WO2019107962A2 - Method for conjugating antibody and physiologically active substance - Google Patents

Method for conjugating antibody and physiologically active substance Download PDF

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Publication number
WO2019107962A2
WO2019107962A2 PCT/KR2018/014939 KR2018014939W WO2019107962A2 WO 2019107962 A2 WO2019107962 A2 WO 2019107962A2 KR 2018014939 W KR2018014939 W KR 2018014939W WO 2019107962 A2 WO2019107962 A2 WO 2019107962A2
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active substance
antibody
physiologically active
peptide
conjugate
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PCT/KR2018/014939
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French (fr)
Korean (ko)
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WO2019107962A3 (en
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유태현
박지수
이유미
Original Assignee
아주대학교 산학협력단
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Priority claimed from KR1020180146289A external-priority patent/KR102037336B1/en
Application filed by 아주대학교 산학협력단 filed Critical 아주대학교 산학협력단
Priority to EP18882347.0A priority Critical patent/EP3719031A4/en
Priority to US16/768,331 priority patent/US11723984B2/en
Priority to CN201880084592.6A priority patent/CN111788215B/en
Priority to JP2020549533A priority patent/JP6969014B2/en
Publication of WO2019107962A2 publication Critical patent/WO2019107962A2/en
Publication of WO2019107962A3 publication Critical patent/WO2019107962A3/en
Priority to US18/338,832 priority patent/US20240016947A1/en

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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/50Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates
    • A61K47/51Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates the non-active ingredient being a modifying agent
    • A61K47/62Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates the non-active ingredient being a modifying agent the modifying agent being a protein, peptide or polyamino acid
    • A61K47/64Drug-peptide, drug-protein or drug-polyamino acid conjugates, i.e. the modifying agent being a peptide, protein or polyamino acid which is covalently bonded or complexed to a therapeutically active agent
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/50Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates
    • A61K47/51Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates the non-active ingredient being a modifying agent
    • A61K47/62Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates the non-active ingredient being a modifying agent the modifying agent being a protein, peptide or polyamino acid
    • A61K47/65Peptidic linkers, binders or spacers, e.g. peptidic enzyme-labile linkers
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/50Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates
    • A61K47/51Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates the non-active ingredient being a modifying agent
    • A61K47/68Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates the non-active ingredient being a modifying agent the modifying agent being an antibody, an immunoglobulin or a fragment thereof, e.g. an Fc-fragment
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K7/00Peptides having 5 to 20 amino acids in a fully defined sequence; Derivatives thereof
    • C07K7/04Linear peptides containing only normal peptide links
    • C07K7/08Linear peptides containing only normal peptide links having 12 to 20 amino acids

Definitions

  • the present invention relates to an Fc position-selective fused peptide in which the 5th, 10th or 11th position of the Fc position-selective binding peptide represented by the amino acid sequence of SEQ ID NO: 1 is substituted with an amino acid having a photoreactive functional group,
  • An active substance an antibody-physiologically active substance conjugate in which an antibody is bound to the physiologically active substance, and a method for producing the antibody-physiologically active substance conjugate.
  • ADC antibody-drug conjugate
  • antibody-biologically active substance conjugates should retain the properties of unbound antibodies and physiologically active substances.
  • the antibody-biologically active substance conjugate should be able to maintain affinity with the antibody prior to binding to the physiologically active substance. That is, the binding of the antibody and the bioactive substance should not inhibit the inherent antigen-antibody binding.
  • the physiologically active substance of the antibody-physiologically active substance conjugate should be able to exhibit activity after reaching the target. That is, in the antibody-physiologically active substance conjugate, the intrinsic properties of each of the monoclonal antibody and the physiologically active substance should be maintained, which is determined by the method of conjugating the two substances.
  • linker used for conjugation should be stable in the blood to prevent the biologically active substance from separating from the antibody and to reach the target tissue / cell.
  • linkers used in antibody-biologically active substance conjugates include acid-labile hydrazone, protease-labile peptide, and disulfide (reducing agent) sensitive to a reducing agent. ).
  • Non-cleavable thioether linkers are also used.
  • a method of introducing a cysteine residue into an antibody by using a functional group (lysine epsilon-amino group or cysteine thiol group) or mutation and using the reactivity of the thiol group is commonly used for conjugation of an antibody and a physiologically active substance .
  • the position where the physiologically active substance is connected can not be adjusted, and the water ratio of the antibody to the physiologically active substance is not constant, so that a heterogeneous antibody-physiologically active substance conjugate is produced.
  • the thiol group of the cysteine introduced into the antibody it is difficult to predict the effect on the structure and activity of the antibody due to the mutation in the antibody.
  • a low-molecular peptide mutant was prepared by substituting a photoreactive artificial amino acid covalently bound to an Fc domain binding peptide (US Patent Publication No. 20040253247 (2004.12.16)) that specifically binds to the Fc domain of an antibody by light irradiation .
  • a method of producing an antibody-drug conjugate in which a drug is bound to the above-prepared low molecular weight peptide mutant has been reported (Korean Patent Publication No. 10-2014-0004530 (Jan.
  • the peptide material used in the present invention must be prepared through chemical synthesis.
  • the conjugation method is limited to the case where a drug is conjugated to an antibody, and it is difficult to use it for conjugation of an antibody and a physiologically active substance such as a protein.
  • a physiologically active substance such as a protein.
  • the non-specific reactivity of the photoreactive amino acids used in the present invention has a problem in developing a conjugate of an antibody-biologically active substance into a drug (Yoshihito Tanaka et al., Molecular BioSystems, 6): 473-480, 2008).
  • an Fc position-selective peptide in which a specific position of an Fc position-selective binding peptide capable of specifically binding to an antibody Fc domain is replaced with an amino acid having a photoreactive functional group (para-benzophenylalanine (pBpa)
  • pBpa para-benzophenylalanine
  • the present invention provides an Fc position-selective fused peptide wherein the 5th, 10th or 11th position of the Fc position-selective binding peptide represented by the amino acid sequence of SEQ ID NO: 1 is substituted with an amino acid having a photoreactive functional group to provide.
  • the present invention also provides a physiologically active substance modified with a conjugate peptide in which a physiologically active substance is directly or linked to the peptide through a linker.
  • the present invention also provides an antibody-physiologically active substance conjugate wherein an antibody is bound to a physiologically active substance formulated with the conjugated peptide.
  • FIG. 1 is a schematic view showing a technique of bonding an antibody of the present invention to a physiologically active substance.
  • FIG. 2 is a result of electrophoresis after photo-reacting an antibody and a physiologically active substance formulated with the peptide to determine the substitution position of p-benzoylphenylalanine of the FcIII peptide of the present invention.
  • FIG. 3 is a schematic representation of ⁇ -lactamase (FcIII- ⁇ -lactamase) -expressing plasmid modified with the FcIII peptide of the present invention and FcIII- ⁇ -lactamase expressed in the plasmid.
  • FIG. 4 schematically shows a plasmid expressing ⁇ -lactamase zymogen (FcIII- ⁇ -lactamase zymogen) modified with the FcIII peptide of the present invention and FcIII- ⁇ -lactamase zymogen expressed in the plasmid.
  • Figure 5 schematically shows the expression plasmid PE24 (FcIII-ß-PE24) expressed in the FcIII peptide of the present invention and FcIII- ⁇ -PE24 expressed in the plasmid.
  • FIG. 6A shows a recombinant tRNA synthetase expression plasmid in the present invention.
  • 6B shows a plasmid expressing proline tRNA synthetase.
  • FIG. 7 shows the binding of the fusion protein of the present invention to the antibody (Cetuximab) by electrophoresis.
  • FIG. 8 shows the position-specific binding of the fusion protein of the present invention and the antibody (Cetuximab) by electrophoresis using a Z-domain.
  • FIG. 9 shows the location of the junction between FcIII and the antibody (Cetuximab) of the present invention by LC-MS / MS.
  • FIG. 10 shows electrophoretic results of Cetuximab-FcIII-PE24 conjugates obtained by binding the fusion protein of the present invention and an antibody (Cetuximab) at a ratio of 1: 1.
  • Figure 11 shows the results of confirming the EF2 ribosylation activity of the Cetuximab-FcIII-PE24 conjugate of the present invention.
  • FIG. 13 shows electrophoretic results of separation of Trastuzumab-FcIII-PE24 conjugate in which a fusion protein of the present invention and an antibody (Trastuzumab) are bound to each other and a fusion protein and an antibody are bound at a ratio of 1: 1.
  • a physiologically active substance which can be specifically bound to an antibody Fc domain and which is modified with an Fc position-selective peptide in which the 5th, 10th or 11th position of the Fc position-selective binding peptide is substituted with an amino acid having a photoreactive functional group (FIG. 2).
  • Fc position-selective peptide in which the 5th, 10th or 11th position of the Fc position-selective binding peptide is substituted with an amino acid having a photoreactive functional group
  • the present invention relates to an Fc position-selective fused peptide wherein the 5th, 10th, or 11th position of the Fc position-selective binding peptide represented by the amino acid sequence of SEQ ID NO: 1 is substituted with an amino acid having a photoreactive functional group will be.
  • the Fc position-selective binding peptide (FcIII) (amino acid sequence SEQ ID NO: 1, gene SEQ ID NO: 2) locally specifically binds to the CH3-CH2 interface region of the Fc domain of the human- (WL DeLano et al, Science , 2000).
  • the peptide shows a U-structure because two cysteines form a disulfide bond with each other.
  • the position substituted with the amino acid having the photoreactive functional group may be 10th.
  • a method for producing an Fc positionally-selected fused peptide substituted with an amino acid having a photoreactive functional group is characterized in that the amino acid sequence of the Fc position-selective binding peptide is identified and expressed in an expression system capable of expressing the peptide
  • a vector may be prepared and transformed into a host cell and expressed by a recombinant technique, or artificially synthesized, followed by substitution or introduction of at least one amino acid residue with an amino acid having a photoreactive functional group by a known method, or Can be synthesized by incorporating an amino acid having at least one photoreactive functional group in the artificial synthesis.
  • the introduction of the gene can be carried out by a commonly known gene manipulation method.
  • a physical method such as a method using a vector such as a virus, a non-viral method using a synthetic phospholipid or a synthetic cationic polymer, or an electrotransfer method in which a gene is introduced by applying temporary electrical stimulation to the cell membrane can be used , but is not limited thereto.
  • " amplification " in the present invention refers to amplification, substitution, or deletion of a part of the gene, introduction of a certain base, or introduction of a gene derived from another microorganism encoding the same enzyme to increase the activity of the corresponding enzyme .
  • the term " vector " means a DNA construct containing a DNA sequence operably linked to a suitable regulatory sequence capable of expressing the DNA in an appropriate host.
  • the vector may be a plasmid, phage particle, or simply a potential genome insert. Once transformed into the appropriate host, the vector may replicate and function independently of the host genome, or, in some cases, integrate into the genome itself. Because the plasmid is the most commonly used form of the current vector, the terms " plasmid " and " vector " are sometimes used interchangeably in the context of the present invention. However, the present invention includes other forms of vectors having functions equivalent to those known or known in the art.
  • &quot expression vector " is usually a recombinant carrier into which a fragment of different DNA is inserted, and generally means a fragment of double stranded DNA.
  • the heterologous DNA means a heterologous DNA that is not naturally found in the host cell.
  • the expression control sequence and the gene are contained within an expression vector containing a bacterial selection marker and a replication origin. If the expression host is a eukaryotic cell, the expression vector should further comprise a useful expression marker in the eukaryotic expression host.
  • &quot integrative vector &quot
  • integrative vector &quot means a vector in which integration or insertion into a nucleic acid is performed through integrase.
  • integrated vectors include retrovirus vector, transposon and adeno-associated viral vector. But is not limited to.
  • a host cell transformed or transfected with the vector constitutes another aspect of the present invention.
  • the term " transformation " means introducing DNA into a host and allowing the DNA to replicate as an extrachromosomal factor or by chromosomal integration. This includes any method of introducing the nucleic acid into an organism, cell, tissue or organ, and can be carried out by selecting a suitable standard technique depending on the host cell as is known in the art.
  • Such methods include electroporation, protoplast fusion, calcium phosphate (CaPO 4 ) precipitation, calcium chloride (CaCl 2 ) precipitation, agitation with silicon carbide fibers, Agrobacterium mediated transformation, PEG, dextran sulfate , Lipofectamine, and dry / inhibition-mediated transformation methods, and the like.
  • the host cell of the invention may be a prokaryotic or eukaryotic cell.
  • a host having high efficiency of introduction of DNA and high efficiency of expression of the introduced DNA is usually used.
  • Known eukaryotic and prokaryotic hosts such as Escherichia coli, Pseudomonas, Bacillus, Streptomyces, fungi and yeast, insect cells such as Spodoptera prolipida (SF9), animal cells such as CHO and mouse cells, COS 1, COS 7, BSC 1, BSC 40 and BMT 10, and tissue cultured human cells are examples of host cells that can be used.
  • the single cell host may be selected from a selected vector, the toxicity of the product encoded by the DNA sequence of the present invention, the secretion characteristics, the ability to fold the protein correctly, the culture and fermentation requirements, the product encoded by the DNA sequence of the invention And ease of purification.
  • one skilled in the art can select various vector / expression control sequences / host combinations that can express the DNA sequences of the invention in fermentation or in large animal cultures.
  • a binding method, a panning method, a film emulsion method, or the like can be applied as a screening method for cloning cDNA of NSP protein by expression cloning.
  • &quot means a technique of fusing two cells having different traits using a protoplast from which cell walls of plant cells or fungi have been removed.
  • Protoplast fusion involves the use of chemical methods such as the addition of metal ions such as calcium and magnesium to high osmotic solutions or physical exposure such as by increasing the DNA absorption of the protoplasts by exposing the protoplasts to temporary pores in the cell membrane, There is a way.
  • the "photoreactive functional group” may be a functional group capable of absorbing light of a specific wavelength upon irradiation with light and forming a covalent bond with an adjacent reactive functional group.
  • the Fc positionally-selective peptide with the photoreactive functional group of the present invention binds to or binds to the Fc domain of the antibody by its specificity as an inherent property when mixed with the antibody. Then, when the mixture is irradiated with light, it can absorb light of a specific wavelength and form a covalent bond with a reactive functional group on the adjacent antibody Fc domain through a photoreactive functional group. That is, the Fc position-selective binding peptide of the present invention can covalently bind to the specific functional group of the Fc domain through the photoreactive functional group upon light irradiation.
  • the amino acid having the photoreactive functional group may be p-benzoyl phenylalanine.
  • the artificial amino acid having a photoreactive functional group may be composed of a photoreceptor, a photomethionine or an azidophenylalanine.
  • the photoreactive functional group used in the present invention has a high wavelength band, that is, a low energy
  • the branch has specificity that the covalent bond is activated through light energy.
  • the p-benzoylphenylalanine of the present invention is represented by the following formula (1).
  • the present invention relates to a physiologically active substance which is formulated with a conjugate peptide in which a physiologically active substance is directly or linked to the peptide through a linker.
  • the physiologically active substance may be a therapeutic agent or a diagnostic agent.
  • the therapeutic agent or diagnostic agent may be an enzyme, hormone, cytokine, antibody, antibody fragment, analgesic agent, antipyretic agent, anti- A substance, an antiviral drug, an antifungal drug, a cardiovascular drug, a central nervous system drug, a kidney function and an electrolytic metabolism drug, and a chemotherapeutic agent.
  • the physiologically active substance of the present invention may be a therapeutic agent or a diagnostic / detection agent.
  • the antibody used as the physiologically active substance may be a therapeutic antibody.
  • Approximately 30 therapeutic antibodies have been approved by the FDA and their safety is very high because they closely resemble those of in vivo IgG.
  • Therapeutic antibodies have been used for a wide range of disease treatments (such as transplant rejection, cancer, autoimmune diseases and inflammation, heart disease and infectious infections, etc.).
  • the Fc domain-containing molecule is a therapeutic antibody
  • the therapeutic antibody recognizes and binds to a receptor protein or an antigenic protein specifically present in a disease-causing tissue, and therefore its specificity is very high.
  • a molecular imaging probe or a drug delivery vehicle when a molecular imaging probe or a drug delivery vehicle is combined with a therapeutic antibody as a physiologically active substance, it can be converted into a theragnosis agent capable of monitoring the therapeutic process together with a drug combination effect.
  • a molecular imaging probe or a drug delivery system by combining a molecular imaging probe or a drug delivery system with a simple targeting antibody, it is possible to develop a teraginosis preparation for diagnosis, treatment, or simultaneous diagnosis and treatment.
  • Non-limiting examples of therapeutic agents include antibodies, antibody fragments, drugs, toxins, nucleic acid hydrolases, hormones, immunomodulators, chelators, boron compounds, photoactive agents or dyes, and radioactive isotopes .
  • diagnostic / detection agents include, but are not limited to, an increase in radioisotopes, dyes (e.g., biotin-streptavidin complexes), contrast agents, fluorescent compounds or molecules and magnetic resonance imaging (MRI) (Paramagnetic ion).
  • the diagnostic agent comprises a radioactive isotope, an enhancer for use in magnetic resonance imaging, and a fluorescent compound.
  • a reactant having a long tail attached to many of the chelating groups to couple the ions.
  • the tail may be a polymer such as polylysine or polacacaride or a polymer such as ethylenediaminetetraacetic acid (EDTA), diethylenetriaminepentaacetic acid (DTPA), porphyrin, polyamine, crown ether, bis-thiosemic A chain having a pendant group capable of bonding with a chelating group such as a thiosemicarbazone, polyoximes, and a group known to be useful for the above purpose.
  • the chelate can normally be coupled to the Fc position-selective peptidic peptide by a minimal loss of immunoreactivity and a functional group capable of forming a bond to the molecule with minimal assembly and / or internal cross-linking.
  • Particularly useful metal-chelate combinations include diagnostic isotopes and 2-benzyl-DTPA and monomethyl and cyclohexyl analogues thereof used in the general energy range of 60 to 4,000 keV, for example, radioisotopes include 125 I , 131 I, 123 I, 124 I, 62 Cu, 64 Cu, 18 F, 111 In, 67 Ga, 99 mTc, 94 mTc, 11 C, 13 N, 15 O, 76 Br.
  • non-radioactive metals such as manganese, iron and gadolinium
  • the same chelate is useful for MRI when used with nanoparticles or antibodies of the present invention.
  • Macrocyclic chelates such as NOTA, DOTA, and TETA are used with a variety of metals and radioactive metals, preferably with radionuclides of gallium, yttrium and copper, respectively.
  • the metal-chelate complex can be made very stable by aligning the ring size with the metal of the object.
  • the present invention makes it possible to produce cyclic chelates such as macrocyclic polyethers useful for stably binding RAIT with nuclides such as 223Ra.
  • Immunoconjugates are conjugates of therapeutic or diagnostic agents and antibody components.
  • the diagnostic agent comprises a radioactive or non-radioactive label, a contrast agent (magnetic resonance imaging, computed tomography, or a contrast agent suitable for ultrasound), and the radioactive label includes gamma-, beta-, alpha-, It may be a positron emission isotope.
  • &quot typically stimulate immune cells that are proliferating or activating in an immune response cascade such as macrophages, B-cells, and / or T-cells.
  • An example of such an immunomodulator is a cytokine.
  • cytokine Those skilled in the art are a type of cytokine in which interleukins and interferons stimulate T-cell or other immune cell activity.
  • DNA deoxyribonucleic acid
  • RNA ribonucleic acid
  • PNA peptide nucleic acid
  • LNA locked nucleic acid
  • An Fc positionally-selected fused peptide in which the DNA, RNA, PNA or LNA is linked can be immobilized on a solid support for use as a biochip, a biosensor, an immune detection kit or a complementary self-addressable chip have.
  • the linker may include a reactive functional group, an amino acid, and a self-cleaving spacer.
  • the linker of the present invention may be in a form of linking a physiologically active substance with a specific residue in an Fc positionally selected binding peptide substituted with a photoreactive functional group and may include a nucleophilic residue For example, cysteine). ≪ / RTI >
  • the linker may comprise, for example, a reactive functional group, an amino acid, and a self-cleaving spacer that binds to an Fc positionally-selective fused peptide substituted with a photoreactive functional group.
  • the functional group may be selected from the group consisting of i) a maleimide group, an acetamide group or a derivative thereof, ii) an aziridine group, an aryl halide, an acryloyl group or a derivative thereof, iii) an alkylation reactor, an arylation reactor, pyridyldisulfide, Lysine, or a derivative thereof.
  • the linker includes, for example, i) a maleimide group or a derivative thereof-valine-citurline-para-aniline benzoic acid (PABA); Or ii) in the form of an acetamide group or a derivative thereof-valine-citurulline-para-aniline benzoic acid (PABA).
  • the binding of the Fc positionally-selective peptide and the physiologically active substance substituted with the photoreactive functional group through the linker can be carried out by a known method, for example, an alkylation, a disulfide interchange method, and a trans-esterification reaction method have.
  • a known method for example, an alkylation, a disulfide interchange method, and a trans-esterification reaction method have.
  • the conjugated peptide and the physiologically active substance can be conjugated to each other through the thiol group of the cysteine residue in the Fc positionally-selective peptide substituted with the photoreactive functional group.
  • the nucleophilic reactivity of the thiol of the cysteine residue to the maleimide group is dependent on the other amino acid functional groups present in the protein, such as the amino group of the lysine residue Terminal amino group, it can be utilized for specific binding to cysteine.
  • a physiologically active substance modulated with a maleimide group, a derivative thereof, or an acetamide group or a derivative thereof, for example, a bromoacetamide group or an iodoacetamide group is a cysteine-thioether bond and a photoreactive functional group It can be seen that the substituted Fc position selective binding peptide and the physiologically active substance are bound.
  • a method for producing a fusion protein comprising the steps of: (a) mixing a physiologically active substance formulated with a conjugated peptide with an Fc domain-containing molecule; (b) irradiating the mixture with light to generate a conjugate of an antibody-physiologically active substance to which a photoreactive functional group of the physiologically active substance modified with the conjugated peptide is bound to an Fc domain-containing molecule; And (c) a step of obtaining a conjugate of the antibody-biologically active substance.
  • the light may be 320 to 380 nm, and preferably 350 to 365 nm.
  • the present invention is not limited thereto.
  • the " Fc domain-containing molecule &quot includes, without limitation, a molecule including an Fc domain and capable of being adjacent or binding specifically recognized by an Fc position-selective junction peptide.
  • the Fc domain containing molecule includes a protein comprising an Fc domain, a peptide, a glycoprotein, a glycopeptide, an antibody, a fragment of an antibody, an immunoglobulin or an immunoglobulin fragment, and the like.
  • the antibody and immunoglobulin are heterotetrameric glycoproteins of about 150 kDa and comprise the same two light chains and the same two heavy chains.
  • Fc domain thereof may be an antibody or immunoglobulin light chain obtained by treating papain and a fragment from which the heavy chain has been removed.
  • the Fc domain-containing molecule may be a target-oriented natural or non-natural antibody capable of specifically binding to a target molecule.
  • the antibody includes both polyclonal and monoclonal antibodies as well as specific recombinant antibodies such as chimeric, humanized or human antibodies.
  • the antibody may be a receptor-specific antibody or a ligand-specific antibody.
  • the antibody may also be a receptor-specific antibody that does not prevent ligand binding but prevents receptor activation.
  • the antibody may be a therapeutic antibody, an antibody capable of binding with a separate therapeutic agent or diagnostic agent, an antibody for targeting without therapeutic effect, or an antibody capable of simply reacting with an antigen- Lt; / RTI >
  • the antibody-biomolecule conjugate can be used to maximize the advantages of antibodies such as specificity, non-toxicity in circulation and pharmacokinetics in the blood circulation, Specifically, it is a technology focused on targeting only specific tissues (for example, cancer cells).
  • an immunoconjugate includes anti-cancer drugs for " targeted chemotherapeutics ".
  • the immunoconjugate is composed of three components including a drug, a monoclonal antibody, and a linker linking the antibody and the drug.
  • the immunoconjugate technique is a technique in which a specific antigen A method for delivering a substance having physiological activity to tumor cells using an antibody that specifically binds to tumor cells.
  • the physiologically active compound is selected from the group consisting of beta-lactamase (TEM-1), beta-lactamase zymogen (Korean Patent No. 1016956840000 (2017.01. 06) and Pseudomonas exotoxin A (PE24) were used.
  • TEM-1 beta-lactamase
  • beta-lactamase zymogen Korean Patent No. 1016956840000 (2017.01. 06)
  • PE24 Pseudomonas exotoxin A
  • " ß-lactamase " (amino acid sequence number 3) is not cytotoxic in itself, but a prodrug having a beta-lactam ring is cleaved to activate the drug As a mechanism, it can be used as an effective tumor treatment drug when treated with an appropriate prodrug.
  • an inactive prodrug such as GC-mel can be used.
  • ⁇ -lactamase zymogen amino acid SEQ ID NO: 5
  • BLIP ⁇ -lactamase inhibitor protein
  • MMP-2 matrix metalloproteinase-2
  • " PE24 " (amino acid sequence number 7) binds EF-2 by ADP-ribosylation of elongation factor-2 (EF-2) And activates to induce apoptosis of cells (U.S. Patent No. 09388222 (Jul. 12, 2016)).
  • the Fc domain-containing molecule may be characterized in that it is selected from the group consisting of immunoglobulin-derived domains, combinations thereof, and Fc regions thereof.
  • IgG is selected from the group consisting of IgG, IgA, IgD, IgE, IgM, combinations thereof, and the Fc region thereof, and more preferably IgG1 or an Fc region thereof But is not limited thereto.
  • step (c) since FcIII binds to the Fc domain of the heavy chain of the antibody, when the fusion protein and the antibody are photoreactive, A form in which a physiologically active substance immobilized on one antibody, a form in which a physiologically active substance immobilized on one antibody, a form in which a physiologically active substance immobilized on one antibody, a form in which a physiologically active substance immobilized on one antibody and a physiologically active substance modulated on two antigenic peptides are bound to an antibody).
  • An antibody-biologically active substance conjugate in which a physiologically active substance formulated with one conjugated peptide is conjugated has a structure in which one neonatal Fc receptor (FcRn) is free, , It can not be decomposed and a high half-life of the drug can be expected.
  • FcRn neonatal Fc receptor
  • Antibodies that do not bind a physiologically active substance formulated with a conjugated peptide can be removed by optimizing the reaction conditions by controlling the reaction ratio of the antibody and the fusion protein and the ultraviolet irradiation time.
  • a conjugate of an antibody-physiologically active substance conjugated with a physiologically active substance conjugated with one conjugated peptide and a conjugate of an antibody-physiologically active substance conjugated with a biologically active substance conjugated with two conjugated peptides is a conjugate between the protein A and the Fc domain of the antibody Can be separated using binding affinity. Since Protein A has specific binding affinity to the CH 2 -CH 3 domain interface of the Fc domain of the antibody, affinity chromatography resins used for purification after antibody expression, .
  • antibody-biologically active substance conjugates in which the biologically active substance formulated with two conjugated peptides are bound to the antibody do not bind to the protein A resin (WL DeLano et al, Science , 287 (5456): 1279-83, 2000) .
  • the form in which the two physiologically active substances are bound to the antibody can be removed by protein A affinity chromatography and then subjected to anion chromatography successively on the resulting product to cause binding due to the difference in isoelectric point
  • a form in which a physiologically active substance formulated with one conjugated peptide is bound to the antibody can be isolated.
  • the present invention relates to a conjugate of an antibody-biologically active substance in which an antibody is bound to a physiologically active substance formulated with the conjugated peptide.
  • WST-8 and MTS essays were performed to confirm the activity of the IgG1-FcIII-PE24 conjugate.
  • the WST-8 and MTS essays are transformed into mitochondrial succinate dehydrogenase, which is produced by bacteria in the medium, into tetrazolium salt (Formazan), which can be measured at a specific absorbance , And the survival of the cells can be confirmed by measuring the absorbance.
  • the absorbance changes were measured while increasing the concentrations of the three antibody-physiologically active substance conjugates within a specific range. As a result, it was observed that cell proliferation and viability decreased as the conjugate of the antibody-biologically active substance conjugated with the physiologically active substance modified with the antibody and the conjugated peptide was treated at a high concentration. Thus, it was confirmed that the antibody-biologically active substance conjugate of the present invention can be used as a therapeutic drug.
  • trastuzumab acts specifically on HER2 that forms a heterodimer with EGFR or HER4 to inhibit the activation of ligands EGFR (EGF, TGFa) or HER4 (NRG1) Lt; / RTI > Cetuximab also inhibits the activation of EGFR, which is dependent on ligands (EGF, TGFa), and prevents its downregulation.
  • human IgG1 and FcIII peptide (amino acid sequence number 11, gene sequence number 12) in which the DNA sequence at the 5th position in the amino acid sequence was substituted with an amber codon
  • FcIII peptide (amino acid sequence SEQ. ID. NO. 13, gene SEQ. ID NO. 14) in which the DNA sequence of the position was replaced with an amber codon
  • FcIII peptide in which the DNA sequence at the 11th position was substituted with an amber codon No. 16
  • the sample was then subjected to a UV hand ramp (Lklab, U01-133-194) on 1xPBS buffer (pH 7.4) And irradiated with ultraviolet light of 365 nm for 2 hours.
  • the FcIII peptide gene in which the gene coding for the 10th amino acid was substituted with an amber codon was digested with NheI in 2.1 NEB buffer, and the gene was cut using a spin column And then cleaved by treatment with BamHI in 3.1 NEB buffer.
  • the composition of the buffer was DDW, 10x NEB buffer 3.1, DNA, restriction enzyme, and the total volume was 50 ⁇ l, and the treatment conditions were 37 ° C for 4 hours, respectively.
  • a pET21-a vector digested with sticky ends at both ends was treated with the same restriction enzymes and the cleaved FcIII gene was mixed at a molar ratio of 1: 3 to make a total volume of 10 mu l. Then, T4 DNA ligase ( NEB, England) for 2 hours at room temperature.
  • the ligation mixture was mixed with 50 ⁇ l of competent cell, E. coli DH10B (Thermosensific, C640003), and electroporation (Bio-Rad, USA) was performed. Then, the transformed strain was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing ampicillin to obtain a transformed strain. FcIII expression plasmid-1 was obtained by DNA prep (GeneAll, mini prep kit) Respectively.
  • a plasmid (pSPEL104) containing the entire sequence of ⁇ -lactamase represented by SEQ ID NO: 4 was amplified by polymerase chain reaction (PCR) using the primer shown in Table 1 as a template, and BamHI and NotI Treated with restriction enzymes, and then ligated to the FcIII expression plasmid-1 of Example 1.
  • PCR is performed in three steps of denaturation, annealing, and amplification, and the method is as follows.
  • the reaction composition of the PCR is DDW, 10x pfu buffer, 0.2mM dNTP, 20pmol primer F / R, template, 5units Pfu polymerase, and the final reaction volume is 50 ⁇ l.
  • the reaction was carried out at 95 ° C for 2 minutes using BamhI -f and TEM1-NotI-r in Table 1, followed by 25 cycles of 95 ° C for 30 seconds, 55 ° C for 30 seconds, and 72 ° C for 1 minute, And then treated at 72 ⁇ for 10 minutes.
  • Table 1 shows PCR primers used in the present invention.
  • the two restriction enzymes were cleaved by treatment with 3.1 NEB buffer.
  • the composition of the buffer was DDW, 10x NEB buffer 3.1, DNA, restriction enzyme, total volume 50 ⁇ l, and treated at 37 ° C for 4 hours.
  • the FcIII-expressing plasmid-1 digested with sticky ends at both ends was mixed with ⁇ -lactamase at a molar ratio of 1: 3, and the total volume was adjusted to 10 ⁇ l.
  • T4 DNA ligase (NEB) Lt; RTI ID 0.0 > 25 C < / RTI > for 2 hours.
  • the ligated DNA mixture solution was added to 50 ⁇ l of competent cell E. coli DH10B (Thermosensific, C640003), followed by mixing and electroporation (Bio-Rad, USA). Then, the transformed strain was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing ampicillin to obtain a transformed strain. FcIII- ⁇ -lactamase (amino acid sequence number 17 , Gene SEQ ID NO: 18) expression plasmids were obtained (Fig. 3).
  • a plasmid (pSPEL166) containing the ß-lactamase zymogen sequence (1353 bp) represented by SEQ ID NO: 6 was amplified by PCR using the primers shown in Table 1 under the same conditions as the above conditions and then PCR was performed using NcoI and NotI restriction After digestion with the enzyme, the FcIII expression plasmid-2 of Example 1 was ligated in the same manner as described above.
  • the ligation mixture was added to 50 ⁇ l of E. coli DH10B (Thermosensific, C640003), followed by electroporation (Bio-Rad, USA). Then, the transformant was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing ampicillin, and the transformed strain was obtained.
  • FcIII- ⁇ -lactamase zymogen amino acid sequence No. 19, gene SEQ. ID No. 20 expression plasmids (FIG. 4).
  • PE24 expressed by de-immunized SEQ ID NO: 8 was obtained by gene synthesis (Bioneer) and then digested with BamHI and NotI restriction enzymes in the same manner as described above, and then ligated to FcIII expression plasmid-1.
  • the ligation mixture was added to 50 ⁇ l of E. coli DH10B (Thermosensific, C640003), followed by electroporation (Bio-Rad, USA). Then, the transformed strain was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing ampicillin to obtain a transformed strain.
  • FcIII-PE24 fusion protein amino acid sequence number 21 , Gene SEQ ID NO: 22 expression plasmid was obtained (Fig. 5).
  • a tRNA sequence recognizing the TAG codon (Jason W. Chin et al., PNAS vol. 99 ) was obtained by digesting SalI and BglII with the p-benzoylphenylalanine tRNA synthetase (amino acid SEQ . , 11020-11024, 2002) was used as a vector (Fig. 6A).
  • the ligation mixture was added to 50 ⁇ l of E. coli DH10B (Thermosensific, C640003), followed by electroporation (Bio-Rad, USA). Then, the transformant was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing chloramphenicol to obtain a transformed strain.
  • the TAG codon was recognized by DNA prep (GeneAll, mini prep kit) And a tRNA synthetase (gene SEQ. ID NO: 23) expression plasmid for inserting benzoyl phenylalanine was obtained.
  • a pBbS2K plasmid containing a proline tRNA synthetase sequence was used (Byeong Sung Lee et al., Biochimica Biophysica Acta , S0304-4165, 2017) (FIG.
  • Example 3 Expression and purification of physiologically active substance formulated with conjugated peptides
  • plasmids containing the FcIII-ß-lactamase expression plasmid, TAG codon cognitive tRNA and p-benzoylphenylalanine tRNA synthetase pair and plasmid containing proline tRNA synthetase were transformed into E. coli BL21 (DE3) (SIGMA aldrich, CMC0016), and then plated on an LB plate containing ampicillin, chloramphenicol, and kanamycin to obtain a transformed strain.
  • the obtained single colonies were seeded at 37 ° C and 180 rpm for 12 hours, seeded at a ratio of 10: 1, and incubated at 37 ° C and 180 rpm for 6 hours.
  • the culture was inoculated at a ratio of 100: 1 to 200 ml of 2xYT (including ampicillin, chloramphenicol, and kanamycin) medium and cultured at 37 ° C and 180 rpm.
  • 2xYT including ampicillin, chloramphenicol, and kanamycin
  • FcIII- ⁇ -lactamase In order to purify the expressed FcIII- ⁇ -lactamase, it was centrifuged at 4 ° C. and 9300 g for 15 minutes. The supernatant was then removed and resuspended in 5 ml of lysis buffer (0.75 M sucrose, 0.1 Tris, pH 8.0), added with 0.05 ml / l of lysozyme and 1 ml of 1 mM EDTA, And rotated for a minute. Then, 1 ml of 0.5 M MgCl 2 was added and the mixture was rotated at 4 ° C for 10 minutes. The mixture was centrifuged at 4 ° C and 9300g for 15 minutes, and the supernatant was separated.
  • lysis buffer (0.75 M sucrose, 0.1 Tris, pH 8.0
  • Example 3-2 Expression and purification of FcIII-ß-lactamase zymogen
  • FcIII-ß-lactamase zymogen For the expression of FcIII-ß-lactamase zymogen, plasmids containing the FcIII-ß-lactamase zymogen expression plasmid, TAG codon cognate tRNA and p-benzoylphenylalanine tRNA synthetase pair and plasmid containing proline tRNA synthetase were transformed into E. coli BL21 DE3) (SIGMA aldrich, CMC0016) and then expressing FcIII- ⁇ -lactamase zymogen in the same manner as the expression of FcIII- ⁇ -lactamase.
  • the purification reaction was performed under the same conditions as those for the purification of FcIII- ⁇ -lactamase to elute the 6 ⁇ His-tagged FcIII- ⁇ -lactamase zymogen.
  • FcIII-PE24 For expression of FcIII-PE24, a plasmid containing the FcIII-PE24 expression plasmid, a pair of TAG codon cognition tRNA and p-benzoylphenylalanine tRNA synthetase, and a proline tRNA synthetase was transformed into E. coli BL21 (DE3) (SIGMA aldrich, CMC0016) and then expressing FcIII-PE24 in the same manner as that of FcIII- ⁇ -lactamase.
  • E. coli BL21 DE3 (SIGMA aldrich, CMC0016)
  • Example 4 Binding of physiologically active substances formulated with cetuximab and conjugated peptides and isolation and activity of conjugates
  • Example 4-1 Confirmation of binding of physiologically active substance formulated with cetuximab and conjugated peptide
  • Example 4-2 Separation of conjugate of antibody-biologically active substance conjugated with physiologically active substance modified with cetuximab and conjugated peptide
  • an antibody-physiologically active substance conjugate conjugated with an antibody to the physiologically active substance formulated with the conjugate peptide of Example 4 After mixing with 5 ml 1 ⁇ PBS (pH 7.4), 1 ml of Protein A 50% resin slurry (CaptivA Protein A resin, Repligen) was added and the mixture was rotated at 4 ° C for 1 hour and 30 minutes. After loading the reaction solution into an empty column, the resin was completely submerged and washed by loading 30 ml of 1 ⁇ PBS (pH 7.4). Then, 5 ml of elution buffer (pH 3.0 0.1 M Glycine) was loaded to obtain a product, and 125 ⁇ l of neutralization buffer (pH 9.0 Tris) was added to titrate the pH.
  • elution buffer pH 3.0 0.1 M Glycine
  • the obtained product was a mixture of an antibody-physiologically active substance conjugate conjugated with a physiologically active substance modulated with one conjugated peptide and an antibody not conjugated (FIG. 10).
  • Example 4-3 Confirmation of EF2 ribosylation activity of Cetuximab-FcIII-PE24 conjugate
  • ADP-ribosylation activity of the Cetuximab-FcIII-PE24 conjugate was measured by the method of Zhang and Snyder.
  • the PE24 and Cetuximab-FcIII-PE24 conjugates were diluted to 1 nM in 20 mM Tris-HCl (pH 7.4), 1 mM EDTA, 1 mM DTT and incubated with wheat germ extract in the presence of 50 nM biotinylated NAD + Lt; / RTI > The reaction was then terminated with 5x sodium dodecyl sulfate (SDS) gel loading buffer. Proteins were separated on SDS-12% (w / v) polyacrylamide gel. Biotinylated EF-2 was detected by Western blot using a streptavidin-horseradish peroxidase (HRP) conjugate. Western blot images were analyzed using a ChemiDoc XRS system.
  • cell viability assay was performed using a cell line overexpressing EGFR, a specific antigen to which Cetuximab binds, on the cell surface.
  • EGFR cell line A431 (SIGMA aldrich, 85090402) was cultured in DMEM medium (10% FBS, streptomycin) and cultured in 96-well plate at 2 ⁇ 10 3 cells / well. After 24 hours, Cetuximab-FcIII-PE24 was treated at a concentration of 0 nM, 0.016 nM, 0.16 nM, 1.6 nM and 16 nM and cultured at 37 ° C, 5% CO 2 for 72 hours. Then, the MTS solution (Promega, G3580) was treated with 20 ⁇ l / well and the absorbance at 490 nm was measured after 2 hours.
  • MTS solution Promega, G3580
  • Example 5 Binding of physiologically active substances formulated with Trastuzumab and conjugated peptides and isolation and activity of conjugates
  • a conjugate of an antibody-biologically active substance conjugated with an antibody to a physiologically active substance formulated with the conjugated peptide of Example 4 (CaptivA Protein A resin, Repligen) was added to 1 ml of a Protein A 50% resin slurry, which was then rotated for 1 hour and 30 minutes at 4 ° C. The reaction solution was transferred to an empty column After loading, the resin was completely submerged and washed by loading 30 ml of 1xPBS (pH 7.4). The product was then loaded by loading 5 ml of elution buffer (pH 3.0 0.1M Glycine), and 125 ⁇ l of The pH was titrated by adding neutralizing buffer (pH 9.0 Tris).
  • the obtained product was a mixture of antibody-biomolecule conjugate conjugated with physiologically active substance modified with one conjugated peptide and antibody not conjugated (FIG. 13).
  • the resultant product was continuously mixed with 20 mM phosphate buffer (pH 7.9) and subjected to anion chromatography (mono-Q column, GE Healthcare Life Science, USA) The form in which the active substance was bound to the antibody was isolated and confirmed (Fig. 13).
  • the cell viability assay (cell viability assay (cell viability assay) was performed using cell lines overexpressing HER2, a specific antigen to which Trastuzumab binds, ) Were performed.
  • HER2 overexpressing cell line MDA-MB-231 (Korean Cell Line Bank, 60062), HCC-1954 (Korean Cell Line Bank, 9S1954), MDA-MB- Korean Cell Line Bank, 30026) were cultured in RPMI medium (10% FBS, streptomycin) and cultured in 3-5 ⁇ 10 3 cells / well on 96-well plates.
  • trastuzumab-FcIII-PE24 was treated at concentrations of 0 nM, 0.0064 nM, 0.032 nM, 0.16 nM, 0.8 nM, 4 nM and 20 nM and cultured at 37 ° C and 5% CO 2 for 72 hours.
  • the WST-8 solution (Dojindo, CK04-11) was treated with 10 ⁇ l / well, and the absorbance at 450 nm was measured after 2 hours.
  • trastuzumab-FcIII-PE24 conjugate As a result, the higher the concentration of Trastuzumab-FcIII-PE24 conjugate was, the lower the absorbance of HER2-overexpressing cells was, and the cell viability was markedly decreased as compared with the wild type trastuzumab and PE24 treated wells. In contrast, it was confirmed that the cytotoxicity of trastuzumab-FcIII-PE24 conjugate did not act in the corresponding concentration range for HER2 non-expressing cells (FIG. 14).
  • a physiologically active substance modified with a conjugated peptide is prepared by using an Fc positionally selected binding peptide in which a specific position according to the present invention is substituted with a photoreactive functional group and then the antibody and the physiologically active substance are bound through a photoreaction
  • the material can be linked to the antibody in a selective and highly efficient manner through a simple photoreaction. Therefore, the present invention can be used for the production of antibody-physiologically active substance conjugates in which various kinds of physiologically active substances and antibodies are linked, and the commercialization thereof can be accelerated.

Abstract

The present invention relates to an antibody-conjugated peptide substituted with an amino acid having a photoreactive functional group, a physiologically active substance formulated with the conjugated peptide, and an antibody-physiologically active substance conjugate having an antibody bound to the physiologically active substance. When the physiologically active substance formulated with the conjugated peptide according to the present invention is bound to the antibody, binding efficiency between the antibody and the physiologically active substance is remarkably improved as compared to that of the conventional art, and thus, the drug may be firmly bound without impairing the specificity of the antibody, thereby making it possible to accelerate commercialization of the antibody-physiologically active substance conjugate.

Description

항체와 생리활성물질의 접합방법Method of conjugating antibody and physiologically active substance
본 발명은 서열번호 1의 아미노산 서열로 표시되는 Fc 위치선택적 결합 펩티드에서 5번째, 10번째 또는 11번째 위치가 광반응성 작용기를 갖는 아미노산으로 치환된 Fc 위치선택적 접합 펩티드, 상기 접합 펩티드로 수식화된 생리활성물질, 상기 생리활성물질에 항체가 결합되어 있는 항체-생리활성물질 접합체 및 상기 항체-생리활성물질 접합체의 제조방법에 관한 것이다.The present invention relates to an Fc position-selective fused peptide in which the 5th, 10th or 11th position of the Fc position-selective binding peptide represented by the amino acid sequence of SEQ ID NO: 1 is substituted with an amino acid having a photoreactive functional group, An active substance, an antibody-physiologically active substance conjugate in which an antibody is bound to the physiologically active substance, and a method for producing the antibody-physiologically active substance conjugate.
지난 20년간 항체공학은 생쥐에서 단클론 항체(monoclonal antibody, mAb)를 개발하는 하이브리도마(hybridoma) 기술을 바탕으로 키메릭 항체(chimeric mAb), 인간화 항체(humanized mAb) 및 인간 항체(fully human mAb)의 제조기술 개발로 거듭났으며, 지금은 항체가 하나의 치료용 약물(therapeutic mAb)로서 인정받고 있다. 현재까지 FDA의 승인을 받은 치료용 항체는 28가지로 이식거부반응, 암, 자가면역질환, 염증, 심장질환, 전염성 감염 등의 광범위한 질병치료제로서 사용되고 있으며, 약 300여 종의 치료용 항체가 현재 임상개발 단계에 있어 앞으로 더 많은 치료용 항체가 개발되는 동시에 상업화될 것으로 전망된다. 또한 나아가 기존의 항체(naked mAb)보다 효능을 향상시킨 차세대 치료용 항체 개발을 위한 많은 연구가 진행 중이다. 이 중 특정 항원에 대한 특이성을 갖는 단클론 항체와 생물학적 활성을 갖고 있는 생리활성물질을 연결한 접합체에 대한 연구는 활발하게 진행되고 있다. 이들 항체-생리활성물질 접합체가 치료용 약물로 개발되었을 때, 항체의 표적 특이성을 통한 생리활성물질의 높은 효능과 낮은 부작용을 기대할 수 있을 뿐만 아니라, 항체의 체내 비독성과 낮은 면역원성, 긴 체내 반감기 등의 특성은 개발된 항체-생리활성물질 접합체 약물의 상업화를 가속화할 수 있는 요소이다. 항체와 세포 독성을 갖는 소분자 약물을 연결한 접합체(ADC: antibody-drug conjugate)는 제약사들에 의해서 이미 개발되어 종양 표적 치료제로 사용되고 있다.Over the last twenty years, antibody engineering has been used to develop chimeric mAbs, humanized mAbs, and fully human mAbs based on hybridoma technology, which develops monoclonal antibodies (mAbs) in mice. ), And now antibodies are recognized as a therapeutic drug. There are 28 therapeutic antibodies approved by the FDA to date, and they are used for the treatment of a wide range of diseases such as graft rejection, cancer, autoimmune disease, inflammation, heart disease, infectious infection, etc. About 300 therapeutic antibodies In the clinical development stage, more therapeutic antibodies are expected to be developed and commercialized in the future. In addition, many studies are underway to develop next-generation therapeutic antibodies that have improved efficacy over conventional antibodies (naked mAbs). Among them, studies on conjugates between monoclonal antibodies having specificity for specific antigens and physiologically active substances having biological activity have been actively conducted. When these antibody-biologically active substance conjugates are developed as therapeutic drugs, not only high efficacy and low side effects of physiologically active substances due to the target specificity of the antibodies can be expected, but also the non-toxicity of antibodies, low immunogenicity, And half-life characteristics are factors that can accelerate the commercialization of the developed antibody-biologically active substance conjugate drug. An antibody-drug conjugate (ADC), which links antibodies and cytotoxic small molecule drugs, has already been developed by pharmaceutical companies and is being used as a tumor-targeting agent.
치료용 약물로 개발함에 있어서, 항체-생리활성물질 접합체는 접합되지 않은 항체와 생리활성물질의 특성을 보유해야 한다. 항체-생리활성물질 접합체는 생리활성물질과 결합되기 전의 항체와 같은 친화력을 유지할 수 있어야 한다. 즉, 항체와 생리활성물질 결합으로 인해 본연의 항원-항체 결합이 저해되어서는 안된다. 또한, 항체-생리활성물질 접합체의 생리활성물질도 표적에 도달한 후 활성을 나타낼 수 있어야 한다. 즉, 항체-생리활성물질 접합체에 있어서 단클론 항체와 생리활성물질 각각의 내재적 특성은 유지되어야 하고, 이는 두 물질을 접합하는 방법에 의해서 결정된다. 또한, 접합에 사용되는 링커는 혈액에서도 안정하여 생리활성물질이 항체로부터 분리되는 것을 방지하고 표적 조직/세포에 도달할 수 있도록 해야 한다. 일반적으로 항체-생리활성물질 접합체에 사용되는 링커로는 산성에 불안정한 히드라존(acid-labile hydrazone), 단백질분해효소에 불안정한 펩티드(protease-labile peptide) 및 환원제(reducing agent)에 민감한 이황화물(disulfide)이 있다. 또한 절단되지 않는(non-cleavable) 티올에테르(thioether) 링커도 사용된다. 항체와 생리활성물질의 접합을 위하여 항체가 갖고 있는 작용기(라이신의 ε-아미노기 또는 시스테인의 티올기)나 돌연변이에 의해 항체에 시스테인 잔기를 도입하고 이의 티올기의 반응성을 이용하는 방법이 일반적으로 사용된다. 항체 자체의 작용기를 이용하는 방법은 생리활성물질이 연결되는 위치를 조정할 수 없고, 항체 대 생리활성물질의 물비도 일정하지 않아 불균일한 항체-생리활성물질 접합체를 만들게 된다. 항체에 인위적으로 도입된 시스테인의 티올기를 이용하는 경우에는 항체에 돌연변이를 일으켜야하고, 이로 인한 항체 자체의 구조와 활성에 영향을 예측하기 어렵다.In the development of therapeutic drugs, antibody-biologically active substance conjugates should retain the properties of unbound antibodies and physiologically active substances. The antibody-biologically active substance conjugate should be able to maintain affinity with the antibody prior to binding to the physiologically active substance. That is, the binding of the antibody and the bioactive substance should not inhibit the inherent antigen-antibody binding. In addition, the physiologically active substance of the antibody-physiologically active substance conjugate should be able to exhibit activity after reaching the target. That is, in the antibody-physiologically active substance conjugate, the intrinsic properties of each of the monoclonal antibody and the physiologically active substance should be maintained, which is determined by the method of conjugating the two substances. In addition, the linker used for conjugation should be stable in the blood to prevent the biologically active substance from separating from the antibody and to reach the target tissue / cell. Generally, linkers used in antibody-biologically active substance conjugates include acid-labile hydrazone, protease-labile peptide, and disulfide (reducing agent) sensitive to a reducing agent. ). Non-cleavable thioether linkers are also used. A method of introducing a cysteine residue into an antibody by using a functional group (lysine epsilon-amino group or cysteine thiol group) or mutation and using the reactivity of the thiol group is commonly used for conjugation of an antibody and a physiologically active substance . In the method using the functional group of the antibody itself, the position where the physiologically active substance is connected can not be adjusted, and the water ratio of the antibody to the physiologically active substance is not constant, so that a heterogeneous antibody-physiologically active substance conjugate is produced. When the thiol group of the cysteine introduced into the antibody is used, it is difficult to predict the effect on the structure and activity of the antibody due to the mutation in the antibody.
최근, 항체의 Fc 도메인에 특이적으로 결합하는 Fc 도메인 결합 펩티드(미국공개특허 제20040253247호(2004.12.16))에 광조사에 의해 공유결합하는 광반응성 인공 아미노산을 치환시켜 저분자 펩티드 변이체를 제조하고, 상기 제조된 저분자 펩티드 변이체에 약물을 결합한 항체-약물 접합체를 제조하는 방법이 보고되었다(대한민국공개특허 제10-2014-0004530호(2014.01.13)). 하지만, 상기 발명에서 사용된 펩티드 물질은 화학합성을 통해서 제조해야 하고, 이 때문에 접합방법은 약물을 항체에 접합하는 경우에 한정되고 단백질 같은 생리활성물질과 항체의 접합에는 사용하기 어렵다. 또한, 발명에서 사용한 광반응성 아미노산(실험예: 포토루신, 포토메티오닌 이용)의 비특이적인 반응성으로 항체-생리활성물질 접합체를 의약품으로 개발하는데 문제점을 가지고 있다(Yoshihito Tanaka et al, Molecular BioSystems, 4(6):473-480, 2008).Recently, a low-molecular peptide mutant was prepared by substituting a photoreactive artificial amino acid covalently bound to an Fc domain binding peptide (US Patent Publication No. 20040253247 (2004.12.16)) that specifically binds to the Fc domain of an antibody by light irradiation , A method of producing an antibody-drug conjugate in which a drug is bound to the above-prepared low molecular weight peptide mutant has been reported (Korean Patent Publication No. 10-2014-0004530 (Jan. However, the peptide material used in the present invention must be prepared through chemical synthesis. Therefore, the conjugation method is limited to the case where a drug is conjugated to an antibody, and it is difficult to use it for conjugation of an antibody and a physiologically active substance such as a protein. In addition, the non-specific reactivity of the photoreactive amino acids used in the present invention (experiment examples: using fluorescein and photomethionine) has a problem in developing a conjugate of an antibody-biologically active substance into a drug (Yoshihito Tanaka et al., Molecular BioSystems, 6): 473-480, 2008).
이에, 본 발명자들은 항체 Fc 도메인에 특이적으로 결합가능한 Fc 위치선택적 결합 펩티드의 특정 위치를 광반응성 작용기를 갖고 있는 아미노산(para-benzophenylalanine(pBpa))으로 치환한 Fc 위치선택적 접합 펩티드를 개발하였고, 상기 접합 펩티드로 수식화된 생리활성물질을 제조한 후, 광반응을 통해 항체와 상기 생리활성물질을 결합시킨 결과, 간단한 광반응을 통해서 생리활성물질이 항체에 위치 선택적이고 고효율로 결합하는 것을 확인하고, 본 발명을 완성하게 되었다.Accordingly, the present inventors have developed an Fc position-selective peptide in which a specific position of an Fc position-selective binding peptide capable of specifically binding to an antibody Fc domain is replaced with an amino acid having a photoreactive functional group (para-benzophenylalanine (pBpa) As a result of binding the antibody and the physiologically active substance through a photoreaction after the preparation of the physiologically active substance modified with the conjugated peptide, it was confirmed that the physiologically active substance binds to the antibody locally and highly efficiently through a simple photoreaction , Thereby completing the present invention.
본 배경기술 부분에 기재된 상기 정보는 오직 본 발명의 배경에 대한 이해를 향상시키기 위한 것이며, 이에 본 발명이 속하는 기술분야에서 통상의 지식을 가지는 자에게 있어 이미 알려진 선행기술을 형성하는 정보를 포함하지 않을 수 있다.The information described in the Background section is intended only to improve the understanding of the background of the present invention and thus does not include information forming a prior art already known to those skilled in the art .
발명의 요약SUMMARY OF THE INVENTION
본 발명의 목적은 광반응을 통해 항체와 생리활성물질을 위치 특이적으로 접합시킬 수 있는 펩티드를 제공하는 데 있다.It is an object of the present invention to provide a peptide capable of specifically binding an antibody and a physiologically active substance through a photoreaction.
본 발명의 다른 목적은 상기 펩티드로 수식화된 생리활성물질을 제공하는 데 있다.It is another object of the present invention to provide a physiologically active substance formulated with the peptide.
본 발명의 또 다른 목적은 상기 생리활성물질과 항체가 연결된 항체-생리활성물질 접합체의 제조방법을 제공하는 데 있다.It is still another object of the present invention to provide a method for producing a conjugate of an antibody-biologically active substance to which the above-mentioned physiologically active substance and an antibody are linked.
본 발명의 또 다른 목적은 상기 제조방법으로 제조된 항체-생리활성물질 접합체를 제공하는 데 있다.It is still another object of the present invention to provide a conjugate of an antibody-biologically active substance produced by the above-described method.
상기 목적을 달성하기 위해서, 본 발명은 서열번호 1의 아미노산 서열로 표시되는 Fc 위치선택적 결합 펩티드에서 5번째, 10번째 또는 11번째 위치가 광반응성 작용기를 갖는 아미노산으로 치환된 Fc 위치선택적 접합 펩티드를 제공한다.In order to achieve the above object, the present invention provides an Fc position-selective fused peptide wherein the 5th, 10th or 11th position of the Fc position-selective binding peptide represented by the amino acid sequence of SEQ ID NO: 1 is substituted with an amino acid having a photoreactive functional group to provide.
본 발명은 또한, 상기 펩티드에 생리활성물질이 직접 또는 링커를 통해 연결되어 있는 접합 펩티드로 수식화된 생리활성물질을 제공한다.The present invention also provides a physiologically active substance modified with a conjugate peptide in which a physiologically active substance is directly or linked to the peptide through a linker.
본 발명은 또한, (a) 상기 접합 펩티드로 수식화된 생리활성물질을 Fc 도메인 함유 분자와 혼합하는 단계; (b) 상기 혼합물에 광을 조사하여 상기 접합 펩티드로 수식화된 생리활성물질의 광반응성 작용기와 Fc 도메인 함유 분자가 결합된 항체-생리활성물질 접합체를 생성시키는 단계; 및 (c) 상기 생성된 항체-생리활성물질 접합체를 수득하는 단계를 포함하는 항체-생리활성물질 접합체의 제조방법을 제공한다.(A) mixing a physiologically active substance formulated with the conjugated peptide with an Fc domain containing molecule; (b) irradiating the mixture with light to generate a conjugate of an antibody-physiologically active substance to which a photoreactive functional group of the physiologically active substance modified with the conjugated peptide is bound to an Fc domain-containing molecule; And (c) a step of obtaining a conjugate of the antibody-biologically active substance as described above.
본 발명은 또한, 상기 접합 펩티드로 수식화된 생리활성물질에 항체가 결합되어 있는 항체-생리활성물질 접합체를 제공한다.The present invention also provides an antibody-physiologically active substance conjugate wherein an antibody is bound to a physiologically active substance formulated with the conjugated peptide.
도 1은 본 발명의 항체와 생리활성물질의 접합기술을 나타낸 모식도이다.BRIEF DESCRIPTION OF THE DRAWINGS FIG. 1 is a schematic view showing a technique of bonding an antibody of the present invention to a physiologically active substance. FIG.
도 2는 본 발명의 FcIII 펩티드의 p-벤조일 페닐알라닌의 치환 위치를 결정하기 위하여, 항체와 상기 펩티드로 수식화된 생리활성물질을 광반응시킨 후 전기영동한 결과이다.FIG. 2 is a result of electrophoresis after photo-reacting an antibody and a physiologically active substance formulated with the peptide to determine the substitution position of p-benzoylphenylalanine of the FcIII peptide of the present invention.
도 3은 본 발명의 FcIII 펩티드로 수식화된 ß-lactamase(FcIII-ß-lactamase) 발현 플라스미드 및 상기 플라스미드에서 발현된 FcIII-ß-lactamase를 개략적으로 나타낸 것이다.FIG. 3 is a schematic representation of β-lactamase (FcIII-β-lactamase) -expressing plasmid modified with the FcIII peptide of the present invention and FcIII-β-lactamase expressed in the plasmid.
도 4는 본 발명의 FcIII 펩티드로 수식화된 ß-lactamase zymogen(FcIII-ß-lactamase zymogen) 발현 플라스미드 및 상기 플라스미드에서 발현된 FcIII-ß-lactamase zymogen을 개략적으로 나타낸 것이다.FIG. 4 schematically shows a plasmid expressing β-lactamase zymogen (FcIII-β-lactamase zymogen) modified with the FcIII peptide of the present invention and FcIII-β-lactamase zymogen expressed in the plasmid.
도 5는 본 발명의 FcIII 펩티드로 수식화된 PE24(FcIII-ß-PE24) 발현 플라스미드 및 상기 플라스미드에서 발현된 FcIII-ß-PE24를 개략적으로 나타낸 것이다.Figure 5 schematically shows the expression plasmid PE24 (FcIII-ß-PE24) expressed in the FcIII peptide of the present invention and FcIII-β-PE24 expressed in the plasmid.
도 6a는 본 발명에서 재조합된 tRNA 합성효소 발현 플라스미드를 나타낸 것이다.6A shows a recombinant tRNA synthetase expression plasmid in the present invention.
도 6b는 프롤린 tRNA 합성효소 발현 플라스미드를 나타낸 것이다.6B shows a plasmid expressing proline tRNA synthetase.
도 7은 본 발명의 융합단백질과 항체(Cetuximab)의 결합을 전기영동으로 관찰한 것이다.FIG. 7 shows the binding of the fusion protein of the present invention to the antibody (Cetuximab) by electrophoresis.
도 8은 Z-domain을 이용하여 본 발명의 융합단백질과 항체(Cetuximab)의 위치특이적 결합을 전기영동으로 관찰한 것이다.FIG. 8 shows the position-specific binding of the fusion protein of the present invention and the antibody (Cetuximab) by electrophoresis using a Z-domain.
도 9는 본 발명의 FcIII와 항체(Cetuximab)의 접합위치를 LC-MS/MS로 확인한 것이다.FIG. 9 shows the location of the junction between FcIII and the antibody (Cetuximab) of the present invention by LC-MS / MS.
도 10은 본 발명의 융합단백질과 항체(Cetuximab)가 1:1로 결합한 Cetuximab-FcIII-PE24 접합체를 분리한 결과를 전기영동으로 관찰한 것이다.FIG. 10 shows electrophoretic results of Cetuximab-FcIII-PE24 conjugates obtained by binding the fusion protein of the present invention and an antibody (Cetuximab) at a ratio of 1: 1.
도 11은 본 발명의 Cetuximab-FcIII-PE24 접합체의 EF2 리보실화 활성을 확인한 결과이다.Figure 11 shows the results of confirming the EF2 ribosylation activity of the Cetuximab-FcIII-PE24 conjugate of the present invention.
도 12는 본 발명의 Cetuximab-FcIII-PE24 접합체의 세포성장저해 활성을 확인한 결과이다.12 shows the results of confirming the cell growth inhibitory activity of the Cetuximab-FcIII-PE24 conjugate of the present invention.
도 13은 본 발명의 융합단백질과 항체(Trastuzumab)가 위치특이적으로 결합한 결과와 융합단백질과 항체가 1:1로 결합한 Trastuzumab-FcIII-PE24 접합체를 분리한 결과를 전기영동으로 관찰한 것이다.FIG. 13 shows electrophoretic results of separation of Trastuzumab-FcIII-PE24 conjugate in which a fusion protein of the present invention and an antibody (Trastuzumab) are bound to each other and a fusion protein and an antibody are bound at a ratio of 1: 1.
도 14는 본 발명의 Trastuzumab-FcII-PE24 접합체의 세포성장저해 활성을 확인한 결과이다.14 shows the results of confirming the cell growth inhibitory activity of the Trastuzumab-FcII-PE24 conjugate of the present invention.
발명의 상세한 설명 및 바람직한 구현예DETAILED DESCRIPTION OF THE INVENTION AND PREFERRED EMBODIMENTS
다른 식으로 정의되지 않는 한, 본 명세서에서 사용된 모든 기술적 및 과학적 용어들은 본 발명이 속하는 기술분야에서 숙련된 전문가에 의해서 통상적으로 이해되는 것과 동일한 의미를 갖는다. 일반적으로 본 명세서에서 사용된 명명법은 본 기술분야에서 잘 알려져 있고 통상적으로 사용되는 것이다.Unless otherwise defined, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. In general, the nomenclature used herein is well known and commonly used in the art.
본 발명에서는 항체 Fc 도메인에 특이적으로 결합가능하고, Fc 위치선택적 결합 펩티드에서 5번째, 10번째 또는 11번째 위치가 광반응성 작용기를 갖는 아미노산으로 치환된 Fc 위치선택적 접합 펩티드로 수식화된 생리활성물질을 항체와 결합시킨 결과, 종래와 다르게 비가역적인 공유결합이 형성되며, 광반응성 작용기의 도입위치에 따라 항체와 접합 펩티드로 수식화된 생리활성물질의 결합 효율이 향상되는 것을 확인하였다(도 2).In the present invention, a physiologically active substance which can be specifically bound to an antibody Fc domain and which is modified with an Fc position-selective peptide in which the 5th, 10th or 11th position of the Fc position-selective binding peptide is substituted with an amino acid having a photoreactive functional group (FIG. 2). As a result, it was confirmed that irreversible covalent bonds were formed unlike the conventional art, and the binding efficiency of the physiologically active substance modified with the antibody and the conjugated peptide was improved according to the position of introduction of the photoreactive functional group.
따라서, 본 발명은 일 관점에서, 서열번호 1의 아미노산 서열로 표시되는 Fc 위치선택적 결합 펩티드에서 5번째, 10번째 또는 11번째 위치가 광반응성 작용기를 갖는 아미노산으로 치환된 Fc 위치선택적 접합 펩티드에 관한 것이다.Accordingly, in one aspect, the present invention relates to an Fc position-selective fused peptide wherein the 5th, 10th, or 11th position of the Fc position-selective binding peptide represented by the amino acid sequence of SEQ ID NO: 1 is substituted with an amino acid having a photoreactive functional group will be.
본 발명에서, 상기 Fc 위치선택적 결합 펩티드(FcIII)(아미노산 서열번호 1, 유전자 서열번호 2)는 인간유래 항체(IgG1)의 Fc 도메인의 CH3-CH2 인터페이스 영역(interface region)에 위치특이적으로 결합하는 13개의 아미노산으로 이루어진 짧은 펩티드이다(W.L. DeLano et al, Science, 2000). 상기 펩티드는 두 개의 시스테인이 서로 이황화 결합을 형성하고 있어 U자 구조를 나타낸다.In the present invention, the Fc position-selective binding peptide (FcIII) (amino acid sequence SEQ ID NO: 1, gene SEQ ID NO: 2) locally specifically binds to the CH3-CH2 interface region of the Fc domain of the human- (WL DeLano et al, Science , 2000). The peptide shows a U-structure because two cysteines form a disulfide bond with each other.
본 발명에 있어서, 상기 광반응성 작용기를 갖는 아미노산으로 치환된 위치가 10번째인 것을 특징으로 할 수 있다.In the present invention, the position substituted with the amino acid having the photoreactive functional group may be 10th.
본 발명에서, 광반응성 작용기를 갖는 아미노산으로 치환된 Fc 위치선택적 접합 펩티드를 제조하는 방법은 Fc 위치선택적 결합 펩티드의 아미노산 서열을 동정하고, 이를 공지의 방법으로 예컨대, 상기 펩티드를 발현할 수 있는 발현벡터를 제조하여 숙주세포에 형질전환시켜 재조합 기법으로 발현시키거나, 인공적으로 합성하여 제조한 후 공지의 방법으로 이중 하나 이상의 아미노산 잔기를 광반응성 작용기를 갖는 아미노산으로 치환하거나 도입하여 제조할 수 있거나 또는 인공 합성시 하나 이상의 광반응성 작용기를 갖는 아미노산을 포함시켜 합성할 수 있다.In the present invention, a method for producing an Fc positionally-selected fused peptide substituted with an amino acid having a photoreactive functional group is characterized in that the amino acid sequence of the Fc position-selective binding peptide is identified and expressed in an expression system capable of expressing the peptide A vector may be prepared and transformed into a host cell and expressed by a recombinant technique, or artificially synthesized, followed by substitution or introduction of at least one amino acid residue with an amino acid having a photoreactive functional group by a known method, or Can be synthesized by incorporating an amino acid having at least one photoreactive functional group in the artificial synthesis.
상기 유전자의 도입은 통상적으로 알려진 유전자 조작방법을 사용할 수 있다. 예를 들어, 바이러스 등의 벡터를 이용하는 방법, 합성 인지질이나 합성 양이온성 고분자 등을 사용하는 비바이러스성 방법 및 세포막에 일시적인 전기 자극을 가하여 유전자를 도입하는 전기투과법 등 물리적인 방법을 사용할 수 있으며, 이에 한정하지 않는다.The introduction of the gene can be carried out by a commonly known gene manipulation method. For example, a physical method such as a method using a vector such as a virus, a non-viral method using a synthetic phospholipid or a synthetic cationic polymer, or an electrotransfer method in which a gene is introduced by applying temporary electrical stimulation to the cell membrane can be used , But is not limited thereto.
본 발명에서 “증폭”이란 해당 유전자의 일부 염기를 변이, 치환, 또는 삭제시키거나, 일부 염기를 도입시키거나, 또는 동일한 효소를 코딩하는 다른 미생물 유래의 유전자를 도입시켜 대응하는 효소의 활성을 증가시키는 것을 포괄하는 개념이다.The term " amplification " in the present invention refers to amplification, substitution, or deletion of a part of the gene, introduction of a certain base, or introduction of a gene derived from another microorganism encoding the same enzyme to increase the activity of the corresponding enzyme .
본 발명에서 “벡터(vector)”는 적합한 숙주 내에서 DNA를 발현시킬 수 있는 적합한 조절 서열에 작동가능하게 연결된 DNA 서열을 함유하는 DNA 제조물을 의미한다. 벡터는 플라스미드, 파지 입자, 또는 간단하게 잠재적 게놈 삽입물일 수 있다. 적당한 숙주로 형질전환되면, 벡터는 숙주 게놈과 무관하게 복제하고 기능할 수 있거나, 또는 일부 경우에 게놈 그 자체에 통합될 수 있다. 플라스미드가 현재 벡터의 가장 통상적으로 사용되는 형태이므로, 본 발명의 명세서에서 “플라스미드(plasmid)” 및 “벡터(vector)”는 때로 상호 교환적으로 사용된다. 그러나, 본 발명은 당업계에 알려진 또는 알려지게 되는 바와 동등한 기능을 갖는 벡터의 다른 형태를 포함한다.As used herein, the term " vector " means a DNA construct containing a DNA sequence operably linked to a suitable regulatory sequence capable of expressing the DNA in an appropriate host. The vector may be a plasmid, phage particle, or simply a potential genome insert. Once transformed into the appropriate host, the vector may replicate and function independently of the host genome, or, in some cases, integrate into the genome itself. Because the plasmid is the most commonly used form of the current vector, the terms " plasmid " and " vector " are sometimes used interchangeably in the context of the present invention. However, the present invention includes other forms of vectors having functions equivalent to those known or known in the art.
본 발명에서 “발현 벡터”는 통상 이종의 DNA의 단편이 삽입된 재조합 캐리어(recombinant carrier)로서 일반적으로 이중 가닥의 DNA의 단편을 의미한다. 여기서, 이종 DNA는 숙주 세포에서 천연적으로 발견되지 않는 DNA인 이형 DNA를 의미한다. 발현 벡터는 일단 숙주 세포내에 있으면 숙주 염색체 DNA와 무관하게 복제할 수 있으며 벡터의 수 개의 카피 및 그의 삽입된 (이종) DNA가 생성될 수 있다. 당업계에 주지된 바와 같이, 숙주세포에서 형질감염 유전자의 발현 수준을 높이기 위해서는, 해당 유전자가, 선택된 발현 숙주 내에서 기능을 발휘하는 전사 및 해독 발현 조절 서열에 작동가능하도록 연결되어야만 한다. 바람직하게는 발현 조절서열 및 해당 유전자는 세균 선택 마커 및 복제 개시점(replication origin)을 같이 포함하고 있는 하나의 발현 벡터 내에 포함되게 된다. 발현 숙주가 진핵세포인 경우에는, 발현 벡터는 진핵 발현 숙주 내에서 유용한 발현 마커를 더 포함하여야만 한다.In the present invention, " expression vector " is usually a recombinant carrier into which a fragment of different DNA is inserted, and generally means a fragment of double stranded DNA. Herein, the heterologous DNA means a heterologous DNA that is not naturally found in the host cell. Once an expression vector is in a host cell, it can replicate independently of the host chromosomal DNA, and several copies of the vector and its inserted (heterologous) DNA can be generated. As is well known in the art, to increase the level of expression of a transfected gene in a host cell, the gene must be operably linked to a transcriptional and detoxification regulatory sequence that functions in the selected expression host. Preferably the expression control sequence and the gene are contained within an expression vector containing a bacterial selection marker and a replication origin. If the expression host is a eukaryotic cell, the expression vector should further comprise a useful expression marker in the eukaryotic expression host.
본 발명에서 “통합 벡터”는 핵산으로의 통합 또는 삽입이 인테그라제(integrase)를 통해 수행되는 벡터를 의미하는 것으로, 통합 벡터의 예로는 레트로바이러스 벡터, 트란스포손 및 아데노 관련 바이러스 벡터 등이 있으나 이에 제한되지는 않는다.In the present invention, " integrative vector " means a vector in which integration or insertion into a nucleic acid is performed through integrase. Examples of integrated vectors include retrovirus vector, transposon and adeno-associated viral vector. But is not limited to.
상기 벡터에 의해 형질전환 또는 형질감염된 숙주 세포는 본 발명의 또 다른 측면을 구성한다. 본 발명에서 사용된 용어 “형질전환”은 DNA를 숙주로 도입하여 DNA가 염색체외 인자로서 또는 염색체 통합완성에 의해 복제가능하게 되는 것을 의미한다. 이는 핵산을 유기체, 세포, 조직 또는 기관에 도입하는 어떤 방법도 포함되며 당 분야에서 공지된 바와 같이 숙주 세포에 따라 적합한 표준 기술을 선택하여 수행될 수 있다. 이러한 방법에는 전기충격유전자전달법(electroporation), 원형질 융합, 인산칼슘(CaPO4) 침전, 염화 칼슘(CaCl2) 침전, 실리콘카바이드 섬유를 이용한 교반, 아그로 박테리아 매개된 형질전환, PEG, 덱스트란 설페이트, 리포펙타민 및 건조/억제 매개된 형질전환 방법 등이 포함되나 이에 제한되지 않는다. 발명의 숙주 세포는 원핵 또는 진핵생물 세포일 수 있다. 또한, DNA의 도입효율이 높고, 도입된 DNA의 발현효율이 높은 숙주가 통상 사용된다. 대장균, 슈도모나스, 바실러스, 스트렙토마이세스, 진균, 효모와 같은 주지의 진핵 및 원핵 숙주들, 스포도프테라 프루기페르다(SF9)와 같은 곤충 세포, CHO 및 생쥐 세포같은 동물 세포, COS 1, COS 7, BSC 1, BSC 40 및 BMT 10과 같은 아프리카 그린 원숭이 세포, 및 조직배양된 인간 세포는 사용될 수 있는 숙주 세포의 예이다.A host cell transformed or transfected with the vector constitutes another aspect of the present invention. As used herein, the term " transformation " means introducing DNA into a host and allowing the DNA to replicate as an extrachromosomal factor or by chromosomal integration. This includes any method of introducing the nucleic acid into an organism, cell, tissue or organ, and can be carried out by selecting a suitable standard technique depending on the host cell as is known in the art. Such methods include electroporation, protoplast fusion, calcium phosphate (CaPO 4 ) precipitation, calcium chloride (CaCl 2 ) precipitation, agitation with silicon carbide fibers, Agrobacterium mediated transformation, PEG, dextran sulfate , Lipofectamine, and dry / inhibition-mediated transformation methods, and the like. The host cell of the invention may be a prokaryotic or eukaryotic cell. In addition, a host having high efficiency of introduction of DNA and high efficiency of expression of the introduced DNA is usually used. Known eukaryotic and prokaryotic hosts such as Escherichia coli, Pseudomonas, Bacillus, Streptomyces, fungi and yeast, insect cells such as Spodoptera prolipida (SF9), animal cells such as CHO and mouse cells, COS 1, COS 7, BSC 1, BSC 40 and BMT 10, and tissue cultured human cells are examples of host cells that can be used.
물론 모든 벡터가 본 발명의 DNA 서열을 발현하는데 모두 동등하게 기능을 발휘하지는 않는다는 것을 이해하여야만 한다. 마찬가지로 모든 숙주가 동일한 발현 시스템에 대해 동일하게 기능을 발휘하지는 않는다. 그러나, 당업자라면 과도한 실험적 부담없이 본 발명의 범위를 벗어나지 않는 채로 여러 벡터, 발현 조절 서열 및 숙주 중에서 적절한 선택을 할 수 있다. 예를 들어, 벡터를 선택함에 있어서는 숙주를 고려하여야 하는데, 이는 벡터가 그 안에서 복제되어야만 하기 때문이다. 벡터의 복제 수, 복제 수를 조절할 수 있는 능력 및 당해 벡터에 의해 코딩되는 다른 단백질, 예를 들어 항생제 마커의 발현도 또한 고려되어야만 한다. 발현 조절 서열을 선정함에 있어서도, 여러 가지 인자들을 고려하여야만 한다. 예를 들어, 서열의 상대적 강도, 조절가능성 및 본 발명의 DNA 서열과의 상용성 등, 특히 가능성있는 이차 구조와 관련하여 고려하여야 한다. 단세포 숙주는 선정된 벡터, 본 발명의 DNA 서열에 의해 코딩되는 산물의 독성, 분비 특성, 단백질을 정확하게 폴딩시킬 수 있는 능력, 배양 및 발효 요건들, 본 발명 DNA 서열에 의해 코딩되는 산물을 숙주로부터 정제하는 것의 용이성 등의 인자를 고려하여 선정되어야만 한다. 이들 변수의 범위 내에서, 당업자는 본 발명의 DNA 서열을 발효 또는 대규모 동물배양에서 발현시킬 수 있는 각종 벡터/발현 조절 서열/숙주 조합을 선정할 수 있다. 발현 클로닝에 의해 NSP 단백질의 cDNA를 클로닝 하려고 할 때의 스크리닝법으로서 바인딩법(binding법), 페닝법(panning법), 필름에멀션법(film emulsion 법) 등이 적용될 수 있다.Of course, it should be understood that not all vectors function equally well in expressing the DNA sequences of the present invention. Likewise, not all hosts function identically for the same expression system. However, those skilled in the art will be able to make appropriate selections among a variety of vectors, expression control sequences, and hosts without undue experimentation and without departing from the scope of the present invention. For example, in selecting a vector, the host should be considered because the vector must be replicated within it. The number of copies of the vector, the ability to control the number of copies, and the expression of other proteins encoded by the vector, such as antibiotic markers, must also be considered. In selecting the expression control sequence, a number of factors must be considered. For example, the relative strength of the sequence, controllability and compatibility with the DNA sequences of the present invention should be considered in relation to particularly possible secondary structures. The single cell host may be selected from a selected vector, the toxicity of the product encoded by the DNA sequence of the present invention, the secretion characteristics, the ability to fold the protein correctly, the culture and fermentation requirements, the product encoded by the DNA sequence of the invention And ease of purification. Within the scope of these variables, one skilled in the art can select various vector / expression control sequences / host combinations that can express the DNA sequences of the invention in fermentation or in large animal cultures. A binding method, a panning method, a film emulsion method, or the like can be applied as a screening method for cloning cDNA of NSP protein by expression cloning.
본 발명에서 “원형질체 융합”은 식물세포 또는 균류 등의 세포벽을 제거한 원형질체(protoplast)를 이용하여 서로 다른 형질을 가진 두 세포를 융합하는 기술을 의미한다. 원형질체 융합에는 고농도의 삼투압 용액에 칼슘, 마그네슘 등의 금속이온을 첨가하는 등의 화학적 방법 또는 전기충격을 주어 세포막에 일시적으로 작은 구멍이 생기도록 원형질체를 노출시켜 원형질체의 DNA흡수를 증가시키는 등의 물리적 방법이 있다.In the present invention, " protoplast fusion " means a technique of fusing two cells having different traits using a protoplast from which cell walls of plant cells or fungi have been removed. Protoplast fusion involves the use of chemical methods such as the addition of metal ions such as calcium and magnesium to high osmotic solutions or physical exposure such as by increasing the DNA absorption of the protoplasts by exposing the protoplasts to temporary pores in the cell membrane, There is a way.
본 발명에서, “광반응성 작용기”는 광조사시 특정 파장의 빛을 흡수하여 인접한 반응성 작용기와 공유결합을 형성할 수 있는 작용기일 수 있다.In the present invention, the "photoreactive functional group" may be a functional group capable of absorbing light of a specific wavelength upon irradiation with light and forming a covalent bond with an adjacent reactive functional group.
본 발명의 광반응성 작용기를 구비한 Fc 위치선택적 접합 펩티드는 항체와 혼합하였을 때, 내재적 특성인 특이성에 의해 항체의 Fc 도메인에 인접 또는 결합한다. 이후, 상기 혼합물에 빛을 조사하면 특정 파장의 빛을 흡수하여 광반응성 작용기를 통해 이와 인접한 항체 Fc 도메인 상의 반응성 작용기와 공유결합을 형성할 수 있다. 즉, 본 발명의 Fc 위치선택적 접합 펩티드는 광조사시 상기 광반응성 작용기를 통해 Fc 도메인의 특정 작용기에 공유결합할 수 있다.The Fc positionally-selective peptide with the photoreactive functional group of the present invention binds to or binds to the Fc domain of the antibody by its specificity as an inherent property when mixed with the antibody. Then, when the mixture is irradiated with light, it can absorb light of a specific wavelength and form a covalent bond with a reactive functional group on the adjacent antibody Fc domain through a photoreactive functional group. That is, the Fc position-selective binding peptide of the present invention can covalently bind to the specific functional group of the Fc domain through the photoreactive functional group upon light irradiation.
본 발명에 있어서, 상기 광반응성 작용기를 갖는 아미노산은 p-벤조일 페닐알라닌(p-benzoyl phenylalanine)인 것을 특징으로 할 수 있다. 광반응성 작용기를 갖는 인공 아미노산은 포토루신이나 포토메티오닌 혹은 아지도페닐알라닌 등으로 구성될 수 있으나, 본 발명에서 사용된 광반응성 작용기는 특정 작용기에 선호도를 가지고 작용하며 높은 파장대를 가지는, 즉 낮은 에너지를 가지는 빛 에너지를 통해 공유결합이 활성화되는 점을 특이성으로 갖는다.In the present invention, the amino acid having the photoreactive functional group may be p-benzoyl phenylalanine. The artificial amino acid having a photoreactive functional group may be composed of a photoreceptor, a photomethionine or an azidophenylalanine. However, the photoreactive functional group used in the present invention has a high wavelength band, that is, a low energy The branch has specificity that the covalent bond is activated through light energy.
본 발명의 p-벤조일 페닐알라닌은 하기 화학식 1로 표시된다.The p-benzoylphenylalanine of the present invention is represented by the following formula (1).
[화학식 1][Chemical Formula 1]
Figure PCTKR2018014939-appb-I000001
Figure PCTKR2018014939-appb-I000001
본 발명은 다른 관점에서, 상기 펩티드에 생리활성물질이 직접 또는 링커를 통해 연결되어 있는 접합 펩티드로 수식화된 생리활성물질에 관한 것이다.In another aspect, the present invention relates to a physiologically active substance which is formulated with a conjugate peptide in which a physiologically active substance is directly or linked to the peptide through a linker.
본 발명에 있어서, 상기 생리활성물질은 치료제 또는 진단제제인 것을 특징으로 할 수 있으며, 상기 치료제 또는 진단제제는 효소, 호르몬(Hormon), 사이토카인, 항체, 항체 단편, 진통제, 해열제, 항염증제, 항생 물질, 항바이러스(virus)제, 항진균약, 심장혈관약, 중추 신경 작용약, 신장 기능 및 전해질 대사 작용약, 화학 요법제로 구성된 군에서 선택되는 것을 특징으로 할 수 있다.In the present invention, the physiologically active substance may be a therapeutic agent or a diagnostic agent. The therapeutic agent or diagnostic agent may be an enzyme, hormone, cytokine, antibody, antibody fragment, analgesic agent, antipyretic agent, anti- A substance, an antiviral drug, an antifungal drug, a cardiovascular drug, a central nervous system drug, a kidney function and an electrolytic metabolism drug, and a chemotherapeutic agent.
본 발명의 생리활성물질은 치료제 또는 진단/검출제제일 수 있다. 구체적으로, 상기 생리활성물질로서 사용되는 항체는 치료용 항체일 수 있다. 치료용 항체는 현재 약 30종이 FDA의 승인을 받았으며, 생체 내 존재하는 IgG와 성질이 거의 흡사하여 그 안전성이 매우 높다. 치료용 항체는 광범위한 질병 치료제(예를 들어, 이식거부반응, 암, 자가면역질환과 염증, 심장질환 및 전염성 감염 등)로 사용되고 있다. 특히, Fc 도메인 함유 분자가 치료용 항체인 경우, 상기 치료용 항체는 질병이 생긴 조직에 특이적으로 존재하는 수용체 단백질 혹은 항원단백질을 인식하여 결합하기 때문에 그 특이성이 매우 높다. 따라서, 치료용 항체에 생리활성물질로서 분자영상프로브나 약물전달체를 결합시키면 약물병용효과와 함께 치료과정을 모니터링할 수 있는 테라그노시스(theragnosis) 제제로 전환할 수 있다. 또한 단순한 표적화 항체에도 분자영상프로브나 약물전달체를 결합시킴으로써 진단, 치료, 혹은 진단과 치료를 동시에 진행하는 테라그노시스 제제를 개발할 수 있다.The physiologically active substance of the present invention may be a therapeutic agent or a diagnostic / detection agent. Specifically, the antibody used as the physiologically active substance may be a therapeutic antibody. Approximately 30 therapeutic antibodies have been approved by the FDA and their safety is very high because they closely resemble those of in vivo IgG. Therapeutic antibodies have been used for a wide range of disease treatments (such as transplant rejection, cancer, autoimmune diseases and inflammation, heart disease and infectious infections, etc.). In particular, when the Fc domain-containing molecule is a therapeutic antibody, the therapeutic antibody recognizes and binds to a receptor protein or an antigenic protein specifically present in a disease-causing tissue, and therefore its specificity is very high. Therefore, when a molecular imaging probe or a drug delivery vehicle is combined with a therapeutic antibody as a physiologically active substance, it can be converted into a theragnosis agent capable of monitoring the therapeutic process together with a drug combination effect. In addition, by combining a molecular imaging probe or a drug delivery system with a simple targeting antibody, it is possible to develop a teraginosis preparation for diagnosis, treatment, or simultaneous diagnosis and treatment.
치료제의 비제한적인 예로는 항체, 항체단편, 약물, 독소, 핵산가수분해효소(nuclease), 호르몬, 면역조절제, 킬레이터, 붕소화합물, 광활성(photoactive)제제 또는 염료, 및 방사성동위원소를 포함한다.Non-limiting examples of therapeutic agents include antibodies, antibody fragments, drugs, toxins, nucleic acid hydrolases, hormones, immunomodulators, chelators, boron compounds, photoactive agents or dyes, and radioactive isotopes .
진단제제/검출제제의 비제한적인 예로는 방사성동위원소, 염료(예를들어, 비오틴(biotin)-스트렙타비딘(streptavidin) 복합체), 조영제, 형광 화합물 또는 분자 및 자기공명 영상화(MRI)에의 증가제(상자성 이온)을 포함한다. 바람직하게, 진단제제는 방사성동위원소, 자기공명 영상에서 사용되는 증가제, 및 형광화합물을 포함한다. 항체성분을 방사성 금속 또는 상자성 이온과 부하하기 위해, 이온을 결합하는데 킬레이트기의 다수와 부착된 긴 꼬리를 갖는 반응물과 반응하는 것이 필요할 수도 있다. 상기의 꼬리는 폴리리신, 폴라사카라이드와 같은 고분자, 또는 에틸렌디아민테트라아세트산(EDTA), 디에틸렌트리아민펜타아세트산(DTPA; diethylenetriaminepentaacetic acid), 포르피린(porphyrin), 폴리아민, 크라운 에테르, 비스-티오세미카르바존(thiosemicarbazone), 폴리옥심(polyoximes)과 같은 킬레이트기와 결합될 수 있는 펜던트기를 갖고 상기 목적에 유용하다고 알려진 기를 갖는 유도화되거나 유도될 수 있는 사슬일 수 있다. 킬레이트는 정상적으로 면역반응성의 최소 손실과 최소 집합체 및/또는 내부 교차연결로 분자에 결합을 형성할 수 있는 작용기에 의해 Fc 위치선택적 접합 펩티드에 연결될 수 있다.Non-limiting examples of diagnostic / detection agents include, but are not limited to, an increase in radioisotopes, dyes (e.g., biotin-streptavidin complexes), contrast agents, fluorescent compounds or molecules and magnetic resonance imaging (MRI) (Paramagnetic ion). Preferably, the diagnostic agent comprises a radioactive isotope, an enhancer for use in magnetic resonance imaging, and a fluorescent compound. In order to load the antibody component with radioactive metal or paramagnetic ions, it may be necessary to react with a reactant having a long tail attached to many of the chelating groups to couple the ions. The tail may be a polymer such as polylysine or polacacaride or a polymer such as ethylenediaminetetraacetic acid (EDTA), diethylenetriaminepentaacetic acid (DTPA), porphyrin, polyamine, crown ether, bis-thiosemic A chain having a pendant group capable of bonding with a chelating group such as a thiosemicarbazone, polyoximes, and a group known to be useful for the above purpose. The chelate can normally be coupled to the Fc position-selective peptidic peptide by a minimal loss of immunoreactivity and a functional group capable of forming a bond to the molecule with minimal assembly and / or internal cross-linking.
특히, 유용한 금속-킬레이트 조합은 진단성 동위원소와 60~4,000keV의 일반적인 에너지 범위에서 사용되는 2-벤질-DTPA 및 이의 모노메틸 및 시클로헥실 유사체를 포함하고, 예를 들어 방사성 영상화제에는 125I, 131I, 123I, 124I, 62Cu, 64Cu, 18F, 111In, 67Ga, 99mTc, 94mTc, 11C, 13N, 15O, 76Br이 있다. 망간, 철 및 가돌리늄과 같은 비-방사성 금속과 복합화될 경우, 같은 킬레이트는 본 발명의 나노입자 또는 항체와 사용될 때 MRI에 유용하다. NOTA, DOTA, 및 TETA와 같은 거대고리(macrocyclic) 킬레이트는 금속 및 방사성 금속의 종류와 사용되고, 바람직하게는 갈륨, 이트륨(yttrium) 및 구리의 방사성핵종과 각각 사용된다. 상기 금속-킬레이트 복합체는 대상의 금속에 고리크기를 맞춤으로써 매우 안정하게 제조될 수 있다. 본 발명에 의해 RAIT에 223Ra와 같은 핵종과 안정하게 결합하는데 유용한 거대고리 폴리에테르류와 같은 고리형 킬레이트를 제조할 수 있다.Particularly useful metal-chelate combinations include diagnostic isotopes and 2-benzyl-DTPA and monomethyl and cyclohexyl analogues thereof used in the general energy range of 60 to 4,000 keV, for example, radioisotopes include 125 I , 131 I, 123 I, 124 I, 62 Cu, 64 Cu, 18 F, 111 In, 67 Ga, 99 mTc, 94 mTc, 11 C, 13 N, 15 O, 76 Br. When complexed with non-radioactive metals such as manganese, iron and gadolinium, the same chelate is useful for MRI when used with nanoparticles or antibodies of the present invention. Macrocyclic chelates such as NOTA, DOTA, and TETA are used with a variety of metals and radioactive metals, preferably with radionuclides of gallium, yttrium and copper, respectively. The metal-chelate complex can be made very stable by aligning the ring size with the metal of the object. The present invention makes it possible to produce cyclic chelates such as macrocyclic polyethers useful for stably binding RAIT with nuclides such as 223Ra.
이뮤노컨쥬게이트(immunoconjugate)는 치료제 또는 진단제제와 항체 성분의 컨쥬게이트이다. 상기 진단제제는 방사성 또는 비방사성 표지, 조영제(자기공명영상화, 컴퓨터단층촬영(computed tomography), 또는 초음파에 적절한 조영제)를 포함하고, 방사성 라벨은 감마-, 베타-, 알파-, 오제 전자- 또는 양전자 방출 동위원소일 수 있다.Immunoconjugates are conjugates of therapeutic or diagnostic agents and antibody components. The diagnostic agent comprises a radioactive or non-radioactive label, a contrast agent (magnetic resonance imaging, computed tomography, or a contrast agent suitable for ultrasound), and the radioactive label includes gamma-, beta-, alpha-, It may be a positron emission isotope.
본 발명에서, “면역조절제”는 전형적으로 대식세포(macrophage), B-세포, 및/또는 T-세포와 같은 면역반응 캐스캐이드(immune response cascade)에서 증식하거나 활성화되는 면역세포를 자극한다. 상기 면역조절제의 예는 사이토카인이다. 당업자들은 인터루킨 및 인터페론이 T-세포 또는 기타 면역 세포 활성을 자극하는 사이토카인의 일종이다.In the present invention, " immunomodulators " typically stimulate immune cells that are proliferating or activating in an immune response cascade such as macrophages, B-cells, and / or T-cells. An example of such an immunomodulator is a cytokine. Those skilled in the art are a type of cytokine in which interleukins and interferons stimulate T-cell or other immune cell activity.
본 발명의 Fc 위치선택적 접합 펩티드에 DNA(deoxyribonucleic acid), RNA(ribonucleic acid), PNA(peptide nucleic acid) 또는 LNA(locked nucleic acid)가 직접 또는 링커를 통해 연결될 수 있다. 상기 DNA, RNA, PNA 및 LNA는 상보적 서열을 갖는 물질과 특이적으로 결합하는 성질을 갖는 중합체이므로 상기 DNA, RNA, PNA 또는 LNA를 연결시킨 Fc 위치선택적 결합 펩티드는 유전자 스크리닝, 바이오센서 등에 사용될 수 있다.DNA (deoxyribonucleic acid), ribonucleic acid (RNA), peptide nucleic acid (PNA), or locked nucleic acid (LNA) can be directly or linked to the Fc position-selective binding peptide of the present invention. Since the DNA, RNA, PNA and LNA are polymers having a property of specifically binding to a substance having a complementary sequence, the Fc position-selective binding peptide linked with DNA, RNA, PNA or LNA can be used for gene screening, .
상기 DNA, RNA, PNA 또는 LNA를 연결시킨 Fc 위치선택적 접합 펩티드를 바이오칩, 바이오센서, 면역검출키트 또는 상보적 자기주소지정칩(complementary self-addressable chip)으로 활용하기 위하여 고체 지지체에 고정시켜 사용할 수 있다.An Fc positionally-selected fused peptide in which the DNA, RNA, PNA or LNA is linked can be immobilized on a solid support for use as a biochip, a biosensor, an immune detection kit or a complementary self-addressable chip have.
본 발명에 있어서, 상기 링커는 반응성 기능기, 아미노산 및 자가 절단 스페이서를 포함하는 것을 특징으로 할 수 있다.In the present invention, the linker may include a reactive functional group, an amino acid, and a self-cleaving spacer.
본 발명의 링커는 광반응성 작용기로 치환된 Fc 위치선택적 접합 펩티드 내의 특정 잔기와 생리활성물질을 연결하는 형태일 수 있으며, 광반응성 작용기로 치환된 Fc 위치선택적 접합 펩티드 상에 존재하는 친핵성 잔기(예를 들어, 시스테인)에 반응하는 친전자성기를 갖는 반응성 부위를 가질 수 있다. 상기 링커는 예를 들어, 광반응성 작용기로 치환된 Fc 위치선택적 접합 펩티드에 결합하는 반응성 기능기, 아미노산 및 자가 절단 스페이서를 포함할 수 있다.The linker of the present invention may be in a form of linking a physiologically active substance with a specific residue in an Fc positionally selected binding peptide substituted with a photoreactive functional group and may include a nucleophilic residue For example, cysteine). ≪ / RTI > The linker may comprise, for example, a reactive functional group, an amino acid, and a self-cleaving spacer that binds to an Fc positionally-selective fused peptide substituted with a photoreactive functional group.
상기 기능기는 i) 말레이마이드기, 아세트아마이드기, 또는 이의 유도체, ii) 아지리딘기, 아릴할라이드, 아크릴로일기, 또는 이의 유도체, iii) 알킬화 반응기, 아릴화 반응기, 피리딜 다이설파이드, 티오니트로벤조익산, 또는 이의 유도체일 수 있다. 구체적으로, 상기 링커는 구체적 예로 i) 말레이마이드기 또는 이의 유도체-발린-시트룰린(valine-citurulline)-파라 아닐린 벤조산(para-aniline benzoic acid: PABA); 또는 ii) 아세트아마이드기 또는 이의 유도체-발린-시트룰린(valine-citurulline)-파라 아닐린 벤조산(para-aniline benzoic acid: PABA)의 형태일 수 있으나, 이에 제한되는 것은 아니다.The functional group may be selected from the group consisting of i) a maleimide group, an acetamide group or a derivative thereof, ii) an aziridine group, an aryl halide, an acryloyl group or a derivative thereof, iii) an alkylation reactor, an arylation reactor, pyridyldisulfide, Lysine, or a derivative thereof. Specifically, the linker includes, for example, i) a maleimide group or a derivative thereof-valine-citurline-para-aniline benzoic acid (PABA); Or ii) in the form of an acetamide group or a derivative thereof-valine-citurulline-para-aniline benzoic acid (PABA).
상기 링커를 통한 광반응성 작용기로 치환된 Fc 위치선택적 접합 펩티드와 생리활성물질의 결합은 공지의 방법, 예를 들어 알킬레이션, 이황화(disulfide) 상호교환 방법 및 트랜스티오에스테르화 반응법이 이용될 수 있다. 이를 통해 광반응성 작용기로 치환된 Fc 위치선택적 접합 펩티드 내 시스테인 잔기의 티올기를 통해 상기 접합 펩티드와 생리활성물질이 접합될 수 있다.The binding of the Fc positionally-selective peptide and the physiologically active substance substituted with the photoreactive functional group through the linker can be carried out by a known method, for example, an alkylation, a disulfide interchange method, and a trans-esterification reaction method have. Whereby the conjugated peptide and the physiologically active substance can be conjugated to each other through the thiol group of the cysteine residue in the Fc positionally-selective peptide substituted with the photoreactive functional group.
하나의 구체예에서, 티올-링커 결합을 위해서 사용되는 말레이미드 기의 경우, 시스테인 잔기의 티올이 말레이미드 기에 대하여 갖는 친핵 반응성이 단백질 중에 존재하는 다른 아미노산 기능기, 예를 들어 리신 잔기의 아미노기 또는 N-말단 아미노기에 비하여 약 1,000배 더 높기 때문에 시스테인에 특이적으로 결합시키는데 활용될 수 있다. 따라서, 말레이미드기, 이의 유도체 또는 아세트아마이드기 또는 이의 유도체, 예를 들어 브로모 아세트아마이드기, 이오도 아세트아마이드기를 통한 접합 펩티드로 수식화된 생리활성물질은 시스테인이 티오에테르 결합으로 광반응성 작용기로 치환된 Fc 위치선택적 접합 펩티드와 생리활성물질이 결합됨을 알 수 있다.In one embodiment, in the case of a maleimide group used for thiol-linker linkage, the nucleophilic reactivity of the thiol of the cysteine residue to the maleimide group is dependent on the other amino acid functional groups present in the protein, such as the amino group of the lysine residue Terminal amino group, it can be utilized for specific binding to cysteine. Therefore, a physiologically active substance modulated with a maleimide group, a derivative thereof, or an acetamide group or a derivative thereof, for example, a bromoacetamide group or an iodoacetamide group, is a cysteine-thioether bond and a photoreactive functional group It can be seen that the substituted Fc position selective binding peptide and the physiologically active substance are bound.
본 발명은 또 다른 관점에서, (a) 상기 접합 펩티드로 수식화된 생리활성물질을 Fc 도메인 함유 분자와 혼합하는 단계; (b) 상기 혼합물에 광을 조사하여 상기 접합 펩티드로 수식화된 생리활성물질의 광반응성 작용기와 Fc 도메인 함유 분자가 결합된 항체-생리활성물질 접합체를 생성시키는 단계; 및 (c) 상기 생성된 항체-생리활성물질 접합체를 수득하는 단계를 포함하는 항체-생리활성물질 접합체의 제조방법에 관한 것이다.According to another aspect of the present invention, there is provided a method for producing a fusion protein comprising the steps of: (a) mixing a physiologically active substance formulated with a conjugated peptide with an Fc domain-containing molecule; (b) irradiating the mixture with light to generate a conjugate of an antibody-physiologically active substance to which a photoreactive functional group of the physiologically active substance modified with the conjugated peptide is bound to an Fc domain-containing molecule; And (c) a step of obtaining a conjugate of the antibody-biologically active substance.
본 발명에 있어서, 상기 광은 320 내지 380nm인 것을 특징으로 할 수 있으며, 바람직하게는 350 내지 365nm인 것을 특징으로 할 수 있으나, 이에 제한되는 것은 아니다.In the present invention, the light may be 320 to 380 nm, and preferably 350 to 365 nm. However, the present invention is not limited thereto.
본 발명에서, “Fc 도메인 함유 분자”는 Fc 도메인을 포함하여 Fc 위치선택적 접합 펩티드에 의해 특이적으로 인식되어 인접 또는 결합할 수 있는 분자를 제한 없이 포함한다. 상기 Fc 도메인 함유 분자는 Fc 도메인을 포함하는 단백질, 펩티드, 글리코프로틴, 글리코펩티드, 항체, 항체의 단편, 면역글로불린 또는 면역글로불린의 단편 등을 포함한다. 상기 항체 및 면역글로불린은 약 150 kDa의 이종 4분자체 당단백질(heterotetrameric glycoprotein)으로, 동일한 두 개의 경쇄 및 동일한 두 개의 중쇄를 포함한다. Fc 도메인을 포함하는 이의 단편은 항체 또는 면역글로불린에 파파인을 처리하여 얻은 경쇄 및 중쇄가 제거된 단편일 수 있다.In the present invention, the " Fc domain-containing molecule " includes, without limitation, a molecule including an Fc domain and capable of being adjacent or binding specifically recognized by an Fc position-selective junction peptide. The Fc domain containing molecule includes a protein comprising an Fc domain, a peptide, a glycoprotein, a glycopeptide, an antibody, a fragment of an antibody, an immunoglobulin or an immunoglobulin fragment, and the like. The antibody and immunoglobulin are heterotetrameric glycoproteins of about 150 kDa and comprise the same two light chains and the same two heavy chains. Fc domain thereof may be an antibody or immunoglobulin light chain obtained by treating papain and a fragment from which the heavy chain has been removed.
본 발명에 있어서, 상기 Fc 도메인 함유 분자는 표적분자에 특이적으로 결합가능한 표적지향형 천연 또는 비천연 항체인 것을 특징으로 할 수 있다.In the present invention, the Fc domain-containing molecule may be a target-oriented natural or non-natural antibody capable of specifically binding to a target molecule.
본 발명에서, 항체는 키메라, 인간화된 또는 인간 항체 등의 특정 재조합 항체뿐만 아니라, 폴리클론 및 단클론 항체를 모두 포함한다. 상기 항체는 수용체-특이적 항체 또는 리간드-특이적 항체일 수 있다. 본 발명에서 항체는 또한 리간드 결합을 방지하지 않으나 수용체 활성화를 방지하는 수용체-특이적 항체일 수 있다. 또한, 상기 항체는 치료용 항체일 수도 있고, 별도의 치료제 또는 진단제제와 결합할 수 있는 항체일 수도 있고, 치료 효과가 없는 표적화를 위한 항체일 수도 있고, 단순히 항원-항체 반응을 할 수 있는 항체일 수도 있다.In the present invention, the antibody includes both polyclonal and monoclonal antibodies as well as specific recombinant antibodies such as chimeric, humanized or human antibodies. The antibody may be a receptor-specific antibody or a ligand-specific antibody. In the present invention, the antibody may also be a receptor-specific antibody that does not prevent ligand binding but prevents receptor activation. In addition, the antibody may be a therapeutic antibody, an antibody capable of binding with a separate therapeutic agent or diagnostic agent, an antibody for targeting without therapeutic effect, or an antibody capable of simply reacting with an antigen- Lt; / RTI >
본 발명에서, 항체-생리활성물질 접합체(antibody-biomolecule conjugate)는 특이성(specificity), 체내 혈액순환시 비독성(non-toxicity in circulation) 및 약동학(pharmacokinetics) 등 항체의 장점을 최대한 활용하여 약물이 구체적으로 특정 조직(예를 들어, 암세포)만을 타겟팅하는데 초점을 맞춘 기술이다. 따라서, 면역콘쥬게이트(immunoconjugate)라고도 불리며 “표적화학요법(targeted chemotherapeutics)”을 위한 항암 약물도 이에 속한다. 면역콘쥬게이트는 약물, 단클론 항체 및 상기 항체와 약물을 연결하는 링커(linker)를 포함하는 세 가지 요소로 구성되며, 구체적으로 항암 목적에 있어서, 면역콘쥬게이트 기술은 암세포의 표면에 발현되는 특정 항원에 특이적으로 결합하는 항체를 사용하여 생리적 활성을 가지는 물질을 종양세포에 전달하는 방법이다.In the present invention, the antibody-biomolecule conjugate can be used to maximize the advantages of antibodies such as specificity, non-toxicity in circulation and pharmacokinetics in the blood circulation, Specifically, it is a technology focused on targeting only specific tissues (for example, cancer cells). Thus, it is also referred to as an immunoconjugate and includes anti-cancer drugs for " targeted chemotherapeutics ". The immunoconjugate is composed of three components including a drug, a monoclonal antibody, and a linker linking the antibody and the drug. Specifically, for anticancer purposes, the immunoconjugate technique is a technique in which a specific antigen A method for delivering a substance having physiological activity to tumor cells using an antibody that specifically binds to tumor cells.
본 발명의 일 실시예에서, 생리활성 화합물은 베타-락타메이즈(ß-lactamase(TEM-1)), 베타-락타메이즈 자이모겐(ß-lactamase zymogen) (대한민국등록특허 제1016956840000호(2017.01.06)) 및 슈도모나스 엑소톡신 A(Pseudomonas exotoxin A(PE24))를 사용하였다.In one embodiment of the present invention, the physiologically active compound is selected from the group consisting of beta-lactamase (TEM-1), beta-lactamase zymogen (Korean Patent No. 1016956840000 (2017.01. 06) and Pseudomonas exotoxin A (PE24) were used.
본 발명에서, “ß-lactamase”(아미노산 서열번호 3)는 그 자체로는 세포독성을 갖지 않지만, 베타-락탐 고리(ß-lactam ring)을 가지는 전구약물(prodrug)을 절단하여 약물로 활성화시키는 기작으로, 적절한 prodrug와 함께 처리했을 때 효과적인 종양치료 약물로 이용될 수 있다. 본 발명에서는 GC-mel이라는 불활성 상태의 prodrug를 이용할 수 있고, ß-lactamase에 의해 GC-Mel의 ß-lactam ring이 절단되면 멜파란(Melphalan) 형태로 전환되어 세포내 DNA에 알킬화(alkylation)되고, 이로 인해 세포 증식이 저해되며 세포의 아포토시스(apoptosis)를 유발한다.In the present invention, " ß-lactamase " (amino acid sequence number 3) is not cytotoxic in itself, but a prodrug having a beta-lactam ring is cleaved to activate the drug As a mechanism, it can be used as an effective tumor treatment drug when treated with an appropriate prodrug. In the present invention, an inactive prodrug such as GC-mel can be used. When the β-lactam ring of GC-Mel is cleaved by β-lactamase, it is converted into Melphalan form and alkylated to intracellular DNA , Which inhibits cell proliferation and induces cell apoptosis.
본 발명에서, “ß-lactamase zymogen”(아미노산 서열번호 5)은 베타-락타메이즈 저해 단백질(ß-lactamase inhibitor protein(BLIP))이 ß-lactamase와 융합되어 함께 발현된 상태로 비활성상태로 발현된다. 그러나 두 단백질 사이를 잇는 링커에 암세포에서 과발현되는 매트릭스 메탈로프로티나제(matrix metalloproteinase-2(MMP-2)) 절단 부위를 도입하어 있어, 암세포 주변에서 BLIP이 절단되어 제거되므로 ß-lactamase가 활성을 나타낸다.In the present invention, "β-lactamase zymogen" (amino acid SEQ ID NO: 5) is expressed in an inactivated state with β-lactamase inhibitor protein (β-lactamase inhibitor protein (BLIP) . However, since the linkage between the two proteins is introduced into the cancer cell-overexpressing matrix metalloproteinase-2 (MMP-2) cleavage site, BLIP is cleaved off around cancer cells, so that β-lactamase is active .
본 발명에서, “PE24”(아미노산 서열번호 7)는 세포내 단백질 합성에 관여하는 신장 인자-2(elongation factor-2(EF-2))를 ADP-리보실화(ribosylation)시켜 EF-2를 불활성화시켜, 세포의 아포토시스를 유발한다(미국특허등록 제09388222호(2016.07.12.)).In the present invention, " PE24 " (amino acid sequence number 7) binds EF-2 by ADP-ribosylation of elongation factor-2 (EF-2) And activates to induce apoptosis of cells (U.S. Patent No. 09388222 (Jul. 12, 2016)).
본 발명에 있어서, 상기 Fc 도메인 함유 분자는 면역글로불린 유래의 도메인, 이들의 조합 및 이들의 Fc 영역으로 이루어진 군에서 선택되는 것을 특징으로 할 수 있다. 바람직하게는, IgG, IgA, IgD, IgE, IgM, 이들의 조합 및 이들의 Fc 영역으로 이루어진 군에서 선택되는 것을 특징으로 할 수 있으며, 더욱 바람직하게는 IgG1 또는 이의 Fc 영역인 것을 특징으로 할 수 있으나, 이에 제한되는 것은 아니다.In the present invention, the Fc domain-containing molecule may be characterized in that it is selected from the group consisting of immunoglobulin-derived domains, combinations thereof, and Fc regions thereof. Preferably, IgG is selected from the group consisting of IgG, IgA, IgD, IgE, IgM, combinations thereof, and the Fc region thereof, and more preferably IgG1 or an Fc region thereof But is not limited thereto.
본 발명에서, (c)단계에서 생성된 항체-생리활성물질 접합체를 수득하는 단계는, FcIII가 항체의 중쇄사슬의 Fc 도메인에 결합하기 때문에 융합 단백질과 항체가 광반응하면, 총 3가지 형태(결합하지 않은 항체, 1개의 접합 펩티드로 수식화된 생리활성물질이 항체에 결합한 형태 및 2개의 접합 펩티드로 수식화된 생리활성물질이 항체에 결합한 형태)의 산물이 생성될 수 있다. 치료적 약물(therapeutic drug)로 이용되기 위해서는 정확한 약동학을 가지는 산물을 수득해야 하므로, 생산된 3가지 형태의 산물을 분리하고 1가지 형태의 산물을 수득해야 한다. 1개의 접합 펩티드로 수식화된 생리활성물질이 결합된 형태의 항체-생리활성물질 접합체는 한쪽의 신생아 Fc수용체(neonatal Fc receptor(FcRn))이 자유로운 상태로, 2개의 융합단백질이 결합된 형태보다 체내에서 혈액순환 할 때, 분해되지 않아 높은 약물의 반감기를 기대할 수 있다.In the present invention, in the step of obtaining the antibody-physiologically active substance conjugate produced in step (c), since FcIII binds to the Fc domain of the heavy chain of the antibody, when the fusion protein and the antibody are photoreactive, A form in which a physiologically active substance immobilized on one antibody, a form in which a physiologically active substance immobilized on one antibody, a form in which a physiologically active substance immobilized on one antibody, a form in which a physiologically active substance immobilized on one antibody and a physiologically active substance modulated on two antigenic peptides are bound to an antibody). In order to be used as a therapeutic drug, products having the correct pharmacokinetics must be obtained, so that the three types of products produced must be isolated and one type of product obtained. An antibody-biologically active substance conjugate in which a physiologically active substance formulated with one conjugated peptide is conjugated has a structure in which one neonatal Fc receptor (FcRn) is free, , It can not be decomposed and a high half-life of the drug can be expected.
접합 펩티드로 수식화된 생리활성물질이 결합하지 않은 항체는 항체와 융합단백질의 반응비율과 자외선 조사시간을 조절하여 반응조건을 최적화하여 제거할 수 있다.Antibodies that do not bind a physiologically active substance formulated with a conjugated peptide can be removed by optimizing the reaction conditions by controlling the reaction ratio of the antibody and the fusion protein and the ultraviolet irradiation time.
1개의 접합 펩티드로 수식화된 생리활성물질이 항체와 결합한 항체-생리활성물질 접합체와 2개의 접합 펩티드로 수식화된 생리활성물질이 항체와 결합한 항체-생리활성물질 접합체는 protein A와 항체의 Fc 도메인 간의 결합 친화성(binding affinity)을 이용하여 분리할 수 있다. Protein A는 항체의 Fc 도메인의 CH2-CH3 도메인 인터페이스(interface)에 특이적인 결합 친화성을 가지기 때문에, 항체를 발현한 후 정제할 때 사용하는 친화 크로마토그래피(affinity chromatography)의 레진(resin)으로 사용된다. 따라서, 2개의 접합 펩티드로 수식화된 생리활성물질이 항체에 결합된 항체-생리활성물질 접합체는 protein A 레진과 결합하지 않는다(W.L. DeLano et al, Science, 287(5456):1279-83, 2000). 2개의 생리활성물질이 항체와 결합한 형태는 protein A 친화 크로마토그래피를 통해 제거될 수 있으며, 이후 수득물에 연속적으로 음이온 크로마토그래피(anion chromatography)를 실시함으로써 등전점(isoelectric point)의 차이로 인해 결합하지 않은 항체와 1개의 접합 펩티드로 수식화된 생리활성물질이 항체에 결합한 형태를 분리할 수 있다.A conjugate of an antibody-physiologically active substance conjugated with a physiologically active substance conjugated with one conjugated peptide and a conjugate of an antibody-physiologically active substance conjugated with a biologically active substance conjugated with two conjugated peptides is a conjugate between the protein A and the Fc domain of the antibody Can be separated using binding affinity. Since Protein A has specific binding affinity to the CH 2 -CH 3 domain interface of the Fc domain of the antibody, affinity chromatography resins used for purification after antibody expression, . Thus, antibody-biologically active substance conjugates in which the biologically active substance formulated with two conjugated peptides are bound to the antibody do not bind to the protein A resin (WL DeLano et al, Science , 287 (5456): 1279-83, 2000) . The form in which the two physiologically active substances are bound to the antibody can be removed by protein A affinity chromatography and then subjected to anion chromatography successively on the resulting product to cause binding due to the difference in isoelectric point And a form in which a physiologically active substance formulated with one conjugated peptide is bound to the antibody can be isolated.
본 발명은 또 다른 관점에서, 상기 접합 펩티드로 수식화된 생리활성물질에 항체가 결합되어 있는 항체-생리활성물질 접합체에 관한 것이다.In another aspect, the present invention relates to a conjugate of an antibody-biologically active substance in which an antibody is bound to a physiologically active substance formulated with the conjugated peptide.
본 발명의 다른 실시예에서, IgG1-FcIII-PE24 접합체의 활성을 확인하기 위하여, WST-8 에세이 및 MTS 에세이를 수행하였다. 상기 WST-8 에세이와 MTS 에세이는 배지 내의 균이 생산하는 사립체 숙신산 탈수소효소(mitochondrial succinate dehydrogenase)에 의해 용액 안의 테트라졸리움 염(tetrazolium salt)이 특정 흡광도에서 측정이 가능한 포르마잔(Formazan)으로 변화하므로, 흡광도 측정을 통하여, 세포의 생존을 확인할 수 있다. 상기 3가지 항체-생리활성물질 접합체의 농도를 특정 범위 내에서 늘려가며 흡광도 변화를 측정하였다. 그 결과, 항체와 접합 펩티드로 수식화된 생리활성물질이 결합된 항체-생리활성물질 접합체를 높은 농도로 처리할수록 세포증식 및 생존능이 감소하는 것을 관찰하였다. 따라서, 본 발명의 항체-생리활성물질 접합체는 치료적 약물로 사용할 수 있다는 것을 확인하였다.In another embodiment of the present invention, WST-8 and MTS essays were performed to confirm the activity of the IgG1-FcIII-PE24 conjugate. The WST-8 and MTS essays are transformed into mitochondrial succinate dehydrogenase, which is produced by bacteria in the medium, into tetrazolium salt (Formazan), which can be measured at a specific absorbance , And the survival of the cells can be confirmed by measuring the absorbance. The absorbance changes were measured while increasing the concentrations of the three antibody-physiologically active substance conjugates within a specific range. As a result, it was observed that cell proliferation and viability decreased as the conjugate of the antibody-biologically active substance conjugated with the physiologically active substance modified with the antibody and the conjugated peptide was treated at a high concentration. Thus, it was confirmed that the antibody-biologically active substance conjugate of the present invention can be used as a therapeutic drug.
본 발명에서, 상업적 휴먼 IgG의 일 실시예로써 세툭시맙(Cetuximab)과 트라스투주맙(Trastuzumab)을 이용하여 생리활성물질 접합체를 형성하고 정제 및 분리하여 활성을 확인하였다. 트라스투주맙(Trastuzumab)은 EGFR이나 HER4와 헤테로다이머(heterodimer)를 형성하는 HER2에 특이적으로 작용하여 리간드들에 의존적인 EGFR(EGF, TGFα)이나 HER4(NRG1)의 활성화를 억제하고 하위 신호전달을 막는다. 또한, 세툭시맙(Cetuximab)은 리간드들(EGF, TGFα)에 의존적인 EGFR의 활성화를 억제시키고, 이의 하위 신호전달을 막는다.In the present invention, as an embodiment of commercial human IgG, cetuximab and trastuzumab were used to form a physiologically active substance conjugate, purified and separated to confirm the activity. Trastuzumab acts specifically on HER2 that forms a heterodimer with EGFR or HER4 to inhibit the activation of ligands EGFR (EGF, TGFa) or HER4 (NRG1) Lt; / RTI > Cetuximab also inhibits the activation of EGFR, which is dependent on ligands (EGF, TGFa), and prevents its downregulation.
이하, 실시예를 통하여 본 발명을 더욱 상세히 설명하고자 한다. 이들 실시예는 오로지 본 발명을 예시하기 위한 것으로, 본 발명의 범위가 이들 실시예에 의해 제한되는 것으로 해석되지 않는 것은 당업계에서 통상의 지식을 가진 자에게 있어서 자명할 것이다.Hereinafter, the present invention will be described in more detail with reference to Examples. It is to be understood by those skilled in the art that these embodiments are only for illustrating the present invention and that the scope of the present invention is not construed as being limited by these embodiments.
실시예 1: Fc 위치선택적 접합 펩티드 제조Example 1: Preparation of Fc-position selective splice peptide
효율적인 광반응 결합이 가능한 p-벤조일 페닐알라닌의 치환 위치를 선정하기 위하여, 서열번호 1의 아미노산 서열 중 5번째, 10번째, 또는 11번째 위치의 DNA 염기서열이 각각 앰버 코돈(amber codon)으로 치환된 FcIII 펩티드를 유전자 합성(Bioneer)한 후, 융합단백질 형태로 발현될 수 있도록 유전자 조작을 수행하였다. FcIII 펩티드의 앰버 코돈 위치에 p-벤조일 페닐알라닌이 삽입되도록 발현한 후 정제하였다. 치환 위치에 따른 광반응 효율 변화를 관찰하기 위하여, 휴먼 IgG1과 상기 아미노산 서열 중 5번째 위치의 DNA 염기서열이 각각 앰버 코돈으로 치환된 FcIII 펩티드(아미노산 서열번호 11, 유전자 서열번호 12), 10번째 위치의 DNA 염기서열이 각각 앰버 코돈으로 치환된 FcIII 펩티드(아미노산 서열번호 13, 유전자 서열번호 14) 및 11번째 위치의 DNA 염기서열이 각각 앰버 코돈으로 치환된 FcIII 펩티드(아미노산 서열번호 15, 유전자 서열번호 16)로 수식화된 생리활성물질을 각각 1:3의 비율로 혼합하여 샘플을 제조한 후, 상기 샘플을 1xPBS 버퍼(pH7.4) 상에서 UV hand ramp(Lklab, U01-133-194)를 이용하여, 365nm의 자외선을 2시간 동안 조사하였다.In order to select the substitution position of p-benzoylphenylalanine capable of efficient photoreactive binding, the DNA sequence at the 5th, 10th, or 11th position in the amino acid sequence of SEQ ID NO: 1 is substituted with an amber codon After FcIII peptide was synthesized (Bioneer), gene manipulation was performed so that it could be expressed in the form of a fusion protein. To express p-benzoylphenylalanine at the amber codon position of the FcIII peptide, followed by purification. In order to observe the change of photoreactivity according to the substitution position, human IgG1 and FcIII peptide (amino acid sequence number 11, gene sequence number 12) in which the DNA sequence at the 5th position in the amino acid sequence was substituted with an amber codon, FcIII peptide (amino acid sequence SEQ. ID. NO. 13, gene SEQ. ID NO. 14) in which the DNA sequence of the position was replaced with an amber codon and FcIII peptide in which the DNA sequence at the 11th position was substituted with an amber codon No. 16) was mixed at a ratio of 1: 3 to prepare a sample. The sample was then subjected to a UV hand ramp (Lklab, U01-133-194) on 1xPBS buffer (pH 7.4) And irradiated with ultraviolet light of 365 nm for 2 hours.
그 결과, 10번째 아미노산인 발린이 p-벤조일 페닐알라닌으로 치환된 FcIII로 수식화된 생리활성물질과 항체의 결합 효율이 가장 우수한 것을 확인하였다(도 2). 따라서, FcIII 펩티드의 10번째 아미노산인 발린 위치에 p-벤조일 페닐알라닌을 치환한 샘플이 가장 높은 광반응 효율을 나타낸다.As a result, it was confirmed that the binding efficiency between the physiologically active substance formulated with FcIII substituted with p-benzoyl phenylalanine and valine, which is the 10th amino acid, was the best (FIG. 2). Therefore, a sample in which p-benzoylphenylalanine is substituted at the valine position, which is the 10th amino acid of the FcIII peptide, exhibits the highest photoreaction efficiency.
FcIII 펩티드 발현 플라스미드를 제조하기 위하여, 10번째 아미노산을 코딩하는 유전자가 앰버 코돈으로 치환된 FcIII 펩티드 유전자는 2.1 NEB 버퍼에서 NheI을 처리하여 절단하고 스핀 컬럼(spin column)을 이용하여 절단된 유전자를 거른 후, 3.1 NEB 버퍼에서 BamHI을 처리하여 절단하였다. 상기 버퍼의 조성은 DDW, 10x NEB buffer 3.1, DNA, 제한효소로, 총 부피는 50μl이며, 처리 조건은 각각 37℃, 4시간 동안 수행하였다. 상기와 동일한 제한효소를 처리하여 양끝을 접착성 말단(sticky end)으로 절단된 pET21-a 벡터와 상기 절단된 FcIII 유전자를 1:3의 몰비로 섞어 총 부피 10μl으로 만든 후, T4 DNA 리가아제(NEB, England)를 이용하여, 상온에서 2시간 반응시켜 라이게이션하였다.In order to prepare an FcIII peptide expression plasmid, the FcIII peptide gene in which the gene coding for the 10th amino acid was substituted with an amber codon was digested with NheI in 2.1 NEB buffer, and the gene was cut using a spin column And then cleaved by treatment with BamHI in 3.1 NEB buffer. The composition of the buffer was DDW, 10x NEB buffer 3.1, DNA, restriction enzyme, and the total volume was 50 μl, and the treatment conditions were 37 ° C for 4 hours, respectively. A pET21-a vector digested with sticky ends at both ends was treated with the same restriction enzymes and the cleaved FcIII gene was mixed at a molar ratio of 1: 3 to make a total volume of 10 mu l. Then, T4 DNA ligase ( NEB, England) for 2 hours at room temperature.
상기 라이게이션된 DNA 혼합용액을 수용성 세포(competent cell)인 E.coli DH10B(Thermo sientific, C640003) 50μl와 혼합하여 일렉트로포레이션(electroporation)(Bio-Rad, USA)을 수행하였다. 이후, 암피실린이 포함된 LB 아가 배지에 도말하여 37℃에서 12~14시간 배양하여 형질전환된 균주를 획득하고, DNA를 프렙(prep)(GeneAll, mini prep kit)하여 FcIII 발현 플라스미드-1을 수득하였다.The ligation mixture was mixed with 50 μl of competent cell, E. coli DH10B (Thermosensific, C640003), and electroporation (Bio-Rad, USA) was performed. Then, the transformed strain was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing ampicillin to obtain a transformed strain. FcIII expression plasmid-1 was obtained by DNA prep (GeneAll, mini prep kit) Respectively.
또한, 벡터로 pET22-b를 사용하고, 삽입 DNA로 10번째 아미노산을 코딩하는 유전자가 앰버 코돈으로 치환된 FcIII 펩티드 시퀀스를 사용하여, 제한효소로 NdeI 및 NcoI를 이용하여, 상기와 동일한 방법으로 FcIII 발현 플라스미드-2를 수득하였다.In addition, using pET22-b as a vector and FcIII peptide sequence in which the gene encoding the tenth amino acid was replaced with an amber codon as an insert DNA, NdeI and NcoI were used as restriction enzymes, and FcIII Expression plasmid-2 was obtained.
실시예 2: 접합 펩티드로 수식화된 생리활성물질 제조Example 2: Preparation of physiologically active substance formulated with conjugated peptides
실시예 2-1: FcIII-ß-lactamase 클로닝Example 2-1: FcIII-β-lactamase cloning
서열번호 4로 표시되는 ß-lactamase 전체 시퀀스를 포함하는 플라스미드(pSPEL104)를 주형으로 표 1의 프라이머를 이용하여 중합효소 연쇄반응(polymerase chain reaction(PCR))을 통해 증폭시킨 다음, BamHI과 NotI를 처리하여 제한효소로 절단한 후, 실시예 1의 FcIII 발현 플라스미드-1에 라이게이션하였다.A plasmid (pSPEL104) containing the entire sequence of β-lactamase represented by SEQ ID NO: 4 was amplified by polymerase chain reaction (PCR) using the primer shown in Table 1 as a template, and BamHI and NotI Treated with restriction enzymes, and then ligated to the FcIII expression plasmid-1 of Example 1.
PCR은 변성(denaturation), 어닐링(Annealing), 증폭(Amplification)의 3단계를 거치고 그 방법은 다음과 같다. PCR의 반응 조성은 DDW, 10x pfu 버퍼, 0.2mM dNTP, 20pmol 프라이머 F/R, template, 5units Pfu 중합효소이며, 최종 반응 부피는 50μl이다. 표 1의 BamhI- -f와 TEM1-NotI-r를 이용하여 95℃조건에서 2분간 반응 후, 95℃ 30초, 55℃ 30초, 72℃ 1분을 한 cycle로 하여 25cycle을 반응시키고, 반응종료 후 72℃조건에서 10분 동안 처리하였다.PCR is performed in three steps of denaturation, annealing, and amplification, and the method is as follows. The reaction composition of the PCR is DDW, 10x pfu buffer, 0.2mM dNTP, 20pmol primer F / R, template, 5units Pfu polymerase, and the final reaction volume is 50μl. The reaction was carried out at 95 ° C for 2 minutes using BamhI -f and TEM1-NotI-r in Table 1, followed by 25 cycles of 95 ° C for 30 seconds, 55 ° C for 30 seconds, and 72 ° C for 1 minute, And then treated at 72 캜 for 10 minutes.
표 1은 본 발명에 사용된 PCR 프라이머를 나타낸 것이다.Table 1 shows PCR primers used in the present invention.
Figure PCTKR2018014939-appb-T000001
Figure PCTKR2018014939-appb-T000001
상기 두 제한효소는 3.1 NEB 버퍼에 함께 처리하여 절단하였다. 버퍼의 조성은 DDW, 10x NEB buffer 3.1, DNA, 제한효소이고, 총 부피는 50μl이며, 37℃조건에서 4시간 동안 처리하였다. 상기 제한효소를 처리하여 양끝을 sticky end로 절단된 FcIII 발현 플라스미드-1와 ß-lactamase를 1:3의 몰비로 혼합하여 총 부피가 10μl가 되게한 후, T4 DNA 리가아제(NEB)를 이용하여 25°C조건에서 2시간 동안 라이게이션하였다.The two restriction enzymes were cleaved by treatment with 3.1 NEB buffer. The composition of the buffer was DDW, 10x NEB buffer 3.1, DNA, restriction enzyme, total volume 50 μl, and treated at 37 ° C for 4 hours. The FcIII-expressing plasmid-1 digested with sticky ends at both ends was mixed with β-lactamase at a molar ratio of 1: 3, and the total volume was adjusted to 10 μl. Then, using T4 DNA ligase (NEB) Lt; RTI ID = 0.0 > 25 C < / RTI > for 2 hours.
라이게이션된 DNA 혼합용액을 수용성 세포(competent cell)인 E.coli DH10B(Thermo sientific, C640003) 50μl에 넣은 후 섞어 일렉트로포레이션(Bio-Rad, USA)을 수행하였다. 이후, 암피실린이 포함된 LB 아가 배지에 도말하여 37℃에서 12~14시간 배양하여 형질전환된 균주를 획득하고, DNA를 prep(GeneAll, mini prep kit)하여 FcIII-ß-lactamase(아미노산 서열번호 17, 유전자 서열번호 18) 발현 플라스미드를 수득하였다(도 3).The ligated DNA mixture solution was added to 50 μl of competent cell E. coli DH10B (Thermosensific, C640003), followed by mixing and electroporation (Bio-Rad, USA). Then, the transformed strain was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing ampicillin to obtain a transformed strain. FcIII-β-lactamase (amino acid sequence number 17 , Gene SEQ ID NO: 18) expression plasmids were obtained (Fig. 3).
실시예 2-2: FcIII-ß-lactamase zymogen 클로닝Example 2-2: FcIII-ß-lactamase zymogen cloning
서열번호 6으로 표시되는 ß-lactamase zymogen 시퀀스(1353bp)를 포함하는 플라스미드(pSPEL166)를 주형으로 상기 조건과 동일한 조건에서, 표 1의 프라이머를 이용하여 PCR을 통해 증폭시킨 다음, NcoI과 NotI과 제한효소로 절단한 후, 실시예 1의 FcIII 발현 플라스미드-2에 상기와 동일한 방법으로 라이게이션하였다.A plasmid (pSPEL166) containing the ß-lactamase zymogen sequence (1353 bp) represented by SEQ ID NO: 6 was amplified by PCR using the primers shown in Table 1 under the same conditions as the above conditions and then PCR was performed using NcoI and NotI restriction After digestion with the enzyme, the FcIII expression plasmid-2 of Example 1 was ligated in the same manner as described above.
라이게이션된 DNA 혼합용액을 E.coli DH10B(Thermo sientific, C640003) 50μl에 넣은 후 섞어 일렉트로포레이션(Bio-Rad, USA)을 수행하였다. 이후, 암피실린이 포함된 LB agar 배지에 도말하여 37℃에서 12~14시간 배양한 후 형질전환된 균주를 획득하고, DNA를 prep(GeneAll, mini prep kit)하여 FcIII-ß-lactamase zymogen(아미노산 서열번호 19, 유전자 서열번호 20) 발현 플라스미드를 수득하였다(도 4).The ligation mixture was added to 50 μl of E. coli DH10B (Thermosensific, C640003), followed by electroporation (Bio-Rad, USA). Then, the transformant was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing ampicillin, and the transformed strain was obtained. FcIII-β-lactamase zymogen (amino acid sequence No. 19, gene SEQ. ID No. 20) expression plasmids (FIG. 4).
실시예 2-3: FcIII-PE24 클로닝Example 2-3: FcIII-PE24 cloning
탈면역화된 서열번호 8로 표시되는 PE24를 유전자 합성(Bioneer)으로 수득한 후, 상기와 동일한 방법으로 BamHI과 NotI의 제한효소로 절단한 후, FcIII 발현 플라스미드-1에 라이게이션하였다.PE24 expressed by de-immunized SEQ ID NO: 8 was obtained by gene synthesis (Bioneer) and then digested with BamHI and NotI restriction enzymes in the same manner as described above, and then ligated to FcIII expression plasmid-1.
라이게이션된 DNA 혼합용액을 E.coli DH10B(Thermo sientific, C640003) 50μl에 넣은 후 섞어 일렉트로포레이션(Bio-Rad, USA)을 수행하였다. 이후, 암피실린이 포함된 LB agar배지에 도말하여 37℃에서 12~14시간 배양하여 형질전환된 균주를 획득하고, DNA를 prep(GeneAll, mini prep kit) 하여 FcIII-PE24 융합단백질(아미노산 서열번호 21, 유전자 서열번호 22) 발현 플라스미드를 수득하였다(도 5).The ligation mixture was added to 50 μl of E. coli DH10B (Thermosensific, C640003), followed by electroporation (Bio-Rad, USA). Then, the transformed strain was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing ampicillin to obtain a transformed strain. FcIII-PE24 fusion protein (amino acid sequence number 21 , Gene SEQ ID NO: 22) expression plasmid was obtained (Fig. 5).
실시예 2-4: Orthogonal TAG 코돈인지 tRNA 및 tRNA 합성효소 클로닝Example 2-4: Orthogonal TAG codon cognition tRNA and tRNA synthetase cloning
서열번호 10으로 표시되는 p-벤조일 페닐알라닌 tRNA 합성효소(아미노산 서열번호 9) 시퀀스에 SalI과 BglII를 처리하여 절단한 후, TAG 코돈을 인지하는 tRNA 시퀀스(Jason W. Chin et al, PNAS vol. 99, 11020-11024, 2002)를 포함하는 pEVOL 플라스미드를 벡터로 이용하여 라이게이션하였다(도 6a).A tRNA sequence recognizing the TAG codon (Jason W. Chin et al., PNAS vol. 99 ) was obtained by digesting SalI and BglII with the p-benzoylphenylalanine tRNA synthetase (amino acid SEQ . , 11020-11024, 2002) was used as a vector (Fig. 6A).
라이게이션된 DNA 혼합용액을 E.coli DH10B(Thermo sientific, C640003) 50μl에 넣은 후 섞어 일렉트로포레이션(Bio-Rad, USA)을 수행하였다. 이후, 클로람페니콜(chloroamphenicol)이 포함된 LB 아가 배지에 도말하여 37℃에서 12~14시간 배양하여 형질전환된 균주를 획득하고, DNA를 prep(GeneAll, mini prep kit)하여 TAG 코돈을 인지하여 p-벤조일 페닐알라닌을 삽입하는 tRNA 합성효소(유전자 서열번호 23) 발현 플라스미드를 수득하였다.The ligation mixture was added to 50 μl of E. coli DH10B (Thermosensific, C640003), followed by electroporation (Bio-Rad, USA). Then, the transformant was cultured at 37 ° C. for 12 to 14 hours on an LB agar medium containing chloramphenicol to obtain a transformed strain. The TAG codon was recognized by DNA prep (GeneAll, mini prep kit) And a tRNA synthetase (gene SEQ. ID NO: 23) expression plasmid for inserting benzoyl phenylalanine was obtained.
본 발명에서는 프롤린(proline) tRNA 합성효소 시퀀스를 포함하는 pBbS2K 플라스미드를 이용하였다(Byeong Sung Lee et al, Biochimica Biophysica Acta, S0304-4165, 2017)(도 6b).In the present invention, a pBbS2K plasmid containing a proline tRNA synthetase sequence was used (Byeong Sung Lee et al., Biochimica Biophysica Acta , S0304-4165, 2017) (FIG.
실시예 3: 접합 펩티드로 수식화된 생리활성물질 발현 및 정제Example 3: Expression and purification of physiologically active substance formulated with conjugated peptides
실시예 3-1: FcIII-ß-lactamase의 발현 및 정제Example 3-1: Expression and purification of FcIII-ß-lactamase
FcIII-ß-lactamase의 발현을 위하여, FcIII-ß-lactamase 발현 플라스미드, TAG 코돈인지 tRNA와 p-벤조일 페닐알라닌 tRNA 합성효소 pair를 포함한 플라스미드 및 프롤린 tRNA 합성효소를 포함한 플라스미드를 E.coli BL21(DE3)(SIGMA aldrich, CMC0016)에 일렉트로포레이션한 후, 암피실린, 클로람페니콜, 카나마이신이 포함된 LB 플레이트에 도말하여 형질전환된 균주를 수득하였다.For the expression of FcIII-ß-lactamase, plasmids containing the FcIII-ß-lactamase expression plasmid, TAG codon cognitive tRNA and p-benzoylphenylalanine tRNA synthetase pair and plasmid containing proline tRNA synthetase were transformed into E. coli BL21 (DE3) (SIGMA aldrich, CMC0016), and then plated on an LB plate containing ampicillin, chloramphenicol, and kanamycin to obtain a transformed strain.
상기 수득한 단일 콜로니를 씨드(seed)로 하여 37℃, 180rpm조건에서 12시간 동안 종균배양하고, 10:1의 비율로 배지에 다시 접종하여 37℃, 180rpm 조건에서 6시간 동안 배양하였다. 상기 배양액을 200ml 2xYT(암피실린, 클로람페니콜, 카나마이신 포함) 배지에 100:1의 비율로 접종한 후 37℃, 180rpm 조건에서 배양하여, 600nm에서의 흡광도가 0.5가 되었을 때 최종 농도가 0.2%가 되도록 아라비노오스(arabinose)를 넣어주고, 20nM이 되도록 무수테트라시클린(anhydrotetracycline(aTc))을 첨가하였다. 흡광도가 1.0이 되면 최종농도가 1mM이 되도록 p-벤조일 페닐알라닌 및 IPTG(Isopropyl-β-D-thio-galactoside)을 첨가한 후에, 37℃, 180rpm 조건에서 12시간 동안 배양하였다.The obtained single colonies were seeded at 37 ° C and 180 rpm for 12 hours, seeded at a ratio of 10: 1, and incubated at 37 ° C and 180 rpm for 6 hours. The culture was inoculated at a ratio of 100: 1 to 200 ml of 2xYT (including ampicillin, chloramphenicol, and kanamycin) medium and cultured at 37 ° C and 180 rpm. When the absorbance at 600 nm reached 0.5, the final concentration was 0.2% Arabinose was added, and anhydrotetracycline (aTc) was added to make 20 nM. When the absorbance was 1.0, p-benzoylphenylalanine and IPTG (Isopropyl-β-D-thio-galactoside) were added to a final concentration of 1 mM and then cultured at 37 ° C. and 180 rpm for 12 hours.
상기 발현된 FcIII-ß-lactamase을 정제하기 위하여, 4℃, 9300g 조건에서 15분 동안 원심분리하였다. 이후, 상등액을 제거하고, 5ml 용해 버퍼(lysis buffer)(0.75M sucrose, 0.1 Tris, pH8.0)에 재현탁시키고, 0.05g/ml의 리소자임 및 1mM EDTA 10ml을 첨가한 후, 4℃에서 20분간 회전(rotating)시켰다. 이후, 0.5M MgCl2 1ml을 넣고 4℃에서 10분 동안 회전시킨 뒤, 4℃, 9300g 조건에서 15분간 원심분리하고, 상등액을 분리하였다.In order to purify the expressed FcIII-β-lactamase, it was centrifuged at 4 ° C. and 9300 g for 15 minutes. The supernatant was then removed and resuspended in 5 ml of lysis buffer (0.75 M sucrose, 0.1 Tris, pH 8.0), added with 0.05 ml / l of lysozyme and 1 ml of 1 mM EDTA, And rotated for a minute. Then, 1 ml of 0.5 M MgCl 2 was added and the mixture was rotated at 4 ° C for 10 minutes. The mixture was centrifuged at 4 ° C and 9300g for 15 minutes, and the supernatant was separated.
이후, 히스티딘 태그 단백질(Histidine tagged protein)을 정제하기 위하여, 상기 상등액 20ml에 50% Ni-NTA Superflow 레진(Clonetech, USA) 슬러리 1ml 첨가하여, 4℃조건에서 1시간 동안 회전시키면서 FcIII-ß-lactamase를 레진과 결합시켰다. 상기 반응액을 빈 컬럼에 로딩한 후, 30ml 세척 버퍼(50mM NaPO3, 300mM NaCl, 40mM 이미다졸)를 로딩하여 세척하고, 5ml 용출 버퍼(50mM NaPO3, 300mM NaCl, 300mM 이미다졸)를 로딩하여 6x His-tag FcIII-ß-lactamase을 용출하였다.Then, 1 ml of a slurry of 50% Ni-NTA Superflow resin (Clonetech, USA) was added to 20 ml of the supernatant to purify the histidine tagged protein. FcIII-β-lactamase Lt; / RTI > with resin. The reaction solution was loaded on an empty column and then washed by loading 30 ml wash buffer (50 mM NaPO 3 , 300 mM NaCl, 40 mM imidazole) and loading 5 ml elution buffer (50 mM NaPO 3 , 300 mM NaCl, 300 mM imidazole) 6x His-tag FcIII-ß-lactamase was eluted.
실시예 3-2: FcIII-ß-lactamase zymogen의 발현 및 정제Example 3-2: Expression and purification of FcIII-ß-lactamase zymogen
FcIII-ß-lactamase zymogen의 발현을 위하여, FcIII-ß-lactamase zymogen 발현 플라스미드, TAG 코돈인지 tRNA와 p-벤조일 페닐알라닌 tRNA 합성효소 pair를 포함한 플라스미드 및 프롤린 tRNA 합성효소를 포함한 플라스미드를 E.coli BL21(DE3)(SIGMA aldrich, CMC0016)에 일렉트로포레이션한 후, 상기 FcIII-ß-lactamase의 발현과 동일하게 배양하여 FcIII-ß-lactamase zymogen을 발현시켰다.For the expression of FcIII-ß-lactamase zymogen, plasmids containing the FcIII-ß-lactamase zymogen expression plasmid, TAG codon cognate tRNA and p-benzoylphenylalanine tRNA synthetase pair and plasmid containing proline tRNA synthetase were transformed into E. coli BL21 DE3) (SIGMA aldrich, CMC0016) and then expressing FcIII-β-lactamase zymogen in the same manner as the expression of FcIII-β-lactamase.
이후, 상기 FcIII-ß-lactamase의 정제반응과 동일한 조건으로 정제반응을 수행하여, 6x His-tag FcIII-ß-lactamase zymogen을 용출하였다.Then, the purification reaction was performed under the same conditions as those for the purification of FcIII-β-lactamase to elute the 6 × His-tagged FcIII-β-lactamase zymogen.
실시예 3-3: FcIII-PE24의 발현 및 정제Example 3-3: Expression and purification of FcIII-PE24
FcIII-PE24의 발현을 위하여, FcIII-PE24 발현 플라스미드, TAG 코돈인지 tRNA와 p-벤조일 페닐알라닌 tRNA 합성효소 pair를 포함한 플라스미드 및 프롤린 tRNA 합성효소를 포함한 플라스미드를 E.coli BL21(DE3)(SIGMA aldrich, CMC0016)에 일렉트로포레이션 후, 상기 FcIII-ß-lactamase의 발현과 동일하게 배양하여 FcIII-PE24을 발현시켰다.For expression of FcIII-PE24, a plasmid containing the FcIII-PE24 expression plasmid, a pair of TAG codon cognition tRNA and p-benzoylphenylalanine tRNA synthetase, and a proline tRNA synthetase was transformed into E. coli BL21 (DE3) (SIGMA aldrich, CMC0016) and then expressing FcIII-PE24 in the same manner as that of FcIII-β-lactamase.
이후, 상기 FcIII-ß-lactamase의 정제반응과 동일한 조건으로 정제반응을 수행하여, 6x His-tag FcIII-PE24을 용출하였다.Then, the purification reaction was carried out under the same conditions as the FcIII-β-lactamase purification to elute 6 × His-tag FcIII-PE24.
실시예 4: 세툭시맙(Cetuximab)과 접합 펩티드로 수식화된 생리활성물질의 결합 및 접합체의 분리와 활성Example 4: Binding of physiologically active substances formulated with cetuximab and conjugated peptides and isolation and activity of conjugates
실시예 4-1: Cetuximab과 접합 펩티드로 수식화된 생리활성물질의 결합 확인Example 4-1: Confirmation of binding of physiologically active substance formulated with cetuximab and conjugated peptide
항체와 실시예 3에서 수득한 접합 펩티드로 수식화된 생리활성물질(FcIII-ß-lactamase, FcIII-ß-lactamase zymogen 및 FcIII-PE24)의 결합을 확인하기 위하여, 1:5의 비율로 Cetuximab과 접합 펩티드로 수식화된 생리활성물질을 혼합하여 pH7.4 1xPBS 버퍼 상에서 UV hand ramp(Lklab, U01-133-194)를 이용하여 365nm의 자외선을 2시간 동안 조사하였다. 그 결과, Cetuximab과 접합 펩티드로 수식화된 생리활성물질(FcIII-ß-lactamase, FcIII-ß-lactamase zymogen 및 FcIII-PE24)이 결합한 것을 확인하였다(도 7).In order to confirm the binding of the antibody to the physiologically active substance (FcIII-ß-lactamase, FcIII-ß-lactamase zymogen and FcIII-PE24) formulated with the conjugate peptide obtained in Example 3, conjugation with Cetuximab at a ratio of 1: The peptide-modified physiologically active substance was mixed and irradiated with ultraviolet light of 365 nm for 2 hours using a UV hand ramp (Lklab, U01-133-194) on pH 7.4 1xPBS buffer. As a result, it was confirmed that a physiologically active substance (FcIII-ß-lactamase, FcIII-ß-lactamase zymogen and FcIII-PE24) modified with cetuximab and conjugated peptide was bound (FIG.
접합 펩티드로 수식화된 생리활성물질이 정확하게 항체의 CH2-CH3 도메인 인터페이스(interface)에 위치특이적으로 결합하는지 확인하기 위하여, 10μM 휴먼 IgG1과와 30μM FcIII-ß-lactamase를 고정된 농도비율로 혼합하고, Z-domain의 농도를 10-35μM까지 5μM간격으로 늘려가며 처리한 후, UV hand ramp를 이용하여 365nm 자외선을 조사하며 2시간 동안 광반응하였다. 상기 Z-domain은 FcIII peptide와 동일한 CH2-CH3 도메인 인터페이스에 결합한다.To confirm whether the physiologically active substance formulated with the conjugated peptide binds specifically to the CH 2 -CH 3 domain interface of the antibody, 10 μM human IgG1 and 30 μM FcIII-β-lactamase were mixed at a fixed concentration ratio After the treatment, the Z-domain concentration was increased to 10-35 μM at 5 μM intervals, and then the UV light was irradiated with 365 nm ultraviolet light for 2 hours. The Z-domain binds to the same CH 2 -CH 3 domain interface as the Fc III peptide.
그 결과, FcIII-ß-lactamase 농도보다 높은 농도인 35μM Z-domain을 처리한 후 광반응하였을 때, 형성되는 휴먼 IgG1-FcIII-ß-lactamase가 현저히 줄어드는 것을 확인하였다. 이는, 간접적으로 FcIII 융합단백질이 위치특이적으로 항체의 Fc 도메인에 결합한다는 것을 의미한다(도 8).As a result, it was confirmed that the formed human IgG1-FcIII-β-lactamase was remarkably reduced when the 35 μM Z-domain, which was higher than the concentration of FcIII-β-lactamase, was photoreactive. This implies that the FcIII fusion protein indirectly binds to the Fc domain of the antibody in a site-specific manner (Fig. 8).
또한, 접합 펩티드로 수식화된 생리활성물질과 항체의 접합위치를 확인하기 위하여, LC-MS/MS를 사용하여 분석을 수행하였다. Cetuximab-FcIII-ß-lactamase 콘쥬게이트를 트립신/글루타밀 엔도펩티다제 혼합물 소화(Trypsin/Glutamyl endopeptidase mixture digestion)처리하여 분석하였다. 그 결과, FcIII의 Val10 위치에 삽입된 pBpa의 작용기가 항체의 Met252의 작용기에 형성하는 공유결합으로 인해 위치특이적으로 생성된 콘쥬게이트 fragment의 peaks를 확인하였다(도 9).In addition, analysis was performed using LC-MS / MS to confirm the junction position of the antibody with the physiologically active substance formulated with the conjugated peptide. The Cetuximab-FcIII-ß-lactamase conjugate was analyzed by trypsin / glutamyl endopeptidase mixture digestion. As a result, the peaks of the conjugate fragment that was locally-specific due to the covalent bond formed by the functional group of pBpa inserted at the Val10 site of FcIII to the functional group of Met252 of the antibody were confirmed (FIG. 9).
실시예 4-2: Cetuximab과 접합 펩티드로 수식화된 생리활성물질이 결합된 항체-생리활성물질 접합체의 분리Example 4-2: Separation of conjugate of antibody-biologically active substance conjugated with physiologically active substance modified with cetuximab and conjugated peptide
1개의 접합 펩티드로 수식화된 생리활성물질이 항체와 결합된 항체-생리활성물질 접합체를 분리하기 위하여, 실시예 4의 접합 펩티드로 수식화된 생리활성물질에 항체가 결합된 항체-생리활성물질 접합체를 5ml 1xPBS(pH7.4)에 혼합한 후, 1ml의 Protein A 50% 레진 슬러리(CaptivA Protein A resin, Repligen)를 첨가하여 4℃ 조건에서 1시간 30분 동안 회전시켰다. 상기 반응액을 빈 컬럼에 로딩한 후 레진이 완전하게 가라앉도록 하고, 30ml의 1xPBS(pH7.4)를 로딩하여 세척하였다. 이후 5ml의 용출 버퍼(pH3.0 0.1M Glycine)를 로딩하여 산물을 수득하고, 125μl의 중화 버퍼(pH 9.0 Tris)를 넣어 pH를 적정하였다.In order to isolate a conjugate of an antibody-physiologically active substance conjugated with an antibody and a physiologically active substance formulated with one conjugated peptide, an antibody-physiologically active substance conjugate conjugated with an antibody to the physiologically active substance formulated with the conjugate peptide of Example 4 After mixing with 5 ml 1 × PBS (pH 7.4), 1 ml of Protein A 50% resin slurry (CaptivA Protein A resin, Repligen) was added and the mixture was rotated at 4 ° C for 1 hour and 30 minutes. After loading the reaction solution into an empty column, the resin was completely submerged and washed by loading 30 ml of 1 × PBS (pH 7.4). Then, 5 ml of elution buffer (pH 3.0 0.1 M Glycine) was loaded to obtain a product, and 125 μl of neutralization buffer (pH 9.0 Tris) was added to titrate the pH.
그 결과, 상기 수득한 산물은 1개의 접합 펩티드로 수식화된 생리활성물질이 결합한 항체-생리활성물질 접합체와 접합되지 않은 항체의 혼합물인 것을 확인하였다(도 10).As a result, it was confirmed that the obtained product was a mixture of an antibody-physiologically active substance conjugate conjugated with a physiologically active substance modulated with one conjugated peptide and an antibody not conjugated (FIG. 10).
실시예 4-3: Cetuximab-FcIII-PE24 접합체의 EF2 ribosylation 활성 확인Example 4-3: Confirmation of EF2 ribosylation activity of Cetuximab-FcIII-PE24 conjugate
Cetuximab-FcIII-PE24 접합체의 ADP-리보실레이션 활성을 측정하기 위하여, Zhang과 Snyder의 방법으로 비오틴화(biotinylated) NAD+에서 EF-2 로의 ADP-ribose 전이 측정를 측정하였다.To measure the ADP-ribosylation activity of the Cetuximab-FcIII-PE24 conjugate, ADP-ribose metastasis from biotinylated NAD + to EF-2 was measured by the method of Zhang and Snyder.
PE24와 Cetuximab-FcIII-PE24 접합체를 각각 20mM Tris-HCl (pH 7.4), 1mM EDTA, 1mM DTT에서 1nM으로 희석시키고, 37℃조건에서 1시간 동안 50nM 비오틴화 NAD+의 존재하에 밀 배아 추출물과 함께 배양하였다. 그 후, 5x 소듐도데실설페이트(sodium dodecyl sulfate(SDS)) 겔 로딩 완충액으로 반응을 종결시켰다. 단백질은 SDS-12%(w/v) 폴리아크릴아미드겔에서 분리하였다. 비오틴화 EF-2는 스트렙타비딘-겨자무과산화효소(streptavidin-horseradish peroxidase(HRP)) 접합체를 이용하여 웨스턴블랏으로 검출하였다. 웨스턴블랏 이미지는 ChemiDoc XRS 시스템을 사용하여 분석하였다.The PE24 and Cetuximab-FcIII-PE24 conjugates were diluted to 1 nM in 20 mM Tris-HCl (pH 7.4), 1 mM EDTA, 1 mM DTT and incubated with wheat germ extract in the presence of 50 nM biotinylated NAD + Lt; / RTI > The reaction was then terminated with 5x sodium dodecyl sulfate (SDS) gel loading buffer. Proteins were separated on SDS-12% (w / v) polyacrylamide gel. Biotinylated EF-2 was detected by Western blot using a streptavidin-horseradish peroxidase (HRP) conjugate. Western blot images were analyzed using a ChemiDoc XRS system.
그 결과, PE24와 마찬가지로, Cetuximab-FcIII-PE24 접합체도 EF-2를 ADP-리보실화시켜 불활성화시키는 것을 확인하였다(도 11).As a result, it was confirmed that the Cetuximab-FcIII-PE24 conjugate similarly to PE24 was inactivated by ADP-ribosylation of EF-2 (FIG. 11).
실시예 4-4: Cetuximab-FcIII-PE24 접합체의 세포성장저해 활성 확인Example 4-4: Confirmation of cell growth inhibitory activity of Cetuximab-FcIII-PE24 conjugate
광반응을 통해 생성된 Cetuximab-FcIII-PE24 접합체의 활성을 확인하기 위하여, Cetuximab이 결합하는 특정 항원인 EGFR을 세포 표면에 과발현하는 세포주를 이용하여 세포 생존력 측정(cell viability assay)를 수행하였다.To confirm the activity of the Cetuximab-FcIII-PE24 conjugate produced through the photoreaction, cell viability assay was performed using a cell line overexpressing EGFR, a specific antigen to which Cetuximab binds, on the cell surface.
EGFR 세포주인 A431(SIGMA aldrich, 85090402)을 DMEM 배지(10% FBS, 스트렙토마이신)에 배양한 후, 96-웰 플레이트에 2X103 cell/well로 종균배양하였다. 24시간 후, Cetuximab-FcIII-PE24를 0nM, 0.016nM, 0.16nM, 1.6nM 및 16nM의 농도로 처리하고, 37℃, 5% CO2 조건에서 72시간 동안 배양하였다. 이후, MTS 용액(Promega, G3580)을 20μl/well로 처리하고, 2시간 후 490nm 흡광도를 측정하였다.EGFR cell line A431 (SIGMA aldrich, 85090402) was cultured in DMEM medium (10% FBS, streptomycin) and cultured in 96-well plate at 2 × 10 3 cells / well. After 24 hours, Cetuximab-FcIII-PE24 was treated at a concentration of 0 nM, 0.016 nM, 0.16 nM, 1.6 nM and 16 nM and cultured at 37 ° C, 5% CO 2 for 72 hours. Then, the MTS solution (Promega, G3580) was treated with 20 μl / well and the absorbance at 490 nm was measured after 2 hours.
그 결과, Cetuximab-FcIII-PE24 접합체를 높은 농도를 처리할수록 흡광도가 낮게 나타났으며, 음성대조군으로 야생형 Cetuximab 및 PE24를 처리한 웰보다 세포 생존능이 현저하게 감소하는 것을 확인하였다(도 12).As a result, the absorbance of the Cetuximab-FcIII-PE24 conjugate was found to be lower as the treatment was conducted at higher concentrations, and the cell viability was markedly decreased as compared with the wild type Cetuximab and PE24 treated wells as a negative control (FIG. 12).
실시예 5: 트라스투주맙(Trastuzumab)과 접합 펩티드로 수식화된 생리활성물질의 결합 및 접합체의 분리와 활성Example 5: Binding of physiologically active substances formulated with Trastuzumab and conjugated peptides and isolation and activity of conjugates
실시예 5-1: Trastuzumab과 FcIII-PE24의 결합 확인Example 5-1 Confirmation of Binding of Trastuzumab and FcIII-PE24
항체와 실시예 3에서 수득한 접합 펩티드로 수식화된 생리활성물질(FcIII-PE24)의 결합을 확인하기 위하여, 1:5의 비율로 Cetuximab과 접합 펩티드로 수식화된 PE24을 혼합하여 pH7.4 1xPBS 버퍼 상에서 UV hand ramp(Lklab, U01-133-194)를 이용하여 365nm의 자외선을 2시간 동안 조사하였다. 그 결과, Cetuximab과 접합 펩티드로 수식화된 생리활성물질(FcIII-PE24)이 결합한 것을 확인하였다(도 13).To confirm the binding of the antibody to the physiologically active substance (FcIII-PE24) modified with the conjugated peptide obtained in Example 3, PE424 modified with Cetuximab and a conjugated peptide at a ratio of 1: 5 was mixed, Was irradiated with ultraviolet light of 365 nm for 2 hours using a UV hand ramp (Lklab, U01-133-194). As a result, it was confirmed that the physiologically active substance (FcIII-PE24) modified with Cetuximab and the conjugated peptide was bound (Fig. 13).
실시예 5-2: Trastuzumab-FcIII-PE24 접합체의 분리Example 5-2: Isolation of Trastuzumab-FcIII-PE24 conjugate
1개의 접합 펩티드로 수식화된 생리활성물질(이 항체와 결합된 항체-생리활성물질 접합체를 분리하기 위하여, 실시예 4의 접합 펩티드로 수식화된 생리활성물질에 항체가 결합된 항체-생리활성물질 접합체를 5ml 1xPBS(pH7.4)에 혼합한 후, 1ml의 Protein A 50% 레진 슬러리(CaptivA Protein A resin, Repligen)를 첨가하여 4℃ 조건에서 1시간 30분 동안 회전시켰다. 상기 반응액을 빈 컬럼에 로딩한 후 레진이 완전하게 가라앉도록 하고, 30ml의 1xPBS(pH7.4)를 로딩하여 세척하였다. 이후 5ml의 용출 버퍼(pH3.0 0.1M Glycine)를 로딩하여 산물을 수득하고, 125μl의 중화 버퍼(pH 9.0 Tris)를 넣어 pH를 적정하였다.In order to isolate a conjugate of an antibody-biologically active substance conjugated with this antibody, a conjugate of an antibody-biologically active substance conjugated with an antibody to a physiologically active substance formulated with the conjugated peptide of Example 4 (CaptivA Protein A resin, Repligen) was added to 1 ml of a Protein A 50% resin slurry, which was then rotated for 1 hour and 30 minutes at 4 ° C. The reaction solution was transferred to an empty column After loading, the resin was completely submerged and washed by loading 30 ml of 1xPBS (pH 7.4). The product was then loaded by loading 5 ml of elution buffer (pH 3.0 0.1M Glycine), and 125 μl of The pH was titrated by adding neutralizing buffer (pH 9.0 Tris).
그 결과, 상기 수득한 산물은 1개의 접합 펩티드로 수식화된 생리활성물질이 결합한 항체-생리활성물질 접합체와 접합되지 않은 항체의 혼합물인 것을 확인하였다(도 13). 연속적으로 상기 수득한 산물에 20mM phosphate buffer(pH7.9)을 혼합하여 음이온 크로마토그래피(mono-Q column, GE Healthcare Life Science, USA)를 실시하여 결합하지 않은 항체와 1개의 접합 펩티드로 수식화된 생리활성물질이 항체에 결합한 형태를 분리하여 확인하였다(도 13).As a result, it was confirmed that the obtained product was a mixture of antibody-biomolecule conjugate conjugated with physiologically active substance modified with one conjugated peptide and antibody not conjugated (FIG. 13). The resultant product was continuously mixed with 20 mM phosphate buffer (pH 7.9) and subjected to anion chromatography (mono-Q column, GE Healthcare Life Science, USA) The form in which the active substance was bound to the antibody was isolated and confirmed (Fig. 13).
실시예 5-3: Trastuzumab-FcIII-PE24 접합체의 세포성장저해 활성 확인Example 5-3: Confirmation of cell growth inhibitory activity of Trastuzumab-FcIII-PE24 conjugate
광반응을 통해 생성된 Trastzumab-FcIII-PE24 접합체의 활성을 확인하기 위하여, Trastuzumab이 결합하는 특정 항원인 HER2을 세포 표면에 과발현하는 세포주들과 미발현하는 세포주를 이용하여 세포 생존력 분석(cell viability assay)을 수행하였다.In order to confirm the activity of the Trastzumab-FcIII-PE24 junction produced by the photoreaction, the cell viability assay (cell viability assay (cell viability assay) was performed using cell lines overexpressing HER2, a specific antigen to which Trastuzumab binds, ) Were performed.
HER2 과발현 세포주인 BT-474(한국세포주은행, 60062), HCC-1954(한국세포주은행, 9S1954), MDA-MB-453(한국세포주은행, 30131)과 HER2 미발현 세포주인 MDA-MB-231(한국세포주은행, 30026)을 RPMI 배지(10% FBS, 스트렙토마이신)에 배양한 후, 96-웰 플레이트에 3-5X103 cell/well로 종균배양하였다. 24시간 후, trastuzumab-FcIII-PE24를 0nM, 0.0064nM, 0.032nM, 0.16nM, 0.8nM, 4nM, 20nM의 농도로 처리하고, 37℃, 5% CO2 조건에서 72시간 동안 배양하였다. 이후, WST-8 용액(Dojindo, CK04-11)을 10μl/well로 처리하고, 2시간 후 450nm 흡광도를 측정하였다.HER2 overexpressing cell line, MDA-MB-231 (Korean Cell Line Bank, 60062), HCC-1954 (Korean Cell Line Bank, 9S1954), MDA-MB- Korean Cell Line Bank, 30026) were cultured in RPMI medium (10% FBS, streptomycin) and cultured in 3-5 × 10 3 cells / well on 96-well plates. After 24 hours, trastuzumab-FcIII-PE24 was treated at concentrations of 0 nM, 0.0064 nM, 0.032 nM, 0.16 nM, 0.8 nM, 4 nM and 20 nM and cultured at 37 ° C and 5% CO 2 for 72 hours. Thereafter, the WST-8 solution (Dojindo, CK04-11) was treated with 10 μl / well, and the absorbance at 450 nm was measured after 2 hours.
그 결과, HER2 과발현 세포에 Trastuzumab-FcIII-PE24 접합체를 농도를 높게 처리할수록 흡광도가 낮게 나타났으며, 음성대조군으로 야생형 trastuzumab 및 PE24를 처리한 웰보다 세포 생존능이 현저하게 감소하는 것을 확인하였다. 대조적으로 HER2 미발현 세포에 대해서는 trastuzumab-FcIII-PE24 접합체의 세포독성이 해당농도범위에서 작용하지 않는 결과를 확인하였다(도 14).As a result, the higher the concentration of Trastuzumab-FcIII-PE24 conjugate was, the lower the absorbance of HER2-overexpressing cells was, and the cell viability was markedly decreased as compared with the wild type trastuzumab and PE24 treated wells. In contrast, it was confirmed that the cytotoxicity of trastuzumab-FcIII-PE24 conjugate did not act in the corresponding concentration range for HER2 non-expressing cells (FIG. 14).
본 발명에 따른 특정 위치가 광반응성 작용기로 치환된 Fc 위치선택적 접합 펩티드를 이용하여 접합 펩티드로 수식화된 생리활성물질을 제조한 후, 광반응을 통해 항체와 상기 생리활성물질을 결합시키면, 생리활성물질을 간단한 광반응을 통해서 항체에 위치 선택적이고 고효율로 연결할 수 있다. 따라서, 다양한 종류의 생리활성물질과 항체를 연결한 항체-생리활성물질 접합체 제조에 이용할 수 있고, 이의 상업화를 가속화시킬 수 있다.When a physiologically active substance modified with a conjugated peptide is prepared by using an Fc positionally selected binding peptide in which a specific position according to the present invention is substituted with a photoreactive functional group and then the antibody and the physiologically active substance are bound through a photoreaction, The material can be linked to the antibody in a selective and highly efficient manner through a simple photoreaction. Therefore, the present invention can be used for the production of antibody-physiologically active substance conjugates in which various kinds of physiologically active substances and antibodies are linked, and the commercialization thereof can be accelerated.
이상으로 본 발명 내용의 특정한 부분을 상세히 기술하였는 바, 당업계의 통상의 지식을 가진 자에게 있어서 이러한 구체적 기술은 단지 바람직한 실시 양태일 뿐이며, 이에 의해 본 발명의 범위가 제한되는 것이 아닌 점은 명백할 것이다. 따라서 본 발명의 실질적인 범위는 첨부된 청구항들과 그것들의 등가물에 의하여 정의된다고 할 것이다.While the present invention has been particularly shown and described with reference to specific embodiments thereof, those skilled in the art will appreciate that such specific embodiments are merely preferred embodiments and that the scope of the present invention is not limited thereto will be. It is therefore intended that the scope of the invention be defined by the claims appended hereto and their equivalents.
전자파일 첨부하였음.I attached an electronic file.

Claims (13)

  1. 서열번호 1의 아미노산 서열로 표시되는 Fc 위치선택적 결합 펩티드에서 5번째, 10번째 또는 11번째 위치가 광반응성 작용기를 갖는 아미노산으로 치환된 Fc 위치선택적 접합 펩티드.An Fc position-selective fused peptide wherein the 5th, 10th, or 11th position of the Fc position-selective binding peptide represented by the amino acid sequence of SEQ ID NO: 1 is substituted with an amino acid having a photoreactive functional group.
  2. 제1항에 있어서, 상기 광반응성 작용기를 갖는 아미노산으로 치환된 위치가 10번째인 것을 특징으로 하는 접합 펩티드.2. The conjugate peptide according to claim 1, wherein the position substituted with the amino acid having the photoreactive functional group is tenth.
  3. 제1항에 있어서, 상기 광반응성 작용기를 갖는 아미노산은 p-벤조일 페닐알라닌(p-benzoyl phenylalanine)인 것을 특징으로 하는 접합 펩티드.The conjugated peptide according to claim 1, wherein the amino acid having the photoreactive functional group is p-benzoyl phenylalanine.
  4. 제1항 내지 제3항 중 어느 한 항의 펩티드에 생리활성물질이 직접 또는 링커를 통해 연결되어 있는 접합 펩티드로 수식화된 생리활성물질.A physiologically active substance modulated with a peptide of any one of claims 1 to 3, wherein the physiologically active substance is directly or via a linker.
  5. 제4항에 있어서, 상기 생리활성물질은 치료제 또는 진단제제인 것을 특징으로 하는 접합 펩티드로 수식화된 생리활성물질.5. The physiologically active substance according to claim 4, wherein the physiologically active substance is a therapeutic agent or a diagnostic agent.
  6. 제5항에 있어서, 상기 치료제 또는 진단제제는 효소, 호르몬(Hormon), 사이토카인, 항체, 항체 단편, 진통제, 해열제, 항염증제, 항생 물질, 항바이러스(virus)제, 항진균약, 심장혈관약, 중추 신경 작용약, 신장 기능 및 전해질 대사 작용약, 화학 요법제로 구성된 군에서 선택되는 것을 특징으로 하는 접합 펩티드로 수식화된 생리활성물질.6. The method of claim 5, wherein the therapeutic agent or diagnostic agent is selected from the group consisting of an enzyme, a hormone, a cytokine, an antibody, an antibody fragment, an analgesic agent, an antitumor agent, an antiinflammatory agent, an antibiotic, an antiviral agent, Wherein the physiologically active substance is selected from the group consisting of central nervous system drugs, kidney function, electrolyte metabolism drugs, and chemotherapeutic agents.
  7. 제4항에 있어서, 상기 링커는 반응성 기능기, 아미노산 및 자가 절단 스페이서를 포함하는 것을 특징으로 하는 접합 펩티드로 수식화된 생리활성물질.5. The physiologically active substance as claimed in claim 4, wherein the linker comprises a reactive functional group, an amino acid and a self-cleaving spacer.
  8. 다음 단계를 포함하는 항체-생리활성물질 접합체의 제조방법:A method for producing an antibody-biologically active substance conjugate comprising the steps of:
    (a) 제4항의 접합 펩티드로 수식화된 생리활성물질을 Fc 도메인 함유 분자와 혼합하는 단계;(a) mixing a physiologically active substance formulated with the conjugated peptide of claim 4 with an Fc domain containing molecule;
    (b) 상기 혼합물에 광을 조사하여 상기 접합 펩티드로 수식화된 생리활성물질의 광반응성 작용기와 Fc 도메인 함유 분자가 결합된 항체-생리활성물질 접합체를 생성시키는 단계; 및(b) irradiating the mixture with light to generate a conjugate of an antibody-physiologically active substance to which a photoreactive functional group of the physiologically active substance modified with the conjugated peptide is bound to an Fc domain-containing molecule; And
    (c) 상기 생성된 항체-생리활성물질 접합체를 수득하는 단계.(c) obtaining the resulting antibody-biologically active substance conjugate.
  9. 제8항에 있어서, 상기 광은 320 내지 380nm인 것을 특징으로 하는 항체-생리활성물질 접합체의 제조방법.9. The method according to claim 8, wherein the light is 320 to 380 nm.
  10. 제8항에 있어서, 상기 Fc 도메인 함유 분자는 표적분자에 특이적으로 결합가능한 표적지향형 천연 또는 비천연 항체인 것을 특징으로 하는 항체-생리활성물질 접합체의 제조방법.9. The method of claim 8, wherein the Fc domain-containing molecule is a target-directed natural or non-natural antibody capable of specifically binding to a target molecule.
  11. 제8항에 있어서, 상기 Fc 도메인 함유 분자는 IgG, IgA, IgD, IgE, IgM, 이들의 조합 및 이들의 Fc 영역으로 이루어진 군에서 선택되는 것을 특징으로 하는 항체-생리활성물질 접합체의 제조방법.9. The method of claim 8, wherein the Fc domain-containing molecule is selected from the group consisting of IgG, IgA, IgD, IgE, IgM, combinations thereof, and Fc regions thereof.
  12. 제11항에 있어서, 상기 Fc 도메인 함유 분자는 IgG1 유래의 도메인 조합 및 이들의 Fc 영역으로 이루어진 군에서 선택되는 것을 특징으로 하는 항체-생리활성물질 접합체의 제조방법.12. The method for producing an antibody-biologically active substance conjugate according to claim 11, wherein the Fc domain-containing molecule is selected from the group consisting of IgG1-derived domain combinations and Fc regions thereof.
  13. 제4항의 접합 펩티드로 수식화된 생리활성물질에 항체가 결합되어 있는 항체-생리활성물질 접합체.An antibody-biologically active substance conjugate wherein an antibody is bound to a physiologically active substance formulated with the conjugated peptide of claim 4.
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