AU2001289811A1 - High throughput method and kit - Google Patents

High throughput method and kit

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AU2001289811A1
AU2001289811A1 AU2001289811A AU2001289811A AU2001289811A1 AU 2001289811 A1 AU2001289811 A1 AU 2001289811A1 AU 2001289811 A AU2001289811 A AU 2001289811A AU 2001289811 A AU2001289811 A AU 2001289811A AU 2001289811 A1 AU2001289811 A1 AU 2001289811A1
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target
surrogate
target protein
proteins
target proteins
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Paul Bernasconi
Ray Donald Carpenter
Jennifer Audrey Hunt
Robert Michael Petrovich
Gary Keith Powell
Kimberly Ann White
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Syngenta Participations AG
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Syngenta Participations AG
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Description

HIGH THROUGHPUT METHOD AND KIT
The present invention is directed to a high throughput method and kit for the discovery of small molecule interactors of target proteins, in particular to a high throughput method and kit for parallel analysis of small molecule interactions with a multitude of target proteins of unknown function.
Single target High Throughput Screens (HTS) are the method of choice to discover small molecule inhibitors, ligands, agonists or antagonists of specific target proteins in both the Agricultural and Pharmaceutical Research communities. These screens are performed on robotic platforms that can test 100,000 to over a million compounds against one target protein. Several detection methods, ranging from radiolabeled tracers to elaborate fluorescence markers, are currently used. For each target protein to be screened, investigators must know its particular enzymatic or regulatory function in order to identify and prepare a proper substrate or ligand, and to develop a proper workable detection method. Gene products that are known to have a useful physiological role, but whose enzymatic or regulatory function is unknown, are not used as targets in HTS. Thus, this approach requires a large investment in assay development and implementation, allowing only a limited number of target protein HTS to be performed in a given time period.
Whole genome sequencing projects are forcing a shift in the traditional approach to the HTS research paradigm. One important outcome of these sequencing efforts is the identification of large collections of validated targets. However, because the current approaches to small molecule discovery are based on the single target HTS model, scientists are unable to efficiently use and exploit the vast amount of genomics information being generated. Thus, only highly validated targets warrant the development of unique screens, i.e. targets of known function. In addition, the function of a large portion of the newly discovered validated targets is unknown, making the development of a single target HTS impossible in these cases. Clearly, current single target HTS approaches have severe economic, feasibility, and logistic limitations Thus, a HTS capable of analyzing more than just a few targets without development of unique screens for each target would provide a significant advantage in the field of genomic analysis. In addition, an HTS capable of analyzing a large number of targets of unknown function would also provide a significant advantage in the field of genomic analysis. The present invention brings together gene cloning and expression, protein purification and modification, ligand identification and synthesis, and assay platform technologies into a novel screen and method that allows for the parallel, massively multiplexed screening of targets on a genomic scale. The present invention further provides a screen and method capable of analyzing in a HTS manner a multitude of targets of unknown function. A protein of unknown function is any protein for which one cannot associate enzymatic, regulatory, structural or receptor activity.
In the preferred embodiment, the method and kit of the present invention use a collection or plurality of gene products, otherwise referred to herein as "target proteins," based on genomics information about their essentiality to a physiological process. The method and kit of the present invention do not require, however, that the enzymatic or regulatory function of the target proteins be known, nor, for that matter, their essentiality.
In accordance with the present invention, the gene coding for each desired target protein is prepared, transferred into an expression vector and moved into an appropriate host organism, for example E. coli, baculovirus, mammalian cells, or yeast. The gene products or target proteins are expressed and then purified.
The purified target proteins are biotinylated and used to pan for phages displaying foreign peptides on their surfaces. Phages containing peptide sequences that bind selectively to the purified target proteins are separately amplified and the DNA encoding the peptides sequenced. The peptide sequences encoded by the DNA are synthesized and used as the surrogate ligands in the method and kit of the present invention.
A target module is prepared by binding selectively a target protein, modified to allow its detection, with a surrogate ligand that is linked to an individually detectable bead. In one embodiment of the present invention, 100 target modules are constructed for 100 target proteins of interest. The 100. target modules are rnixed together in each chamber of a multi- chamber container. A compound or collection of compounds to be tested is added to each chamber, and the interaction of a compound with each target module is observed. In the preferred embodiment, analysis of the interaction is implemented by flow cytometry. A compound that is specific for a particular target protein will displace that protein from its target module. The identity of the target module so disrupted is deteπnined by identifying the particular bead to which the surrogate ligand is attached. In more detail, the method of the present invention includes the steps of obtaining a pluraUty of target proteins; obtaining a first set of surrogate ligands, wherein each surrogate ligand in the set of surrogate ligands binds selectively to a first target protein; binding the first set of surrogate ligands to first detectable beads to form a first set of surrogate ligand-bead complexes, wherein the first detectable beads can all be detected by the optical characteristics of the first detectable beads; combining the first set of surrogate ligand-bead complexes with the target protein labeled for detection to form a first target module; repeating the above steps, either concurrently or subsequently with a different set of surrogate ligands and detectable beads, and with either the first target protein or a different target protein, to form sets of target modules; adding the sets of target modules to each chamber of a multi-chamber container; adding a test compound, or a collection of test compounds, to each chamber of the multi- chamber container; detecting displacement of a target protein with a test compound; and deteirnining the identity of each target protein that is displaced with a test compound. The method of the invention further includes obtaining each said set of surrogate ligands by obtaining a phage library, wherein each phage of the library displays foreign peptides; mixing the phage library with each target protein of the pluraUty of target proteins; isolating phages displaying the foreign peptides that bind selectively to each target protein; isolating DNA encoding the foreign peptides that bind selectively to each target protein; sequencing the DNA; and synthesizing the set of surrogate ligands based on the sequencing.
The method of the invention further includes obtaining the pluraUty of target proteins by selecting target genes from a genome; expressing each of the target genes to produce the pluraUty of target proteins; and purifying the target proteins.
The method includes biotinylating the target proteins and linking the target proteins with avidin-phycoerythrin.
The invention further provides target proteins by selecting target genes from a genome, expressing each of the target genes to produce the set of target proteins, and purifying the target proteins.
The invention further provides using a surrogate Ugand selected from the group including a peptide, RNA aptamer, and β-peptide. Surrogate Ugands may also be selected from smaU molecules derived from combinatorial chemistry or from natural compound collections. The invention also provides screening target proteins having unknown function. The invention further provides labehng each individual bead with a defined combination of two dyes, with a defined combination of three dyes, or with a defined population of quantum dots. The invention also provides screening with 100 beads such that 100 target proteins are screened in each chamber of a multi-chamber container or with 1000 beads such that 1000 target proteins are screened in each chamber of a multi-chamber container. The invention further provides screening with an amount of test compound per chamber within the range of 0.1 ng to 100 ng.
The invention also provides for a kit that screens a pluraUty of target proteins derived from a genome the kit comprising sets of target modules, wherein each set of the sets of target modules comprises individuaUy detectable beads; a set of surrogate Ugands attached to the detectable beads, wherein the surrogate ligands of the set of surrogate Ugands are bound selectively to the same or different target protein of the pluraUty of target proteins; wherein the target proteins are labeled for detection; and a multi-chamber container, wherein the sets of target modules are stored in each chamber of the multi-chamber container. The invention also provides for a method for high throughput screening using individually detectable beads, surrogate Ugands, and a pluraUty of target proteins comprising: combining in a chamber a pluraUty of target modules, each target module comprising a Ugand-bead complex and a target protein labeled for detection; wherein the Ugand-bead complex comprises a surrogate Ugand coupled to an individuaUy detectable bead; wherein each surrogate Ugand is selected for use in the method according to a peptide sequence thereof that is known to bind selectively to one of the target proteins; adding to each of the pluraUty of detection chambers a test compound, whereby the compound displaces the target proteins from the target modules to which target compounds interact, detecting displacement of a target protein with a test compound; and determining the identity of each target protein that is displaced with a test compound.
It being understood that the order of the steps of the method of the present invention is not critical and that other orders are possible.
BRIEF DESCRIPTION OF THE FIGURES FIG. 1 A is a graph which shows the inhibition constants of a surrogate Ugand identified for a target protein as measured by enzyme inhibition. FIG IB is a graph which shows the affinity constant for the same surrogate Ugand and same protein Ulustrated in FIG1A as measured in a Lurninex™ bead set-up in which the Ugand is bound to the bead.
Gene Cloning And Expression Of Targets
Table II, Section A illustrates the general steps for cloning genes of interest and expression and purification of the corresponding target proteins. Gene products or proteins are considered to be target proteins when they have shown potential as targets for pesticide or drug design work, as determined by knock-out, mis-expression, or gene disruption experiments. In the preferred embodiment of the invention, a coUection of genes of interest may consist of the whole genome of a particular organism. A useful coUection might consist of 96 genes of interest or multiples thereof, since they can be processed in paraUel using microtiter plate based equipment. A set of two PCR primers for each of these genes is derived from the sequence and used to amplify the corresponding cDNA. The template can be a first strand cDNA obtained by reverse transcription of a population of mRNAs or double stranded cDNA prepared by purifying DNA from a plasmid or phage Ubrary. The ampUfied material is used in a versatile cloning system such as Echo™ Cloning System which uses Cre recombinase for directional cloning from a universal donor vector into a variety of expression vectors (InNitrogen, Carlsbad, CA), or GATEWAY Cloning Technology (LifeSciences, GIBCO-BRL, RockviUe, MD) which uses bacteriophage lambda-based site-specific recombination for cloning into a variety of expression vectors. (Current Bio. (1998), 8:1300; Ann. Rev. Biochem. (1989), 58:913; and Ptashe, (1992) A Genetic Switch, CeU Press, Cambridge) The proper orientation is checked by PCR with external and internal primers.
Using the Echo™ Cloning System, genes of interest are transferred into an E. coli, baculovirus, mammaUan ceU or yeast expression vector. For ease of target protein purification, the expression vectors can contain an affinity tag such as GST (glutathione-S-transferase), aUowing purification by GSH-agarose chromatography (Smith et al. (1986) PNAS 83:8703- 8707), 6xHistidine, allowing protein purification on metal chelate chromatography (Porath et al. (1975) Nature 258:598), or other affinity tags (Ausubel et al., Current Protocols in Molecular Biology, John Wley and Sons (1995)) Alternatively, the expression vector may not provide any tag and the protein is purified either by differential centrifugation (using inclusion bodies), hydrophobic interaction, or ion exchange chromatography. The whole process is run in a paraUel fashion in 96-weU plates, which are used for the primer preparation, PCR reactions, E. coli transformation and DNA template preparations. A robotic Uquid handler such as Tecan Genesis (Tecan AG, Switzerland) or Qiagen Biorobot 9600 (Qiagen GmbH, Germany) is used for the formatting of the PCR reactions. Colony picking is handled by a robot such as Genetix Q-bot (Genetix Ltd, UK).
In one embodiment of the invention, the cloned target protein is expressed in E. coli using conventional inducible promoters such as the tac promoter, arabinose promoter, or T7 promoter (Ausubel et al., Current Protocols in Molecular Biology, John Wiley and sons, 1995). Expression in E.coli is achieved in a wide range of possible genetic backgrounds. The lack of proteases is a weU know way of improving expression level (Messing (1983) Methods Enzymol 101:20-78), this system has been recently improved by the suppression of the lonA protease, an ATP dependent enzyme responsible for most of the proteolytic activity in the bacterial cytoplasm. Thomas et al. (1993) Gene 136:237-242 Other genetic characteristics are also useful, such as the ones in the so-caUed "Origami™" strains which have mutations in both thioredoxin reductase (trxB) and glutathione reductase (gor) genes, which greatly enhances disulfide bond formation in the cytoplasm of E. coli (Aslund et al. (1999) inNovations 10, 11- 12). The cloned target can also be expressed in yeast using a galactose inducible promoter (Johnston and Davis (1984) Mol. Cell. Biol. 4:1440-1448), in baculovirus infected insect ceUs using the polyhedrin promoter (MaioreUa et al. (1988) Bio/Technology 6:1406-1410) or in mammaUan ceUs using the CMV promoter (Kaufman (1990) Meth. Enzymol. 185:487-511). The target protein encoded and expressed by each gene of interest is purified using existing paraUel one-step techniques such as the ones offered by Pierce (Rockford, II) and Qiagen. The expected molecular weight of the target proteins are confirmed by SDS-PAGE or by mas spectrometry methods such as MALDI-TOF. Since the method of the present invention is also appUcable to proteins of unknown function, some indication that the protein is folded properly is needed. In absence of an activity to measure, the presence of target protein folding is confirmed by CD spectroscopy. For that purpose highly sensitive instruments such as π*-180 (AppUed Photophysics, UK) is used. When inclusion bodies are used for purification of the protein, the protein is completely denatured by incubation with 6 M guanidine-HCl and then refolded by dialysis against guanidine-HCl free buffer or by serial dilutions in buffers containing decreasing concentrations of guanidine-HCl. Refolding is foUowed by CD spectroscopy. In another embodiment of the present invention, PCR ampUfication of targets can be substituted by the use of a fuU-length cDNA Ubrary of the organism of interest. As genomics advances, it is expected that these libraries in the universal vectors described above wiU be available. Such a Ubrary is arrayed in a series of 96-weU plates, each containing a defined cDNA. For example, the complete complement of the 6000 yeast expressed proteins can be arrayed, according the present invention, in less than 65 96-weU plates.
Surrogate Ligand Preparation
A surrogate Ugand is a peptide, RNA, beta-peptide or other molecule that has been identified as having an affinity for a given protein. The surrogate Ugand acts as a replacement for the physiologicaUy relevant Ugand in displacement assays, thereby aUowing the design of high throughput displacement assays of the invention without knowing the identify of the physiological Ugand.
The Ugand preparation procedure, briefly iUustrated in Section B of Table II, used by the present invention is based on Phage Display of Peptides and Proteins: A Laboratory Manual (1996) Acad. Press NY. eds. Kay, B., Winter, J., and McCafferty; J.; Cwirla, S.E., et al. (1990) PNAS USA, 87:6378-6382; and Barrett, R.W. et al. (1992) Anal. Biochem. 204:357- 364, aU of which are incorporated herein by reference. In this procedure, biotinylation of target proteins, phage panning, phage purification, estimation of peptide-phage affinity for target protein, and preparation and purification of phage DNA for sequencing are performed in 96-weU format.
In one embodiment of the invention, solution phase panning foUowed by capture of phage on rnicrotiter plates is used. For solution phase panning, the target proteins obtained and purified as described above and iUustrated in Section A of Table II are biotinylated using sulfb-NHS- LC-LC-biotin according to the procedure recommended by the manufacturer (Pierce, Rockford, IL). Free biotin may be removed by passing through a gel filtration using D-Salt polyacrylamide 6000 columns (Pierce Chemical Co.). The extent of biotinylation of target proteins may be estimated by the [2-(4'-hycroxyazobenzene) benzoic acid] (HABA) method (Green, N.M. (1965) Biochem. J., 94, 23c-24c), or proteins may be used without measurement of biotinylation. Using sulfo-NHS-LC-LC-biotin according to the procedure recommended by Pierce (Rockford, IL), target proteins are routinely biotinylated to the extent of 1- 10 biotin molecules per target protein. Multiple proteins may be biotinylated in polypropylene rnicrotiter dishes and separated from free biotin by passing through Sephadex G-50 (Pharmacia Biotech) packed into 96-weU Multiscreen Minicolumns (MilUpore Corporation). Referring again to Table II, Section B, biotinylated target proteins (0.05 ug - 1.0 ug) in 90 ul 50mM Tris-HCL, 150 mM HaCl, pH 7.5, containing 0.5% Tween-20 (wash buffer A) are added to phage (10π pfu) from a peptide phage Ubrary such as those available from New England Biolabs, Beverly, MA (for example, Ph.D.- 12, Ph.D.-7, or Ph.D.-cyc7) in a 96-weU polypropylene rnicrotiter plate (one protein per weU) and incubated for 1 hour at room temperature. The phage Ubrary can be prepanned against streptavidin to eUminate the phages that are specific for this protein. Each solution corresponding to each protein is then transferred to a weU of a 96-weU streptavidin coated plate (one solution per weU). These streptavidin coated plates are either obtained from Pierce, or prepared by incubating Nunc Maxisorp plates overnight at 4 C with 15 ug streptavidin in 150 ul of 0.1M NaHCO3 pH 8.6, foUowed by incubation with blocking). Prepared Nunc Maxisorp plates are capable of binding 0.025 ug of biotinylated target protein as measured by binding of horseradish peroxidase- labeled biotin (Pierce Chemical Co.). After a 20 minute incubation, biotin is added to each weU solution to a final concentration of 0.1 mM and incubation continued for 5 minutes. The plate is washed with several volumes of wash buffer A and phage bound to the protein target are eluted by adding 100 ul of 0.2 M glycine HC1, pH 2.2, to each weU and incubating for ten minutes. The acid solution containing the released phage is removed from each weU and transferred to a weU of a 96 weU polypropylene rnicrotiter plate containing 15 ul of 1 M Tris- HCl, pH 9.1.
Alternatively, panning is carried out essentiaUy foUowing the protocol of New England Biolabs recommended for Phage Display Peptide Library Kit. Target proteins (5 ug in 150 ul 0.1M NaHCO3, pH 8.6) are added to each weU of a 96 well rnicrotiter plate (Costar 9017 or Nunc Maxisorp) and incubated at 4 C overnight with gentle shaking. The protein solution is then removed, and weUs are filled with blocking buffer (0.1 M NaHCO3, 5 mg/ml BSA, pH 8.6). The plate is incubated three hours at 4 C then the blocking buffer is removed and the plate washed with wash buffer A. Next, 10u plaque forming units (pfu) from a peptide phage Ubrary are suspended in wash buffer A and incubated for one hour at room temperature. The rnicrotiter plate is washed with wash buffer A. To elute the phage, 100 ul of 0.2 M glycine HC1, pH 2.2, is added to each weU and incubated ten minutes. The acid solution is removed from each weU and added to the weUs of a 96 weU polypropylene rnicrotiter plate containing 15 ul of l M Tris-HCl, pH 9.1.
From each of the 96 weUs, the eluted phage (now in a total volume of 100 ul) is ampUfied in 2 ml of LB media containing 1:100 dUution of overnight culture of E. coli strain ER2738 (New England Biolabs) (or other E. coli strain containing the F-factor). This amplification is performed in eight sterile 12-weU plates, using Qiagen Air Pore strips (Qiagen, Valencia, CA) to prevent spiUage. After 4.5 hours, the samples are transferred to a 96-weU deep weU plate (one sample per weU) and centrifuged at 3,000 x g to peUet the E.coli ceUs. The 96 supernatants containing the phage are transferred to a 96 deep weU plate (one supernatant per weU) and a 1/6 volume of PEG/NaCl (20% w/v polyethylene glycol 8000, 2.5 M NaCl) is added. The solution is incubated at 4°C overnight. After overnight precipitation at 4°C, samples are spun for 30 minutes at 5600 x g in a Qiagen 4-15°C centrifuge to peUet the phage. Each of the 96 supernatants is removed and the phage are resuspended in 100 ul wash buffer A. Phage yields of 1010- 1011 pfu are routinely obtained by propagation of eluted phage in 2 ml of ceU culture, which provides an adequate number of phage for subsequent rounds of panning. Alternatively, E.coli ceUs can be removed and the supernatant containing the phage coUected by filtration instead of centrifugation as is known in the art.
AmpUfied phage is used in second and third rounds of panning and 100 ul of each ampUfied phage (typicaUy 1010 to 1011 pfu) are added to its corresponding target protein as described above. Panning is carried out in identical manner except that wash buffer may contain concentrations of Tween-20 up to 0.5% (v/v). Phage may be titered as described below or the entire 100 ul of ampUfied phage may be used for panning without estimation of phage titer. After the third round of affinity panning, phage may be titered.
The titer of a phage stock may be estimated after each of the amplification steps, or the titer of phage eluted after panning may be estimated. To estimate phage titer, phage may be seriaUy diluted in polypropylene rnicrotiter plates and spotted onto a cell lawn. WeUs of a rnicrotiter plate are filled with 90 ul TBS (50 mM Tris HCl, pH 7.5, 0.15 M NaCl). Ten microUters of phage are transferred by multichannel pipettor to the first row of the plate, mixed by pipetting up and down multiple times. From this row 10 ul is transferred to the next row until the last row is reached. Phages are thus diluted over a 108-fold range. In this method, the 96 phage samples may be diluted for titering using 8 rnicrotiter plates. Using a multichannel pipettor, 2 ul of solution are removed from a column of weUs in the rnicrotiter plate and spotted onto LB agar plates that contain IPTG (200 uM) and Xgal (190 uM) and that are overlaid with top agar mixed with a saturated culture of E. coli ER2738 (New England Biolabs), or other E. coli strain containing F-factor. Sixteen such agar plates are necessary to estimate the titer of the 96 phage samples. Agar plates are incubated approximately 16 hours at 37°C and phage are visualized as blue plaques to estimate titer of the phage stock. Phage titer is calculated by observing the greatest phage dUution that produced individual phage plaques on the agar plate. FoUowing three rounds of affinity panning, individual plaques are isolated by pipetting an appropriate dilution, based on the phage titer described above, of eluted phage from the third round of affinity panning onto LB/IPTG X-gal agar plates described above. One agar plate is needed for each eluted phage sample (i.e. 96 agar plates are required to obtain individual phage from panning against 96 targets). Plates are incubated overnight at 37°C to produce blue plaques. As many as twelve individual plaques from each plate are transferred separately into 500 ul of a 1:100 saturated culture of E. coli ER2738 dUuted in LB in 96-deep weU plates and ampUfied at 37°C with vigorous shaking for 4.5 hours. Twelve 96-weU deep plates are needed for the 96 targets. Phage may be separated from ceUs using a Uniplate filter plate as described above. Phage in the ceU-free media may be titered as described above and used for a phage ELISA.
To determine which individual phage binds most tightly to a target protein, a phage ELISA is used. The ELISA is carried out essentiaUy the same as the NEB protocol except 3,3\5,5'- tetramethylbenzidine (TMB) (KPL, Gaithersburg, MD) is used as the horseradish peroxidase (HRP) substrate. ELISA signals are read at 600nm in a mitrotiter plate reader such as Spectrafluor (Tecan). Individual phage are dUuted so that aU phage samples are at equal concentration (typicaUy 2 x 108 to 2 x 109 pfu in 50 ul of wash buffer A). The individual phage are transferred to weUs coated with the target protein as described in the direct panning method described above. In the case of solution phase panning, biotinylated target proteins are added to streptavidin plates and then phage are added to rnicrotiter plate. Phage are aUowed to bind as described in panning steps above except that after washing unbound phage from the plate, 150 ul of a 1:5000 dilution of HRP-labeled anti-M13 antibody (Pharmacia Biotech, Piscataway, NJ) is added to each well and incubated, then removed and the weUs are washed. The HRP substrate TMB (KPL, Gaithersburg, MD) is added and absorbance at 600nm is monitored. Preferably, only those phage which show the highest affinity, are used in the method and kit of the present invention. Individual phages with the highest affinity for their corresponding target protein are sequenced by propagating the phage in 96-weU deep weU plates, whereby phage DNA is prepared in the 96-weU format using an existing kit (Qiaprep 96 M13 kit; Qiagen, Valencia, CA) according to the manufacturer's recommended procedure. In the case of NEB phage hbraries, phage DNA is sequenced using the primer suppUed with the Ph.D. Phage Display Kits.
TABLE I Table I shows examples of surrogate ligand sequences obtained by foUowing the panning protocol described above. The Ubrary used is HyB, obtained from Display Systems Biotech, Vista. CA. Phage ELISA performed using direct coating of rnicrotiter weUs with 5 ug target protein and 109 pfu of individual phage results in ELISA signals above background weUs (containing no target protein) for the two target proteins.
Target Protein #1: Arabidopsis GDP-mannose-pyrophosphorylase
Phage ID Sequence
1M2 SGRVRPAG (SEQIDNO:l) lel2 GRKLERNR (SEQIDNO:2) lf3 GRKLERNR (SEQ ID NO:3) lfl2 IRRKTEGT (SEQ ID NO:4)
la3 GGGTFGGA (SEQIDNO:5)
Target Protein #2: Bacillus thurineensis vip2
Phage ID Sequence lf8 AGRFKAFR (SEQIDNO:6)
2b5 MGPGGRLG (SEQ ID NO:7)
2g5 AARSGRSD (SEQ ID NO:8)
2a5 AEGLRGWG (SEQIDNO:9) la8 ERAIWDRD (SEQIDNO:10) lb8 SVRRETMD (SEQIDNO:ll) These two examples of Table 1 show how surrogate ligands cluster around a consensus sequence (G R K L E (SEQ ID NO: 12) for target protein #1, A X G G/L R D (SEQ ID NO: 13) for target protein #2). They also show how outsiders that have no physiological significance are identified by their lack of consensus sequence (phage ID la3 in target #1).
Using the method of the present invention, sets of surrogate Ugands are obtained, where each surrogate Ugand in each set of surrogate Ugands binds selectively to one of the desired target proteins. Thus, a set of surrogate Ugands is generated for each desired target protein. In one embodiment of the present invention, the surrogate Ugands bind selectively to a pluraUty of target proteins of unknown function.
A surrogate Ugand "binds selectively" when it binds to its target in such a way that the binding can be readUy distinguished from its binding to other targets because a) the signal generated is higher than the background signal and b) the binding is of much higher affinity for the specific target than it is for non-specific ones (the signal obtained from binding to non-specific targets is weaker or non-existent).
As an alternative to phage Ubraries displaying multiple copies of a peptide on a single phage, monovalent phage that display one or less peptides/phage may be used by the method of the present invention. Using monovalent phage may result in higher affinity phage. Lowman, H.B. (1997) Annu. Rev. Biophys. Biomol. Struct. 26:401-24 One such phage Ubrary, HyB, can be obtained from Display Systems Biotech, Vista. CA. Using the HyB Ubrary, phage can be panned and propagated as described above except that helper phage M13KO7 must be added during phage amplification for production of phages. In this phagemid system, the displayed peptide is linked to the human secretory trypsin inhibitor, (PSTI) which is in turn displayed on the g3 protein of the filamentous phage. Rottgen, P., and Collins, J. (1995) Gene 164:243-250. Such a system may result in peptide phage of higher affinity than polyvalent display. Green, N.M. (1965) Biochem. J., 94:23c-24c Also in this system, the PSTI protein displaying the selected peptide may be transferred to an expression vector and purified in ilUgram quantities from one Uter ceU culture. Maywald, F. et al. (1988) Gene 68:357-369)
In another embodiment of the present invention, the peptidic surrogate Ugand can be replaced by a RNA aptamer. The method for selection and preparation of such RNA aptamers has been pubUshed (for review see: Famulok, M (1999) Curr. Opin. Struct. Biol. 9:324; Herman, T and Patel, D.J. Science (2000), 287:820-825); KeUy, JA, Feigon, J, Yeates, (1996) J. Mol. Biol. 256:417; and Feigon, J, Dieckmann, T and Smith, F.W. (1996) Chem. Biol. 3: 611). The peptidic surrogate Ugand can also be replaced by a beta-peptide. Beta-peptides are composed of beta-amino acids, which contain an additional methylene group in the peptidic backbone (Seebach, D and Matthews, J.L. (1997) Chem. Comm. 2015-2022; GeUman, S (1998) Ace. Chem. Res. 31:173-180). Because of the expected increased stabiUty of beta-peptide versus natural peptides, the surrogate Ugands thus generated are expected to be shorter than natural peptide surrogate Ugands and therefore might simplify the complexity of the pool of surrogate Ugands that need to be screened to identify a Ugand for each of the target proteins. The selection of the appropriate beta-peptide surrogate Ugand for each target protein can be based on protocols used for some coUections of natural peptides such as Yaffe et al. (1997) CeU, 91:961-971. These protocols select the specific Ugand by presenting the coUection of Ugands to the protein target and subsequent separation of the complex by gel filtration. The selected Ugand is then identified by mass-spectrometry.
High Throughput Multiplexed Displacement Assay
The multiplexed HTS displacement assay of the present invention incorporates the technology developed by Luminex Corporation, Austin TX. This technology provides a coUection of one hundred 5 um microspheres ("beads" or "particles") individuaUy labeled by a defined combination of two dyes. The surfaces of the beads are modified to aUow coupling of an analyte (nucleic acid, protein, or other such material) to the beads. The analyte is also labeled, preferably with a fluorescent molecule (nucleic acid, protein, or other such material). The bead identity, and therefore the identity of the analyte coupled to it, is determined by flow cytometry. Since one hundred different beads are avaUable, the interaction of one hundred different analytes with their corresponding fluorescent label can be measured at the same time. The Luminex multiplex assay is described in US Pat. No. 5,981,180, which is incorporated herein by reference. While current Luminex beads carry two dyes, aUowing the encoding of one hundred beads, three dyes are possible and would allow the simultaneous encoding of one thousand beads and corresponding target proteins.
Once the surrogate Ugands are identified and sequenced by the method of the present invention as described above, they may be synthesized by and obtained from a commercial suppUer of peptides. In the preferred embodiment of the present invention, the surrogate Ugands have a N or C terminal cysteine residue. For cost saving reasons, it is preferred to have the cysteine as C-terrninal rather than N-teπriinal. The Merrifield peptide synthesis procedure starts at the C- terrninal and a large amount of Cys-resin can be prepared and used for aU the peptide synthesis work. An amount of 1 mg of peptide is sufficient for use by the method of the present invention.
According to the method of the present invention, each surrogate Ugand of the present invention is coupled to individuaUy labeled and detectable Luminex beads to form what is referred to herein as a Ugand-bead complex. The term "complex" refers to the structure formed upon connection of Ugand to bead. Target proteins bind selectively to their respective Ugand-bead complexes to form sets of target modules of the invention. For example, a particular target protein binds selectively with a particular Ugand-bead complex to form a first target module. Another target protein binds selectively with another (or the same) Ugand-bead complex to form a second target module, and so on.
One embodiment of the method of the present invention uses avidin-Unked phycoerythrin to label the target proteins. The symbols λexι, λεmι indicate the excitation and emission wavelengths for bead identification. The symbols λeX2, λem2 indicate the wavelengths for measuring the fluorescence associated with the bead. Alternatively, the target proteins can be labeled with a fluorescent group compatible with the Luminex technology. An example of such group is the Alexa 532 dye (Molecular Probes, Eugene, OR) or Cy5 (Pharmacia). The assay of the present invention is performed by incubating the sets of target modules in each weU of a rnicrotiter plate (either 96 or 384-weU format). The reaction volume can be between 10 and 100 ul. The buffer used can be adapted to each instance but is typicaUy PBS or 100 mM Tris-HCl at pH 7.5 with 0.1 M NaCl. In one embodiment, 1000 to 5000 beads comprise each set of specific target modules and are present, with 0.1 to 100 nM of a target protein and 0.1 to 100 pM of avidin-phycoerythrin, in each weU of a rnicrotiter plate. In addition, the weU contains 1 to 10 uM of test compound in a final concentration of DMSO of 1 to 5 % . Thus, in one embodiment, 100,000 to 500,000 beads (representing the sets of target modules) are present in the same final volume of 10 to 100 ul. The reaction mixtures are incubated at room temperature for 1 to 30 minutes and analyzed using a Luminex detection apparatus.
The present invention recognizes that the physical entity analyzed and measured by the present invention is the selective binding of the target protein to its corresponding surrogate Ugand. Steps were taken to ensure that this physical entity was biochemicaUy meaningful. As an example, the inhibition potency of a surrogate Ugand, as defined by its K and measured by an enzymatic assay was compared to its affinity for the target protein, as defined as its KD and measured in a Lurninex bead assay set-up. This comparison, shown in FIGS 1A and IB, demonstrates that the two values are essentiaUy identical.
The present invention also recognizes that the target proteins will often present more than one relevant binding site, for example, kinases have a catalytic site which binds the substrate and ATP and a protein interaction site that interacts with the protein directly upstream in the signal transduction pathway. Surrogate Ugands are identified for each of these sites. By binding each of these surrogate Ugands to a different bead, the different sites are probed simultaneously. For some appUcations, the present invention also recognizes that it is advantageous to have the target protein rather than the surrogate ligand bound to the bead. In this case, the target protein is linked to the bead by covalent bound formation with the reactive groups present on the bead surface or by interaction with avidin coated beads. The surrogate Ugand is free in solution and labeled either with biotin, for detection via avidin-phycoerythrin, or with a fluorescent dye such as Alexa 532 or Cy3 for direct detection.
The present invention also recognizes that the Lurninex technology can be replaced with technologies that also identify beads with a specific marker. For example, one such marker system is referred to as the Quantum Dot™ (Quantum Dot Corporation, Palo Alto, CA). The Quantum Dot™ is a 2-10 nm CdSe crystal which, depending on its size, emits a single wavelength Ught ranging from ultraviolet to infrared when excited with UV Ught (Chan and Nie (1998), Science 281 :p2016-2018). In this approach, each bead, either a polymer bead or a glass bead, is identified by a defined population of quantum dots. The complexity of the quantum dot population defines the total number of distinct beads that can be encoded. The complexity of a set-up defined by the presence of absence of a given quantum dot is calculated by: complexity = 2(number of different quantum dots)-l. For example, if five quantum dots are used, 31 beads can be encoded. The complexity of a set-up defined by the absence, low amount or high amount of a given quantum dot is given by: complexity = 3(number of different quantum dots)-l. For example, if five quantum dots are used, 242 beads can be encoded. It can be seen that, even with a smaU number of quantum dots, a larger coUection of beads can be encoded. This aUows the use of quantum dots with weU separated emission, which in turn aUows the detection and identification of the bead to be performed by a low cost imaging system. Such a system can be a microscope with a UV Ught source, a mechanical stage holding a 96-weU plate controUed by a computer and a color digital camera such as the ones used for computer work. The reaction in each weU is composed of the same elements as for the Luminex approach but with the quantum dot encoding beads replacing the Lurninex bead. After aUowing the beads to settle at the bottom of the weU, the 96-weU plate is scanned on the microscope, the image captured and analyzed by computer. This setup needs only to discriminate between the five quantum dot colors and a six color for the fluorescence associated with the bead due to the bound fluorescent Ugand. This last source of fluorescence can also be a six quantum dot of a color different from the bead encoding.
Alternatively, a microfluidics set-up such as the one avaUable from CaUper Technologies (CaUper, Mountain View, CA) can be used by the present invention. In this case, both the surrogate Ugand and the target protein are free in solution. The surrogate Ugand is labeled with a fluorescent such as fluorescein, tetramethylrhodamine or other. The detection of the interaction is done by fluorescence polarization as is known in the art. Fluorescence polarization methods suffer from a lack of sensitivity and the need for a large amount of target protein. A typical concentration of such protein is 10 to 50 uM. In the case of a 50 kDa protein assayed in a 25 ul assay volume, 1.25 to 6.25 grams of protein are needed to assay 100,000 compounds. These large amounts are incompatible with a Genomics based HTS. By using a microfluidics set-up, the reaction volume is reduced to 10 nl or less, requiring 500 ug or less of the target protein. In this case, each compound is sampled against each target in a serial fashion.
The present invention also includes a screening kit comprising a set of target modules representing the whole complement of expressed proteins in a given organism, or for a subset thereof such as the proteins involved in a specific metaboUc or signaling pathway. The Ugand- bead complexes are stably stored in a sterUe fashion at 4° C. The corresponding pluraUty of protein targets are stored as aUquots in a sterUe fashion at -80C. Alternatively, the sets of target modules are constructed and stored in the individual chambers of a multi-chamber container. The kit of the invention is used, in part, to associate potentiaUy useful protein targets with test compounds.
One advantage of the present invention is that it provides for a huge increase in datapoints coUected per day compared to traditional HTS of target proteins. Since the method and kit of the invention are formatted for 96 or 384 weU plates, the process is adapted to a robotic platform consisting, for example, of a TomTec Quadra 96plus (TomTec, Hamden, CT) for assembling the reactions and a Hudson PlateCrane (Hudson Control Systems) to deUver the assembled plates to a Luminex/HTS detection apparatus. Thus, the method and kit of the present invention analyzes one 384- well plate every 20 minutes. When one-hundred targets are multiplexed and a single smaU molecule is present per weU, the output of the present invention is 115,200 datapoints per hour. When 24 plates are assayed in a da y cycle of 10 hours, the method and kit of the present invention coUects 1.1 miUion datapoints per day. As a comparison, a survey of forty-three Life Science companies involved in HTS showed that the estimated datapoint coUection is between 135,000 to 175,000 each month for 1999 and expected to grow to 490,000 to 615,000 monthly in the year 2002 (High Throughput Screening: 1999-2000 Market analysis for Life Science Manufacturers, Clinical Marketing Consultants, Boulder, CO). In the same survey, these companies do not expect a decrease in price per datapoint, making the coUection of data on a genome size coUection of targets out of reach economicaUy.
Furthermore, the method of the present invention makes a very efficient use of the compounds to be screened: only a very smaU amount of each compound is consumed to test a large number of targets. As an example of the present method and kit, a 100 ul assay volume containing 100 targets and a compound coUection with an average MW of 500 tested at 2 uM, a 100 target test would require 100 ng of compound (or 1 ng per target). Based on the survey mentioned above, a typical assay uses a 384-weU format using 50 ul volume per weU. Since only one target is assayed per weU, the equivalent amount of compound that would be needed to run 100 targets, in the traditional HTS format, is 5 ug (or 50 ng per target). Another advantage of the present invention, is that it provides a HTS method and kit that screens for proteins of unknown function.
The above-disclosed embodiments are iUustrative. This disclosure of the invention wiU place one skilled in the art in possession of many variations of the invention. All such obvious and foreseeable variations are intended to be encompassed by the appended claims. TABLE II: flow diagram of the method of the present invention.
B
Target genes coUection from Genomics ϊ
PCR amplification or arrayed fuU length cDNAs pECHO cloning phage display Ubrary linear, cycUc, fusion protein
I cre-lox recombination in expression vectors ϊ
(E.coli, baculo virus, mammaUan, yeast) Panning
1 solid phase or solution phase
Protein purification via 6xHis, GST i or HA tags SLidentification by sequencing chemical synthesis
I
Protein characterization (MW) secondary i structure via CD bead coupling via activated COOH or i Protein biotinylation maleimide groups
1 ϊ
Displacement assay fluorescently labeled protein biotinylated protein, avidin-phycoerythrin
I
Multiplexing by encoding SL identity with bead color
( 100 theoretical points)
I
100 assays
t compound sourcing packaging

Claims (1)

  1. What is claimed is:
    1) A method comprising: a) obtaining a pluraUty of target proteins; b) obtaining a first set of surrogate Ugands, wherein each surrogate Ugand in said set of surrogate Ugands binds selectively to a first target protein; c) binding said first set of surrogate Ugands to first detectable beads to form a first set of surrogate Ugand-bead complexes, wherein said first detectable beads can aU be detected by the optical characteristics of said first detectable beads; d) combining said first set of surrogate Ugand-bead complexes with said first target protein labeled for detection to form a first target module; e) repeating steps a, b, c and d, either concurrently or subsequently with a different set of surrogate Ugands and detectable beads, and with either said first target protein or a different target protein, to form sets of target modules; f) adding said sets of target modules to each chamber of a multi-chamber container; g) adding a test compound, or a coUection of test compounds, to each chamber of said multi-chamber container; h) detecting displacement of a target protein with a test compound; and i) determining the identity of each target protein that is displaced with a test compound.
    2) The method according to claim 1 , wherein obtaining each said set of surrogate Ugands comprises: a) obtaining a phage Ubrary, wherein each phage of said Ubrary displays foreign peptides; b) mixing said phage Ubrary with each said target protein of said pluraUty of target proteins; c) isolating phages displaying said foreign peptides that bind selectively to each said target protein; d) isolating DNA encoding said foreign peptides that bind to each said target protein; e) sequencing said DNA; and f) synthesizing said set of surrogate Ugands based on said sequencing. 3) The method according to claim 1 , wherein said set of target proteins are obtained by: a) selecting target genes from a genome; b) expressing each of said target genes to produce said set of target proteins; and c) purifying said target proteins.
    4) The method according to claim 1, wherein the target protein in step (e) is said first target protein.
    5) The method according to claim 1, wherein the target protein in step (e) is a target protein different from said first target protein.
    6) The method according to claim 1, comprising: a) biotinylating said target proteins; and b) Unking said target proteins with avidin-phycoerythrin.
    7) A method comprising: a) obtaining a pluraUty of target proteins; b) obtaining a first set of surrogate Ugands, wherein each surrogate Ugand in said set of surrogate Ugands binds selectively to a first target protein; c) binding said first target protein to first detectable beads to form a first set of target protein-bead complexes, wherein said first detectable beads can aU be detected by the optical characteristics of said first detectable beads; d) combining said first set of target protein-bead complexes with said first set of surrogate Ugands labeled for detection to form a first target module; e) repeating steps a, b, c, and d, either concurrently or subsequently with a different set of surrogate Ugands and detectable beads, and either said first target protein or a different target protein, to form sets of target modules; f) adding said sets of target modules to each chamber of a multi-chamber container; g) adding a test compound, or a coUection of test compounds, to each said chamber of said multi-chamber container; h) detecting displacement of a surrogate Ugand with a test compound; and i) determining the identity of each surrogate Ugand that is displaced with a test compound.
    8) A method according to claim 7, wherein obtaining each said set of surrogate Ugands comprises: a) obtaining a phage library, wherein each phage of said Ubrary displays foreign peptides; b) mixing said phage Ubrary with each said target protein of said pluraUty of target proteins; c) isolating phages displaying said foreign peptides that bind to each said target protein; d) isolating DNA encoding said foreign peptides that bind selectively to each said target protein; e) sequencing said DNA; and f) synthesizing said set of surrogate Ugands based on said sequencing.
    9) A method according to claim 7, wherein said set of target proteins are obtained by: a) selecting target genes from a genome; b) expressing each of said target genes to produce said set of target proteins; and c) purifying said target proteins.
    10) The method according to claim 16, wherein the target protein in step (e) is said first target protein.
    11) The method according to claim 16, wherein the target protein in step (e) is a target protein different from said first target protein.
    12) The method according to claim 16, comprising: a) biotinylating said target proteins; and b) Unking said target proteins with avidin-phycoerythrin.
    13) A method according to claim 1 or 7, wherein said surrogate Ugand is a peptide a RNA aptamer or a beta-peptide.
    14) A method according to claim 1 or 7, comprising labeling each said individual bead with a defined combination of two dyes, with a defined combination of three dyes or with a defined population of quantum dots
    15) A method according to claim 14, comprising labeling each said individual bead with a defined combination of two dyes, wherein the number of said individual beads is 100 such that 100 target proteins are screened in each said chamber.
    16) A method according to claim 1 or 7, wherein the amount of said compound used per said chamber faUs within the range of 0.1 to 100 ng. 17) A method according to claim 1 or 7, wherein the enzymatic or regulatory function of each said target protein of said pluraUty of target proteins is unknown.
    18) A kit for screening a pluraUty of target proteins from a genome comprising: a) sets of target modules, wherein each set of said sets of target modules comprises:
    ( 1 ) individuaUy detectable beads ;
    (2) a set of surrogate Ugands attached to said detectable beads, wherein the surrogate Ugands of said set of surrogate Ugands are bound selectively to the same or different target protein of said pluraUty of target proteins;
    (3) wherein said target proteins are labeled for detection; and b) a multi-chamber container, wherein said sets of target modules are stored in each chamber of said mult-chamber container.
    19) A kit according to claim 18, wherein said pluraUty of target proteins are of unknown function;
    20) A kit for screening a pluraUty of target proteins from a genome comprising: a) a set of Ugand-bead complexes, wherein each said Ugand-bead complex comprises:
    (1) a detectable bead;
    (2) a surrogate Ugand attached to said detectable bead; b) a pluraUty of target proteins, each said target protein of said pluraUty of target proteins is capable of selectively binding to a surrogate Ugand; and c) a multi-chamber container, wherein said pluraUty of ligand-bead complexes are stored in each chamber of said multi-chamber container, said target proteins being stored separately from said Ugand-bead complexes.
    21) A kit according to claim 20, wherem said target proteins are of unknown function;
    22) A kit according to claim 18 or 20, wherein the number of said target proteins is greater than 50.
    23) A kit according to claim 18 or 20, wherein the number of said target proteins is greater than 500.
    24) In a method for high throughput screening using individuaUy detectable beads, surrogate Ugands, and a pluraUty of target proteins, the improvement comprising, a) combining in each chamber of a multi-chamber container sets of target modules, i) wherein each target module within each set of said sets of target modules comprises a Ugand-bead complex and a target protein labeled for detection;
    U) wherein said Ugand-bead complex comprises a surrogate Ugand coupled to an individuaUy detectable bead; in) wherein each said surrogate Ugand binds selectively to one of said target proteins; b) adding to each said chamber of said multi-chamber container a test compound, whereby said compound displaces said target proteins from said target modules to which said target compounds interact; c) detecting displacement of a target protein with a test compound; and d) determining the identity of each target protein that is displaced with a test compound.
    25) The method according to claim 24, wherein the function of said pluraUty of target proteins are unknown.
    26) The method according to claim 24, wherein obtaining each said set of surrogate Ugands comprises: a) obtaining a phage Ubrary, wherein each phage of said Ubrary displays foreign peptides; b) mixing said phage Ubrary with each said target protein of said pluraUty of target proteins; c) isolating phages displaying said foreign peptides that bind selectively to each said target protein; d) isolating DNA encoding said foreign peptides that bind to each said target protein; e) sequencing said DNA; and f) synthesizing said set of surrogate Ugands based on said sequencing.
    27) The method according to claim 24, wherein said set of target proteins are obtained by: a) selecting target genes from a genome; b) expressing each of said target genes to produce said set of target proteins; and c) purifying said target proteins.
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