JP2001505194A - Branched peptide linker - Google Patents

Abstract

  (57) [Summary] The present invention relates to conjugates comprising a target ligand, such as an antibody, a therapeutically active drug and a branched peptide linker, and provides the branched peptide linker. The branched peptide linker of the invention contains two or more amino acid components that provide an enzyme cleavage site. The number of drugs that can be attached to the branching linker varies by a factor of two for each generation of branching.

Description

DETAILED DESCRIPTION OF THE INVENTION                          Branched peptide linker Background art   Bifunctional compounds (ie, “linkers”) that link a cytotoxic reagent to an antibody are: Are known in the art. These compounds are particularly directed against tumor-associated antigens. Useful for the formation of immunoconjugates. Take Immunoconjugates enable selective delivery of toxic drugs to tumor cells [ For example, Harmentin & Sailor's "Behring Insti. Mitl." 2: 197-215, 1988), "Monoclonal antibody-drug conjugate. Research on Gallego et al., "Int. J. Cancer" (33: 737-744, 19). 1984), four daunomycin-monoclonal antibodies 791T with antitumor activity / 36 Conjugate Production "; Arnon et al.," Immunological Rev. "(62 : 5-27, 1982), "Conjugation of daunomycin and antitumor antibody. In Vitro and In Vivo Efficacy "].   Greenfield et al. Disclose at the 13-keto position of the anthracycline molecule. On the other hand, acid-sensitive immunity containing acylhydrazide bound via acylhydrazone bond Formation of epidemic conjugates and conjugation of this anthracycline derivative to antibody molecules European Patents by Greenfield et al. Application Publication No. EP 0328147 (published August 16, 1989), which is disclosed in US Pat. Patent application No. 07/270509 (filed on November 16, 1988) and U.S. Pat. S. Patent Application No. 07/155181 (filed on February 11, 1988), Abandoned now]. The latter references also include specific thioether-containing linkers and Conjugates (including immunoconjugates containing hydrazine thioether) are also available It is shown.   Also, U.S. Patent Application No. 07 / 522,996 (Kaneko et al., May 1, 1990) (Filed on April 4) (European Patent Application Publication No. EP A0457250, 1991) Corresponding to the publication on November 21, 2011) contains the acyl at the C-13 position of the anthracycline molecule. Anthracycline antibiotic linked to a bifunctional linker by hydrazone linkage The formation of the containing conjugate is described. In their invention, the linker Contains a reactive pyridinyldithio or ortho-nitrophenyldithio group The group allows the linker to react with the appropriate group attached to the cell-reactive ligand. To form a complete conjugate.   Conjugates rely on simple acid hydrolysis to release drug prematurely You. Therefore, it has conjugates that release the active drug in a highly site-specific manner Is desired. In European Patent Application Publication No. 94 107501.2, A lysosomal enzyme-cleaving antitumor drug that can be selectively activated at the site of a tumor Product conjugates are disclosed. However, conventional immunoconjugates One of the problems is that drugs and target ligands (eg, immunoglobulins) (Phosphorus) is relatively low. Can be activated at the tumor site and More demand for immunoconjugates that increase the proportion of target ligands .                                Summary of the Invention   The present invention provides novel branched peptide linkers. Offer. This new linker is used to produce new drug / linker molecules, and And targeting ligands, therapeutically active drugs and branched peptide phosphorus Manufacture biologically active conjugates consisting of Kerr. this The new conjugate is a site in the selected target cell population that is recognized by the target ligand Can be selectively activated.   As used herein, the phrase “drug / linker” or “linker / drug” The branched peptide linker is coupled to more than one therapeutically active drug molecule And the phrase "conjugate" refers to the drug / linker molecule And the one coupled with the command.   The branched peptide linker of the present invention is a protein peptide spacer (protein pe). ptide spacer) and self-sacrifice spacing between the protein peptide sequence and the drug (Self-immolating) spacers may also be included. The linker of the invention is branched Therefore, more than one drug molecule per linker is coupled to the target ligand. To run. The number of drugs attached to each linker depends on the number of branches (or branches) In multiples of two. Thus, the number of drug molecules per linker molecule The numbers would be 2, 4, 8, 16, 32, 64, etc. The branching factor is mathematically 2ⁿ(N is a positive integer). The first branching linker is the first Branching or two¹Ie, potentially two per linker Contains drug molecules. The bi-branched linker is a second-generation branched or Is 2^TwoIe, potentially containing 4 drug molecules per linker You.   As n rises from n = 1, the immunoconjugate Solubility tends to decrease. Use highly water-soluble peptides or Solubilizing components, for example charged species such as polyethylene glycol or β-alanine Is added to the drug and released from the drug by enzymes in a low pH or liposome environment. By doing so, the solubility can be increased.   The invention relates to linking a thiol group derived from a targeting ligand to two or more drug moieties. The branched peptide linker to be linked to the target peptide. A thiol group (also referred to as a sulfhydryl group) derived from Consisting of a compound having a terminal containing an acceptor; a polyvalent atom (eg, carbon Atom or nitrogen atom) is 2ⁿ(Where n is positive Taking into account the degree of branching of at least two amino acids per branch. The minutes provide at least one enzyme site per branch, and at least Both ends are covalently linked with chemically reactive functional groups derived from the drug component It contains a group capable of forming Preferably n is 1, 2, 3 or 4, more preferably Is 1, 2 or 3, most preferably 1 or 2. The target ligand is an antibody Or a fragment thereof.   As used in the previous paragraph, the phrase "thiol group derived from the target ligand" The thiol group is already present in the target ligand, or Is modified to contain a thiol group (if necessary, the denaturing agent A thiol spacer group between the thiol and thiol groups). You. Similarly, the phrase “a chemically reactive functional group derived from a drug component” refers to a chemical If a reactive functional group is already present on the drug or the drug is chemically modified , Containing chemically reactive functional groups. Such chemically reactive functionalities A group is a group that can form a covalent bond with the linker terminus. Of chemically reactive functional groups Concrete example As primary or secondary amino, hydroxyl, sulfhydroxyl, Boxyl, aldehyde, ketone and the like can be mentioned.   The present invention also provides a linker, drug / linker, and / or conjugate. An intermediate to be produced; and administering the conjugate of the invention to a patient. And methods for treating or preventing a selected disease state.   The selected target cell population recognized by the target ligand is preferably a tumor cell population. It is.   The present invention provides, in one aspect, drug-activated enzyme cleavage by one or more tumor-associated enzymes. Provide tumor-specific conjugates that are highly selective substrates for cleavage.   In another aspect, the present invention provides a method wherein the activating enzyme has a cytotoxic level of free drug near the tumor. Tumor-specific drug conduit that is present in the tumor in an amount sufficient to cause Provide a courier.   In another aspect, the present invention provides a tumor-specific, stable, Provide a drug conjugate.   Furthermore, the present invention, in other respects, is significantly less toxic than activated drugs. The present invention provides a tumor-specific conjugate of the present invention.   In yet another aspect, the present invention relates to a method wherein the mutation in a biological process is, for example, cancer. Provide a method to deliver the conjugate to target cells, which is desired for the treatment of any disease. Offer.   The present invention also provides a conjugate according to the present invention, which is administered to a warm-blooded animal. And a method for delivering an active antitumor agent to a site of a tumor cell of the warm-blooded animal.   An object of the above and other aspects of the present invention is to suppress the pharmacological activity of an antitumor drug, Thus, the antineoplastic agent is converted to a pharmacologically inactive peptidyl derivative conjugate Therefore, at an appropriate reactive site, a protein peptide sequence and a self-immolative spacer Drugs that are linked to ligands via peptide linkers (For example, an antitumor agent). The above peptide linker Has at least two amino acid residue sequences, in particular, a peptidyl derivative By one or more lysosomal proteases, such as cathepsins B, C, D or L It is adapted to be a selective substrate for drug-activated enzyme cleavage. enzyme The cleavage reaction removes the peptide linker component from the drug conjugate and Selectively at the site of the tumor, resulting in the release of a pharmacologically active form of the antineoplastic agent. Drug release Compared to a ligand-drug linker that relies on simple acid hydrolysis for The new method is based on premature linker hydrolysis in the blood, resulting in significantly lower systemic toxicity So that a large amount of the drug is transported to the tumor site, and the method comprises Produces a longer shelf life and simplifies the handling conditions of the conjugate.   The conjugate of the present invention comprises a biparte conjugate and a free drug. Shows much lower systemic toxicity compared to The conjugate of the invention was selected It possesses both specificity and therapeutic activity for treatment of a target cell population. Such a The conjugate can be used in a pharmaceutical composition, for example, For example, a pharmaceutically effective amount of a compound of formula (III) below, and a pharmaceutically acceptable carrier, Consists of a diluent or excipient.   The present invention relates to a linker molecule of formula (I):   [Wherein A is a thiol acceptor;   W is a bridging moiety;   c is 0 or 1;   a is an integer of 2 to 12;   Q is O, NH or N-lower alkyl;   p is 0 or 1;   d is 0 or 1;   E is a polyvalent atom;   Each b is an integer from 1 to 10;   Each X is a group of the formula: -CO-Y-Zm-Gn, where   Y is two L-type amino acid residues,   Z is one or two amino acid residues,   m is 0 or 1,   G is a self-immolative spacer, and   n is 0 or 1, provided that when G is 0, -Y-Zm is ala-leu-ala-leu or Is gly-phe-leu-gly; or   Each X is of the formula: The base of here   Each X¹Is a group of the formula: -CO-Y-Zm-Gn, Y, Z, Q, E, G, m, d, p, a, b and n are as defined above, or   Each X¹Is the formula: Group of each X^TwoIs a group of the formula: -CO-Y-Zm-Gn, Y, Z, G, Q, E, m, d, p, a, b and n are as defined above, or each X^TwoIs the formula: Group of each X^ThreeIs a group of the formula: -CO-Y-Zm-Gn, Y, Z, G, Q, E, m, d, p, a, b and n are as defined above, or each X^ThreeIs the formula: Group of each X^FourIs a group of the formula: -CO-Y-Zm-Gn, Y, Z, G, Q, E, m, d, p, a, b and n are as defined above.   The present invention also relates to drug / linker molecules of formula (II):   Wherein A is a thiol acceptor;   W is the bridge;   c is 0 or 1;   a is an integer of 2 to 12;   Q is O, NH or N-lower alkyl;   p is 0 or 1;   d is 0 or 1;   E is a polyvalent atom;   Each b is an integer from 1 to 10;   Each X is a group of the formula: -CO-Y-Zm-GnD, where   Y is two L-type amino acid residues,   Z is one or two amino acid residues,   m is 0 or 1,   G is a self-sacrifice spacer,   n is 0 or 1, provided that when G is 0, -Y-Zm is ala-leu-ala-leu or Is gly-phe-leu-gly, and   D has a main chain and at least one chemically reactive functional group hanging from the main chain. The functional group is a self-immolative spacer or a terminal amino acid residue. Reacts with a group to form a covalent bond and the functional group is a primary or secondary amino group. , Hydroxyl, sulfhydryl, carboxyl, aldehyde or ketone group Selected from; or   Each X is of the formula: The base of here   Each X¹Is a group of the formula: -CO-Y-Zm-Gn-D, Y, Z, G, D, Q, E, m, d, p and n are as defined above, or   Each X¹Is the formula: Group of each X^TwoIs a group of the formula: -CO-Y-Zm-Gn-D, Y, Z, G, D, Q, E, m, d, p, a, b and n are as defined above, or each X^TwoIs the formula: Group of each X^ThreeIs a group of the formula: -CO-Y-Zm-Gn-D, Y, Z, G, D, Q, E, m, d, p, a, b and n are as defined above, or each X^ThreeIs the formula:Group of each X^FourIs a group of the formula: -CO-Y-Zm-Gn-D, Y, Z, G, D, Q, E, m, d, p, a, b and n are as defined above.   Furthermore, the present invention relates to a conjugate of the following formula (III):   [Wherein L is a ligand;   q is an integer of 1 to 10;   A is a thiol acceptor;   W is the bridge;   c is 0 or 1;   a is an integer of 2 to 12;   Q is O, NH or N-lower alkyl;   p is 0 or 1;   d is 1 or 2;   E is a polyvalent atom;   Each b is an integer from 1 to 10;   Each X is a group of the formula: -CO-Y-Zm-Gn-D, where   Y is two L-type amino acid residues,   Z is one or two amino acid residues,   m is 0 or 1,   G is a self-immolative spacer, and   n is 0 or 1, provided that when G is 0, -Y-Zm is ala-leu-ala-leu or Is gly-phe-leu-gly;   D has a main chain and at least one chemically reactive functional group hanging from the main chain. The functional group reacts with the self-immolative spacer and Form a bond and the functional group is a primary or secondary amino, hydroxyl, Selected from the group of xyl, sulfhydryl, aldehyde or ketone; or   Each X is of the formula: The base of here   Each X¹Is a group of the formula: -CO-Y-Zm-Gn-D, Y, Z, G, D, Q, E, m, d, p, a, b and n are as defined above, or   Each X¹Is the formula: Group of each X^TwoIs a group of the formula: -CO-Y-Zm-Gn-D, Y, Z, G, D, Q, E, m, d, p, a, b and n are as defined above, or each X^TwoIs the formula: Group of each X^ThreeIs a group of the formula: -CO-Y-Zm-Gn-D, Y, Z, G, D, Q, E, m, d, p, a, b and n are as defined above, or each X^ThreeIs the formula:Group of each X^FourIs a group of the formula: -CO-Y-Zm-Gn-D, Y, Z, G, D, Q, E, m, d, p, a, b and n are as defined above.   The phrase "lower alkyl" as used herein is an alkyl group having 1 to 3 carbon atoms. . The polyvalent atom is preferably carbon or nitrogen.   In one embodiment, the drug components are an anthracycline antibiotic, and a target drug. Gand is an antibody.   In a preferred embodiment, the anthracycline is the amino group of anthracycline. It is linked to the linker at the sugar group. The sugar component is preferably daunosamine. next The antibody binds to the anthracycline compound via the linker. Particularly preferred tool In one embodiment, the linkage is a reducing disulfide group (ie, the free sulfhydryl group of the antibody). Via the drill group (-SH)).   In a most preferred embodiment, the anthracycline drug component is doxorubicin; The thiol acceptor is the Michael Addition accessor. Puter (Michael Addition Adduct from the acceptor) Adduct) is derived), more preferably a maleimide group; and the antibody component is A chimeric or humanized antibody, wherein the linker The point of attachment is the amino group of the sugar component of the drug.   The conjugates of the invention have specificity for the treatment of a selected target cell population. Retains both therapeutic activity. Such conjugates can be used in pharmaceutical compositions. The pharmaceutical composition includes, for example, a pharmaceutically effective amount represented by the following formula (III): And a pharmaceutically acceptable carrier, diluent or excipient.                             Detailed description of the invention   The present invention relates to a ligand capable of targeting a selected cell population. (Target ligand), and connected to the ligand by a branched peptide linker A novel drug-linker-ligand conjugate comprising a drug is provided. The linker is a thiol acceptor (for example, Michael Addition Accessor). ), Bridges, branch points and enzymes of enzymes such as cathepsins B, C, D or L Per branch, providing a cleavage site and containing at least two amino acid components Of the peptide sequence. The branched peptide linker is a self-immolative spacer The spacer may also space the drug and protein peptide sequence. Peptide arrangement If the sequence (ie, YZm) is ala-leu-ala-leu or gly-phe-leu-gly The presence of the self-immolative spacer was found to be optional. These peptides The reason for not requiring a self-immolative spacer for the sequence is not fully understood, This appears to be based on responses to various enzymes.   The target ligand molecule is an immunoreactive protein such as an antibody or a fragment thereof. Non-immunoreactive proteins; peptide ligands such as bombesin; A binding ligand that recognizes a vesicle-related receptor; or a reactive sulfhydryl group (- SH) or modified to contain such sulfhydryl groups. It can be any protein or peptide that can be used. Thiolak Scepter-carboxyl compounds are linked to ligands via thioether bonds Drugs include primary or secondary amino, hydroxyl, sulfhydryl, carbohydrate Linked to a linker via a functional group selected from xyl, aldehyde or ketone You.   For a more specific understanding of the invention, drugs, ligands, peptides and Discuss sir individually. Next, the synthesis of the conjugate will be described.   Abbreviations and terminology used in the following detailed description and the appended claims. Is common in amino acid and peptide chemistry, and It will be understood that all of the amino acids are in the L-form unless otherwise specified.   Some abbreviations used in the present invention are as follows unless otherwise indicated. You.   AcOH: acetic acid, Alloc: allyloxy-carbonyl, Boc: t-butyloxycal Bonyl, DBU: diazobicycloundecene, DCC: dicyclohexylcarbo Diimide, DCI: direct chemical ionization, DCU: dicyclohexylurea, D IEA: diisopropylethylamine, DMAP: 4-dimethylaminopi Lysine, DME: 1,2-dimethoxyethane, DOX: doxorubicin, DTT : Dithiothreitol, EEDQ: N-ethoxycarbonyl-2-ethoxy-1 , 2-Dihydroquinoline, EtOAc: ethyl acetate, FAB: fast atom bombardment, Fmoc: full Oleynylmethoxycarbonyl, GABA: γ-aminobutyric acid, HOBt: N-hydrido Roxybenzotriazole, HRMS: High resolution mass spectroscopy, LD L: low density lipoprotein, MC: 6-maleimidocaproyl, MP: 3-maleimide Propionyl, MPr-BHP: maleimidopropyl-bis-hydroxypropyl , MPr-Mal: maleimidopropyl-malonyl, MEt-IBHE: maleimidoethyl Ru-imino-bis-hydroxyethyl, MMA: mitomycin A, MMC: Itomycin C, Mtr: 4-methoxytrityl, NHS: N-hydroxysuccine Imido, NMP: N-methylpyrrolidinone, PABC: p-aminobenzylca Rubamoyl, PAB-OH: p-aminobenzyl alcohol, PNP: p-nit Rophenol, TFA: trifluoroacetic acid, THF: tetrahydrofuran   Peptide residue(-Y-Zm-)   The peptide linkers of the present invention have 2, 3 or 4 amino acids per branch Self-immolative spacer that provides one or more enzymatic cleavage sites, if present, for acid residues -Included with The amino acid components assemble to form a peptide sequence.   The amino acid residues constituting the peptide residues are each independently an amino acid, Or from the group of naturally occurring amino acids. Naturally occurring amino acids are alanine (Al a), arginine (Arg), asparagine (Asn), aspartic acid (Asp), cis Tein (Cys), glutamic acid (Glu), glutamine (Gln), glycine (Gly), Histidine (His), isoleucine (Ile), leucine (Leu), lysine (Lys), Methionine (Met), ornithine (Orn), phenylalanine (Phe), proline (Pro), Serine (Ser), Threonine (Thr), Tryptophan (Trp), Tyrosine (Tyr) and valine (Val). Preferred naturally occurring amino acids are Ala, V al, Leu, Lys, Ile, Met, Phe, Trp and Pro. Also, certain non-naturally occurring Mino acids can also be part of the peptide residues. Such non-naturally occurring amino acids include , Citrulline (Cit), and protected Amino acids such as acetyl, formyl, tosyl, nitro, etc. Naturally occurring amino acids are mentioned. Specific amino acids are used herein as part of the peptide sequence. When the acids are indicated, they are in the L-form unless otherwise specified. “ The amino acid residues that make up the “Y” component must be L-type. The amino acid residue to be formed may be either L-type or D-type. More preferred Amino acids include Lys, acetyl or formyl protected Lys, Arg, Arg, His, Orn, acetyl or formyl protected with a sil or nitro group Orn, Phe, Val, Ala and Cit protected by Most preferred is Lys And Cit.   The amino acid residue sequence may be a peptidyl derivative drug-conjugate to be formed. Adapted to be selectively enzymatically cleaved by one or more tumor-associated proteases Have been. The amino acid residue chain length of each branch of the peptide linker is preferably It varies from peptide to tetrapeptide chain length.   The first amino acid residue (ie, reading from left to right, the first Is a basic amino acid (eg, Lys or Arg); or Preferably, it has a strong hydrogen bonding ability (eg, Cit). Second amino acid residue (Ie, the second amino acid that, when read from left to right, constitutes "Y") Preferably having a hydrophobic side chain (eg Phe, Val, Ala, Leu or Ile) .   To further illustrate the conjugates of the present invention, specific peptides The groups of linker groups are exemplified below.   Phe-Lys, Val-Lys, Phe-Phe-Lys, Lys-Phe-Lys, Gly-Phe-Lys, Ala- Lys, Val-Cit, Phe-Cit, Leu-Cit, Ile-Cit, Trp-Cit, Phe-Ala, Gly-Ph e-Leu-Gly, Ala-Leu-Ala-Leu, Phe-Ng-tosyl-Arg, Phe-Ng-nitro- Arg, Lys-Lys, Lys-Cit, and Cit-Cit.   Specific preferred examples of peptide sequences include Phe-Lys, Val-Lys, Val-C it and D-Phe-Phe-Lys.   Many of the specific peptide linker molecules suitable for use in the present invention are Design and maximize the selectivity of enzyme cleavage by tumor-associated proteases Can be used (optimized). Preferred peptide linkers used in the present invention Is optimized for proteases, cathepsins B, C, D and L You.   spacer("G")   In the molecule according to the present invention, the drug component and the protein peptide component are spaced apart, and An intermediate, self-immolative spacer component covalently bonded with these may be used. Self Self-immolative spacers can be defined as bifunctional chemical components, which are bifunctional chemical components. Covalently bound with two spaced chemical components to form a generally stable tripartate ( tripartate) molecule: by enzymatic cleavage from the tripartate molecule. To release one of the spaced chemical components; then, following enzymatic cleavage, Dynamically cleaves from the rest of the molecule, releasing the other of the spaced chemical components . According to the present invention, the self-immolative spacer is shared at one end with the protein peptide component. Binds to the chemical reaction site where the pharmacological activity is suppressed by derivatization of the drug component at the other end Because of the covalent bond, the protein peptide component and the drug component Is covalently bound with and is stable and pharmacologically inactive in the absence of the target enzyme, The above-described target enzyme in a covalent bond linking a spacer component and a protein peptide component A tripartate molecule capable of enzymatic cleavage by The release of the protein peptide component from the tate molecule is effected. Take Enzymatic cleavage in turn activates the self-immolative properties of the spacer component and Initiates a spontaneous cleavage of the covalent bond linking the moiety to the drug component, This results in the release of the drug in a physiologically active form.   In the molecules of formulas I, II and III above,   G is the self-spaced and covalently linked drug component and amino acid A sacrificial spacer component, wherein the spacer is a T component (used in the formula shown below) "T" represents a nucleophilic atom already contained in the drug) And a structure of the following formula (IV), (V), (VI), (VII) or (VIII) Can be represented by  (Where T is O, N or S)   Where T is O, N or S, and R¹Is C₁-C_FiveAlkyl)   (J. Med. Chem., 27: 1447, 1984) (where T is O, N or S and R^TwoIs H or C₁-C_FiveAlkyl)   (Where T is O, N or S) Or   (Where T is O, S or N)   As used herein, "C₁-C_Five“Alkyl” means 1 unless stated otherwise. Meant to include branched or unbranched hydrocarbon chains having up to 5 carbon atoms. For example, but not limited to, methyl, ethyl, isopropyl , N-propyl, sec-butyl, isobutyl, n-butyl and the like.   Preferred self-immolative spacer components G suitable for use in the present invention are of the formula (IVa) : It is a PABC shown by.   Other preferred self-immolative spacer components G suitable for use in the present invention are of the formula (V a): Is a GABA represented by.   Another preferred self-immolative spacer component G suitable for use in the present invention is of the formula (V b): Is α, α-dimethyl GABA.   Yet another preferred self-immolative spacer component G suitable for use in the present invention is: Formula (Vc): Is β, β-dimethyl GABA.Thiol acceptor   In the molecules of formulas I, II and III, the thiol acceptor "A" is Binds to the ligand via a sulfur atom derived from the ligand. Thiol acceptors , After binding to a ligand via a thiol group, Rule adduct. Thiol acceptors are, for example, α-substituted acetyl groups. May be. Such a group has the formula:   (Wherein Y is a removable group) Indicated by Specific examples of the leaving group include Cl, Br, I, mesylate, and tosylate. And the like. When the thiol acceptor is an α-substituted acetyl group, After binding to the thiol adduct, -S-CH_TwoForming a bond;   Preferably, the thiol acceptor is a Michael Addition acceptor It is.   A representative Michael Addition acceptor of the present invention has the formula: Indicated by   After binding to the thiol group of the ligand, the Michael Addition Acceptor For example, formula A:   Where L is a ligand Michael Addition Adduct.Bridge(“W”)   The bridge is a bifunctional chemical component that is covalently bonded with two spaced chemical components Thus, a stable tripartate molecule can be formed. A specific example of the bridge is SS Wong's “Chemistry of Protein Conjugation and Crosslinking” Conjugation and Crosslinking Chemistry) "(CRC Press, Florida, 1991); and GE Means and RE Finy's "Bioconjugate Chemistry" (vol. 1, pages 2-12, 1990). The bridge “W” is clearly And covalently binds to the keto component. One example of a bridge is the formula:       − (CH_Two) f- (Z) g- (CH_Two) h- Where:   f is an integer of 0 to 10,   h is an integer of 0 to 10,   g is 0 or 1, provided that when g is 0, f + h is 1 to 10, and   Z is S, O, NH, SO_Two, Phenyl, naphthyl, polyethylene glycol, An alicyclic hydrocarbon ring having 3 to 10 carbon atoms, or 3 to 6 carbon atoms and O, N or Or a heteroaromatic hydrocarbon containing one or two heteroatoms selected from S It is a ring.   Preferred alicyclic components include cyclopropyl, cyclobutyl, cyclopentene And cyclohexyl. Preferred heteroaromatic components include Jill, polyethylene glycol (repeating unit 1 to 20), furanyl, pyranyl, Pyrimidinyl, pyrazinyl, pyridazinyl, oxazinyl, pyrrolyl, thiazolyl And morpholinyl.   In the bridge, when g is 0, f + h is 2 to 6, preferably 2 to 4, and more preferably. More preferably, it is 2. When g is 1, f is 0, 1 or 2 and h Is preferably 0, 1 or 2.   The preferred bridge to couple to thiol acceptors is the Pierce Catalog (Pierce Catalog) E-12, E-13, E-14, E-15, E-16 and And E-17 (1992).Drug   The drug conjugate of the present invention is suitable for ordinary uses where the corresponding drug is effective. Ligands that deliver drugs to certain cells that are effective and particularly beneficial It has excellent medicinal properties due to its inherent ability. Further, the conjugate of the present invention Because gates can be used to modify certain biological responses, Should not be construed as limited to For example, a drug component may have a desired biological activity. It may be a protein or polypeptide having the property. Such proteins include For example, proteins such as tumor necrosis factor are included.   Preferred drugs for use in the present invention are cytotoxic drugs, especially those used in cancer therapy It is. Such drugs generally include DNA toxicants, antimetabolites, natural products and And their analogs. Preferred types of cytotoxic drugs include, for example, Dihydrofolate reductase inhibitor and thymidylate synthase inhibitor Enzyme inhibitors such as DNA intercalators, DNA Cleaver, topical isomerase inhibitor, anthracycline drug , Vinca drugs, mitomycin, bleomycin, cytotoxic nucleoti , Pteridine family of drugs, diynenes, podophyllotoxin, Causative factors, and taxanes. Especially useful among these types Examples of useful substances include methotrexate, metopterin, and dichloromethotate. Lexate, 5-fluorouracil, 6-mercaptopurine, cytosine arabi Noside (arabinosylcytosine), melphalan, leurosine, Leurosideine, actinomycin, daunorubicin, doxo Rubicin, mitomycin C, mitomycin A, carminomycin, aminop Terin, tallysomycin, podophyllotoxin and podophyll Rotoxin derivatives (eg etoposide or etoposide phosphate), bottles Blastin, vincristine, vindesine, taxol, taxo Tele (taxotere), retinoic acid, butyric acid, N⁸-Acetyl spermidine, camptothe Syn and their analogs.   As mentioned above, those skilled in the art will appreciate the To carry out the reaction of a good compound, a given compound can be chemically modified.   In the conjugate of formula I,   D is a drug component having a chemically reactive functional group hanging from its main chain, The functional group links the drug backbone to the protein peptide linker, and the functional group Is a primary or secondary amino, hydroxyl, sulfhydryl, carboxyl, It is selected from the group of aldehyde or ketone. A typical example of the amino-containing drug is my Tomycin C, Mitomycin A, Daunorubicin, Doxorubicin, Aminop Terin, actinomycin, bleomycin, 9-aminocamptothecin, N⁸ -Acetyl spermidine, 1- (2-chloroethyl) -1,2-dimethanesulfo Nylhydrazide, talisomycin, cytarabine and derivatives thereof. Up Representative examples of the alcohol-containing drug include etoposide, camptotensin, and taxo. Esperamicin, 1,8-dihydroxy-bicyclo [7.3.1] trideca- 4,9-diene-2,6-diyn-13-one (U.S. Patent No. 5198560) , Dofilotoxin, angudin, vincristine, vinblastine, morpholine -Doxorubicin, n- (5,5-diacetoxy-pentyl) doxorubicin, And derivatives thereof.   Representative examples of the sulfhydryl-containing drug include esperamicin, 6-mercaptob Phosphorus and its derivatives.   Representative examples of the carboxyl-containing drug include methotrexate, camptothecin ( Lactones), butyric acid, retinoic acid, and derivatives thereof.   Representative examples of the above aldehyde- and ketone-containing drugs are angidin, anthracic Phosphorus (eg, doxorubicin), and derivatives thereof.   A very preferred group of cytotoxic drugs for use as the drug of the present invention include: Embedded image   Mitomycin group of formula (1):  (Where R¹Is hydrogen or methyl;   Is)   Bleomycin group of formula (2):   (Where R¹Is hydroxy, amino, C₁-C_ThreeAlkylamino, di (C₁-C_Three Alkyl) amino, C_Four-C₆Polymethyleneamino,Is)   Methotrexate group of formula (3):   (Where R¹Is amino or hydroxy;   R^TwoIs hydrogen or methyl;   R^ThreeIs hydrogen, fluoro, chloro, bromo or iodo;   R^FourIs a component forming a hydroxy or carboxylic acid salt Is)   Melphalan of formula (4):   6-mercaptopurine of formula (5):  Cytosine arabinoside of formula (6):   Podophyllotoxins of formula (7):   (Where R^TwoIs hydrogen;   R¹Is hydrogen or  R^ThreeIs NH_Two, OH, OCH_Three, NH (C₁-C_ThreeAlkyl) or N (C₁-C_ThreeA Lequil)_Two;   R^FourIs OH or NH_Two;   R^FiveIs methyl or thienyl;   R⁶Is hydrogen or methyl, or a phosphate salt thereof, and is used herein. Do “(C₁-C_ThreeAlkyl) "is a straight or branched chain having 1 to 3 carbon atoms. A branched carbon chain means, for example, methyl, ethyl, n-propyl and isopropyl. Pill)   Drugs of the Vinca alkaloid group of formula (8):   (Where R¹Is H, CH_ThreeOr CHO;   R^TwoAnd R^ThreeAre independent of each other, R^ThreeIs H and R^FourAnd R^TwoOne of them is ethyl The other is H or OH;   R^TwoAnd R^ThreeTogether with the carbon to which they are attached, R^TwoAnd R^ThreeIs R^FourBut d Forms an oxirane ring in the case of tyl;   R^FiveIs hydrogen, (C₁-C_ThreeAlkyl) -CO or chloro-substituted (C₁-C_TwoAl Kill) -CO, which is used herein as "C₁-C_Three“Alkyl” means 1 to 3 Means a straight or branched carbon chain having carbon atoms, for example methyl, ethyl , N-propyl and isopropyl)   Difluoronucleosides of the formula (9);   (Where R¹Is the formula: One base of:   R^TwoIs hydrogen, methyl, bromo, fluoro, chloro or iodo;   R^ThreeIs OH or NH_Two;   R^FourIs hydrogen, bromo, chloro or iodo Is)   Taxols of formula (10):  (Where R¹Is hydroxy;   R^TwoIs hydrogen or hydroxy;   R^Two'Is hydrogen, hydroxy or acetoxy;   R⁷Is hydrogen or hydroxy;   R^ThreeIs hydrogen, hydroxy or acetoxy;   R^FourIs aryl, substituted aryl, C_1-6Alkyl, C_2-6Alkenyl, C_2-6Al Quinyl or t-butoxy;   R^FiveIs C_1-6Alkyl, C_2-6Alkenyl, C_2-6Alkynyl, or -ZR⁶ :   Z is a single bond, C_1-6Alkyl or C_2-6Alkenyl;   R⁶Is aryl, substituted aryl, C_3-6Cycloalkyl, thienyl or furyl Wherein "alkyl" as used herein refers to a straight chain having from 1 to 6 carbon atoms Or a branched carbon chain such as methyl, ethyl, n-propyl, iso- Propyl, n-butyl, sec-butyl, isobutyl, t-butyl, n-pliers Alkenyl, sec-butyl, isopentyl and n-hexyl; "" Has at least one carbon-carbon double bond and 2 to 6 carbon atoms. A straight or branched carbon chain, such as ethenyl, propenyl, And propenyl, butenyl, isobutenyl, pentenyl, and hexenyl, "Alkynyl" means at least one carbon-carbon triple bond and 2-6 Means a straight or branched carbon chain having carbon atoms of, for example, ethynyl, “Aryl” includes 6-10, lopinyl, butynyl and hexynyl. Means an aromatic hydrocarbon having two carbon atoms, such as phenyl and naph "Substituted aryl" refers to C_1-6Alkanoyloxy, hydroxy Si, halogen, C_1-6Alkyl, trifluoromethyl, C_1-6Alkoxy, ally Le, C_2-6Alkenyl, C_1-6Choose from alkanoyl, nitro, amino and amide Means aryl substituted with at least one of the following groups:   Argidines of formula (11):   (Where R¹Is OH or O;   R^TwoIs H or O)   Argidine can be used as an ester or hydrazone as C-3, C-4, C-4 The -8 or C-15 position can be targeted.   Phenylenediamine mustard (12):     H_TwoN-C₆H_Four-N (CH_TwoCH_TwoCl)_Two   Anthracycline antibiotics of formula (13):   (Where R¹Is -CH_Three, -CH_TwoOH, -CH_TwoOCO (CH_Two)_ThreeCH_ThreeOr -CH_TwoOCOCH (OC_TwoH_Five)_Two;   R^TwoIs -OCH_Three-, -OH or -H;   R^ThreeIs -NH_Two, -NHCOCF_Three, 4-morpholinyl, 3-cyano-4-mol Folinyl, 1-piperidinyl, 4-methoxy-1-piperidinyl, benzylamido , Dibenzylamine, cyanomethylamine, 1-cyano-2-methoxyethyl Amine, or NH- (CH_Two)_Four-CH (OAc)_Two;   R^FourIs -OH, -OTHP, or -H; and   R^FiveIs -OH or -H, provided that R^FourIs -OH or -OTHP, R^FiveIs Not -OH)   Those skilled in the art will recognize that structural formula (13) may include a drug or various common names in the art. Understand that a compound that is a derivative of a drug with a common name is included. You. Table I below lists some anthracyclines that are particularly preferred for use in the present invention. Indicates the drug and its common or common name.   Among the compounds shown in Table I, the most preferred drug is doxorubicin. Doxo Rubicin (also referred to herein as "DOX") has the formula¹Is -C H_TwoOH, R^TwoIs -OCH_Three, R^ThreeIs -NH_Two, R^FourIs -OH and R^FiveIs -H Anthracycline.  The most preferred drugs are taxol, mitomycin C, and formula (13) as described above. A) anthracycline antibiotic.   Ligand   "Ligand" means within its scope a receptor associated with a given target cell population. Specially binds or reacts or associates with other or other acceptable components Includes any molecule. This cell-reactive molecule (to which a drug reagent Attached via a linker on the plate) requires therapeutic or other biological modification Can be any molecule that binds, complexes, or reacts with the cell population; Having a free reactive sulfhydryl (-SH) group, or It can be modified to contain a drill group. Cell-reactive molecules are ligands Plays a role in delivering therapeutically active drug components to individual target cell populations that respond You. Such molecules include, but are not limited to, for example, antibodies and the like. High molecular weight proteins, small molecular weight proteins, polypeptides or peptide ligands , And non-peptidyl ligands.   Non-immunoreactive proteins and polypeptides that can be used to form the conjugates of the present invention Alternatively, peptide ligands include, but are not limited to, Spherin, epidermal growth factor ("EGF"), bombesin, gastrin, gastrin Release peptide, platelet-derived growth factor, 1L-2, 1L-6, tumor growth factor (" TGF ") (eg, TGF-α and TGF-β), vaccinia growth factor (" VGF "), insulin and insulin-like growth factors I and II. Non-peptidyl ligands include, for example, carbohydrates, lectins, and low-density Apoproteins from lipoproteins.   Immunoreactive ligands include antigen-recognizing immunoglobulins (also referred to as "antibodies"), Or an antigen-recognition fragment thereof. Particularly preferred immunoglobulins are It is an immunoglobulin that can recognize tumor-associated antigens. "Immune group used "Robulin" is an approved reticulum or subretinal immunoglobulin, such as IgG. , IgA, IgM, IgD or IgE. Preferred immunoglobulins Belongs to the IgG class of immunoglobulins. Immunoglobulin It can also derive from shrimp species. However, immunoglobulins are not human, murine or murine. Ha It is preferably of the heron source. In addition, immunoglobulins are polyclonal Or it may be monoclonal, preferably monoclonal.   It should be noted that those skilled in the art will also appreciate that the invention It will be appreciated that this also includes the use of fragments. Such immunoglobulin fragments For example, Fab ', F (ab')_Two, Fv or Fab fragment Or other antigen-recognizing immunoglobulin fragments. Such exemption Immunoglobulin fragments can be digested with pepsin or papain, Produced by proteolytic enzyme digestion such as it can. Materials and methods for producing such immunoglobulin fragments include [Generally, Parham J. et al. "Immunology" (13 1, 2895, 1983); Ramoi et al., "J. Immunological Methods" (5. 6, 235, 1983); Parham's "id." (53, 133, 198). 2 years); and Matthew et al., "Id." (50, 239, 1982)]. .   An immunoglobulin may be a "chimeric antibody," which term is art-recognized. Have been. Immunoglobulins are also “bifunctional” or “hybrid” antibodies, That is, one antigenic site, for example, one arc with specificity for a tumor-associated antigen The antibody may have an arm. The other arm is another target, For example, haptens or antigens that bind to them-lethal to bearing tumor cells Recognize active agents. Alternatively, bifunctional antibodies are used in which each arm is therapeutically or lively. Specific for another epitope of a tumor-associated antigen of a cell that is physically degenerated There may be. In any case, hybrid antibodies are bispecific and are preferred Or one or more binding sites or target antigens specific for the selected hapten, such as tumors One or more binding sites specific for an antigen associated with a tumor, infected organism or other disease state Have.   Biological bifunctional antibodies are described, for example, in European patent applications referenced by those skilled in the art. No. EPA 0105360. Such hybrid or two As noted, functional antibodies can be used biologically by cell fusion or by chemical Especially by using crosslinking agents or disulfide bridge-forming reagents And may be composed of whole antibodies and / or fragments thereof. Or A method for obtaining such a hybrid antibody is described in, for example, PCT Patent Application Publication No. WO8 3/03679 (published October 27, 1983) and European patent application published No. EPA 0217577 (published April 8, 1987). Special Preferred bifunctional antibodies for are "polydoma" or "quadroma (q uadroma) ”or biologically produced from bis- (maleimi) C) a cross-linking agent such as -methyl ether or other cross-linking agents familiar to those skilled in the art. And synthesized.   In addition, the immunoglobulin may be a single chain antibody ("SCA"). They are , Variable light (“V_L”) And variable heavy ("V_H") Domains are linked by peptide bridges or disulfide bonds Single-chain Fv fragment ("scF_V”). Globulin is a single V with antigen-binding activity_HDomain (dAbs) [G. Winter and C.I. Millstein's "Nature" (3 49, 295, 1991); "Biochemislry" by Glockschwaer et al. ( 29, 1362, 1990); S. Ward et al. “Nature” (34 1, 544, 1989)].   Particularly preferred for use in the present invention are chimeric monoclonal antibodies, preferably tumors. It is a chimeric antibody having specificity for a tumor-associated antigen. As used herein, the phrase "ki" "Mella antibody" refers to a protein derived from a single source, usually produced by recombinant DNA technology. At least the variable portion, i.e., the binding portion and the constant portion derived from another species source. Partial monoclonal antibody is designated. Murine variable and human constant parts Are particularly suitable for certain uses of the invention, preferably for human therapy. However, it is well known that such antibodies are easily produced and that murine alone monoclonal antibodies This is because the immunity is lower than that of Such a murine / human chimeric antibody is a murine Expression immunoglobulin comprising a DNA segment encoding an immunoglobulin constant portion It is the product of the Brin gene. Other forms of chimeric antibodies encompassed by the present invention include: A net or sub-net is denatured or altered from that of the original antibody. Heel Such "chimeric" antibodies are sometimes referred to as "class-switched" antibodies. is there. A method for producing a chimeric antibody is performed by using a conventional recombinant DNA and a gene known in the art. Requires transfection methods [eg, Morrison S. et al. L. "Proc. Na t'l Acad. Sci. "(81, p. 6851, 1984)].   The phrase “chimeric antibody” is used in the concept of “humanized antibody”, ie, a substrate or antibody. Indicates that the complementarity determining portion ("CDR") has a different specificity compared to the parent immunoglobulin Comprising an antibody that has been modified to include a CDR of an immunoglobulin having is there. In a preferred embodiment, the murine CDRs are implanted into the substrate portion of a human antibody. Manufactures “humanized antibodies” [see, eg, L. et al. Leachman's "Nature (332, 323, 1988); S. "Nature" by Nyberger et al. 314, 268, 1985)]. Particularly preferred CDRs are chimeras and This corresponds to a bifunctional antibody showing a sequence that recognizes the antigen. CDR modified antibody For teaching, refer to the teaching of EPA 0239400 (published September 30, 1987). Teru.   One of skill in the art will appreciate that the low immunogenicity of chimeric or human-directed antibodies, as well as Bifunctional-textures of the described bifunctional antibodies which have the advantage of being particularly adaptable to therapeutic treatment It will be appreciated that antibodies can be produced. Such bifunctional-chimeric antibodies are, for example, For example, by chemical synthesis using crosslinkers of the type described above and / or recombinant methods, Can be achieved. In any case, the present invention relates to bifunctional, chimeric, bifunctional-textured La, human-oriented, or antigen-recognition fragments or derivatives thereof. Nevertheless, if the technical scope is limited by the individual production method of the antibody, Should not be understood.   In addition, the present invention contemplates within its technical scope active proteins, such as Neuberger et al. PCT Patent Application Publication No. WO86 / 01533 (released on March 13, 1986) Immunoglobulin (as described above) or immunity fused with an enzyme of the type disclosed in It contains globulin fragments. The disclosure of such products is for reference only. Introduce in the specification.   Note that "bifunctional", "fused", "chimeric" (including human), And "bifunctional-chimeric" (including human) antibody structures include their individual The wording also includes a structure consisting of an antigen recognition fragment. By those skilled in the art As will be appreciated, such fragments are intact bifunctional, textured By conventional enzymatic cleavage of human or bifunctional-chimeric antibodies Could be manufactured. However, the intact antibody is of a structural nature in question. The immunoglobulin fragment if it is not susceptible to the cleavage Can be used as a source to produce the structure of interest; When used, when expressed, in vivo by chemical or biological means. Or combined in vitro to obtain the ultimately desired intact immunoglobulin "flag" To encode the desired “fragment” that can produce In addition, the DNA sequence itself can be adapted. Thus, in this context, the word Use the phrase "fragment".   Furthermore, as described above, the immunoglobulin (antibody) or its flag used in the present invention. The mention may be polyclonal or monoclonal in nature. But Thus, monoclonal antibodies are the preferred immunoglobulins. Such polyclonality Or monoclonal antibodies are now well known to those of skill in the art, and Can produce sufficient useful immunoglobulin that can be used in the present invention. For example, G. Kohler and C.I. Millstein's "Nature" (256, 495, 1975)]. In addition, hybridomas and / or such hybrids Monoclonal antibodies produced by humans and useful in the practice of the present invention are Type Culture Collection ("ATCC"), Maryland 20 852, Rockville, Percrow Drive 12301), or Commercially, for example, Boerlinger-Manniheim Biochemicals (Ind. Ana 46250, Indianapolis, P.O. Box 50816) Are generally available.   Particularly preferred monoclonal antibodies for use in the present invention recognize tumor-associated antigens Things. Such monoclonal antibodies are not limited to these. However, for example, the following are included.   In a most preferred embodiment, the ligand-containing conjugate is a U.S.A. S. Patent Application No. 07/544246 (filed on June 26, 1990) [PCT patent application Publication No. WO91 / 00295 (released January 10, 1991)] From a chimeric antibody BR96 ("Chi BR96"). Chi BR96, Endogenous murine / human chimeric antibodies that should be kept in mind for breast, lung, colon and Fucosylation expressed by human carcinoma cells, such as those derived from ovarian carcinoma Reacts with Lewis Y antigen. Hybridoma expression chimera BR96 (Chi (Same as BR96), on May 23, 1990 under the terms of the Budapest Treaty. , American Type Culture Collection ("ATCC") Deposited at 12301 Percrow Drive, Rockville, 20852, India Was. This hybridoma sample was deposited under accession number ATCC 10460. It is possible. Chi BR96 is obtained, in part, from its parent BR96 source. Yes BR96-expressed BR96 was found in the terms of the Budapest Treaty on February 2, 1989. It is deposited at the ATCC on the 1st and is available under accession number HB10036. Place The desired hybridoma is cultured and produced using standard methods currently known in the art. Antibodies are isolated from cell culture supernatants [Harrell, “Single Clone Hybridization”. Doma Antibodies: Techniques and Applications "(CRC Press, 1982)].   Thus, the term "immunoglobulin" or "antibody" as used herein has its meaning. And all of the immunoglobulin / antibody forms or structures described above.   Synthesis of each compound of the present invention   The linkers, drugs / linkers and conjugates of the present invention are publicly known in the art. It is described and / or described herein by techniques known in the art or as guidance. Alternatively, they can be prepared via routine experimentation using techniques known in the art. Attachment of the drug to the linker causes the nucleophilic atom (O, N or S) of the drug to be self-immolative. This is done by reacting with the carboxy terminus of the spacer or peptide. This reaction is shown as follows.  Here, X = Cl, Br, tosylate, N-hydroxysuccinimide, etc. Leavable group   y = OH, NH_Two, Nucleophilic groups such as SH and NH-lower alkyl   R = residue of linker   The bond to the aldehyde or ketone can be an enol or N-lower alkyl enantiomer. This can be done by having an aldehyde or ketone in the form of an olefin. Play Upon release of the released enamine, it spontaneously adds to the aldehyde or ketone. Expected to hydrolyze.   The reaction formulas shown below are examples of the production method (compound No. is Example N). o. Corresponding to).                                 Reaction formula 1                                Reaction formula 2                          Reaction Scheme 3 (Part I)                         Reaction formula 3 (Part II)                          Scheme 4 (Part I)                         Scheme 4 (Part II)                                Reaction formula 5                                Reaction formula 6                                Reaction formula 7                                Reaction formula 8                          Reaction Scheme 9 (Part I)                         Scheme 9 (Part II)                               Reaction formula 10                               Reaction formula 11                               Reaction formula 12  Next, the present invention will be described specifically with reference to examples, but is not limited to these examples. Should not be interpreted as   Example 1   Fmoc-Lys (Mtr):   Fmoc-Lys hydrochloride (23.78 g) in dry methylene chloride (250 ml) , 56.42 mmol) was stirred at rt (room temperature) under argon at room temperature. Lucylyl chloride (15 ml, 2.1 eq) and DIEA (10.3 ml, 1 . 05 equivalents). The mixture was heated to reflux for 1 h (hour), during which time it was And then cooled to 0 ° C. After adding DIEA (31 ml, 3.1 eq), Add p-anisyldiphenylmethyl chloride (18.29 g, 1.05 eq) You. The reaction is stirred at rt for 14 h. The solvent was evaporated and the residue was taken up in ethyl acetate and pH 5 Partition between buffer (0.05M biphthalate). Add organic phase to pH 5 buffer Wash with water and brine, dry over sodium sulfate and evaporate to give a pale yellow foam (34.71 g, 96%).   HRMS     Calculated value: 641.3015     Obtained: 641.3001   Example 2   Lys (Mtr):   Fmoc-Lys in methylene chloride / acetonitrile (1: 1, 80 ml) Mtr) 1 (5.25 g, 8.19 mmol) at RT with diethylamine (8 0 ml). After 1.5 h, the solvent is evaporated. The residue was acetonitrile at 60 ° C. Flush with tril (50 ml x 2), then triturate with ether (80 ml). To chelate. The solid obtained is filtered, washed with ether and then methylene chloride. / Methanol (1: 1) as much as possible. Filtering off some by-product solids, The filtrate is concentrated under reduced pressure. The light yellow-brown solid obtained is dried under reduced pressure for 4 h (3.2 221 g, 94%).   Example 3   Fmoc-Lys (Mtr) -OSu:   Fmoc-Lys (Mtr) in DME (100 ml)_Two(5.5567 g, 8.672 mmol) and N-hydroxysuccinimide (1.0978 g, 1.1 eq.) At 0 ° C. with 0.5 M DCC / methylene chloride (19. (1 ml, 1.1 eq). The mixture is gradually warmed to rt. 14 hours later The DCU solids are filtered off and the filtrate is evaporated to dryness. Use crude active ester without purification I have.   Example 4   Fmoc-Lys (Mtr) -Lys (Mtr):   Fmoc-Lys (Mtr) -OSu3 (about 8.67) in DMF (70 ml) Stirred solution of Lys (Mtr) 2 (3.6294 g, 1 eq) Is treated with DIEA (4.5 ml, 3 eq) at rt. After 4 h, the mixture is vinegared Dilute with ethyl acid (250 ml). Transfer the solution to pH 4 buffer (0.05M biphthale Washed twice with water and brine, dried over sodium sulfate and evaporated. The residue was flushed with methylene chloride (400 ml) to give a pale yellow foam, which was Use without purification.   Example 5   Fmoc-Lys (Mtr) -Lys (Mtr) -PABOH:   Fmoc-Lys (Mtr) -Lys (Mt) in methylene chloride (100 ml) r) 4 (about 8.672 mmol) and di-t-butyl dicarbonate (2.8 A stirred solution of 390 g (1.5 eq) was stirred at rt with pyridine (0.736 ml, . 05 equivalents). After 20 minutes, p-aminobenzyl alcohol (1.60) 20 g, 1.5 equivalents). Stirring is continued for 16 h, then the solvent is evaporated and the residue Is dried under reduced pressure for 2 h. The crude product is used without purification.  Elemental analysis (C₇₄H₇₅N_FiveO₇・ 2H_TwoAs O)   Calculated values: C75.17, H6.73, N5.92   Obtained: C74.89, H6.37, N5.75   Example 6   Lys (Mtr) -Lys (Mtr) -PABOH:   Fmoc-Lys (Mtr) -Lys (M in acetonitrile (100 ml) tr) -PABOH5 (about 8.672 mmol) at RT with diethylamine ( 75 ml). After 2 h, the solvent is rotovap (rotovap) At 40 ° C., and the residue was dried under reduced pressure for 1 h. ml) as much as possible. The solid is filtered off and the filtrate is concentrated under reduced pressure. Residue 1) 2.5%, 2) 3% and 3) 3.5% methanol / methylene chloride The product is obtained as a colorless foam by chromatography eluting with (2.84) 03g, 35% (4 steps)).   Elemental analysis (C₅₉H₆₅N_FiveO_Five・ H_TwoAs O)   Calculated values: C75.21, H7.17, N7.43   Obtained: C75.37, H6.96, N7.24   Example 7a   Fmoc-Phe-OSu:   Fmoc-Phe (5.1033 g, 13.1 g) in methylene chloride (100 ml). 17 mmol) and NHS (1.592 g, 1.05 eq) at 0 ° C. with DC Treat with C (2.854 g, 1.05 eq). Let the ice bath warm to rt and mix. The mixture is stirred for 14 h. DCU is filtered off and the filtrate is evaporated. Colorless glass obtained The crude product is used without purification.   Example 7b   Fmoc-Val-OSu 7b:   This was performed according to the description in Example 7a, using Fmoc-Val (7.02 g, 20.7 g). Mmol).   Example 7c   Fmoc-Ala-OSu:   This was performed according to the description in Example 7a, using Fmoc-Ala (5.0414 g, 15 31 mmol).   Example 8a   Fmoc-Phe-Lys (Mtr):   Lys (Mtr) 2 (4.6 in water (100 ml) and DME (50 ml) 86 g, 11.20 mmol) and NaHCO_Three(941.0 mg, 1 equivalent) Of Fmoc-Phe-OSu 7a in DME (50 ml) (11. (20 mmol). Then, THF (25 ml) was added to dissolve. help. The mixture is stirred at rt for 2 days, then as much DME as possible (Bath temperature 30 ° C). The resulting rubber suspension is diluted with ethyl acetate to pH 5 Partition between the powders. Wash the organic phase with water and brine, dry and evaporate to a pale yellow foam Get things. This is flushed with methylene chloride (100 ml). By TLC, The product was found to be sufficiently pure and was used without purification (8.5 59 g, 97%).   Elemental analysis (C₅₀H₄₉N_ThreeO₆・ H_TwoAs O)   Calculated values: C74.51, H6.38, N5.21   Obtained: C74.17, H6.57, N5.41   Example 8b   Fmoc-Val-Lys (Mtr):   This is based on Fmoc-Val-OSu 7b (20. Prepared from 7 mmol) and Lys (Mtr) 2 (9.09 g, 1.05 eq) (15.28 g, 100%).   HRMS     Calculated value: 740.3700     Obtained: 740.3712   Example 8c   Fmoc-Ala-Lys (Mtr):   Fmoc-Ala-OSu 7c (15.31 mm) in DME (100 ml) Mol) solution in water / DME (2: 1, 150 ml) with Lys (Mtr) 2 ( 6.4080 g, 1 eq) and potassium bicarbonate (1.5331 mg, 1 eq) To the stirred solution. After 16 h, the DME was removed under reduced pressure and the resulting suspension was quenched. Treat with acid (3.22 g, 1.1 eq) / water (25 ml). The mixture is treated with ethyl acetate Extract with Wash the organic phase with water (2 times) and brine, dry over sodium sulfate Concentrate in vacuo to give a yellow foam which is used without purification.   Example 9a   Fmoc-Phe-Lys (Mtr) -PAB-OH:   Fmoc-Phe-Lys (Mtr) 8a (7 in methine chloride (100 ml) . 728 g, 9.808 mmol) and p-aminobenzyl alcohol (1. A stirred solution of 450 g, 1.2 eq) was stirred at rt with EEDQ (3.640 g, 1. 5 equivalents). After 20 h, the solvent is evaporated (water bath 30 ° C.). Remove solid residue Triturate with water (200 ml) and sonicate the resulting suspension for 15 minutes Wave treatment and leave at rt for 2 h. The solid obtained is filtered and washed thoroughly with ether. And dried under reduced pressure (7.6140 g, 87%).   Elemental analysis (C₅₇H₅₆N_FourO₆・ H_TwoAs O)   Calculated values: C75.14, H6.42, N6.15   Obtained: C75.25, H6.02, N6.49   Example 9b   Fmoc-Val-Lys (Mtr) -PABOH: This is based on Fmoc-Val-Lys (Mtr) 8b ( 15.28 g, 20.65 mmol) (14.24 g, 82%).   Elemental analysis (C₅₃H₅₆N_FourO₆・ 0.5H_TwoAs O)   Calculated values: C73.76, H6.77, N6.49   Obtained: C74.01, H6.68, N6.63   Example 9c   Fmoc-Ala-Lys (Mtr) -PABOH:   This is based on the description in Example 9a, Fmoc-Ala-Lys (Mtr) 8c (1.0885 g, 15.31 mmol) (11.0073 g, 88%).   Elemental analysis (C₅₁H₅₂N_FourO₆・ H_TwoAs O)   Calculated values: C73.36, H6.52, N6.71   Obtained: C73.02, H6.72, N6.54   Example 10a   Phe-Lys (Mtr) -PAB-OH:   Fmoc-Phe-Lys (Mtr) -PAB in methylene chloride (35 ml) -OH9a (4.2857 g, 4.80 mmol) was added at RT with diethylamine (50 ml). Sonicate the mixture briefly and stir at rt for 4 h . After that no starting material was seen by TLC. Evaporate the solvent and salt the residue Flash with methylene chloride and on silica 1) 2%, 2) 3% and 3) 4% meta Chromatography eluting with toluene / methylene chloride gave the product as a colorless foam. (2.230 g, 69%).   Elemental analysis (C₄₂H₄₆N_FourO_Four・ 1 / 2H_TwoAs O)   Calculated values: C74.20, H6.97, N8.24   Found: C 74.28, H 7.00, N 8.34   Example 10b   Val-Lys (Mtr) -PABOH:   Fmoc-Val-Ly in methylene chloride / methanol (5: 1, 75 ml) Solution of a (Mtr) -PABOH 9b (13.94 g, 16.50 mmol) Is treated with diethylamine (150 ml). Sonicate the reaction for 30 minutes And then let stand at rt for 3 h. Evaporate the solvent and flush the residue with methylene chloride You. The remaining material was converted on silica to 1) 2%, 2) 3%, 3) 3.5% and 4) 4 The product was chromatographed eluting with Obtained as a colorless foam (6.2510 g, 61%).   HRMS (C₃₈H₄₇N_FourO_FourAs)     Calculated value: 623.3598     Obtained value: 623.3606   Elemental analysis (C₃₈H₄₆N_FourO_Four・ H_TwoAs O)   Calculated values: C71.22, H7.55, N8.74   Found: C 71.41, H 7.51, N 8.66.   Example 10c   Ala-Lys (Mtr) -PABOH:   Fmoc-Ala-Lys (Mtr) -PABOH9 in DMF (50 ml) c (11.0073 g, 13.47 mmol) at RT with diethylamido. (25 ml). After 2.5 h, the mixture was concentrated under high vacuum and the residue was Flash with methylene chloride (100 ml x 2) and then with toluene (150 ml) . The remaining substance was purified on silica using methylene chloride / (ethyl acetate / methanol = 5: 1). ) = 1) 4: 1, 2) 1: 1, 3) 1: 1.6 and 4) 1: 3 The product is obtained as a pale yellow foam by chromatography (5.7817 g). , 72%).   Example 11   N, N-bis-carbobenzyloxyethylenediamine:   Ethylenediamine (9.4 ml, 1 M NaOH (310 ml, 1 equivalent) 0.5 eq.) At 0 ° C. in a strongly stirred solution of benzyl chloroformate (40 ml, (280 mmol) over 45 minutes. A dark white precipitate forms and the mixture Is stirred for 4 h after the dropwise addition. The solid product obtained is filtered off, washed with water and then with hexane. Air dry overnight (46.17 g, 100%).   Example 12   N-carbobenzyloxyethylenediamine hydrochloride:   N, N-bis-carbobenzyloxyethylenedia in glacial acetic acid (100 ml) Min 11 (23.91 g, 72.8 mmol) was added to 12M HCl (12.1 m 1, 2 equivalents). The stirred mixture was heated at reflux for 1 h, then at rt overnight Let stand still. A small amount of solid was filtered off, the filtrate was diluted with ether (700 ml) and rt And let stand for 2h. The white solid product obtained is filtered off, washed repeatedly with ether and reduced. Dry overnight in a pressure desiccator (9.2440 g, 55%).   Example 13   N-carbovenyloxy-N ', N'-bis- (t-butoxycarbonyl Chill) ethylenediamine:   N-carbobenzylo in methanol / methylene chloride (3: 1, 100 ml) Stirring of xyethylenediamine hydrochloride 12 (5.009 g, 21.68 mmol) Stir the stirred solution at rt with t-phthyl acrylate (64 ml, 20 eq.) Treat with ethylamine (3.3 ml, 1.1 eq). Two days later, remove the solvent Remove with a pump. The residue was dried under reduced pressure for 30 minutes and then 30% ethyl acetate / ether And 50% saturated NaHCO_ThreeDistribute between. Wash the organic phase with water and brine, add sodium sulfate Dry over thorium and evaporate. The residue is purified on silica with 20% ethyl acetate / hex Chromatography eluting the product with a thick colorless oil (9.3801 g, 96%).   Elemental analysis (C_{twenty four}H₃₈N_TwoO₆・ 0.5H_TwoAs O)   Calculated values: C 62.72, H 8.55, N 6.09   Obtained values: C62.54, H8.27, N5.95   Example 14   N, N-bis- (t-butoxycarbonylethyl) ethylenediamine dihydrochloride salt:   N-carbobenzyloxy-N ', N'-bis-t-butoxypropionyl Tilenediamine 13 (18.3640 g, 40.76 mmol) was filtered through glass. Pass through the Raney Nickel floor in the vessel. The filtrate was degassed with nitrogen and 10% Pd / C ( 1 g) and 12M HCl (6.8 ml, 2 equiv.). Pearl mixture (Parr) Hydrogenate with a shaker at 50 psi for 16 h and degas again with nitrogen You. The catalyst is filtered off on a celite bed. The filtrate was concentrated under reduced pressure, and the residue was treated with methyl chloride. Flash with ren (twice) to obtain an off-white foam (15.8696 g, 100%).  Example 15   N-Maleoyl-N ', N'-bis- (t-butoxycarbonylethyl) ethyl Rangeamine:   N, N-bis-t-butoxypropionyl ether in acetonitrile (30 ml) Stirring of tylenediamine dihydrochloride 14 (5.3363 g, 13.70 mmol) The solution was treated with DIEA (4.77 ml, 2 eq.) And anhydrous Treat with formic acid (1.4111 g, 1.05 eq). Reaction solution slowly to rt Heat. After 16 h, trimethylsilyl chloride (5.2 ml, 3 eq) and Add DIEA (7.2 ml, 3 eq). The mixture is heated at reflux for 4 h. Under cooling The solvent is removed under reduced pressure and the residue is dissolved in ethyl acetate. The solution is saturated NaHCO_Three,water And washed with brine, dried over sodium sulfate and evaporated. Residue on silica The product was chromatographed eluting with hexane / acetic acid (2.5: 1). As a pale yellow oil (2.9986 g, 55%).   Elemental analysis (C₂₀H₃₂N_TwoO₆As)   Calculated values: C60.59, H8.13, N7.07   Obtained values: C60.65, H7.98, N6.88   Example 16   N-Maleoyl-N ', N'-bis- (carboxyethyl) ethylenediamine -P-toluenesulfonic acid:   N-Maleoyl-N ', N'-bis-t-butyl in methylene chloride (100 ml) Toxipropionyl ethylenediamine 15 (3.9934 g, 10.07 mmol G) at rt to give p-toluenesulfonic acid monohydrate (5.75 g, 3 equivalents) To process. Stir the reaction at rt overnight. Evaporate the solvent at rt and remove the rubbery residue Dry under reduced pressure for 3 h. By NMR the signal of the complete loss of t-butyl ester is Admitted. The crude product is used without purification.¹H-NMR (DMSO-d₆) Δ (Containing 3 equivalents of p-toluenesulfonic acid) 2.29 (s, 9H), 2.76 ( m, 4H), 3.39 (m, 6H), 3.81 (brt, 2H), 7.11 (s , 2H), 7.17 (d, 6H), 7.49 (d, 6H), 9.27 (br, 1 H)   Example 17   N-Maleoyl-N ', N'-bis- (succinimidyloxycarbonyl Chill) ethylenediamine:   N-Maleoyl-N ', N'-bis-propyl in acetonitrile (90 ml) Onylethylenediamine / p-toluenesulfonate 16 (approx. Toluene, containing 2 equivalents of p-toluenesulfonic acid), triethylamine (4.4 ml, 3.1 equivalents) and N-hydroxysuccinimide (2.5502 g, 2 . (2 eq.) At 0 ° C. in 0.5 M DCC / methylene chloride (45.3). ml, 2.25 equivalents). After 14 hours, the reaction solution was concentrated under reduced pressure, and the residue was Partition between ethyl and water. The aqueous phase is re-extracted with ethyl acetate. Yu combined The phases are washed with water (twice) and brine, dried over sodium sulfate and evaporated. Remaining The residue was chromatographed on silica eluting with ethyl acetate / methylene chloride (1: 1). Filtration gives the product as a pale yellow foam (1.2043 g, 25%, 2 Tep).   Example 18a   MEt-IDP- (Lys (Mtr) -Lys (Mtr) -PABOH)_Two:   Lys (Mtr) -Lys (Mtr) -PABOH6 in DME (30 ml) (2.0903 g, 2.262 mmol) and N-maleyl-N ', N'- Bis-succinimidyloxypropionylethylenediamine 17 (541.0 (0.5 mg, 0.5 eq) is stirred at rt for 2 days. The reaction solution was concentrated under reduced pressure at 30 ° C. And dissolve the residue in ethyl acetate. Wash the solution with water (twice) and brine and add sulfuric acid Dry over sodium and evaporate to give the product as a colorless glass (2.3623 g, 99%). Example 18b   MEt-IDP- (Phe-Lys (Mtr) -PABOH)_Two:   N-Maleoyl-N ', N'-bis- (carboxye) in DME (50 ml) Tyl) ethylenediamine / p-toluenesulfonic acid 16 (1.0643 g, 1. 696 mmol) at 0 ° C. with triethylamine (0.6 ml, 2 ml). 5 eq), Phe-Lys (Mtr) -PABOH10a (2.2750 g, 2 Eq), NHS (439.0 mg, 2.25 eq) and DCC (methylene chloride). 0.5 M, 8.5 ml, 2.5 eq.). Add the reaction solution slowly to rt Warm up. After 16 h, the DCU by-product is filtered off and the filtrate is concentrated under reduced pressure. A residue Triturate with tel, filter the resulting solid, wash with ether and dry under reduced pressure. Dry (2.0494 g, 76%).   Example 18c   MEt-IDP- (Ala-Lys (Mtr) -PABOH)_Two:   This is N-maleoyl-N ', N'-bis-succinimidyloxypropyl Prepared from onylethylenediamine 17.   HRMS (C₈₄H₉₆N_TenO₁₂As Na)     Calculated value: 1459.7107     Obtained value: 1459.707   Example 19a   MEt-IDP- (Lys (Mtr) -Lys (Mtr) -PABC-PNP )_Two:   MEt-IDP- (Lys (Mtr) -L in dry methylene chloride (60 ml) ys (Mtr) -PABOH)_Two18a (2.3623 g, 1.127 mmol) ) And bis-p-nitrophenylenocarbonate (1.5424 g, 4.5 equivalents) Amount) with freshly activated 4% powdered sieve (8.5 g) and DIEA (0.8 g). 83 ml, 4.5 eq.). The mixture is stirred for 16 h and then filtered. The filtrate was concentrated under reduced pressure to give a yellow solid, which could be made up into ether (200 ml). Dissolve. The suspension is sonicated and stirred at rt overnight. The resulting white solid It is filtered off, washed repeatedly with ether and dried under reduced pressure (2.4084 g, 88%).   Elemental analysis (C₁₄₄H₁₄₈N₁₄O_{twenty two}・ 2H_TwoAs O)   Calculated values: C70.23, H6.22, N7.96   Obtained values: C70.11, H6.22, N7.96   Example 19b   MEt-IDP- (Phe-Lys (Mtr) -PABC-PNP)_Two:   This is based on the description of Example 19a, MEt-IDP- (Phe-Lys (M tr) -PABOH)_TwoMade from 18b (517.8 mg, 0.326 mmol) (509.1 mg, 74%).   Example 19c   MEt-IDP- (Ala-Lys (Mtr) -PABC-PNP)_Two:   This is based on the description of Example 19a, MEt-IDPO (Ala-Lys (M tr) -PABOH)_TwoPrepared from 18c (6.24 g, 4.34 mmol) (6.00 g, 74%).   Example 20a   MEt-IDP- (Lys (Mtr) -Lys (Mtr) -PABC-DOX )_Two:   MEt-IDP- (Lys (Mtr) -Lys (Mt) in DMF (25 ml) r) -PABC-PNP)_Two19a (753.0 mg, 0.3103 mmol) And a stirred solution of DOX hydrochloride (377.9 mg, 2.1 eq.) At rt with D Treat with IEA (0.114 ml, 2.1 eq). After 3 days, the mixture was washed with ethyl acetate. (200 ml), wash the solution with water (4 times) and brine, and add sodium sulfate. Dry on top and evaporate to give an orange glass. This is ether (200m l) with trituration, the solid obtained is filtered off and then chlorided on silica. The crude product was chromatographed eluting with methylene / methanol (16: 1). The product is obtained as an orange solid (803.8 mg, 80%).   Example 20b   MEt-IDP- (Phe-Lys (Mtr) -PABC-DOX)_Two:   This is based on the description of Example 20a, MEt-IDP- (Phe-Lys (M tr) -PABC-PNP)_Two19b (340.8 mg, 0.161 mmol) (411.2 mg, 93%).   Example 20c   MEt-IDP- (Ala-Lys (Mtr) -PABC-DOX)_Two:   This is based on the description of Example 20a, MEt-IDP- (Ala-Lys (M tr) -PABC-PNP)_TwoMade from 19c (6.00 g, 3.39 mmol) (620 mg, 7%).   Example 21a   MEt-IDP- (Lys-Lys-PABC-DOX)_Two・ 5Cl_TwoCHCO_Two H:   MEt-IDP- (Lys (Mtr) -Lys in methylene chloride (21 ml) (Mtr) -PABC-DOX)_Two20a (318.7 mg, 0.0985 mm Mol) at rt with anisole (3.2 ml, 300 eq.) Treat with chloroacetic acid (0.244 ml, 30 eq). After 2.5 h, ethyl acetate (50 ml). The mixture is stored at 4 ° C. for 2 h. The resulting solid is collected by filtration, Wash repeatedly with ethyl acetate and then ether, then air dry (274.5 mg, 99.8%).   Example 21b   MEt-IDP- (Phe-Lys-PABC-DOX)_Two・ 3Cl_TwoCHCO_Two H:   This is based on the description of Example 21a, MEt-IDP- (Phe-Lys (M tr) -PABC-DOX)_Two20b (280.0 mg, 0.103 mmol) (237.1 mg, 90%).   Example 21c   MEt-IDP- (Ala-Lys-PABC-DOX)_Two・ 3Cl_TwoCHCO_Two H:   This is based on the description of Example 21a, and MEt-IDP- (Ala-Lys (M tr) -PABC-DOX)_TwoFrom 20c (569 mg, 0.248 mmol) Manufactured (455 mg, 80%).   Example 22   N-carbobenzyloxy-N ', N'-bis- (t-butoxycarbonyl Chill) ethylenediamine:   N-carbobenzyloxyethylenediamine hydrochloride in DMF (100 ml) 12 (13.95 g, 60.48 mmol) and potassium bicarbonate (24.22 g, 4 equiv.) at 0 ° C. with t-butyl bromoacetate (22 ml). , 2.25 equiv.) Over 10 minutes. Warm the mixture to rt. Stirring was continued for 12 h, then the mixture was 50% saturated with ether / ethyl acetate (3: 1). Partition between sodium bicarbonate. Wash the organic phase with water (3 times) and brine, and add sodium sulfate Dry over lium and evaporate to give a thick oil. Hep it at 60 ° C Flash several times with tan to remove excess t-butyl bromoacetate, then On silica, 1) hexane, 2) 5% ethyl acetate / hexane, and 3) 25% Purify the product by chromatography, eluting with ethyl acetate / hexane. Obtained as a filtered colorless oil (18.53 g, 73%).   Example 23   N, N-bis- (t-butoxycarbonylmethyl) ethylenediamine dihydrochloride salt:   N-carbobenzyloxy-N ', N'-bis- in ethanol (75 ml) (T-Butoxyacetyl) ethylenediamine 22 (15.02 g, 35.54 mi) ) Is filtered over a Raney nickel bed. Acetic acid (6.1 ml, 3 equivalents ) Is added and the mixture is hydrogenated as described in Example 4. Without purification of the crude product use.   Example 24   N-Maleoyl-N ', N'-bis- (t-butoxycarbonylmethyl) ethyl Rangeamine:   CHCl_ThreeN, N-bis- (t-butoxyacetyl) ethyl in (150 ml) Diamine 25 dihydrochloride 23 (about 35.54 mmol) was treated with anhydrous maleic acid at rt. Treat with acid (3.83 g, 1.1 eq). The mixture was stirred for 14 h and then dissolved. Evaporate the medium. The residue is CHCl_Three(200 ml), then flush with argon Dissolve in lower acetonitrile (200 ml). The stirred mixture was cooled to 0 ° C. Methylsilyl chloride (18 ml, 4 equivalents) and triethylamine (20 ml , 4 equivalents). Remove the ice bath and heat the mixture to reflux for 2.5 h. Solvent Decrease Remove the pressure and partition the residue between ether and 30% saturated sodium bicarbonate. Organic phase Is washed with water, brine, dried and evaporated. The residue is treated on silica with hexane / ethyl acetate. The product was waxy by chromatography eluting with Obtain as a solid (8.25 g, 63%, 3 steps).   Example 25   N-Maleoyl-N ', N'-bis- (carboxymethyl) ethylenediamine -P-toluenesulfonic acid:   N-Maleoyl-N ', N'-bis- (t-butyl) in methylene chloride (70 ml). (Toxicarbonylmethyl) ethylenediamine 24 (2.6718 g, 7.25 Of the stirred solution of p-toluenesulfonic acid monohydrate (4.1 (400 g, 3 equivalents). After 30 h, the resulting white solid was filtered and washed with methyl chloride. Wash repeatedly with styrene and ether, then dry under reduced pressure. By NMR, raw 1.4 to 1.5 equivalents of p-toluenesulfonic acid was observed per equivalent of the product (raw (Product: 3.7531 g, 100%).   Elemental analysis (C_TenH₁₃N_TwoO₆・ 1.3C₇H₇O_ThreeS ・ 2H_TwoAs O)   Calculated values: C44.48, H5.10, N5.43   Obtained: C44.51, H4.96, N5.20   Example 26a   MEt-IDA- (Phe-Lys (Mtr) -PABOH)_Two:   Phe-Lys (Mtr) -PABOH10a (2 in DME (150 ml) . 5179 g, 3.753 mmol), N-maleoil-N ', N'-bis- ( Carboxymethyl) ethylenediamine / p-toluenesulfonic acid 25 (804. 0 mg, 0.5 eq) and N-hydroxysuccinimide (475.2 mg, 1 eq.) At 0 ° C. with DIEA (0.33 ml, 0.5 eq.) And 0. Treat with 5M DCC / methylene chloride (9.0 ml, 1.2 eq). Six hours later, The DCU is filtered off and the filtrate is concentrated under reduced pressure. The residue is partitioned between ethyl acetate and water. Yes The organic phase is washed with water (twice) and brine, dried over sodium sulfate and concentrated under reduced pressure . The residue is dissolved as much as possible in methylene chloride (100 ml) and the mixture is then eluted. Dilute with Tell (100 ml). After standing overnight, filter the resulting solid and air dry (2.6295 g, 90%).  Example 26b   MEt-IDA- (Val-Lys (Mtr) -PABOH)_Two:   This was determined according to the description in Example 26a, using N-maleoil-N ', N'-bis- ( Carboxymethyl) ethylenediamine / p-toluenesulfonic acid 25 (500 m g, 1.16 mmol) and Val-Lys (Mtr) -PABOH10b ( 1.44 g, 2 equiv.) (1.68 g, 95%).   Elemental analysis (C₈₆H₁₀₀N_TenO₁₂・ 2H_TwoAs O)   Calculated values: C68.78, H6.98, N9.33   Obtained: C 68.87, H 7.54, N 9.48   Example 27a   MEt-IDA- (Phe-Lys (Mtr) -PABC-PNP)_Two:   MEt-IDA- (Phe-Lys (Mtr) in methylene chloride (25 ml) -PABOH)_Two26a (471.5 mg, 0.319 mmol) and bis- A stirred suspension of p-nitrophenyl carbonate (971.0 mg, 10 equiv.) Treat with DIEA (0.611 ml, 11 eq) at rt under argon. 16 After h, the solvent is removed under reduced pressure and the residue is dried under reduced pressure for 3 h. The residue was treated with methylene chloride (15 ml), to which ether (30 ml) is added under slow stirring. Get Allow the suspension to stand overnight. The solid was collected by filtration and ether / methylene chloride (2: 1). And dried under reduced pressure (411.5 mg, 68%).  Example 27b   MEt-IDA- (Val-Lys (Mtr) -PABC-PNP)_Two:   This is based on the description in Example 27a, MEt-IDA- (Val-Lys (M tr) -PABOH)_TwoPrepared from 26b (300 mg, 0.205 mmol) (347.7 mg, 94%).   Example 28a   Met-IDA- (Phe-Lys (Mtr) -PABC-DOX)_Two:   MEt-IDA- (Phe-Lys (Mtr) -PA in NMP (10 ml) BC-PNP)_Two27a (410.3 mg, 0.217 mmol) and doxo A solution of rubicin hydrochloride (283.0 mg, 2.25 eq) was added to DIEA (0.0 94 ml, 2.5 eq.). After 48 h, the mixture is poured into ethyl acetate. Dissolution Wash the solution with water (3 times) and evaporate under reduced pressure. In each case the product is contained by TLC Some orange solids are formed. This is filtered and then Combine with organic soluble components and then chromatograph. Combine The resulting substance was converted to methylene chloride / (ethyl acetate / methanol = 5: 1) = 1 on silica. ) 6: 4, and 2) chromatography, eluting 1: 1 with the product As an orange solid (351.8 mg, 60%).  Example 28b   MEt-IDA- (Val-Lys (Mtr) -PABC-DOX)_Two:   This is based on the description of Example 28a, MEt-IDA- (Val-Lys (M tr) -PABC-PNP)_Two27b (6.351 g, 3.536 mmol) (2.79 g, 30%).   Example 29a   MEt-IDA- (Phe-Lys-PABC-DOX)_Two・ 2Cl_TwoCHCO_Two H:   MEt-IDA- (Phe-Lys (Mtr)-in methylene chloride (15 ml) PABC-DOX)_Two28a (192.0 mg, 0.071 mmol) with stirring The solution was treated at rt with anisole (1.54 ml, 200 equivalents) and dichloroacetic acid ( 0.117 ml, 20 eq.). One hour later, ethyl acetate (15 ml) was added. I can. The resulting solid is collected by filtration, washed with ethyl acetate and ether, and dried under reduced pressure (181.0 mg, 100%).  Example 29b   MEt-IDA- (Val-Lys-PABC-DOX)_Two・ 2Cl_TwoCHCO_Two H:   This is based on the description in Example 29a, MEt-IDA- (Val-Lys (M tr) -PABC-DOX)_Two28b (232 mg, 0.0891 mmol) (171 mg, 78%).   Example 30   MEt-IDA- (Phe-Lys (Mtr) -PABC-MMC)_Two:   MEt-IDA- (Phe-Lys (Mtr) -PAB in NMP (6 ml) C-PNP)_Two27a (183.8 mg, 0.0971 mmol), mitomai Syn-C (73.1 mg, 2.25 equivalents), N-hydroxybenzotriazole Monohydrate (131.3 mg, 10 eq) and freshly activated 4% powdered seed (0.5 g) in DIEA (0.17 ml, 10 equivalents). After 40 h, the mixture was filtered and the filtrate was ethyl acetate (80 m Dilute in 1). Wash the solution with water (4 times), brine, dry over sodium sulfate, Evaporate. The residue was purified on silica using methylene chloride / (ethyl acetate / methanol = 5: 1) Chromatography eluting with = 2: 1 to give the product as a light purple solid (201.7 mg, 91%).   Example 31   Met-IDA- (Phe-Lys-PABC-MMC)_Two・ 2Cl_TwoCHCO_Two H:   MEt-IDA- (Phe-Lys (Mtr)-in methylene chloride (3 ml) PABC-MMC)_Two30 (134.6 mg, 0.0590 mmol) in solution , Anisole (1.28 ml, 200 equivalents) and 1M chloroacetic acid / methyl chloride (1.18 ml, 20 equivalents). After 3.5 h, ethyl acetate (30 ml ). The resulting purple solid is collected by filtration, washed with ethyl acetate and air-dried (97. 8 mg, 82%). By HPLC, the products are decomposed in solution to one product It seems to be.   Example 32   2'-methoxytrityl-paclitaxel:   Paclitaxel (0.51 g, 0.597 mm) in methylene chloride (14 ml) Mol) and p-methoxytrityl chloride (4.63 g, 25 equivalents) Treat the solution with pyridine (1.23 ml, 25 eq) at rt under nitrogen. at rt After 16 h, the solvent is evaporated and the residue is dissolved in ethyl acetate. Put the solution in cold pH5 buffer (100 ml × 2), wash with water and brine, dry and evaporate. Residue on silica And purified by chromatography eluting with 3% methanol / methylene chloride. The product is obtained as a white solid (482 mg, 72%).   Example 33   MEt-IDA- (Phe-Lys (Mtr) -PABC-7-paclitaxe Le)_Two:   Paclitaxel-2'-Mtr32 (789.3) in methylene chloride (5 ml). mg, 0.701 mmol) in DIEA (0.12 2 ml, 1 equivalent), pyridine (0.057 ml, 1 equivalent) and diphosgene (0 . 043 ml, 0.5 eq.). The mixture was warmed to rt for 1.5 h. Then, this was injected with a syringe into MEt-IDA- (Phe-Lys (Mtr) -PABO). H)_Two26a (547.3 mg, 0.5 eq) / methylene chloride (5 ml) and Add to a stirred suspension of DIEA (0.122 ml, 1 eq) at rt. 16 hours later , The mixture was diluted with ethyl acetate, pH 5 buffer (0.5 M biphthalate), water and And brine, dried over sodium sulfate and concentrated in vacuo. Residue on silica Methylene chloride / (ethyl acetate / methanol = 5: 1) = 1) 5: 1 and 2) Chromatography eluting 3: 1 gives the product as a colorless glass (859.2 mg, 63%). A small amount of monotaxol adduct (172.0 mg, 18%).  Example 34   MEt-IDA- (Phe-Lys-PABC-7-paclitaxel)_Two・ 2 ClCH_TwoCO_TwoH:   MEt-IDA- (Phe-Lys (Mtr)-in methylene chloride (3 ml) PABC-7-paclitaxel)_Two33 (333.0 mg, 0.0861 mmol ) With anisole (1.87 ml, 200 equivalents) and 1 M chloroacetic acid / chloride Treat with methylene (1.72 ml, 20 eq). After 4 h, the mixture was washed with ether ( 30 ml). The resulting suspension is sonicated for a few minutes and then the solid is filtered. Take and wash with ether (256.3 mg, 97%). Product slowly in solution Decomposition is observed.   Example 35   N-carbobenzyloxy-N ', N'-bis- (t-butoxycarbonyl Chill) propylene diamine:   This was performed according to the description in Example 22 using N-carbobenzyloxypropylene diadia. Prepared from min hydrochloride (3.4624 g, 14.15 mmol) (5.301). 7 g, 86%).  Example 36   N, N-bis- (t-butoxycarbonylmethyl) propylenediamine / divinegar acid:   N-carbobenzyloxy-N ', N'-bis- in ethanol (75 ml) (T-butoxycarbonylmethyl) propylenediamine 35 (5.3017 g, 12.144 mmol) of acetic acid (2.14 mmol) via a Raney nickel bed. (3 ml) / ethanol (75 ml). Gas the filtrate with nitrogen Drain and treat with 10% palladium on activated carbon (0.4 g). Pearl dressing the mixture The catalyst is hydrogenated at 50 psi for 16 h and then filtered off through a bed of celite. Filtration The solution is concentrated under reduced pressure, and the residue is flushed with chloroform (150 ml). Crude product Used without purification.   Example 37   N-Maleoyl-N ', N'-bis- (t-butoxycarbonylmethyl) pro Pyrene diamine:   This was performed according to the description in Example 24, using N, N-bis- (t-butoxycarbonyl). Methyl) Propylenediamine. Prepared from diacetic acid 36 (12.14 mmol). . Chromatography of the crude product on silica, eluting with hexane / ethyl acetate (3: 1) Upon chromatography, the product is obtained as a pale yellow oil (2.0653 g, 44%, 3 steps).   Example 38   N-Maleoyl-N ', N'-bis- (carboxymethyl) propylene diamine N-p-toluenesulfonic acid:   N-Maleoyl-N ', N'-bis- (t-butyl) in methylene chloride (25 ml) Toxicarbonylmethyl) propylenediamine 37 (2.06 g, 5.39 mm Mol) is stirred at rt to give p-toluenesulfonic acid monohydrate (3.07 g, 3 equivalents). After 16 h, the solvent is removed under reduced pressure. Residue with ether Triturate four times (each time decant the ether). Obtained The semi-solid material is flushed with chloroform (150 ml × 2). By NMR 1.4 to 1.5 moles of p-toluenesulfonic acid per mole of product (Product: 2.68 g, 97%).   Example 39   MPr-IDA- (Phe-Lys (Mtr) -PABOH)_Two:   This was determined according to the description in Example 26a, using N-maleoil-N ', N'-bis- ( (Carboxymethyl) propylenediamine-p-toluenesulfonic acid 38 (2.6 842 g, 5.25 mmol) and Phe-Lys (Mtr) -PABOH1 Oa (7.0432 g, 2 eq). However, the crude product is silica Methylene chloride / (ethyl acetate / methanol = 5: 1) = 1) 2: 1 and 2) 1 . Chromatography eluting with 5: 1 gives the product as a white solid (4 . 5253 g, 55%).   Example 40   MPr-IDA- (Phe-Lys (Mtr) -PABC-PNP)_Two:   This was performed according to the description in Example 27a, using MPr-IDA- (Phe-Lys (M tr) -PABOH)_TwoPrepared from 39 (1.7793 g, 1.143 mmol) (1.8909 g, 87%).   Example 41   MPr-IDA- (Phe-Lys (Mtr) -PABC-DOX)_Two:   This is based on the description in Example 28a, MPr-IDA- (Phe-Lys (M tr) -PABC-PNP)_Two40 (722.7 mg, 0.379 mmol) Manufactured. The crude product was purified on silica using methylene chloride / methanol = 1) 20: 1. And 2) Chromatography eluting 15: 1 to give the product as an orange Obtained as a colored solid (869.4 mg, 84%).   Example 42   MPr-IDA- (Phe-Lys-PABC-DOX)_Two・ 2Cl_TwoCHCO_Two H:   This is based on the description in Example 29a, MPr-IDA- (Phe-Lys (M tr) -PABC-DOX)_Two41 (714.3 mg, 0.263 mmol) (645.9 mg, 96%).  Example 43   Di-t-butyliminodiacetate:   Glycine t-butyl ester hydrochloride (5.0811) in DMF (40 ml). g, 30.31 mmol) and potassium bicarbonate (6.3730 g, 2.1 equivalents) ) Was stirred at 0 ° C in t-butyl bromoacetate (4.9 ml, 1 equivalent) ). Remove the ice bath and stir the mixture at rt for 14 h. Reduce solvent at 30 ° C Remove the pressure and partition the residue between ethyl acetate and 50% saturated sodium bicarbonate. Organic The phases are washed with water (3 times) and brine, dried over sodium sulfate and concentrated in vacuo. The residue was dissolved in silica with ethyl acetate / hexane = 1) 5% and 2) 25%. Chromatography on separation gives the product as a colorless oil (4.9310). g, 66%).   Example 44   N-Maleoyl-N ', N'-bis- (t-butoxycarbonylmethyl) pro Pionamide:   2-maleimidopropionic acid (1.007 g) in methylene chloride (12 ml) , 5.916 mmol) at rt with oxalyl chloride (1.2 ml, 2 ml). . (1 equivalent) and DMF (1 drop). After 4 h, the solvent is evaporated. The residue Flush with dry methylene chloride (20 ml x 2) and dissolve in methylene chloride (2 ml). Understand. To this was added di-tert-butyliminodiacetate in methylene chloride (6 ml). To 43 (1.4510 g, 1 eq) and DIEA (1.24 ml, 1.2 eq) ) Is added dropwise over 15 minutes. After 14 h, the mixture was diluted with ethyl acetate Wash with 15% citric acid, water and brine, dry the organic phase over sodium sulfate, Concentration under reduced pressure gave a pale yellow glass, which by NMR was used for the next step. Pure enough (2.3448 g, 100%).   Example 45   N-Maleoyl-N ', N'-bis- (carboxymethyl) propionamide :   N-Maleoyl-N ', N'-bis- (t-butyl) in methylene chloride (40 ml) Toxicarbonylmethyl) propionamide 44 (1.9100 g, 4.82 mi) ) Is treated with trifluoroacetic acid (20 ml) at rt. The mixture is sonicated at rt for 20 minutes and then left for 3.5 h. Decompress the reaction solution Concentrate, flush the residue with chloroform (50 ml × 2), then add ether Triturate together. The resulting pale yellow solid is filtered and washed with ether (1. 2273 g, 90%).   HRMS     Calculated value: 285.0723     Obtained value: 285.0712   Example 46   MP-IDA- (Phe-Lys (Mtr) -PABOH)_Two:   This was determined according to the description in Example 26a, using N-maleoil-N ', N'-bis- ( Carboxymethyl) propionamide 45 (142.1 mg, 0.500 mmol ) And Phe-Lys (Mtr) -PABOH10a (671.0 mg) 2 Equivalent). However, the crude product was converted to methylene chloride / (ethyl acetate) using silica. / Methanol = 5: 1) = 1) 2: 1 and 2) Chromatography eluting with 1.5: 1 Upon chromatography, the product is obtained as a white solid (349.7 mg, 44%).   Example 47   MP-IDA- (Phe-Lys (Mtr) -PABC-PNP)_Two:   This is based on the description in Example 27a, MP-IDA- (Phe-Lys (Mt r) -PABOH)_Two46 (225.4 mg, 0.142 mmol) (195.5 mg, 72%).   Example 48   MP-IDA- (Phe-Lys (Mtr) -PABC-DOX)_Two:   This is based on MP-IDA- (Phe-Lys (Mt r) -PABC-PNP)_Two47 (195.0 mg, 0.102 mmol) Manufactured. The crude product was purified on silica with methylene chloride / methanol = 1) 20: 1 and And 2) Chromatography eluting 15: 1 gives the product as an orange Obtained as a solid (117.7 mg, 42%).  Example 49   MP-IDA- (Phe-Lys-PABC-DOX)_Two・ 2Cl_TwoCHCO_Two H:   This is based on the description in Example 29a, MP-IDA- (Phe-Lys (Mt r) -PABC-DOX)_Two48 (91.0 mg, 0.033 mmol) (76.4 mg, 94%).   Example 50   Z-βAla:   Β-alanine (50.10 g, 0.562) in 2M NaOH (281 ml) Mol) at 0 ° C. with benzyl chloroformate (88 ml, 1.1 equivalents). Volume) for 1 h. Stir at 0 ° C. for 1.5 h then at rt for 1.5 h. h Continue. The resulting mixture is extracted with ether (500ml x 4). Aqueous phase Is acidified with 5M HCl (120 ml). The resulting white precipitate is filtered off, Wash and dissolve in methylene chloride. Dry the solution over sodium sulfate and concentrate under reduced pressure To give a white solid (114.95 g, 92%).  Example 51   Z-βAla-OSu:   Z-βAla50 (37.42 g, 0.16 in methylene chloride (700 ml)) 8 mol) and N-hydroxysuccinimide (19.34 g, 1 equivalent) Stir at 0 ° C. and treat with DCC (34.69 g, 1 eq). The reaction solution Heat to t. After 16 h, the DCU was filtered off and the filtrate was concentrated in vacuo to remove a white foam. (53.80 g, 100%).   Example 52   Z-βAla-IDA:   Iminodiacetic acid (16.84 g, 84.32 mmol) and water (240 ml) And a stirred solution of lithium hydroxide monohydrate (10.62 g, 2 equivalents) at 0 ° C And Z-βAla-OSu51 (27.01 g, 0.1 mL) in DME (130 ml). 667 equivalents). After 15 minutes, the ice bath was removed and the reaction solution was left at rt for 16 hours. Stir. The mixture is concentrated on a rotary evaporator to a volume of 200 ml. can get The suspension was extracted with ethyl acetate (250 ml × 2), then the aqueous phase was extracted with 85% phosphoric acid And acidify to pH 1-2. The mixture was treated with 10% isopropanol / ethyl acetate (2 00 ml × 3). Wash the combined organic phases with 2% phosphoric acid and brine Dried over sodium sulfate and evaporated to give a colorless glass which was Flush to give a foam (21.36 g, 75%).  Elemental analysis (C_FifteenH₁₈N_TwoO₇・ H_TwoAs O)   Calculated values: C50.56, H5.66, N7.86   Obtained values: C50.56, H5.45, N8.21   Example 53   Z-βAla-IDA- (OSu)_Two:   This was performed according to the description in Example 51, using Z-βAla-IDA52 (21.36 g). , 63.12 mmol).   Elemental analysis (C_{twenty three}H_{twenty four}N_FourO₁₁・ 0.5H_TwoAs O)   Calculated values: C51.02, H4.65, N10.35   Obtained values: C50.83, H5.13, N10.75   Example 54   Z-βAla-IDA- (βAla-Ot-Bu)_Two:   Z-βAla-IDA- (OSu) in DME (250 ml)_Two53 (about 63 . 12 mmol) and β-alanine t-butyl ester hydrochloride (25.80) g, 2.25 eq) of the stirred suspension at rt with DIEA (24.7 ml, 2.2 5 equivalents). After 12 h the solvent was evaporated and the residue was ethyl acetate (400 ml) And 2% phosphoric acid. Wash the organic phase with water and brine, add sodium sulfate Dry on and evaporate. The residue was purified on silica. 1) Ethyl acetate, ethyl acetate / meta No. 2) 15: 1 and 3) 10: 1. To give the product as a thick colorless oil (26.56 g, 71%).  Elemental analysis (C₂₉H₄₄N_FourO₉・ H_TwoAs O)   Calculated values: C57.04, H7.59, N9.17   Obtained: C57.15, H7.36, N9.46   Example 55   βAla-IDA- (βAla-Ot-Bu)_Two:   Z-βAla-IDA- (Ot-Bu)_Two54 (16.93 g, 28.56 (Mmol) / absolute ethanol (100 ml) by blowing nitrogen for 30 minutes To Carefully add 10% palladium / activated carbon (1 g) and mix the mixture with pearl And hydrogenate at 50 psi for 16 h. The catalyst is then filtered off on a bed of celite, The filtrate is concentrated under reduced pressure. The residue is flushed with methylene chloride to give a colorless foam ( 13.11 g, 100%).   Elemental analysis (C_{twenty one}H₃₈N_FourO₇・ 2.5H_TwoAs O)   Calculated values: C50.09, H8.61, N11.12.   Obtained values: C50.17, H8.61 and N10.51   Example 56   Maleoyl-βAla-IDA- (βAla-Ot-Bu)_Two:   ΒAla-IDA- (Ot-Bu) in chloroform (100 ml)_Two55 (6.20 g, 13.5 mmol) was added to a stirred solution of maleic anhydride (1.46 g). , 1.1 equivalents). After 1.5 h, the mixture is concentrated under reduced pressure. Hex residue Flash and use without purification.  Example 57   MP-IDA- (βAla-Ot-Bu)_Two:   Maleoyl-βAla-IDA- (βAl in acetonitrile (150 ml) a-Ot-Bu)_Two56 (7.50 g, 13.5 mmol) in solution with argon At 0 ° C. below, trimethylsilyl chloride (8.6 ml, 5.02 eq.) Followed by Treat with triethylamine (9.4 ml, 5.02 eq). Heat mixture for 4h Reflux, cool to rt, then store at -20 ° C overnight. Triethyl obtained The amine hydrochloride solid is removed by filtration, and the filtrate is concentrated under reduced pressure. The residue was partitioned between ethyl acetate and water. Distribute. The aqueous phase is further extracted with ethyl acetate. Combine the organic phase with sodium sulfate Dry over thorium and evaporate. Residue on silica 1) 5%, 2) 7% and 3) Chromatography eluting with 10% methanol / methylene chloride The product is obtained as a pale yellow gum (4.83 g, 66%).   Elemental analysis (C_{twenty five}H₃₈N_FourO₇・ 1.5H_TwoAs O)   Calculated values: C53.09, H7.30, N9.91   Found: C 53.13, H 6.98, N 10.05   Example 58   MP-IDA- (βAla)_Two:   MP-IDA- (βAla-Ot-Bu) in methylene chloride (40 ml)_Two 57 (3.50 g, 6.50 mmol) at rt with trifluoroacetic acid ( 3Oml). The mixture is sonicated for 10 minutes and then left for 1 h. The solvent was evaporated on a rotovap and the residue was chloroform (3 times) and ether (4 times) ) To flash. The crude product is used without purification.   Elemental analysis (C₁₇H_{twenty two}N_FourO₉・ 3H_TwoAs O)   Calculated values: C42.50, H5.87, N11.66   Found: C42.44, H5.92, N11.54   Example 59   MP-IDA- (βAla-OSu)_Two:   MP-IDA (βAla) in DMF (2 ml)_Two58 (136.0 mg, 0 . 319 mmol) was stirred at rt for DCC (265.0 mg, 4.01). (Equivalent). The mixture was stirred at rt for 16 h, then without isolation of the product Used in the next step as it is.   Example 60   MP-IDA- (βAla-Phe-Lys (Mtr) -PABOH)_Two:   MP-IDA- (βAla)_TwoCrude reaction mixture containing 58 (about 0.319 mmol) The mixture was diluted with DMF (5 ml) and then Phe-Lys (Mtr) -PABO Treat with H10a (429.1 mg, 2.0 eq). After stirring at rt for 5 h, the solvent Are removed under high vacuum and the residue is triturated with ether. The resulting solid Are filtered off and then on silica 5% methanol / ethyl acetate to remove impurities, And chromatographed eluting with 10% methanol / methylene chloride Elute the product (220.1 mg, 40%).   Example 61   MP-IDA- (βAla-Phe-Lys (Mtr) -PABC-PNP)_Two :   MP-IDA- (βAla-P in DMF / methylene chloride (1: 1, 6 ml) he-Lys (Mtr) -PABOH)_Two60 (95 mg, 0.0548 mmol) The stirred solution of bis-p-nitrophenyl carbonate (100 m g, 6 equiv.) and DIEA (0.057 ml, 6.0 equiv.). 16 After h the solvent is removed under high vacuum and the residue is taken up with methylene chloride / ether (1: 1) Triturate until it is solid. This suspension was stored in the freezer for 1.5 hours. The solid is then filtered off and washed with ether (105 mg, 95%).   Example 62   MP-IDA- (βAla-Phe-Lys (Mtr) -PABC-DOX)_Two :   MP-IDA- (βAla-Phe-Lys (Mtr) -PABC-PNP)_Two 61 (1.445 g, 0.701 mmol) and doxorubicin hydrochloride (1 . 010 g, 2.48 equivalents) / DMF (55 ml) was added to DIEA (0.31 ml , 2.50 equiv.). After 40 h at rt, the solvent was evaporated under high vacuum and the residue With methylene chloride / ether (1: 1). The resulting suspension The liquid is sonicated briefly, then the solid is filtered off and washed with ether. 10 solids Dissolve as much as possible in 100% methanol / chloroform (100 ml). Filter the mixture And the filtrate is concentrated on a rotovap to about 50 ml. Chloroform (50ml) And repeat the operation twice more. The resulting solid is collected by filtration, chloroform and then And wash with ether (1.22 g, 61%).  Example 63   MP-IDA- (βAla-Phe-Lys-PABC-DOX)_Two・ 2Cl_Two CHCO_TwoH:   MP-IDA- (βAla-Phe-Lys (M) in methylene chloride (8 ml) tr) -PABC-DOX)_Two62 (132 mg, 0.0459 mmol) The stirred suspension was mixed with anisole (1 ml, 200 equivalents) and dichloroacetic acid (0.07 6 ml, 20 eq.). The mixture becomes homogeneous immediately. Orange after 5 minutes A color precipitate begins to form. After 2 h, ethyl acetate (25 ml) was added and the suspension was Stir for a minute. The solid was collected by filtration and washed with ethyl acetate and then with ether (89 mg, 80%).   Example 64   M-Et-IDA- (Phe-Lys-PABC-DOX = β-Ala-mT EG)_Two:   MTEG-β-Ala hydrazide (254 mg, 866 μmol) was added to 50 μL Dissolve in 10 ml of methanol with 1 TFA. This solution was added to M-Et-I DA- (Phe-Lys-PABC-DOX)_Two(276 mg, 108 μmol) / Suspended in 40 ml of anhydrous methanol. The reaction was allowed to proceed at room temperature (rt) for 3.5 h. Stir. The reaction mixture is rotary evaporated to the point of precipitation, then 1 ml CH 2_TwoCl_TwoAdd And redissolve. This was added dropwise to 250 ml of ether to precipitate a red solid. You. The solid is filtered off, washed with ether and dried under high vacuum to give M-Et-IDA- ( (Phe-Lys-PABC-DOX = β-Ala-mTEG)_Two(300 mg, 90%).   Mass spectrum: FAB 1354.6 (M + 2H)²⁺   Elemental analysis (C₁₃₂H₁₆₄N₁₈O₄₄・ 4.0H_TwoO as 3.0 TFA)   Calculated values: C53.11, H5.65, N8.08   Obtained values: C52.99, H5.96, N8.64   FTIR: 3412, 2938, 1702, 1681, 1616, 1520, 1412, 832, 696cm^-1   Example 65   M-Et-IDA- (Phe-Lys-PABC-DOX = β-Ala)_Two:   β-Ala hydrazide trifluoroacetate (578 mg, 1.75 mm Is dissolved in 10 ml of methanol with 50 μl of TFA. This solution To M-Et-IDA- (Phe-Lys-PABC-DOX)_Two(111mg , 43.6 μmol) / 15 ml of anhydrous methanol. Reaction solution is rt And stir for 1.5 h. The reaction mixture was rotary evaporated to a volume of 3 ml and then 200 m A red solid precipitates by dropwise addition to 1 liter of acetonitrile. The solid is filtered off and It was washed with nitrile, dried under high vacuum, and treated with M-Et-IDA- (Phe-Lys- PABC-DOX = β-Ala)_Two(117 mg, 99%).   ¹H-NMR (d⁶-DMSO): (selected peak) δ 1.13 (d, 6H), 3 . 95 (s, 6H), 6.96 (s, 2H)   Example 66   Nt-butoxycarbonyl-3-aminopropanol:   3-Aminopropanol (15 ml, 0.20 ml) in methylene chloride (50 ml) Mol) solution at rt in t-butyl pyrocarbonate (42.02 g, 1 equivalent ) / Methylene chloride (25 ml) dropwise over 2 h. After stirring overnight, mix Evaporate the material, flush with heptane (3 times), dry under reduced pressure and slurry the product Obtained as an oil (34.31 g, 100%).   Elemental analysis (C₈H₁₇NO_ThreeAs)   Calculated values: C54.84, H9.78, N7.99   Found: C54.80, H9.82, N7.97   Example 67   Nt-butoxycarbonyl-3-aminopropyl mesylate:   Protected amino alcohol 64 (6.601 g, 37.67 mmol) / salt Methylene chloride (45 ml) was treated with methanesulfonyl chloride (2 . 92 ml, 1.0 equivalent) and triethylamine (5.25 ml, 1.0 equivalent) ) For 30 minutes. The mixture is stirred for 16 h, then the solvent is evaporated You. The residue was partitioned between ether (200ml) and water (250ml) and the organic phase was 10% Wash with citric acid, water and brine, dry over sodium sulfate and evaporate. The residue Chromatography on silica eluting with 2% methanol / methylene chloride You. The product was unstable over time at rt (5.800 g, 61%).   Example 68   Diethyl 2- (Nt-butoxycarbonylaminopropyl) -malonate :   Sodium hydride (60% in mineral oil, 1.84 g, 46 mmol) was added under argon The suspension in THF (20 ml) at 0 ° C. was added to diethyl malonate (7 ml, 1 ml). . (0 eq) and warm the mixture to rt. It became homogeneous When the mesylate 65 (5.84 g, 0.5 equivalent) / THF (15 ml) is once Add to The mixture was heated at reflux overnight, diluted with hexane / ethyl acetate (1: 1). Wash with water, brine, dry over sodium sulfate and evaporate. Residue on silica And chromatographed eluting with 25-35% EtOAc / hexane ( 5.751 g, 79%).   Elemental analysis (C_FifteenH₂₇NO₆As)   Calculated values: C56.77, H8.57, N4.41   Obtained: C56.65, H8.45, N4.42   Example 69   Nt-butoxycarbonyl-5-amino-2-hydroxymethylpentano Le:   Diester 66 (4.957 g, 15.62 mmol) / ether (100 m l) at 0 ° C under argon with lithium borohydride (2M in TMF, 24 ml, 3 ml) Eq.) Followed by methanol (1.9 ml, 3 eq.). Mix 2.5 h. Heat to reflux, then carefully add methanol (25 ml), then cool to rt Instead, add acetic acid (2.7 ml, 3 eq) to quench the reaction. Evaporate the mixture and salt Flush with methylene chloride (twice). Dissolve the residue in methanol (100 ml) The mixture is heated to reflux overnight and then evaporated. The resulting oil is sonicated Dissolve in chloroform (100 ml) as much as possible, then filter off inorganic solids You. The filtrate is evaporated and the residue is eluted on silica with 9% methanol / methylene chloride The product is obtained as a thick oil by chromatography (2.77). 0 g, 76%).   Elemental analysis (C₁₁H_{twenty three}NO_FourAs)   Calculated values: C56.63, H9.94, N6.00   Obtained: C56.16, H9.83, N5.94   Example 70   5-amino-2-hydroxymethylpentanol / CF_ThreeCO_TwoH:   A solution of 5% water in 50% TFA / methylene chloride (4 ml) was added to diol 67 ( 0.145 g, 0.621 mmol) and the mixture is stirred for 1 h. Steam solvent Emitted and flush the residue with methylene chloride (twice) (0.153 g, 100%) .   Example 71   5-maleimido-2-hydroxymethylpentanol:   Aminodiol 68 / dry acetonitrile was treated with anhydrous maleic acid at 0 ° C. under argon. Treat with acid (1 eq) and DIEA (1 eq). Stir the mixture at rt for 4 h I do. The reaction was recooled to 0 ° C. and trimethylsilyl chloride (3 equivalents) and D Treat with IEA (3 equivalents). The mixture was heated at reflux for 4 h, then cooled to rt And then evaporate. The residue is partitioned between ethyl acetate and water. 10% citrate organic phase Wash with acid, water and brine, dry over sodium sulfate and evaporate. Silica residue Chromatography on the gel gives the product.   Example 72   5-maleimido-2-hydroxymethylpentanol bis-chloroforme G:   A solution of diol 69 / dry methylene chloride was mixed with 1M phosgene / toluene (20 equivalents). ) At 0 ° C. After the addition, the mixture was stirred at rt for 16 h. Then, the solvent is removed by a rotary evaporator. The residue is washed with dry methylene chloride. Rush and dry under reduced pressure. The crude bis-chloroformate is used without purification.   Example 73   MPr-BHP- (Phe-Lys (MMT) -PABOH)_Two:   A stirred solution of the crude bis-formate 70 in dry methylene chloride at 0 ° C. Phe-Lys (MMT) -PABOH10a (2 equivalents) in DI and DI A solution of EA (2 eq) is added all at once. The mixture was stirred at rt for 16 h, then Evaporate the medium. The residue is partitioned between ethyl acetate and water. Wash the organic phase with brine and add sulfuric acid Dry over sodium and evaporate. The product is analyzed by column chromatography using silica gel. Purify by chromatography.   Example 74   MPr-BHP- (Phe-Lys (MMT) -PABC-PNP)_Two:   71, bis-p-nitrophenyl carbonate (6 equivalents) in dry methylene chloride ) And the freshly activated 4Å powdered sieve stirring mixture at rt under argon Treat with DIEA (6 equivalents). After stirring was continued for 16 h, the mixture was filtered and filtered. Evaporate the liquid. The residue is dried under reduced pressure for several hours and then dissolved in a minimum amount of methylene chloride. You. To this is added 2 volumes of ether. The solid obtained is filtered off and ether / Wash with methylene chloride (2: 1) and dry under reduced pressure.   Example 75   MPr-BHP- (Phe-Lys (MMT) -PABC-DOX)_Two:   Bis-p-nitrophenyl carbonate 72 and DOX hydrochloride (1.1 equivalents ) / DMF is treated with DIEA (1.1 eq). After stirring for 2 h, mix The mixture is diluted with ethyl acetate. Wash the solution with water (4 times) and brine, add sodium sulfate Dry over um and evaporate. The residue was chromatographed on silica gel, Obtain the product.   Example 76   MPr-BHP- (Phe-Lys-PABC-DOX)_Two・ 2Cl_TwoCHCO_Two H:   A stirred solution of compound 73 / methylene chloride was added to anisole (100 equivalents) followed by Treat with dichloroacetic acid (10 equivalents). After 1.5 h, dilute the mixture with ethyl acetate I do. The resulting suspension was stirred at rt for 1 h, then the orange solid product was filtered off Wash with ethyl acetate and dry under reduced pressure.   Example 77   N-Adpoc-3-hydroxyaminopropane:   Of 3-hydroxyaminopropane and sodium bicarbonate (1 equivalent) in water The stirred solution was stirred at rt to give 1- (1'-adamantyl) -1-methyl-ethoxycarbo. Treat with nil chloride (1 equivalent). After 6 h, the resulting solid product is filtered off and washed with water Wash and lyophilize under reduced pressure. The crude product is used without purification.   Example 78   N-Adpoc-3-methanesulfonyloxyaminopropane:   Methanol sulfonyl chloride was added to a stirred solution of alcohol 75 / methylene chloride at 0 ° C Lido (1.05 eq) is added, followed by triethylamine (1.05 eq). Mixed The mixture is warmed to rt and stirred at rt overnight. Evaporate the solvent and elute the residue with ethyl acetate. And pH5 buffer (biphthalate). Wash the organic phase with water and brine, Dry over sodium sulfate and evaporate to give the product, which is used without purification.   Example 79   t-butyl-N-adpoc-5-amino-2-t-butoxycarbonyl-penta Noate:   A stirred suspension of sodium hydride in dry tetrahydrofuran at 0 ° C. under argon Carefully treat with di-t-butyl malonate (1 equivalent). Rt the mixture Warm up gradually. When the mixture is homogeneous, recool to 0 ° C and then Treat all at once with a solution of rate 76 (0.8 eq) / tetrahydrofuran. mixture Warm the material to rt and then heat to reflux for 16 h. Cool to rt and allow the mixture to And wash the solution with saturated ammonium chloride, water and brine, and add sodium sulfate. Dry over lium and evaporate. The residue was chromatographed on silica gel. , To obtain the product.   Example 80   t-butyl-5-amino-2-t-butoxycarbonyl-pentanone:   Adpoc substance 77 was treated with 5% trifluoroacetic acid / anisole (100 equivalents) Dissolve in methylene chloride. After 30 minutes, the solvent was removed under high vacuum at rt and the residue was removed. Dry under reduced pressure for several hours. The crude product is used immediately without purification.   Example 81   t-butyl-5-maleimido-2-t-butoxycarbonyl-pentanoate :   Amino diester 78 / dry acetonitrile was treated with anhydrous maleic acid at 0 ° C under argon. Treat with formic acid (1 equivalent) and stir the stirred mixture at rt for 4 h. Bring the mixture to 0 ° C Recool and treat with trimethylsilyl chloride (3 equivalents) and DIEA (3 equivalents). Manage. The mixture is heated at reflux for 4 h, then cooled to rt and evaporated. Residue Is partitioned between ethyl acetate and water. Wash the organic phase with 10% citric acid, water and brine , Dried over sodium sulfate and evaporated. The residue is chromatographed on silica. To give the product.   Example 82   2- (3'-maleimidopropyl) -malonic acid:   Di-t-butyl ester 79 is dissolved in 20% trifluoroacetic acid and the mixture is dissolved. Stir at rt for 5 h. The solvent is evaporated and the residue is flushed several times with methylene chloride. The residue was triturated with ether and the resulting solid product was filtered off and ether And dried under reduced pressure.   Example 83   MPr-Mal- (Phe-Lys (MMT) -PABOH)_Two:   A stirred solution of diacid 80 / dimethoxyethane was added at 0 ° C to n-hydroxysuccinine. With imide (2.2 eq) and 0.5 M DCC / methylene chloride (2.2 eq) To process. Warm the mixture to rt. After 4 h, Phe-Lys (MMT) -P A solution of ABOH 10a (2 equivalents) / dimethoxyethane was added and the mixture was allowed to stand at rt for 1 hour. Stir for 6 h. Then the mixture is filtered and the filtrate is evaporated. Ethyl acetate and water Distribute between. Phase is washed with water and brine, dried over sodium sulfate and evaporated I do. The product is purified by chromatography on silica gel.   Example 84   MPr-Mal- (Phe-Lys (MMT) -PABC-PNP)_Two:   81, bis-p-nitrophenyl carbonate (6 equivalents) in dry methylene chloride ) And the freshly activated 4Å powdered sieve stirring mixture at rt under argon Treat with DIEA (6 equivalents). After stirring was continued for 16 h, the mixture was filtered and filtered. Evaporate the liquid. The residue is dried under reduced pressure for several hours and then dissolved in a minimum amount of methylene chloride. You. To this is added 2 volumes of ether. The solid obtained is filtered off and ether / Wash with methylene chloride (2: 1) and dry under reduced pressure.   Example 85   MPr-Mal- (Phe-Lys (MMT) -PABC-DOX)_Two:   Bis-p-nitrophenyl carbonate 82 and DOX hydrochloride (1.1 equivalents ) / DMF is treated with DIEA (1.1 eq). After 2h of stirring, Dilute the mixture with ethyl acetate. Wash the solution with water (4 times) and brine, add sodium sulfate Dry over lium and evaporate. The residue was chromatographed on silica gel. , To obtain the product.   Example 86   MPr-Mal- (Phe-Lys-PABC-DOX)_Two・ 2Cl_TwoCHCO_Two H:   A stirred solution of compound 83 / methylene chloride was added to anisole (100 equivalents) followed by Treat with dichloroacetic acid (10 equivalents). After 1.5 h, dilute the mixture with ethyl acetate I do. The resulting suspension was stirred at rt for 1 h, then the orange solid product was filtered off Wash with ethyl acetate and dry under reduced pressure.   Example 87   N-carbobenzyloxy-N ', N'-bis- (carboxymethyl) ethyl Diamine:   Di-t-butyl ester 22 was dissolved in 20% trifluoroacetic acid and the mixture was r Stir for 5 h at t. The solvent is evaporated and the residue is flushed several times with methylene chloride. Remaining The residue was triturated with ether, and the resulting solid product was collected by filtration and washed with ether. And dried under reduced pressure.   Example 88   N-carbobenzyloxy-N ', N'-bis- (2-hydroxyethyl) Tylenediamine:   A solution of bis-carboxylic acid 85 / diglyme at 0 ° C. Treat with xysuccinimide (2.2 eq) and DCC (2.2 eq). Mixed The mixture is warmed to rt and then stirred for 16 h. The solid obtained is filtered off. Filtrate Is cooled to 0 ° C. under an argon atmosphere and then 0.5M sodium borohydride / jig Process on the rim. The mixture is warmed to rt for 16 h, then poured into ice water. can get The mixture is extracted with ethyl acetate. Wash the organic phase with water and brine, add sodium sulfate Dry on top and evaporate to give the product, which is used without purification.   Example 89   Bis- (2-hydroxyethyl) ethylenediamine hydrochloride:   Nitrogen was added to a solution of diol 86 and concentrated HCl (1 equivalent) / methanol for 30 minutes. Degas by blowing for a while. To this, 10% palladium / activated carbon (5% by weight) was added. I can. The resulting mixture was shaken with a Parr apparatus under 50 psi of hydrogen gas for 16 h. Go ahead. Then the mixture is filtered and the filtrate is evaporated. The residue was washed several times with chloroform. Rush and drive off traces of methanol. The crude product is used without purification.   Example 90   Bis- (2-hydroxyethyl) -2'-maleimidoethylamine:   Aminodiol 87 / dry acetonitrile was treated with anhydrous maleic acid at 0 ° C. under argon. Treat with acid (1 eq) and DIEA (1 eq). Stir the mixture at rt for 4 h I do. The mixture was recooled to 0 ° C. and trimethylsilyl chloride (3 eq.) And D Treat with IEA (3 equivalents). Heat the reaction to reflux for 4 h, then cool to rt Then evaporate. The residue is partitioned between ethyl acetate and water. Organic phase is 10% citric acid Wash with water, brine, dry over sodium sulfate and evaporate. Silica gel residue Le To give the product.   Example 91   Bis- (2-chlorocarbonyloxyethyl) -2'-maleimidoethylamido N:   Diol 88 / dry methylene chloride solution was added to 1 M phosgene / toluene (20 equivalents). ) At 0 ° C. After the addition, the mixture was stirred at rt for 16 h. Then, the solvent is removed by a rotary evaporator. The residue is washed with dry methylene chloride. Rush and dry under reduced pressure. The crude bis-chloroformate is used without purification.   Example 92   MEt-IBHE- (Phe-Lys (MMT) -PABOH)_Two:   A stirred solution of crude bis-chloroformate 89 / dry methylene chloride at 0 ° C. he-Lys (MMT) -PABOH10a (2 equivalents) and DIEA (2 equivalents) ) / Methylene chloride solution all at once. The mixture was stirred at rt for 16 h, then Evaporate the solvent. The residue is partitioned between ethyl acetate and water. Wash the organic phase with brine and Dry over sodium acid and evaporate. The product is purified by column chromatography using silica gel. Purify by chromatography.   Example 93   MEt-IBHE- (Phe-Lys (MMT) -PABC-PNP)_Two:   90, bis-p-nitrophenyl carbonate (6 equivalents) in dry methylene chloride ) And the freshly activated 4Å powdered sieve stirring mixture at rt under argon Treat with DIEA (6 equivalents). After stirring was continued for 16 h, the mixture was filtered and filtered. Evaporate the liquid. The residue is dried under reduced pressure for several hours and then dissolved in a minimum amount of methylene chloride. You. To this is added 2 volumes of ether. The solid obtained is filtered off and ether / Wash with methylene chloride (2: 1) and dry under reduced pressure.   Example 94   MEt-IBHE- (Phe-Lys (MMT) -PABC-DOX)_Two:   Bis-p-nitrophenyl carbonate 91 and DOX hydrochloride in DMF ( (1.1 eq.) Is treated with DIEA (1.1 eq.). After 2 hours of stirring The mixture is diluted with ethyl acetate. Wash the solution with water (4 times) and brine, add sulfuric acid Dry over sodium and evaporate. The residue is chromatographed on silica gel. To give the product.   Example 95   MEt-IBHE- (Phe-Lys-PABC-DOX)_Two・ 2Cl_TwoCHC O_TwoH:   A stirred solution of compound 92 / methylene chloride was added to anisole (100 equivalents) followed by Treat with dichloroacetic acid (10 equivalents). After 1.5 h, dilute the mixture with ethyl acetate You. The resulting suspension was stirred at rt for 1 h, then the orange solid product was filtered off , Washed with ethyl acetate and dried under reduced pressure.   Example 96   114  (257 mg, 0.25 mmol) and doxorubicin HCl (3 (77 mg, 0.65 mmol) in 25 ml of dry methanol for 24 h You. The reaction was concentrated to 4 ml by rotary evaporation and then bisected into Sephadex (Sephdex). adex) Purify with LH-20 (1 "x 18") using methanol. Including pure product The fractions with the pool are pooled, rotary evaporated and dried under high vacuum,115(222 mg, 50%).   Example 97   Conjugation of BR96 or IgG with a branched peptide linker:   Thiolation:   BR96 and IgG were previously reported¹(Reduction) by a modified method of You. In a typical embodiment, 1.27 g of BR96 (75 m at 105.7 μM) 1, 7.93 μmol) by performing several cycles of exchanging the reduced pressure and the Ar atmosphere several times. Oxygenate. This was then combined with 7.4 mM DTT (6 in PBS with Ar blowing). (3.6 μmol, 8.6 ml, pH 7.0) and stirred under Ar at 37 ° C. for 3 h. You. Against PBS at pH 6.0 in an Amicon stirred cell at 4 ° C. The low molecular weight compounds are removed by ultrafiltration. 400 ml Amiconse Attach Amicon YM30 filter (Molecular weight cut-off 30000) Load r to 40 psi. Ellman's reagent^Two(Ellman's reagent) The thiol content of the cell eluent is monitored until a baseline reading of 12 nm is obtained. Protein and thiol group concentrations as previously reported¹Measure according to this In the example, 1.10 g of reduced BR96 (85 ml with 80.8 μM MAb, 619 . 1 μM thiol) gave a 87% yield and a thiol titer of 7.7 mol thiol groups. / BR96 (mol).   Example 98   Conjugation:   BR96 and M-Et-IDA- (Phe-Lys-PABC-DOX = β-A la-mTEG)_TwoProcedure for Conjugation (Conjugation)¹Is β-Ala All branched peptides modified with mTEG hydrazone or β-Ala hydrazone It is a typical example of the procedure used in the case of the tide linker.   Reduced BR96 (83 ml, 6.70 μmol MAb, 51.6 μmol thiol At 0 ° C. under Ar at 0 ° C. in 4.0 ml of DMSO in M-Et-IDA- (Ph e-Lys-PABC-DOX = β-Ala-mTEG)_Two(239 mg, 77 . (3 μmol) is added dropwise. After stirring for 30 minutes, the reaction solution was Filter on a filter. Conjugate at 4 ° C. with 1 ″ × 24 ″ Bio-Beads Columns (prepared by swelling and packing in methanol first, then H_TwoFlat in O And finally percolation (approximately 2 ml / min) via PBS, pH 7.4 ). The purified conjugate is again filtered through a 0.22μ sterilizing filter. 95 ml of BR96-S-Et-IDA- (Phe-Lys-PABC -DOX = β-Ala-mTEG)_Two(BR96 76.1 μM; DOX   1.11 mM; MR 14.6 mol DOX / BR96 (mol); 100% yield ). Conjugate with liquid N_TwoAnd store at -80 ° C.   For further guidance, see Wilner D. , Trail P. A. , Hofstead ・ S. J. King H. D. , Rash Braslowski G. R. , Gree Infield R. S. , Kaneko T. , Firestone R. A. "Bioc onjugate "(p. 4521, 1993)," (6-maleimide of doxorubicin) Caproyl) hydrazone: for the production of immunoconjugates of doxorubicin New derivatives "; and Redres PW, Blakeley RL, Zeana -. B. "Anal. Biochem." (94, 75, 1979), "L. Mann's reagent: 5,5'-dithiobis (2-nitrobenzoic acid)-retest ".

──────────────────────────────────────────────────続 き Continued on the front page (51) Int.Cl. ⁷ Identification symbol FI Theme coat ゛ (Reference) A61K 39/395 C07K 7/00 A61P 35/00 A61K 37/02 43/00 105 37/24 C07K 5/00 37/36 7/00 37/54 (81) Designated country EP (AT, BE, CH, DE, DK, ES, FI, FR, GB, GR, IE, IT, LU, MC, NL, PT, SE ), OA (BF, BJ, CF, CG, CI, CM, GA, GN, ML, MR, NE, SN, TD, TG), AP (GH, KE, LS, MW, SD, SZ, UG, ZW), EA (AM, AZ, BY, KG, KZ, MD, RU, TJ, TM), AL, AM, AT, AU, AZ, BB, BG, BR, BY, CA, CH, CN, CZ, DE DK, EE, ES, FI, GB, GE, HU, IL, IS, JP, KE, KG, KP, KR, KZ, LK, LR, LS, LT, LU, LV, MD, MG, MK, MN , MW, MX, NO, NZ, PL, PT, RO, RU, SD, SE, SG, SI, SK, TJ, TM, TR, TT, UA, UG, UZ, VN (72) Gene M United States 06455 Spring Street 65, Middlefield, Connecticut

Claims (1)

[Claims] 1. A branched peptide linker linking a thiol group derived from a target ligand to two or more drug components, the compound comprising a compound having a terminus containing a thiol acceptor bound to the thiol group derived from the target ligand; At least one branch point that is a valence atom takes into account a degree of branching of 2 ^n, where n is a positive integer, at least two amino acid components provide an enzyme cleavage site, and other A branched peptide linker, characterized in that at least two termini contain a group capable of forming a covalent bond with chemically reactive functional groups derived from the drug component. 2. 2. The branched peptide linker according to claim 1, wherein n is 1, 2, 3 or 4. 3. 2. The branched peptide linker according to claim 1, wherein n is 1, 2 or 3. 4. 2. The branched peptide linker according to claim 1, wherein n is 1 or 2. 5. 2. The branched peptide linker according to claim 1, which is linked to an antibody or a fragment thereof. 6. 2. The branched peptide linker according to claim 1, wherein the polyvalent atom is nitrogen or carbon. 7. 2. The branched peptide linker according to claim 1, wherein the polyvalent atom is nitrogen. 8. 2. The branched peptide linker according to claim 1, wherein the polyvalent atom is carbon. 9. 2. The branched peptide linker of claim 1, which is linked to a drug component that is anthracycline. Ten. The branched peptide linker according to claim 1, wherein n is 1 or 2, the target ligand is an antibody or a fragment thereof, the polyvalent atom is nitrogen, and the drug component is anthracycline. 11． formula: Wherein A is a thiol acceptor; W is a bridge; c is 0 or 1; a is an integer of 2 to 12; Q is O, NH or N-lower alkyl; p is 0 or 1; 1; E is a polyvalent atom; each b is an integer from 1 to 10; and each X is a group of the formula -CO-Y-Zm-Gn, where Y is two L-amino acid residues, Z is 1 or Two amino acid residues, m is 0 or 1, G is a self-immolative spacer, and n is 0 or 1, provided that when G is 0, -Y-Zm is ala-leu-ala-leu or gly-phe- leu-gly; or each X is of the formula: Wherein each X ¹ is a group of the formula: —CO—Y—Zm—Gn, Y, Z, Q, E, G, m, d, p, a, b and n are as defined above, or Each X ¹ is of the formula: And each X ² is a group of the formula: —CO—Y—Zm—Gn, Y, Z, G, Q, E, m, d, p, a, b, and n are as defined above, or each X ² is the formula: And each X ³ is a group of the formula: —CO—Y—Zm—Gn, Y, Z, G, Q, E, m, d, p, a, b and n are as defined above, or each X ³ is the formula: And each X ⁴ is a group of the formula: —CO—Y—Zm—Gn, and Y, Z, G, Q, E, m, d, p, a, b, and n are as defined above. The indicated compound. 12． 12. The compound according to claim 11, wherein each X is a group of the formula: -CO-Y-Zm-Gn, wherein Y, m, Z and n are as defined above. 13. 12. The compound according to claim 11, wherein each X ¹ is a group of the formula: —CO—Y—Zm—Gn, and Y, m, Z and n are as defined above. 14. Each X ² has the formula: -CO-Y-Zm-Gn group, Y, m, compounds described in the scope 11 according Z and n are as defined above. 15． Each X ³ has the formula: -CO-Y-Zm-Gn group, Y, m, as described in the scope 11 according Z and n are as defined above compound. 16． -YZm is alanine, valine, leucine, isoleucine, methionine, phenylalanine, tryptophan, proline, lysine, lysine protected with acetyl or formyl, arginine, arginine protected with a tosyl or nitro group, histidine, ornithine, acetyl 12. The compound according to claim 11, which is a dipeptide, tripeptide or tetrapeptide containing an amino acid selected from the group of ornithine protected with formyl and citrulline. 17． 12. The compound according to claim 11, wherein the -Y-Zm group is phenylalanine-lysine. 18． 12. The compound according to claim 11, wherein the -YZM group is valine-citrulline. 19. 12. The compound according to claim 11, wherein the -Y-Zm group is valine-lysine. 20. 12. The compound according to claim 11, wherein E is nitrogen. twenty one. 12. The compound according to claim 11, wherein E is carbon. twenty two. formula: Wherein A is a thiol acceptor; W is a bridge; c is 0 or 1; a is an integer of 2 to 12; Q is O, NH or N-lower alkyl; p is 0 or 1; 1; E is a polyvalent atom; each b is an integer from 1 to 10; and each X is a group of the formula: -CO-Y-Zm-GnD, where Y is two L-amino acid residues, Z is 1 or Two amino acid residues, m is 0 or 1, G is a self-immolative spacer, n is 0 or 1, provided that when G is 0, -Y-Zm is ala-leu-ala-leu or gly-phe-leu -Gly and D are a drug component having a main chain and at least one chemically reactive functional group suspended from the main chain, wherein the functional group reacts with a self-immolative spacer or a terminal amino acid residue. Form a covalent bond, and the functional group is Or a secondary amine, hydroxyl, sulfhydryl, carboxyl, aldehyde or ketone; or each X is of the formula: Wherein each X ¹ is a group of the formula: —CO—Y—Zm—Gn—D, Y, Z, G, D, Q, E, m, d, p and n are as defined above, or Each X ¹ is of the formula: And each X ² is a group of the formula: —CO—Y—Zm—Gn—D, Y, Z, G, D, Q, E, m, d, p, a, b, and n are as defined above. Or each X ² is of the formula: And each X ³ is a group of the formula: —CO—Y—Zm—Gn—D, and Y, Z, G, D, Q, E, m, d, p, a, b, and n are as defined above. Or each X ³ is of the formula: And each X ⁴ is a group of the formula: —CO—Y—Zm—Gn—D, and Y, Z, G, D, Q, E, m, d, p, a, b, and n are as defined above. Is a compound represented by the formula: twenty three. 23. The compound according to claim 22, wherein each X is a group of the formula: -CO-Y-Zm-Gn-D, wherein Y, m, Z, n and D are as defined above. twenty four. Each X ¹ has the formula: -CO-Y-Zm-Gn -D group, Y, m, Z, compounds described in the scope 22 of claims n and D are as defined above. twenty five. Each X ² has the formula: -CO-Y-Zm-Gn -D group, Y, m, Z, compounds described in the scope 22 of claims n and D are as defined above. 26. Each X ³ has the formula: -CO-Y-Zm-Gn -D group, Y, m, Z, compound according to claim 22 of claim n and D are as defined above. 27. -YZm is alanine, valine, leucine, isoleucine, methionine, phenylalanine, tryptophan, proline, lysine, lysine protected with acetyl or formyl, arginine, arginine protected with a tosyl or nitro group, histidine, ornithine, acetyl 23. The compound according to claim 22, which is a dipeptide, a tripeptide or a tetrapeptide containing an amino acid selected from the group of ornithine protected with formyl and citrulline. 28. 23. The compound according to claim 22, wherein the -Y-Zm group is phenylalanine-lysine. 29. 23. The compound according to claim 22, wherein the -Y-Zm group is valine-citrulline. 30. 23. The compound according to claim 22, wherein the -YZM group is valine-lysine. 31. 23. The compound according to claim 22, wherein E is nitrogen. 32. 23. The compound according to claim 22, wherein E is carbon. 33. D is mitomycin-C, mitomycin-A, daunorubicin, doxorubicin, N- (5,5-diacetoxypentyl) doxorubicin, aminopterin, actinomycin, bleomycin, 9-aminocamptothecin, N8-acetylspermidine, 1- (2- 23. The compound according to claim 22, which is an amino-containing drug component selected from the group consisting of (chloroethyl) -1,2-dimethanesulfonylhydrazide, talisomycin, and derivatives thereof. 34. 23. The compound according to claim 22, wherein D is doxorubicin. 35. 23. The compound according to claim 22, wherein D is mitomycin-C. 36. 23. The compound according to claim 22, wherein D is mitomycin-A. 37. 23. The compound according to claim 22, wherein D is talisomycin. 38. 23. The compound according to claim 22, wherein D is N- (5,5-diacetoxypentyl) doxorubicin. 39. D is etoposide, camptothecin, taxol, esperamicin, 1,8-dihydroxy-bicyclo [7.3.1] trideca-4-en-2,6-diyn-13-one, angidine, doxorubicin, morpholine-doxorubicin, N- 23. The compound according to claim 22, which is a hydroxyl-containing drug component selected from the group of (5,5-diacetoxypentyl) doxorubicin, vincristine, vinblastine, and derivatives thereof. 40. 23. The compound according to claim 22, wherein D is a sulfhydryl-containing drug component selected from the group of esperamicin, 6-mercaptopurine, and derivatives thereof. 41. 23. The compound according to claim 22, wherein D is a carboxyl-containing drug component selected from the group consisting of methotrexate, camptothecin (a ring-opened form of lactone), butyric acid, retinoic acid, and derivatives thereof. 42. 23. The compound according to claim 22, wherein D is anthracycline. 43. G is 23. The compound according to claim 22, which is 44. 23. The compound according to claim 22, wherein G is p-aminobenzylcarbonyl. 45. G has the formula: -HN-R ¹ -CO- (wherein, R ¹ is C ₁ -C ₅ alkyl, T is O, N or S) compound of according to claim 22 claims represented by. 46. G is the formula: (Wherein, R ² is H or C ₁ -C ₅ alkyl) compounds described in the scope 22 of claims indicated by. 47. G is the formula: 23. The compound according to claim 22, which is represented by the formula: 48. A is the formula: 23. The compound according to claim 22, which is represented by the formula: 49. formula: [Wherein L is a ligand; q is an integer of 1 to 10; A is a thiol acceptor; W is a bridge; c is 0 or 1; a is an integer of 2 to 12; P is 0 or 1; d is 1 or 2; E is a polyvalent atom; each b is an integer from 1 to 10; and each X is a group of the formula -CO-Y-Zm-Gn-D, wherein Y is two L-type amino acid residues, Z is one or two amino acid residues, m is 0 or 1, G is a self-immolative spacer, and n is 0 or 1, provided that when G is 0, -Y- Zm is ala-leu-ala-leu or gly-phe-leu-gly; D is a drug component having a main chain and a chemically reactive functional group hanging from the main chain, wherein the functional group is self-immolative. Reacts with the spacer to form a covalent bond and the functional group is Ku second amino, hydroxyl, carboxyl, sulfhydryl, selected from the group consisting of aldehyde or ketone; or each X is the formula: Wherein each X ¹ is a group of the formula: —CO—Y—Zm—Gn—D, Y, Z, G, D, Q, E, m, d, p, a, b and n are as defined above. And each X ¹ is a group of the formula: And each X ² is a group of the formula: —CO—Y—Zm—Gn—D, Y, Z, G, D, Q, E, m, d, p, a, b, and n are as defined above. Or each X ² is of the formula: And each X ³ is a group of the formula: —CO—Y—Zm—Gn—D, and Y, Z, G, D, Q, E, m, d, p, a, b, and n are as defined above. Or each X ³ is of the formula: And each X ⁴ is a group of the formula: —CO—Y—Zm—Gn—D, and Y, Z, G, D, Q, E, m, d, p, a, b, and n are as defined above. Is a compound represented by the formula: 50. 50. The compound according to claim 49, wherein L is an immunoglobulin or a fragment thereof. 51. 50. The immunoglobulin selected from the group consisting of BR96, BR64, L6, relaxed BR96, relaxed BR64, chimera L6, relaxed chimera BR96, relaxed chimera BR64, relaxed chimera L6, and fragments thereof, according to claim 49. Compound. 52. L is bombesin, EDG, transferrin, gastrin, gastrin releasing peptide, platelet derived growth factor, IL-2, 11-6, TGF-α, TGF-β, VGF, insulin, insulin-like growth factors I and II, carbohydrate, 50. The compound according to claim 49, which is a ligand selected from the group of lectins and apoproteins from low density lipoproteins. 53. 50. A pharmaceutical composition comprising the compound of claim 49 and a pharmaceutically acceptable carrier. 54. 50. A method for controlling undesired cell growth, comprising administering to a host in need of such treatment a compound as defined in claim 49. 55. 55. The method according to claim 54, wherein the undesired cells are cancer cells. 56. 50. A method for treating a warm-blooded animal, comprising administering to the warm-blooded animal a compound according to claim 49 in an amount effective for tumor suppression. 57. 50. A method of targeting a pharmaceutical agent to a host or a predetermined site of a sample, comprising administering to the host or contacting the compound of claim 49 with the sample.