometric analysis of coomassie-stained gels indicated purity in excess of 95% for both dual-labeled eGFP and UCHL3. [00456] References for Example 4
[00457] (1) Zumbuehl, A.; Jeannerat, D.; Martin, S. E.; Sohrmann, M.; Stano, P.; Vigassy,
T.; Clark, D. D.; Hussey, S. L.; Peter, M.; Peterson, B. R.; Pretsch, E.; Walde, P.; Carreira, E.
M. Angew Chem Int Ed Engl 2004, 43, 5181-5.
[00458] (2) Kottani, R.; Valiulin, R. A.; Kutateladze, A. G. Proc Natl Acad Sci USA
2006, 103, 13917-21.
[00459] (3) Race, P. R.; Bentley, M. L.; Melvin, J. A.; Crow, A.; Hughes, R. K.; Smith,
W. D.; Sessions, R. B.; Kehoe, M. A.; McCafferty, D. G.; Banfield, M. J. J Biol Chem 2009,
284, 6924-33.
[00460] (4) Ton-That, H.; Liu, G.; Mazmanian, S. K.; Faull, K. F.; Schneewind, O. Proc.
Natl. Acad ScL U.S.A. 1999, 96, 12424-9.
[00461] (5) Jobling, M. G.; Palmer, L. M.; Erbe, J. L.; Holmes, R. K. Plasmid 1997, 38,
158-73.
[00462] (6) Antos, J. M.; Miller, G. M.; Grotenbreg, G. M.; Ploegh, H. L. JAm Chem Soc
2008, 130, 16338-43.
[00463] (7) Tsien, R. Y. Annu. Rev. Biochem. 1998, 67, 509-544. [00464] (8) Popp, M. W.; Artavanis-Tsakonas, K.; Ploegh, H. L. Journal of Biological
Chemistry 2008, 284, 3593-3602.
[00465] (9) Maresso, A. W., Chapa, T. J. and Schneewind, O. J. Bacteriol 2006, 188,
8145- 8152
[00466] (10) Mazmanian, S. K., Ton-That, H., Su, K. and Schneewind, O. Proc. Natl.
Acad. Sci. U.S.A. 2002, 99, 2293- 2298
[00467] (11) Race, P. R., Bentley, M. L., Melvin, J. A., Crow, A., Hughes, R. K., Smith,
W. D., Sessions, R. B., Kehoe, M. A., McCafferty, D. G. and Banfield, M. J. J. Biol. Chem.
2009, 284, 6924- 6933
[00468] (12) Kruger, R. G., Otvos, B., Frankel, B. A., Bentley, M., Dostal, P. and
McCafferty, D. G. Biochemistry 2004, 43, 1541- 1551
[00469] (13) Δ59-SrtAstaPh is a truncated form of SrtAstaph that has identical reactivity
[00470]
Example 5: Site-Specific PEGylation Using SrtAstaph
[00471] This example describes PEGylation of the four-helix bundle cytokine interferon α at the C-terminus using sortase and demonstrates that the PEGylated version retains activity and has enhanced in vivo circulating time. We cloned into the pET28a+ vector (Novagen) a version of interferon alpha lacking the leader sequence and fused to LPETGG, the SrtAstaph recognition site, separated from the body of the protein by two glycines (Fig 39A). For purification, we added a 6-His tag following the SrtAstaph cleavage site; this tag is lost upon transpeptidation. We expressed this protein in Rosetta-gami(DE3)pLysS cells (Novagen) and purified soluble protein by Ni-NTA IMAC chromatography (Qiagen), followed by size exclusion chromatography on a Superdex 75 column (GE) at pH 5.0. [00472] We constructed a GIy3K-PEG(IOkDa) nucleophile compatible with SrtAstaph • The GIy3K peptide scaffold was constructed by standard Fluorenylmethoxycarbonyl (Fmoc) solid phase peptide chemistry on rink amide resin. Fmoc protected peptide was liberated from the resin by treatment with 95% TFA/3%TIPS/2%H2O, precipitated with cold ether and lyophilized. Methyl-capped 10 kDa PEG succinimidyl ester (1 equivalent, Nanocs) was mixed with peptide (2equivalents), 1 equivalent N-hydroxysuccinimide (NHS, Sigma) and 1 equivalent l-ethyl-3-(3-dimethylaminopropyl) carbodiimide (EDC, Pierce) in N- Methylpyrrolidone (NMP, Fluka) for 24 hours at room temperature, followed by precipitation in cold ether. The resulting solid was resuspended in 20% piperidine/NMP for 30 minutes, followed by re-precipitation in cold ether. This material was resuspended in
H2O and dialyzed extensively against H2O to remove free peptide.
[00473] Sortase labeling was conducted as described previously (see, e.g., other Examples herein). PEGylated protein was purified by cation exchange chromatography on a Mono-S column (GE) at pH 5.0 or 4.5. Protein concentrations were measured by the Bradford method.
[00474] To compare in-vitro activity of interferon alpha conjugates, a standard Daudi cell proliferation inhibition assay was used. The site-specifically PEGylated interferon alpha conjugate is extremely potent in inhibiting Daudi cell proliferation (Fig. 40, Table C), despite conjugation to the large 1OkDa PEG chain. The PEG moiety, positioned away from the receptor binding site prolongs the time the interferon alpha conjugate spends in circulation, as assessed by ELISA performed on mice injected with lOμg of interferon alpha, followed by retro-orbital collection of serum at different time points (Fig. 41). Thus, by PEGylating interferon alpha at a site distant from the receptor binding site, we can extend the circulating half-life with minimal sacrifice in potency.
[00475] Table C*: Inhibition of Daudi cell proliferation by IFNα and IFNα variants
Figure imgf000145_0001
[00476] * See Figs. 39 and 40 legend for details regarding the IFNα2 sequences [00477] As described herein, we have extended the sortase methodology to N-terminal labeling. Since the N-terminus lies in close proximity to the C-terminus in four-helix bundle cytokines, we expect PEG conjugation using N-terminal probes (e.g., Fig. 47) to yield similar results.
Example 6: Sortase-Mediated Circularization of IFNα
[00478] We have shown that proteins bearing an LPXTG motif at the C-terminus and an N-terminal glycine can be covalently cyclized after incubation with sortase A, provided that the N and C terminus are in close apposition to one another, as they are in the four helix bundle cytokines. We constructed an interferon alpha variant by inserting two glycine residues between the initiating methionine and the body of the interferon alpha sequence used for PEGylation (Fig. 39A). When incubated with sortase, this protein cyclizes, as shown unambiguously by MS/MS sequence identification of the junction peptide between the N and C-termini following chymotrypsin digestion (Fig. 39B). The circular interferon alpha was purified by cation exchange chromatography and tested in the cell based interferon alpha activity assay. Again, the engineered protein is as potent as the recombinant standard (Fig 40, Table C).
[00479] To test the thermal stability of the circular protein, we turned to a dye-based thermal denaturation assay, Thermofluor. When denatured, proteins expose hydrophobic residues that bind to and increase fluorescence of the dye Sypro Orange (Invitrogen). The circular interferon alpha has a significantly higher Tm than any other variant tested (Fig 42). We conclude that covalently clamping the termini of interferon alpha together stabilizes the protein by preventing premature fraying of the ends, without sacrificing activity.
Example 7: Circular Site-specfically PEGylated Proteins
[00480] Combining the insertion of a non-genetically encoded PEG moiety at the terminus of interferon alpha and subsequently joining the resulting termini will impart both increased circulating half-life and thermal stability. This is accomplished by two subsequent transacylation steps (Fig. 43), the first joining a peptide bearing the PEG moiety as well as another distinct sortase recognition element to the candidate protein. The second transacylation step is accomplished by a different sortase and results in covalent closure of the protein. However, because the sortase reactions are equilibrium reactions and the sortases SrtAstrep and SrtAstaph are orthogonal in one direction only (SrtAstrep cleaves both LPXTG and LPXTA sites but SrtAstaph attacks only LPXTG), we sought to render the sortase cleavage site on the nucleophile refractory to cleavage during the initial installation of the probe. To that end, we have generated a nucleophile bearing an LPXtG sequence, where t is a phosphorylated threonine residue. Based on the crystal structures of SrtAstaph and SrtAstrep, phosphothreonine will not fit into the substrate recognition groove. Thus, the first transpeptidation step can be accomplished without premature cleavage of the SrtAstaph site on the PEG nucleophile. The resulting conjugate can then be dephosphorylated and incubated with SrtAstaph (which will not cleave the LPETAA junction between the protein and nucleophile) to join the termini.
[00481] Our experiments demonstrate the feasibility of this scheme. We installed a peptide bearing an N-terminal AA sequence (compatible with SrtAstrep) followed by a lysine for conjugating to a non-genetically encoded moiety of choice, an LPEtG SrtAstaph cleavage site, and a hexahistidine epitope tag onto interferon alpha (Fig. 43). The reaction product was confirmed by LC ESI-MS. We then dephosphorylated the protein by incubating with Antarctic phosphatase (NEB), exposing the SrtAstaph cleavage site. This site is competent to undergo the second transacylation step; we installed a triglycine nucleophile onto this site by incubating with SrtAstaph and GIy3 peptide (Sigma) (Fig. 44). Thus, we can accomplish two successive transacylation steps by controlling the accessibility of two orthogonal sortase enzymes to their respective cleavage sites.
Example 8: Sortase-Mediated Installation of a Non-Genetically Encoded Element Between Two Proteins
[00482] The strategy described in Example 7 can be used to install a non-genetically encoded element between two proteins or protein domains as shown, e.g., in Fig. 45. A specific example is the construction of a cytokine variant joined to the Fc region of an antibody, with a non-genetically encoded moiety in the intervening region. Genetic fusions of cytokines to Fc regions can be delivered non-invasively into the bloodstream by Fc receptor bearing epithelial cells in the lungs, after which the half-life of the molecule is prolonged. Implicit in this mechanism is the requirement for an Fc region that is able to bind to its cognate Fc receptor, and thus chemical conjugation of a molecule to the C-terminus or an internal lysine of the Fc portion would likely decrease binding capacity. Using two transacylation steps, we will install a PEG moiety onto the C-terminus of the cytokine portion, followed by installation of an unhindered Fc region. Such a conjugate may show even greater gains in half-life relative to the genetic Fc fusion, as kidney filtration of the molecule is predicted to be further reduced. Other applications include installing a detectable label, e.g., for diagnostic purposes or to monitor the distribution or elimination of the molecule in vivo. [00483]
[00484] The foregoing written specification is considered to be sufficient to enable one skilled in the art to practice the invention. The present invention is not to be limited in scope by examples provided, since the examples are intended as a single illustration of one aspect of the invention and other functionally equivalent embodiments are within the scope of the invention. Various modifications of the invention in addition to those shown and described herein will become apparent to those skilled in the art from the foregoing description and fall within the scope of the appended claims. The advantages and objects of the invention are not necessarily encompassed by each embodiment of the invention.

Claims

CLAIMSWhat is claimed is:
1. A method of ligation comprising the step of contacting an acyl donor compound of formula:
Figure imgf000148_0001
wherein the transamidase recognition sequence is any peptide motif recognized by a transamidase enzyme; X is -0-, -NR-, or -S-; R is hydrogen, substituted or unsubstituted aliphatic, or substituted or unsubstituted heteroaliphatic; A1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; R1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, or substituted or unsubstituted heteroaryl; and with a nucleophilic compound of formula:
Figure imgf000148_0002
wherein
B1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; and n is an integer from O to 6, inclusive; in the presence of a transamidase enzyme under suitable conditions to form a compound of formula:
Figure imgf000149_0001
2. The method of claim 1, wherein X is -O-.
3. The method of claim 1 , wherein the recognition sequence is LPXT, wherein the X of the recognition sequence is any natural or unnatural amino acid.
4. The method of claim 3, wherein the recognition sequence is LPXT, wherein the X of the recognition sequence is D, E, A, N, Q, K, or R.
5. The method of claim 1, wherein the recognition sequence is selected from LPXT, SPXT, LAXT, LSXT, NPXT, VPXT, IPXT, and YPXR wherein the X of the recognition sequence is a natural or unnatural amino acid.
6. The method of claim 1, wherein the recognition sequence is selected from: LPKT, LPIT, LPDT, SPKT, LAET, LAAT, LAET, LAST, LAET, LPLT, LSRT, LPET, VPDT, IPQT, YPRR, LPMT, LPLT, LAFT, LPQT, NSKT, NPQT, NAKT, and NPQS.
7. The method of claim 1, wherein the recognition sequence is XiPX2X3, where Xi is leucine, isoleucine, valine or methionine; X2 is any amino acid; X3 is threonine, serine or alanine; P is proline.
8. The method of claim 7 wherein the transamidase is sortase A.
9. The method of claim 1, wherein the recognition sequence NPXiTX2, where Xi is glutamine or lysine; X2 is asparagine or glycine; N is asparagine; P is proline and T is threonine.
10. The method of claim 9, wherein the transamidase is sortase B.
11. A method of ligation comprising the step of contacting an acyl donor compound of formula:
Figure imgf000150_0001
wherein
A1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; X is -O-, -NR-, or -S-; R is hydrogen, substituted or unsubstituted aliphatic, or substituted or unsubstituted heteroaliphatic; R1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, or substituted or unsubstituted heteroaryl; and
R2 is a natural or unnatural amino acid side chain; with a nucleophilic compound of formula:
Figure imgf000150_0002
wherein
B1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; and n is an integer from 0 to 100, inclusive; in the presence of a transamidase enzyme under suitable conditions to form a compoundormula:
Figure imgf000151_0001
12. The method of claim 11 , wherein X is -O-.
13. The method of claim 11 , wherein X is -NR-.
14. The method of claim 11, wherein X is -NH-.
15. The method of claim 11, wherein X is -S-.
16. The method of claim 11 , wherein R1 is substituted or unsubstituted aliphatic.
17. The method of claim 16, wherein R1 is substituted aliphatic.
18. The method of claim 16, wherein R1 is unsubstituted aliphatic.
19. The method of claim 16, wherein R1 is Ci-I2 aliphatic.
20. The method of claim 19, wherein R1 is Ci-6 aliphatic.
21. The method of claim 20, wherein R1 is butyl.
22. The method of claim 20, wherein R1 is propyl.
23. The method of claim 20, wherein R1 is ethyl.
24. The method of claim 20, wherein R1 is methyl.
25. The method of claim 11, wherein R1 is substituted or unsubstituted aryl.
26. The method of claim 25, wherein R1 is substituted or unsubstituted phenyl.
27. The method of claim 12, wherein R1 is substituted or unsubstituted aliphatic.
28. The method of claim 27, wherein R1 is substituted aliphatic.
29. The method of claim 27, wherein R1 is unsubstituted aliphatic.
30. The method of claim 27, wherein R1 is CM2 aliphatic.
31. The method of claim 27, wherein R1 is C^ aliphatic.
32. The method of claim 31 , wherein R1 is butyl.
33. The method of claim 31 , wherein R1 is propyl.
34. The method of claim 31 , wherein R1 is ethyl.
35. The method of claim 31 , wherein R1 is methyl.
36. The method of claim 12, wherein R1 is substituted or unsubstituted aryl.
37. The method of claim 36, wherein R1 is substituted or unsubstituted phenyl.
38. The method of claim 11, wherein R2 is a natural amino acid side chain.
39. The method of claim 38, wherein R2 is the side chain group of aspartic acid, glutamic acid, alanine, asparagine, glutamine, lysine, or arginine.
40. The method of claim 39, wherein R2 is the side chain group of arginine.
41. The method of claim 39, wherein R2 is the side chain group of glutamic acid.
42. The method of claim 39, wherein R2 is the side chain group of lysine.
43. The method of claim 11, wherein R2 is an unnatural amino acid side chain.
44. The method of claim 11, wherein A1 is an amino acid.
45. The method of claim 11 , wherein A1 is a protein or peptide.
46. The method of claim 45, wherein A1 is green fluorescent protein.
47. The method of claim 45, wherein A1 is selected from the group consisting of an antibody, an antibody chain, an antibody fragment, an antibody epitope, a recombinant protein, a peptide comprising one or more D-amino acids, a branched peptide, a therapeutic protein, an enzyme, a polypeptide subunit of a multisubunit protein, a transmembrane protein, a cell surface protein, a methylated peptide or protein, an acylated peptide or protein, a lipidated peptide or protein, a phosphorylated peptide or protein, and a glycosylated peptide or protein.
48. The method of claim 11 , wherein A1 is a lipid.
49. The method of claim 48, wherein A1 is a saturated hydrocarbon.
50. The method of claim 49, wherein A1 is a Ci-40 hydrocarbon chain.
51. The method of claim 48, wherein A1 is adamantyl.
52. The method of claim 11, wherein A1 is a bioactive small molecule.
53. The method of claim 11, wherein A1 is steroid or analog thereof.
54. The method of claim 11, wherein A1 is a label.
55. The method of claim 54, wherein A1 comprises a fluorescent label, a radiolabel, a chemiluminescent label, or a phosphorescent label.
56. The method of claim 54, wherein A1 is biotin, streptavidin, or fluorescein.
57. The method of claim 1 1 , wherein B1 is a protein or peptide.
58. The method of claim 57, wherein B1 is green fluorescent protein.
59. The method of claim 1 1, wherein B1 is selected from the group consisting of an antibody, an antibody chain, an antibody fragment, an antibody epitope, a recombinant protein, a peptide comprising one or more D-amino acids, a branched peptide, a therapeutic protein, an enzyme, a polypeptide subunit of a multisubunit protein, a transmembrane protein, a cell surface protein, a methylated peptide or protein, an acylated peptide or protein, a lipidated peptide or protein, a phosphorylated peptide or protein, and a glycosylated peptide or protein.
60. The method of claim 1 1, wherein B1 is a lipid.
61. The method of claim 11 , wherein B1 is a saturated hydrocarbon.
62. The method of claim 1 1, wherein B1 is a C MO hydrocarbon chain.
63. The method of claim 11, wherein B1 is adamantyl.
64. The method of claim 11, wherein B1 is a bioactive small molecule.
65. The method of claim 11, wherein B1 is a steroid or analog thereof.
66. The method of claim 11, wherein B1 is a label.
67. The method of claim 66, wherein B1 comprises a fluorescent label, a radiolabel, a chemiluminescent label, or a phosphorescent label.
68. The method of claim 66, wherein B1 is biotin, streptavidin, or fluorescein.
69. The method of claim 11, wherein n is 0.
70. The method of claim 11 , wherein n is 1.
71. The method of claim 11 , wherein n is 2.
72. The method of claim 11 , wherein n is 3.
73. The method of claim 11 , wherein n is 4.
74. The method of claim 11, wherein the acyl compound is of formula:
Figure imgf000154_0001
75. The method of claim 74, wherein the acyl compound is of formula:
Figure imgf000154_0002
76. The method of claim 75, wherein the acyl compound is of formula:
Figure imgf000155_0001
77. The method of claim 76, wherein the acyl compound is of formula:
Figure imgf000155_0002
78. The method of claim 76, wherein the acyl compound is of formula:
Figure imgf000155_0003
79. The method of claim 76, wherein the acyl compound is of formula:
Figure imgf000155_0004
80. The method of claim 11, wherein the transamidase enzyme is a sortase.
81. The method of claim 80, wherein the sortase is sortase A.
82. The method of claim 80, wherein the sortase is sortase B.
83. The method of claim 81, wherein the sortase A further comprises an affinity tag.
84. The method of claim 1 or 1 1, wherein the suitable conditions comprise pH in the range of 6 to 8.5.
85. The method of claim 84, wherein the suitable conditions comprise pH in the range of 7.3 to 7.8.
86. The method of claim 1 or 11, wherein the suitable conditions include a buffer solution comprising calcium ions.
87. The method of claim 1 or 11, wherein the ligation is performed at a temperature ranging from about 15 0C to about 50 0C.
88. The method of claim 1 or 11, wherein the ligation is performed at a temperature ranging from about 23 0C to about 37 0C.
89. The method of claim 1 or 11, wherein the acyl donor is present in a concentration ranging from about 100 μM to about 5 mM.
90. The method of claim 89, wherein the acyl donor is present in a concentration ranging from about 400 μM to about 600 μM.
91. The method of claim 1 or 11, wherein the nucleophilic acyl acceptor is present in a concentration ranging from about 15 μM to about 150 μM.
92. The method of claim 91, wherein the nucleophilic acyl acceptor is present in a concentration ranging from about 40 μM to about 60 μM.
93. The method of claim 1 or 11 , wherein the transamidase is a sortase present in a concentration ranging from about 15 μM to about 150 μM.
94. The method of claim 93, wherein the sortase is present in a concentration ranging from about 40 μM to about 60 μM.
95. A compound of formula:
Figure imgf000157_0001
wherein
A1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; X is -O-, -NR-, or -S-; R is hydrogen, substituted or unsubstituted aliphatic, or substituted or unsubstituted heteroaliphatic; R1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, or substituted or unsubstituted heteroaryl; and R2 is a natural or unnatural amino acid side chain.
96. An acyl compound of formula:
O
.1— Transamidase recognition sequence XR1 wherein the transamidase recognition sequence is any peptide motif recognized by a transamidase enzyme; X is -O-, -NR-, or -S-; A1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; and R1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, or substituted or unsubstituted heteroaryl.
97. A kit comprising a compound of claim 95 or 96.
98. A compound obtained by performing a transamidase-mediated reaction in which the compound of claim 95 or 96 is reacted with a nucleophile, wherein either (i) Al is not a polypeptide or (ii) the nucleophile is not a polypeptide.
99. The compound of claim 98, wherein either (i) Al does not comprise a polypeptide or (ii) the nucleophile does not comprise a polypeptide.
100. The compound of claim 98 or 99, wherein the transamidase is a sortase.
101. The kit of claim 95, further comprising a transamidase.
102. The kit of claim 101, wherein the transamidase is a sortase.
103. The kit of claim 102, wherein the sortase is sortase A.
104. A kit comprising a nucleophilic compound of formula:
Figure imgf000158_0001
wherein
B1 acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; and n is an integer from 0 to 100, inclusive.
105. The kit of claim 104, further comprising instructions for ligation with a nucleophilic compound.
106. The kit of any of claims 95, 96, 97, 101, 102, 103, 104, 105, further comprising at least one item selected from the group consisting of: buffers, material(s) for removing the transamidase from a reaction.
107. A transgenic, non-human animal comprising cells whose genome comprises a DNA segment comprising a portion that encodes a polypeptide of interest and a portion that encodes a sortase recognition motif.
108. The transgenic non-human animal of claim 107, wherein the sortase recognition motif has a sequence selected from the group consisting of: LPXTG, LPXTA, SPXTG, LAXTG, LSXTG, NPXTX, NPXTA, NPXTG, VPXTG, IPXTG, YPXRG, LPXTS, wherein X is a standard or non-standard amino acid.
109. The transgenic non-human animal of claim 107, wherein X is a standard amino acid.
110. The transgenic non-human animal of claim 107, wherein X is selected to match a naturally occurring sortase recognition motif.
111. The transgenic non-human animal of claim 107, wherein the sortase recognition motif has a sequence selected from the group consisting of: LPKTG, LPITG, LPDTA, SPKTG, LAETG, LAATG, LAHTG, LASTG, LAETG, LPLTG, LSRTG, LPETG, VPDTG, IPQTG, YPRRG, LPMTG, LPLTG, LAFTG, LPQTS, NSKTA, NPQTG, NAKTN, and NPQSS.
1 12. The transgenic non-human animal of claim 107, wherein the sortase recognition motif has a sequence LPXTG.
113. The transgenic non-human animal of claim 107, wherein the DNA segment encodes a polypeptide in which the C-terminal amino acid residue of the sortase recognition motif is joined to the N-terminal amino acid residue of the polypeptide of interest.
114. The transgenic non-human animal of claim 107, wherein the DNA segment encodes a polypeptide in which the N-terminal amino acid of the sortase recognition motif is joined to the C-terminal amino acid residue of the polypeptide of interest.
115. The transgenic non-human animal of claim 107, wherein the DNA segment encodes a polypeptide in which the sortase recognition motif is located within the polypeptide of interest.
1 16. The transgenic non-human animal of claim 107, wherein the DNA segment further comprises a portion that encodes a spacer peptide between 1 and 50 amino acids long, wherein the portion that encodes the spacer peptide is located between the portion that encodes the sortase recognition motif and the portion that encodes the polypeptide of interest.
117. The transgenic non-human animal of claim 107, wherein the animal is a mouse.
118. The transgenic non-human animal of claim 107, wherein the animal is a chicken.
119. The transgenic non-human animal of claim 107, wherein the polypeptide of interest comprises an immunoglobulin (Ig) domain.
120. The transgenic non-human animal of claim 1 19, wherein the Ig domain is a heavy chain Ig domain.
121. The transgenic non-human animal of claim 119, wherein the Ig domain is a light chain Ig domain.
122. The transgenic non-human animal of claim 119, wherein the Ig domain is a constant domain.
123. The transgenic non-human animal of claim 119, wherein the Ig domain is a constant domain and the sortase recognition motif is located at or within 20 amino acids of the C-terminus of the Ig domain.
124. The transgenic non-human animal of claim 119, wherein the Ig domain is a domain of a class or isotype of antibody that is secreted.
125. The transgenic non-human animal of claim 119, wherein the Ig domain is an IgG domain.
126. The transgenic non-human animal of claim 119, wherein an endogenous genomic immunoglobulin gene has been genetically modified to encode a polypeptide that comprises an immunoglobulin domain fused to or comprising a sortase recognition motif.
127. A cell derived from the transgenic non-human animal of claim 119.
128. A hematopoietic cell derived from the transgenic non-human animal of claim 119.
129. A pre-B cell, B cell, or plasma cell derived from the transgenic non-human animal of claim 1 19.
130. An antibody-producing cell derived from the transgenic non-human animal of claim 119.
131. An embryonic stem cell or induced pluripotent stem cell derived from the transgenic animal of claim 119.
132. The transgenic animal of claim 119, wherein the animal has been immunized or otherwise contacted with an antigen of interest or infected with an infectious agent of interest.
133. The transgenic animal of claim 119, wherein the animal has a genetic susceptibility to developing an autoimmune disease or has an immunodeficiency.
134. An offspring of the transgenic animal of claim 119 and a second animal, wherein the second animal has a phenotype of interest or is transgenic, or a descendant of the offspring.
135. An antibody or antibody chain produced by the transgenic animal of claim 132, wherein the antibody or antibody chain comprises the sortase recognition motif.
136. A solid support having the antibody or antibody chain of claim 135 attached thereto.
137. A collection of antibodies or antibody chains produced by the transgenic animal of claim 132, wherein (i) members of the collection have variable regions that differ in sequence; (ii) at least some members of the collection comprise the sortase recognition motif; and (iii) at least some members of the collection specifically bind to the antigen.
138. A solid support having the collection of antibodies of claim 137, attached thereto, wherein optionally different antibodies or antibody chains are attached at discrete locations on the surface of the solid support.
139. An antibody or antibody chain produced by the transgenic animal of claim 119.
140. A hybridoma generated by fusing a B-lineage cell derived from the transgenic animal of claim 1 19 with an immortal cell.
141. An antibody or antibody chain produced by the hybridoma of claim 140.
142. A solid support having the antibody or antibody chain of claim 141 attached thereto.
143. A collection of hybridomas of claim 140, wherein (i) members of the collection produce antibodies comprising variable regions that differ in sequence; (ii) at least some members of the collection produce antibodies that comprise the sortase recognition motif; and (iii) at least some members of the collection produce antibodies specifically bind to the antigen.
144. An antibody or antibody chain produced by the transgenic animal of claim 1 19.
145. A method of producing an antibody or antibody chain comprising a sortase recognition motif, the method comprising: (i) immunizing the transgenic animal of claim 119 with an antigen of interest or infecting the transgenic animal with an infectious agent of interest; and (ii) isolating antibodies or antibody chains from the animal.
146. The method of claim 145, further comprising separating antibodies or antibody chains comprising a sortase recognition motif from antibodies or antibody chains that do not comprise a sortase recognition motif.
147. A method of generating a cell capable of producing an antibody or antibody chain comprising a sortase recognition motif, the method comprising: (i) immunizing the transgenic animal of claim 119 with an antigen of interest or infecting the transgenic animal with an infectious agent of interest; and (ii) isolating a B-lineage cell from the animal.
148. The method of claim 147, further comprising generating a hybridoma from the B- lineage cell.
149. A method of ligation comprising the step of contacting an acyl donor compound of formula:
Figure imgf000163_0001
wherein transamidase recognition sequence is a sequence recognized by a transamidase; j is an integer between 0 and 10, inclusive; k is an integer between 0 and 10, inclusive; m is an integer between 0 and 10, inclusive; p is 1 or 2;
X is -O-, -NR-, or -S-;
R is hydrogen; substituted or unsubstituted aliphatic; or substituted or unsubstituted heteroaliphatic; each occurrence of R1 is independently hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl; each occurrence of R3 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl;
R4 is the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; each occurrence of R5 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; and each occurrence of R6 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; and with a nucleophilic compound of formula:
Figure imgf000164_0001
wherein
B1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer, a recognition element, a small molecule, a lipid, or a label; and n is an integer from 0 to 6, inclusive; in the presence of a transamidase enzyme under suitable conditions to form a compound of formula:
Figure imgf000164_0002
150. The method of claim 149, wherein p is 1.
151. The method of claim 149, wherein R1 is hydrogen.
152. The method of claim 149, wherein -XR1 is -OCH3.
153. The method of claim 149, wherein each occurrence of R3 and R5 is independently the side chain of a natural amino acid.
154. The method of claim 149, wherein R4 is a modified side chain of a natural amino acid.
155. The method of claim 149, wherein R4 is a modified side chain of a natural amino acid selected from the group consisting of serine, threonine, lysine, aspartate, glutamate, arginine, asparagine, glutamine, and tyrosine.
156. The method of claim 149, wherein R4 is of the formula:
Figure imgf000165_0001
wherein RD is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl.
157. The method of claim 156, wherein RD is of the formula:
Figure imgf000165_0002
wherein i is an integer between 1 and 100, inclusive.
158. The method of claim 149, wherein m is 0, and -XR1 is -OCH3.
159. The method of claim 149, wherein m is 1, R6 is hydrogen, and -XR1 is -OH.
160. The method of claim 149, wherein m is 1, R6 is methyl, and -XR1 is -OH.
161. The method of claim 149, wherein n is 0.
162. The method of claim 149, wherein n is 1.
163. The method of claim 149, wherein n is i.
164. The method of claim 149, wherein n is 2.
165. The method of claim 149, wherein the transamidase recognition sequence is LPXT, wherein the X of the recognition sequence is any natural or unnatural amino acid.
166. The method of claim 149, wherein the transamidase recognition sequence is LPET.
167. The method of claim 149, wherein the transamidase recognition sequence is LPXTG, wherein the X of the recognition sequence is any natural or unnatural amino acid.
168. The method of claim 149, wherein the transamidase recognition sequence is LPETG.
169. The method of claim 149, wherein the transamidase recognition sequence is LPXTA, wherein the X of the recognition sequence is any natural or unnatural amino acid.
170. The method of claim 149, wherein the transamidase recognition sequence is LPETA.
171. The method of claim 149, further comprising performing a transamidase-mediated ligation on the product of the ligation.
172. A compound prepared by the method of any of claims 149 - 171.
173. The compound of claim 172, wherein the compound comprises a polypeptide.
174. A method of ligation comprising the step of contacting an acyl donor compound of formula:
Figure imgf000166_0001
wherein transamidase recognition sequence is a sequence recognized by a transamidase; j is an integer between 0 and 100, inclusive; m is an integer between 0 and 10, inclusive; p is 1 or 2;
X is -O-, -NR-, or -S-;
R is hydrogen; substituted or unsubstituted aliphatic; or substituted or unsubstituted heteroaliphatic;
R1 is independently hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl; R2 is independently hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl; each occurrence of R3 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; and each occurrence of R6 is independently the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; and with a nucleophilic compound of formula:
Figure imgf000167_0001
wherein j is an integer between 0 and 10, inclusive; k is an integer between 0 and 10, inclusive;
X is -O-, -NR-, or -S-;
R is hydrogen; substituted or unsubstituted aliphatic; or substituted or unsubstituted heteroaliphatic;
R7 is hydrogen; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic, branched or unbranched, substituted or unsubstituted, cyclic or acyclic aryl, or branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaryl;
R4 is the side chain of a natural or unnatural amino acid, optionally modified or substituted; substituted or unsubstituted acyl; branched or unbranched, substituted or unsubstituted, cyclic or acyclic aliphatic; branched or unbranched, substituted or unsubstituted, cyclic or acyclic heteroaliphatic; substituted or unsubstituted aryl; or substituted or unsubstituted heteroaryl; and each occurrence of R is independently the side chain of a natural or unnatural amino acid; in the presence of a transamidase enzyme under suitable conditions to form a compound of formula:
Figure imgf000168_0001
175. The method of claim 174, wherein R1 is hydrogen.
176. The method of claim 174, wherein each occurrence of R4 is the side chain of a natural amino acid.
177. The method of claim 174, wherein j is an integer between 1 and 50, inclusive.
178. The method of claim 174, wherein the transamidase recognition sequence is LPXT, wherein the X of the recognition sequence is any natural or unnatural amino acid.
179. The method of claim 174, wherein the transamidase recognition sequence is LPET.
180. The method of claim 174, wherein the transamidase recognition sequence is LPXTG, wherein the X of the recognition sequence is any natural or unnatural amino acid.
181. The method of claim 174, wherein the transamidase recognition sequence is LPETG.
182. The method of claim 174, wherein the transamidase recognition sequence is LPXTA, wherein the X of the recognition sequence is any natural or unnatural amino acid.
183. The method of claim 174, wherein the transamidase recognition sequence is LPETA.
184. The method of claim 174, wherein p is 1.
185. The method of claim 174, wherein m is 1.
186. The method of claim 174, wherein m is 0.
187. The method of claim 174, wherein m is 0, and -XR2 is -OCH3.
188. The method of claim 174, wherein m is 1, R6 is hydrogen, and -XR2 is -OH.
189. The method of claim 174, wherein m is 1 , R6 is methyl, and -XR2 is -OH.
190. The method of claim 174, wherein each occurrence of R5 is independently the side chain of a natural amino acid.
191. The method of claim 174, wherein R4 is a modified side chain of a natural amino acid.
192. The method of claim 174, wherein R4 is a modified side chain of a natural amino acid selected from the group consisting of serine, threonine, lysine, aspartate, glutamate, arginine, asparagine, glutamine, and tyrosine.
193. The method of claim 174, further comprising performing a transamidase-mediated ligation on the product of the ligation.
194. A compound prepared by the method of any of claims 174 - 193.
195. The compound of claim 194, wherein the compound comprises a polypeptide.
196. A compound comprising a masked transamidase recognition sequence.
197. The compound of claim 196, wherein the masked transamidase recognition sequence comprises a phosphorylated amino acid residue.
198. The compound of claim 196, wherein the masked transamidase recognition sequence comprises a glycosylated amino acid residue.
199. The compound of claim 196, wherein the compound comprises a polypeptide having the masked transamidase recognition sequence at or near its C terminus.
200. The compound of claim 196, wherein the masked transamidase recognition sequence is LPEtG, and wherein t is phospho threonine.
201. A circular protein comprising a sequence having the formula: TRS 1— SP- TRS2, wherein TRSl and TRS2 are first and second transamidase recognition sequences, which are optionally different, and wherein SP is a linker peptide comprising a side chain that comprises a moiety D1 , wherein D1 is acyl, substituted or unsubstituted aliphatic, substituted or unsubstituted heteroaliphatic, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, a peptide, a protein, a polynucleotide, a carbohydrate, a tag, a metal atom, a contrast agent, a catalyst, a non-polypeptide polymer,a particle, a recognition element, a small molecule, a lipid, or a label.
202. The circular protein of claim 201 , wherein the circular protein comprises a therapeutic polypeptide.
203. The circular protein of claim 201 , wherein the circular protein comprises a four-helix bundle.
204. The circular protein of claim 201 , wherein the circular protein comprises a cytokine:
205. The circular protein of claim 201 , wherein the circular protein comprises an interleukin, interferon, colony-stimulating factor, erythropoietin, growth hormone, or neurotrophin.
206. The circular protein of claim 201 , wherein D1 comprises a moiety that enhances protein or peptide solubility, stability, or circulating time, and/or decreases immunogenicity when the circular polypeptide is administered to a subject.
207. The circular protein of claim 201, wherein D1 comprises a polyethylene glycol or a derivative thereof.
208. The circular protein of claim 201, wherein TRSl and TRS2 are recognition sequences for different transamidases.
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