AU2002313471A1 - Cytotoxic CD44 antibody immunoconjugates - Google Patents
Cytotoxic CD44 antibody immunoconjugatesInfo
- Publication number
- AU2002313471A1 AU2002313471A1 AU2002313471A AU2002313471A AU2002313471A1 AU 2002313471 A1 AU2002313471 A1 AU 2002313471A1 AU 2002313471 A AU2002313471 A AU 2002313471A AU 2002313471 A AU2002313471 A AU 2002313471A AU 2002313471 A1 AU2002313471 A1 AU 2002313471A1
- Authority
- AU
- Australia
- Prior art keywords
- compound
- antibody molecule
- antibody
- conjugate
- maytansinoid
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Abandoned
Links
Description
Cytotoxic CD44 Antibody Immunoconjugates
The invention relates to novel conjugates of antibodies with cytotoxic compounds, pharmaceutical compositions comprising such compounds, and their use in tumor therapy.
There have been numerous attempts to improve the efficacy of antineoplastic drugs by conjugating such drugs to antibodies against tumor-associated antigens in order to elevate local concentration of the drug by targeted delivery to the tumor. Many of these approaches have met limited success, and several reasons have been discussed in the literature to explain the failure. For anticancer drugs acting stoichometrically, like e.g. doxorubicin or methotrexate, relatively high intracellular concentrations are necessary to exert the required cytotoxicity. These concentrations are thought to be difficult to achieve with many antibody-drug conjugates because of (a) insufficient potency of many common anticancer drugs, (b) low cell surface concentration of antigen targets, (c) inefficient internalization of antigen-antibody complexes into the target cell, and (d) inefficient release of free drug from the conjugate inside the target cell (Chari et al., 1992).
Two of the aforementioned drawbacks, namely (a) and (d), have been adressed by the work of Chari and coworkers (Chari et a., 1992; Liu et al., 1996; U.S. Patent No. 5,208,020). They have developed antibody conjugates wherein the antibody is linked to a maytansinoid via a disulfide linkage. Maytansines belong to the class of Ansa macrolide antibiotics, which derive from Nocardia sp.. The maytansine ansamitocin P-3, produced by bacterial fermentation, is used as a precursor molecule to manufacture maytansinoid DM1. Maytansine and derivatives act as anti-mitotic agents (inhibitors of tubulin polymerization), similar as vincristine, but with markedly higher potency than vincristine or other established chemotherapeutic agents (DM1 is toxic to cells in vitro at ~10"10 M concentration). In contrast to the high cytotoxicity of free maytansinoid, the antibody conjugate has a toxicity which is several orders of magnitude lower on antigen-negative cells compared to antigen-positive cells. The linkage by disulfide bonding has the advantage that these bonds are readily cleaved inside the target cells by intracellular glutathione, releasing highly toxic free drug. This approach has been applied to antibodies against tumor-associated antigens, for example the C242-DM1 conjugate (Liu et al., 1996; Lambert et al., 1998), and HuN901-DMl (Chari et al., 2000). However, the application of
these conjugates is restricted due to the limited expression of the respective target antigens. For example, the antigen recognized by N901 (CD56, N-CAM) is predominanttly expressed by tumors of neuroendocrine origin, the expression of the C242 antigen (CanAg) is mostly limited to tumors derived from the GI tract.
There is, however, still the need to improve this approach by finding suitable tumor- associated antibodies with favorable antigen expression pattern, high and specific cell surface antigen concentration within the target tissue, and efficient internalization process transporting the antigen complexed-antibody conjugate into the cells.
CD44 is a protein which is expressed in several different isoforms on the surface of a wide variety of cell types. The smallest isoform, standard CD44 (CD44s), which is expressed by a variety of different cells, is thought to mediate cell attachment to extracellular matrix components and may transmit a co-stimulus in lymphocyte and monocyte activation. In contrast, expression of splice variants of CD44 which contain the domain v6 (CD44v6) in the extracellular region, is restricted to a subset of epithelia. The physiological role of CD44v6 is not yet fully understood.
CD44v6, as well as other variant exons (CD44v3, CD44v5, CD44v7/v8, CD44vl0) has been shown to be a tumor-associated antigen with a favorable expression pattern in human tumors and normal tissues (Heider et al., 1995; Heider et al., 1996; Dall et al., 1996; Beham-Schmid et al., 1998; Tempfer et al., 1998; Wagner et al., 1998) and has been subject to antibody-based diagnostic and therapeutic approaches, in particular radioimmunotherapy (RIT) of tumors (Verel et al, 2002; Stromer et al., 2000; WO 95/33771; WO 97/21104).
However, a prerequisite for efficient killing of tumor cells by antibody maytansinoid conjugates is sufficient internalization of the target antigen. Only few data on the internalization of CD44 are available. Bazil et Horejsi reported that downregulation of CD44 on leukocytes upon stimulation with PMA is caused by shedding of the antigen rather than by internalization (Bazil et Horejsi, 1992). Shedding of CD44 is also supported by several reports on soluble CD44 in the serum of tumor patients and normal individuals (Sliutz et al., 1995; Guo et al., 1994; Martin et al., 1997). In a recent paper by Aguiar et al.
the amount of internalized CD44 on matrix-intact chondrocytes was determined to be approximately 6% in 4 hours (Aguiar et al., 1999). Similar low levels of internalized CD44v6 on tumor cells were found in experiments performed by BIA. Taken together, these data suggest that CD44 receptors are more likely subject to shedding than to internalization, and thus CD44 specific antibodies are not to be regarded as suitable candidates for the maytansinoid conjugate approach. This has been supported by in vitro cell proliferation assays wherein AbcD44v6-D l showed only slightly elevated cytotoxicity against antigen-presenting cells as compared to cells lacking the antigen.
It now has been unexpectedly found that CD44 specific antibodies conjugated to highly cytotoxic drugs through a linker which is cleaved under intracellular conditions are very efficient tumor therapeutics in vivo.
The present invention provides novel compounds consisting of a CD44 specific antibody molecule conjugated to a highly cytotoxic drug through a linker which is cleaved under intracellular conditions.
In particular, the present invention provides a compound of formula A(LB)n (Formula (I)) wherein
A is an antibody molecule which is specific for CD44;
L is a linker moiety;
B is a compound which is toxic to cells; and n is a decimal number with n = 1 to 10
The antibody molecule A has a binding specificity for CD44, preferably variant CD44.
The term „antibody molecule" shall encompass complete immunoglobulins as they are produced by lymphocytes and for example present in blood sera, monoclonal antibodies secreted by hybridoma cell lines, polypeptides produced by recombinant expression in host cells which have the binding specificity of immunoglobulins or monoclonal antibodies, and molecules which have been derived from such immunoglobulins, monoclonal antibodies, or polypeptides by further processing while retaining their binding specificity. In particular,
the term „antibody molecule" includes complete immunoglobulins comprising two heavy chains and two light chains, fragments of such immunoglobulins like Fab, Fab', or F(ab)2 fragments (Kreitman et al, 1993), recombinantly produced polypeptides like chimeric, humanised or fully human antibodies (Breitling et Duebel, 1999; Shin et al, 1989; Gϋssow et Seemann, 1991, Winter et al, 1994, EP 0 239 400; EP 0 519 596; WO 90/07861 EP 0 368 684; EP 0 438 310; WO 92/07075; WO 92/22653; EP 0 680 040; EP 0 451 216), single chain antibodies (scFv, Johnson et Bird, 1991), and the like. Today, antibodies may also be produced without immunising a laboratory animal, e.g. by phage display methods (Aujame et al., 1997; US 5,885,793; US 5,969,108; US 6,300,064; US 6,248,516, US 6,291,158). Fully human antibodies may be produced using transgenic mice carrying functional human Ig genes (EP 0 438 474 ; EP 0 463 151; EP 0 546 073). From the aforementioned literature references, the expert knows how to produce these types of antibody molecules, employing state of the art methods like automated peptide and nucleic acid synthesis, laboratory animal immunisation, hybridoma technologies, polymerase chain reaction (PCR), vector and expression technologies, host cell culture, and protein purification methods. In the following, the terms „antibody" and „antibody molecule" are used interchangeably.
„Specific for CD44" shall mean that the antibody molecule has specific binding affinity for an epitope present in CD44. In a preferred embodiment, the antibody molecule of the invention has a binding specificity for the amino acid sequence coded by variant exon v6 of the human CD44 gene. The sequence of variant exon v6 as well as of the other variant exons is known in the art (Screaton et al, 1992; Tδlg et al, 1993; Hofmann et al, 1991). A preferred antibody molecule of the invention specifically binds to peptides or polypetides having or containing the amino acid sequence SEQ ED NO: 1 of the accompanying sequence listing, or an allelic variant of said sequence. Preferably, said antibody molecule has binding specificity for an epitope within said sequence. More preferably, the antibody molecule specifically binds to a peptide having the amino acid sequence SEQ ID NO: 2, even more preferably having the amino acid sequence SEQ ID NO: 3. Such antibody molecules may be easily produced with methods known in the art (WO 95/33771 , WO 97/21104), e.g. by immunising laboratory animals with chemically synthesised peptides having the aforementioned sequences, e.g. bound to a hapten, or immunising with a recombinantly produced fusion protein including said sequences, and proceeding according
to methods known in the art (Harlow 1988; Catty 1988; Koopman et al, 1993; Heider et al, 1993).
Preferably, an antibody molecule according to the invention is the murine monoclonal antibody with the designation VFF-18 which is produced by a hybridoma cell line which has been deposited on 07 June 1994 under the accession number DSM ACC2174 with the DSM-Deutsche Sammlung fur Mikroorganismen und Zellkulturen GmbH, Mascheroder Weg lb, D-38124 Braunschweig, Deutschland/Germany. Also preferred are Fab, Fab', or F(ab)2 fragments of said monoclonal antibody VFF-18. In another preferred embodiment, the antibody molecule is a humanised recombinant antibody, wherein the complementarity determining regions (CDR's) of VFF-18 have been grafted into the respective genes of human immunoglobulin heavy and light chains.
"Complementarity determining regions" of a monoclonal antibody are understood to be those amino acid sequences involved in specific antigen binding according to Kabat et al. , 1991, in connection with Chothia and Lesk, 1987.
In another preferred embodiment, appropriate framework residues of such a CDR-grafted antibody are reverted to murine residues to improve binding affinity. From methods pertinent to the art, the experts knows how to obtain the CDR's of VFF-18, starting with the aforementioned hybridoma with the accession number DSM ACC2174, to choose and obtain appropriate human immunoglobulin genes, to graft the CDR's into these genes, to modify selected framework residues, to express the CDR-grafted antibody in appropriate host cells, e.g. Chinese hamster ovary (CHO) cells, and to test the resulting recombinant antibodies for binding affinity and specificity (see e.g. literature references above). In another preferred embodiment of the invention, the antibody molecule is a recombinant antibody having the CDR's of the antibody VFF-18. Preferably, such a recombinant antibody is a humanised antibody and is a complete immunoglobulin consisting of two complete light and two complete heavy chains. In another preferred embodiment of the invention, the antibody molecule is a recombinant antibody having the same idiotype as the antibody VFF-18. In another preferred embodiment of the invention, the antibody molecule is a recombinant antibody binding to the same epitope as the antibody VFF-18.
In a particular preferred embodiment, the antibody molecule A is an antibody comprising light chains having the amino acid sequence SEQ ID NO: 4, and heavy chains having the amino acid sequence SEQ ID NO: 6. This antibody is called BIWA 4. It is a humanised version of antibody VFF-18 mentioned above, having the complementary determining regions of the murine monoclonal antibody VFF-18 in a completely human framework, and human constant regions. It is therefore an antibody of very low immunogenicity in man, which is a favorable trait. However, as it has no murine framework residues to optimise antigen binding, it has a significanty lower antigen binding affinity as its parent antibody VFF-18, and therefore would not have been regarded as a good candidate for a therapeutic drug. Unexpectedly, it has been found that BIWA 4, despite its poor binding affinity, has a very favorable biodistribution and tumor uptake in vivo, making it superior to other humanised versions of VFF-18 with higher binding affinity (Verel et al, 2002). In a further preferred embodiment, the antibody molecule A is an antibody comprising light chains having the amino acid sequence SEQ ID NO: 8, and heavy chains having amino acid sequence SEQ ID NO: 6. This antibody has higher binding affinity than BIWA 4 and is called BIWA 8.
These antibodies may be produced as follows. Nucleic acid moelcules coding for the light chain and the heavy chain may be synthesised chemically and enzymatically by standard methods. First, suitable oligonucleotides can be synthesized with methods known in the art (e.g. Gait, 1984), which can be used to produce a synthetic gene. Methods to generate synthetic genes from oligonucleotides are known in the art (e.g. Stemmer et al. 1995; Ye et al. 1992; Hayden et Mandecki 1988; Frank et al. 1987). Preferably, the nucleic acid molecules encoding the light and heavy chains of BIWA 4 have the nucleotide sequences of SEQ ID NO: 5 and SEQ ID NO: 7, respectively. These sequences include sequences coding for leader peptides which are cleaved by the host cell (SEQ ID NO: 5: the first 60 nucleotides; SEQ ID NO: 7: the first 57 nucleotides). In a further embodiment, the nucleic acid molecules encoding the light and heavy chains of an antibody molecule according to the invention have the nucleotide sequences of SEQ ID NO: 9 and SEQ ID NO: 7, respectively. These nucleic acid molecules encoding the antibody heavy and light chains then may be cloned into an expression vector (either both chains in one vector molecule, or each chain into a separate vector molecule), which then is introduced into a host cell. Expresssion vectors suitable for immunoglobulin expression in prokaryotic or eukaryotic
host cells and methods of introduction of vectors into host cells are well-known in the art. In general, the immunoglobulin gene therein is in functional connection with a suitable promoter, like for example a human cytomegalovirus (CMV) promoter, hamster ubiquitin promoter (WO 97/15664), or a simian virus SV40 promoter located upstream of the Ig gene. For termination of transcription, a suitable termination/polyadenylation site like that of the bovine growth hormone or SV40 may be employed. Furthermore, an enhancer sequence may be included, like the CMV or SV40 enhancer. Usually, the expression vector furthermore contains selection marker genes like the dihydrofolate reductase (DHFR), glutamine synthetase, adenosine deaminase, adenylate deaminase genes, or the neomycin, bleomycin, or puromycin resistance genes. A variety of expression vectors are commercially available from companies such as Stratagene, La Jolla, CA; Invitrogen, Carlsbad, CA; Promega, Madison, WI or BD Biosciences Clontech, Palo Alto, CA. For example, expression vectors pAD-CMVl (NCBI GenBank Accession No. A32111) or pAD-CMV19 (NCBI GenBank Accession No. A32110) may be used for expression.. The host cell preferably is a mamalian host cell, e.g. a COS, CHO, or BHK cell, more preferably a Chinese hamster ovary (CHO) cell, e.g. a CHO-DUKX (Urlaub and Chasin, 1980), CHO-DG44 (Urlaub et al., 1983), or CHO-K1 (ATCC CCL-61) cell. The host cell then is cultured in a suitable culture medium under conditions where the antibody is produced, and the antibody is then isolated from the culture according to standard procedures. Procedures for production of antibodies from recombinant DNA in host cells and respective expression vectors are well-known in the art (see e.g. WO 94/11523, WO 97/9351, EP 0481 790, EP 0 669 986).
In order to link the antibody molecule A to the compound B which is toxic to cells, a linking moiety L is used. In the most simple case, the linking moiety L is a chemical bond, preferably a covalent bond which is cleaved under intracellular conditions. In one embodiment of the invention, the bond is between a sulfur atom present in the antibody molecule, e.g. in the side chain of a cystein residue, and another sulfur atom present in the toxic compound. In another embodiment, the linking moiety L consists of one or more atoms or chemical groups. Suitable linking groups are well known in the art and include disulfide groups, thioether groups, acid labile groups, photolabile groups, peptidase labile groups and esterase labile groups. Preferred are disulfide groups and thioether groups.
Conjugates of the antibody molecules of the invention and toxic compound can be formed using any techniques presently known or later developed. The toxic compound can be modified to yield a free amino group and then linked to the antibody molecule via an acid- labile linker, or a photolabile linker. The toxic compound can be condensed with a peptide and subsequently linked to an antibody molecule to produce a peptidase-labile linker. The toxic compound can be treated to yield a primary hydroxyl group, which can be succinylated and linked to an antibody molecule to produce a conjugate that can be cleaved by intracellular esterases to liberate free drug. Most preferably, the toxic compound is treated to create a free or protected thiol group, and then one or many disulfide or thiol- containing toxic compounds are covalently linked to the antibody molecule via disulfide bond(s).
For example, antibody molecules can be modified with crosslinking reagents such as N- succinimidyl 3-(2-pyridyldithio)propionate (SPDP), 4-succinimidyl-oxycarbonyl-α-methyl- α-(2-pyridyldithio)-toluene (SMPT), N-succinimidyl-3-(2-pyridyldithio)-butyrate (SDPB), N-succinimidyl-4-(2-pyridyldithio)pentanoate (SPP), N-succinimidyl-5-(2- pyridyldithio)pentanoate, 2-iminothiolane, or acetylsuccinic anhydride by known methods. See, Carlsson et al, 1978; Blattler et al 1985; Lambert et al, 1983; Klotz et al, 1962; Liu et al, 1979; Blakey and Thorpe, 1988; Worrell et al, 1986. In a preferred embodiment, the linker moiety is a 4-thiopentanoate derived from SPP, or 5-thiopentanoate. The antibody molecule containing free or protected thiol groups thus derived is then reacted with a disulfide- or thiol-containing toxic compound to produce conjugates. The conjugates can be purified by HPLC or by gel filtration.
„Toxic" is a compound that inhibits or prevents function of cells and/or causes cell destruction. Toxic compounds used for coupling may act either cytostatic or cytotoxic and lead to cell cycle arrest or cell death. These compounds may act at different stages during the cell cycle, e.g. by interference with nucleic acid synthesis, inactivation of nucleic acids, or by binding to tubulin.
In a preferred embodiment, the compound B which is toxic to cells is a maytansinoid, i.e. a derivative of maytansine (CAS 35846538). In a preferred embodiment, it is a C-3 ester of maytansinol. Maytansinoids suitable for conjugating to antibodies for use in cancer
therapy, including preparation of said maytansinoids and their linkage to antibody molecules, have been described by Chari and Coworkers (Chari et al., 1992; Liu et al., 1996; U.S. Patent No. 5,208,020). These maytansinoids may be used for the present invention. In a preferred embodiment, the toxic compound is N -deacetyl- N -(3- mercapto-l-oxopropyl)-Maytansine (CAS Number 139504-50-0), also referred to as DM1. Preferably, said maytansinoid is a maytansinol derivative linked to the antibody molecule via a disulfide bridge at the C-3 position of maytansinol. In a particularly preferred embodiment, the antibody/maytansinoid conjugate may be prepared from a maytansinoid of formula
Formula (ET)
wherein Ri represents H or SR , wherein R4 represents methyl, ethyl, linear alkyl, branched alkyl, cyclic alkyl, simple or substituted aryl, or heterocyclic;
R2 represents Cl or H;
R3 represents H or CH3; and m represents 1, 2, or 3. Preferably, R] is H, CH3, or SCH3, R2 is Cl, R3 is CH3, and m = 2.
The compound with Ri = H, R2 = Cl, R3 = CH3, and m = 2 is designated DM1 in the literature.
In a preferred embodiment, the compund of the invention has the formula
(Formula IH) wherein
A is an antibody molecule which is specific for CD44, preferably specific for the variant exon v6, preferably specific for the amino acid sequence SEQ ED NO: 3; (L') is an optional linker moiety p is a decimal number with p = 1 to 10.
Preferably, p is 3 to 4, more preferably about 3.5.
Methods for preparing such maytansinoids are known in the art (see in particular US 5,208,020, Example 1). Conveniently, in a first step the maytansinoid C-3 ester ansamitocin P3 may be produced by bacterial fermentation of microorganisms belonging to the genus Nocardia or Actinosynnema, e.g. ATCC 31565, ATCC 31281 (US 4,356,265;
US 4,450,234; WO 01/77360). Ansamitocin P3 may be extracted from the culture using organic solvents like ethyl acetate or toluene, and further purified by adsorption chromatography using e.g. silica gel. It may then be reduced to maytansinol using LiAlH4 (US 4,360,462) or, as suggested more recently, LiAl(OMe)3H or other LiAl or NaAl hydrids (WO 02/16368). The maytansinol may then be esterified at the C-3 position with N-methyl-L-alanine or N-methyl-L-cysteine derivatives to yield a disulfide-containing maytansinoid (US 5,208,020; US 5,416,064; US 6,333,410), for example using dicyclohexylcarbodiimide(DCC) and catalytic amounts of zinc chloride (US 4,137,230; US 4,260,609). In a preferred embodiment, the maytansinol is esterified with the compound N- methyl-N-(3 -methyldithiopropanoyl)-L-alanine of formula
to yield the maytansinoid of Formula (Et) with with R = SR , t = CH3, R2 = Cl, R3 CH3, and m = 2.
The free thiol group may then be released by cleavage of the disulfide bond with dithiothreitol (DTT), to yield e.g. DM1.
Upon intracellular cleavage, the free toxic compound is released from the conjugate A(LB)n. The free drug released from the compound A(LB)n may have the formula B-X, wherein X is an atom or a chemical group, depending on the nature of the cleaving reaction. Preferably, X is a hydrogen atom, as for example when the linker moiety is just a covalent bond between two sulfur atoms, or a hydroxyl group. The cleavage site may also be within the linker moiety if the linker moiety is a chemical group, generating free drug of formula B-L"-X upon cleavage, wherein X is an atom or a chemical group, depending on the nature of the cleaving reaction. Preferably, X is a hydrogen atom or a hydroxyl group.
In a preferred embodiment, the compound of formula (I) is less toxic than the toxic compound B, B-X or B-L"-X released upon intracellular cleavage. Methods of testing cytotoxicity in vitro are known in the art (Goldmacher et al., 1985; Goldmacher et al.,
1986; see also US 5,208,020, Example 2). Preferably, the compound (I) is 10 times or more, more preferably 100 times or more, or even 1000 times or more less toxic than the free drug released upon cleavage.
Preferably, antibody molecule/maytansinoid conjugates are those that are joined via a disulfide bond, as discussed above, that are capable of delivering maytansinoid molecules. Such cell binding conjugates are prepared by known methods such as modifying monoclonal antibodies with succinimidyl pyridyl-dithiopropionate (SPDP) or pentanoate (SPP) (Carlsson et al, 1978). The resulting thiopyridyl group is then displaced by treatment with thiol-containing maytansinoids to produce disulfide linked conjugates. Alternatively, in the case of the aryldithiomaytansinoids, the formation of the antibody conjugate is effected by direct displacement of the aryl-thiol of the maytansinoid by sulfhydryl groups previously introduced into antibody molecules. Conjugates containing 1 to 10 maytansinoid drugs linked via a disulfide bridge are readily prepared by either method. In this context, it is understood that the decimal number n in the formula A(LB)n is an average number as not all conjugate molecules of a given preparation may have the identical integer of LB residues attached to the antibody molecule.
More specifically, a solution of the dithiopyridyl modified antibody at a concentration of 1 mg/ml in 0.1M potassium phosphate buffer, at pH 7.0 containing 1 mM EDTA is treated with the thiol-containing maytansinoid (1.25 molar equivalent/dithiopyridyl group). The release of pyridine-2-thione from the modified antibody is monitored spectrophotometrically at 343nm and is complete in about 30 min. The antibody- maytansinoid conjugate is purified and freed of unreacted drug and other low molecular weight material by gel filtration through a column of Sephadex G-25. The number of maytansinoids bound per antibody molecule can be determined by measuring the ratio of the absorbance at 252 nm and 280 nm. An average of 1-10 maytansinoid molecules/antibody molecule can be linked via disulfide bonds by this method.
In a further aspect, the present invention relates to a conjugate of a CD44v6 specific antibody molecule and a maytansinoid. Herein, „CD44v6 specific" shall mean that the antibody has specific binding affinity to an epitope which is present in a peptide having the amino acid sequence encoded by variant exon v6 of CD44, preferably human CD44. A
preferred antibody molecule of the invention specifically binds to peptides or polypetides having or containing the amino acid sequence SEQ ED NO: 1 of the accompanying sequence listing, or an allelic variant of said sequence. Preferably, said antibody molecule has binding specificity for an epitope within said sequence. More preferably, the antibody molecule specifically binds to a peptide having the amino acid sequence SEQ ID NO: 2, even more preferably having the amino acid sequence SEQ ID NO: 3.
Preferably, the antibody molecule in said conjugate is the monoclonal antibody VFF-18 (DSM ACC2174) or a recombinant antibody having the complementary determining regions (CDRs) of VFF-18. More preferably, the said antibody comprises light chains having the amino acid sequence SEQ ED NO: 4, or, alternatively, SEQ ED NO: 8, and heavy chains having the amino acid sequence SEQ ED NO: 6.
The maytansinoid is preferably linked to the antibody by a disulfide moiety and has the formula
Formula (TV)
wherein the link to the antibody is through the sulfur atom shown in formula TV to a second sulfur atom present in the antibody molecule. To create such a sulfur atom available for bonding, an antibody molecule may be modified by introduction of a suitable linker as
outlined above. Preferably, the maytansinoid is linked to the antibody molecule through a - S-CH2CH2-CO-, a -S-CH2CH2CH2CH2-CO-, or a -S-CH(CH3)CH2CH2-CO- group. The sulfur atom in such a linker group forms the disulfide bond with the maytansinoid, while the carbonyl function may be bonded to an amino function present on the side chain of an amino acid residue of the antibody molecule.
That way, one or more maytansinoid residues may be linked to an antibody molecule. Preferably, 3 to 4 maytansinoid residues are linked to an antibody molecule.
Most preferred is a conjugate of a CD44v6 specific antibody molecule and a maytansinoid, wherein the antibody comprises light chains having the amino acid sequence SEQ ID NO: 4, and heavy chains having the amino acid sequence SEQ ID NO: 6, and wherein the maytansinoid has the formula
(Formula IV)
and is linked to the antibody through a disulfide bond. Preferably, the linking group is -S- CH2CH2CH2CH2-CO- or -S-CH(CH3)CH2CH2-CO-, and the number of maytansinoid residues bound per antibody molecule is 3 to 4.
In a further embodiment, the present invention relates to a method of production of a compound of formula (I) comprising the steps:
(a) introducing free or protected thiol groups into an antibody molecule which is specific for CD44;
(b) reacting the antibody molecule of step (a) with a compound which is toxic to cells, said compound having one or more disulfide or thiol groups; and
(c) recovering the resulting conjugate.
Preferably, the antibody molecule is specific for CD44v6, more preferably specific for the amino acid sequence SEQ ED NO: 3. The compound which is toxic to cells is preferably a maytansinoid, more preferably of formula (IE), most preferably with R\ = H, R2 = Cl, R3 = CH3, and m = 2. In a further preferred embodiment, the antibody comprises light chains having the amino acid sequence SEQ ID NO: 4 or SEQ ID NO: 8, and heavy chains having the amino acid sequence SEQ ED NO: 6.
In preferred embodiments of such a method, (2-pyridyl)-3-dithiopropanoic acid N-hydroxy succinimid ester (N-succinimidyl-3-(2-pyridyldithio)-propionate), (2-pyridyl)-4- dithiopentanoic acid N-hydroxy succinimid ester (N-succinimidyl-4-(2-pyridyldithio)- pentanoate), or (2-pyridyl)-5-dithiopentanoic acid N-hydroxy succinimid ester (N- succinimidyl-5-(2-pyridyldithio)-pentanoate) are used to introduce the free or protected thiol groups into the antibody molecule. The invention also relates to compounds obtainable by a method as described.
In a further embodiment, the present invention relates to a pharmaceutical composition comprising a compound of formula (I), or a conjugate as described, preferably together with a pharmaceutically acceptable carrier, excipient, or diluent.
Suitable pharmaceutically acceptable carriers, diluents, and excipients are well known and can be determined by those of skill in the art as the clinical situation warrants. Examples of suitable carriers, diluents and/or excipients include: (1) Dulbecco's phosphate buffered saline, pH about 7.4, containing about 1 mg/ml to 25 mg/ml human serum albumin, (2) 0.9% saline (0.9% w/v NaCl), and (3) 5% (w/v) dextrose.
More preferably, the antibody molecule present in the pharmaceutical composition is the monoclonal antibody VFF-18, or a recombinant antibody having the CDR's of the antibody VFF-18, preferably in a human framework. In a further preferred embodiment, the antibody comprises light chains having the amino acid sequence SEQ ED NO: 4 or SEQ ED NO: 8, and heavy chains having the amino acid sequence SEQ ED NO: 6. Preferably, the toxic compound is the maytansinoid of formula (IE).
The compounds of the invention may be used for all kinds of clinical or non-clinical applications wherein a toxic compound is to be targeted to cells expressing CD44, preferably CD44v6 on the cell surface.
The conjugate may for example be clinically used ex vivo to remove tumor cells from bone marrow prior to autologous transplantation in cancer treatment. Treatment can be carried out as follows. Bone marrow is harvested from the patient or other individual and then incubated in medium containing serum to which is added the compound of formula (I) according to the invention, concentrations range from about 10 μM to 1 pM, for about 30 minutes to about 48 hours at about 37°C. The exact conditions of concentration and time of incubation (=dose) are readily determined by the skilled artisan. After incubation, the bone marrow cells are washed with medium containing serum and returned to the patient by i.v. infusion according to known methods. In circumstances where the patient receives other treatment such as a course of ablative chemotherapy or total-body irradiation between the time of harvest of the marrow and reinfusion of the treated cells, the treated marrow cells are stored frozen in liquid nitrogen using standard medical equipment.
En a further embodiment, the present invention relates to a method of treatment of cancer comprising applying a pharmaceutical composition as described before to a patient. In particular, this aspect of the invention relates to a method of treatment of cancer in a patient in need thereof comprising administering to the patient a therapeutically effective amount of a compound as described above, or a pharmaceutical composition as described above. Preferably, the cancer is head and neck squamous cell carcinoma (SCC), esophagus SCC, lung SCC, skin SCC, breast adenocarcinoma (AC), lung AC, cervix SCC, pancreas AC, colon AC, or stomach AC.
For clinical treatment of cancer, the compound of formula (I) according to the invention will be supplied as solutions that are tested for sterility and for endotoxin levels. Examples of suitable protocols of conjugate administration are as follows. Conjugates maybe given weekly for 1 to 6 weeks either as an i.v. bolus , or as a continuous infusion for 5 days. Bolus doses can be given in 50 to 100 ml of normal saline to which 5 to 10 ml of human serum albumin has been added. Continuous infusions can be given in 250 to 500 ml of normal saline, to which 25 to 50 ml of human serum albumin has been added, per 24 hour period. Dosages will generally be 10 mg to 400 mg/m of body surface area per application. The dose applied to the patient per administration has to be high enough to be effective, but must be below the dose limiting toxicity (DLT). In general, a sufficiently well tolerated dose below DLT will be considered maximum tolerated dose (MTD). The expert knows how to determine the MTD (Lambert et al., 1998). For weekly administrations, the MTD can be expected to be in the range of 100 to 200 mg/m2. Alternatively, intervals between applications may be longer, e.g. two to four weeks, preferably three weeks. In this case, the MTD can be expected to be in the range of 200 to 300 mg/m . Alternatively, application may be in 5 daily doses, followed by a break of several weeks after which treatment may be repeated. In this case, the MTD per administration can be expected to be lower than 100 mg/m2. For example, conjugates can be administered as a single i.v. infusion with a rate of 3 mg/min every 21 days. Up to 7 cycles of treatment were applied. It is to be understood that the applied doses may well be out of the ranges given above if the clinical situation requires. For example, if the MTD is found to be higher than indicated, single administration may be at a higher dose than 400 mg/m2, or weekly may be at more than 200 mg/m2.
Dose, route of administration, application scheme, repetition and duration of treatment will in general depend on the nature of the disease (type, grade, and stage of the tumor etc.) and the patient (constitution, age, gender etc.), and will be determined by the medical expert responsible for the treatment. Besides treatment of solid tumors, therapeutic application according to the invention may be particularly advantageous as an adjuvant to surgical intervention, to treat minimal residual disease.
In a further embodiment, the invention relates to the use of a compound of formula (I) for the preparation of a pharmaceutical composition for the treatment of cancer. More preferably, the antibody molecule present in the pharmaceutical composition is the monoclonal antibody VFF-18, or a recombinant antibody having the CDR's of the antibody VFF- 18, preferably in a human framework. Most preferred is an antibody molecule comprising a light chain having SEQ ID NO: 4 or SEQ ED NO: 8, and a heavy chain having SEQ ED NO: 6. Preferably, the toxic compound has the formula (IE). Preferably, the cancer is head and neck squamous cell carcinoma (SCC), esophagus SCC, lung SCC, skin SCC, breast adenocarcinoma (AC), lung AC, cervix SCC, pancreas AC, colon AC, or stomach AC.
References
Aguiar DJ, Knudson W, and Knudson CB. Internalization of the hyaluronan receptor CD44 by chondrocytes. Exp.Cell.Res. 252: 292-302, 1999.
Aujame L, Geoffroy F, Sodoyer R. High affinity human antibodies by phage display. Hum Antibodies 8(4):155-68 (1997).
Bazil V and Horejsi V. Shedding of the CD44 adhesion molecule from leukocytes induced by anti-CD44 monoclonal antibody simulating the effect of a natural receptor ligand. J Immunol 149 (3):747-753, 1992.
Blattler et al, Biochem. 24: 1517-1524 (1985).
Breitling F, Duebel S: Recombinant Antibodies. John Wiley, New York 1999.
Carlsson et al, Biochem. J. 173: 723-737 (1978).
Catty D. Antibodies. Oxford IR Press 1988.
Chari RVJ, Martell BA, Gross JL, Cook SB, Shah SA, Blattler WA, McKenzie S J, Goldmacher VS. Immunoconjugates containing novel maytansinoids: promising anticancer drugs. Cancer Research 52: 127-31, 1992.
Chari RVJ, Derr SM, Steeves RM, Widdison WC: Dose-response of the anti-tumor effect of HUN901-DM1 against human small cell lung cancer xenografts. Proceedings of the American Association of Cancer Research (2000) 41 (April 1-5) Abs 4405.
Chothia and Lesk. J. Mol. Biol. 196: 901-917 (1987).
Frank et al. Methods Enzymol. 154: 221-249 (1984)
Gait,M.J., Oligonucleotide Synthesis. A Practical Approach. IRL Press, Oxford, UK (1984).
Goldmacher et al., J Immunol 135: 3648-3651, 1985.
Goldmacher et al., J Cell Biol 102: 1312-1319, 1986.
Giissow D, Seemann G. Humanization of monoclonal antibodies. Methods Enzymol. 203: 99-121 (1991)
Guo YJ, Liu G, Wang X, Jin D, Wu M, Ma J, and Sy MS. Potential use of soluble CD44 in serum as indicator of tumor burden and metastasis in patients with gastric or colon cancer. Cancer Res 54 (2): 422-426, 1994.
Harlow L D. Antibodies. Cold Spring Harbor Lab.1988
Hayden et Mandecki. Gene synthesis by serial cloning of oligonucleotides. DNA 7(8): 571- 7 (1988).
Heider, K.-H., Hofmann, M., Horst, E., van den Berg, F., Ponta, H., Herrlich, P., and Pals, S.T. A human homologue of the rat metastasis-associated variant of CD44 is expressed in colorectal carcinomas and adenomatous polyps. J. Cell Biol. 120: 227-233 (1993).
Heider KH, Mulder JWR, Ostermann E,Susani S, Patzelt E, Pals ST, Adolf GRA. Splice variants of the cell surface glycoprotein CD44 associated with metastatic tumor cells are expressed in normal tissues of humans and cynomolgus monkeys. Eur. J. Cancer 31 A: 2385-2391, 1995.
Heider KH, Sproll M, Susani S, Patzelt E, Beaumier P, Ostermann O, Ahorn H, Adolf GRA. Characterization of a high affinity monoclonal antibody antibody specific for CD44v6 as candidate for immunotherapy of squamous cell carcinomas. Cancer Immunology Immunotherapy 43: 245-253, 1996.
Hofmann, M., Rudy, W., Zδller, M., Tόlg, C, Ponta, H., Herrlich P., and Gϋnthert, U.
CD44 splice variants confer metastatic behavior in rats: homologous sequences are expressed in human tumor cell lines. Cancer Res. 51: 5292-5297 (1991).
Johnson S, Bird R E. Construction of single-chain derivatives of monoclonal antibodies and their production in Escherichia coli. Methods Enzymol. 203: 88-98 (1991).
Kabat E. A., Wu T. T., Perry H. M., Gottesman K. S. and Foeller C. Sequences of Proteins of Immunological Interest (5th Ed.). NIH Publication No. 91-3242. U.S. Department of Health and Human Services, Public Health Service, National Institutes of Health, Bethesda, MD (1991).
Klotz et al, Arch. Biochem. Biophys. 96: 605 (1962).
Koopman, G., Heider, K.-H., Horts, E., Adolf, G. R., van den Berg, F., Ponta, H., Herrlich, P., Pals, S. T. Activated human lymphocytes and aggressive Non-Hodgkin's lymphomas express a homologue of the rat metastasis-associated variant of CD44. J. Exp. Med. 177: 897-904 (1993).
Kreitman R J Hansen H J, Jones A L, FitzGerald D J P, Goldenberg D M, Pastan I. Pseu- domonas exotoxin-based immunotoxins containing the antibody LL2 or LL2-Fab' induce regression of subcutaneous human B-cell lymphoma in mice. Cancer Res. 53: 819-825 (1993).
Lambert et al, Biochem. 22: 3913-3920 (1983).
Lambert JM, Derr SM, Cook S, Braman G, Widdison W, Chari RVJ. Pharmacokinetics, in vivo stability, and toxicity of the Tumor-activated prodrug, C242-DM1, a novel colorectal cancer agent. Proceedings of the American Association of Cancer Research (1998) 39: Abs 3550
Liu et al, Biochem. 18: 690 (1979), Blakey and Thorpe, Antibody, Immunoconjugates and Radiopharmaceuticals, 1: 1-16 (1988).
Liu C, Tadayoni BM, Bourret LA, Mattocks KM, Derr SM, Widdison WC, Kedersha NL, Ariniello PD, Goldmacher VS, Lambert JM, Blattler WA, Chari RVJ. Eradication of large colon tumor xenografts by targeted delivery of maytansinoids. Proc Natl Acad Sci USA 93: 8618-23, 1996.
Martin S, Jansen F, Bokelmann J, and Kolb H. Soluble CD44 splice variants in metastasizing human breast cancer, frit J Cancer 74 (4): 443-445, 1997.
Screaton, G.R., Bell, M.V., Jackson, D.G., Cornells, F.B., Gerth, U., and Bell, J. I. Geno- mic structure of DNA encoding the lymphocyte homing receptor CD44 reveals at least 12 alternatively spliced exons. Proc. Natl. Acad. Sci. U.S.A. 89: 12160-12164 (1992).
Shin S-U, Morrison S L. Production and properties of chimeric antibody molecules. Methods Enzymol. 178: 459-476 (1989).
Sliutz G, Tempfer C, Winkler S, Kohlberger P, Reinthaller A, and Kainz C. Immunohistochemical and serological evaluation of CD44 splice variants in human ovarian cancer. Br.J.Cancer 72: 1494-1497 (1995).
Stemmer et al. Single-step assembly of a gene and entire plasmid from large numbers of oligodeoxyribonucleotides, Gene 164(1): 49-53 (1995).
Sfroomer JW, Roos JC, Sproll M, Quak JJ, Heider KH, Wilhelm BJ, Castelijns JA, Meyer R, Kwakkelstein MO, Snow GB, Adolf GR, van Dongen GA. Safety and biodistribution of 99mTechnetium-labeled anti-CD44v6 monoclonal antibody BIWA 1 in head and neck cancer patients. Clin Cancer Res 6 (8):3046-55, 2000
Tδlg, C, Hofmann, M., Herrlich, P., and Ponta, H. Splicing choice from ten variant exons establishes CD44 variability. Nucleic Acids. Res. 21: 1225-1229 (1993).
Tolcher AW et al. SB-408075, a maytansinoid immunoconjugate directed to the C242 antigen: a phase I pharmacokinetic and biologic correlative study. Poster presented at 11th Symp. on new drugs in cancer therapy (Nov 7-10, 2000 in Amsterdam).
Urlaub and Chasin. Proc. Natl. Acad. Sci. U.S.A. 77(7): 4216-20 (1980)
Urlaub et al., Cell 33: 405-412 (1983)
Verel I, Heider KH, Siegmund M, Ostermann E, Patzelt E, Sproll M, Snow GB, Adolf GR, van Dongen GMS. Tumor targeting properties of monoclonal antibodies with different affinity for target antigen CD44v6 in nude mice bearing head-and-neck cancer xenografts. Int. J. Cancer 99: 396-402 (2002).
Winter, G., Griffith, A. D., Hawkins, R. E., Hoogenboom, H. R. Making antibodies by phage display technology. Ann. Rev. Immunol. 12: 433-455 (1994).
Worrell et al, Anti-Cancer Drug Design 1: 179-184 (1986).
Ye et al. Gene synthesis and expression in E. coli for pump, a human matrix metalloproteinase. Biochem Biophys Res Commun 186(1): 143-9 (1992).
Examples
1. Material and Methods
1.1. In vitro cell proliferation assay
For determination of viable cells the Cell Titer 96® AQueous non-radioactive cell proliferation assay (Promega) was used. 5000 cells per well were seeded into 96-well plates in 90 μl medium without phenole red. Cells were allowed to settle down for 1 to 3 h and then serial dilutions of the immunoconjugate in 10 μl PBS were added. Cells without immunoconjugate served as negative control. Cells were incubated for 4 days at 37°C in a humified 5% CO2 atmosphere and then 20 μl MTS/ PMS were added according to the manufacturer's recommendation. After additional 1 to 4 h incubation at 37°C the absorbance at 490 nm was recorded using an ELISA plate reader. For each cell line triplicates were analyzed. The percentage of the surviving cell fraction and the IC50 value were calculated using the GraphPad Prism® (Version 3.0) software.
1.2. Manufacturing of BI I 1
Humanised recombinant antibodies BIWA 4 and BIWA 8 which have binding specificity for an epitope within SEQ ED NO: 1 were linked to the maytansinoid DM1 as described below. The conjugate of BIWA 4 with DM1 was designated BIWI 1.
Generation of stably transfected cell lines. The genes coding for the light and heavy chains of BIWA 4, SEQ ID NO: 5 and SEQ ID NO: 7, were ligated into expression vector pAD-CMVl (WO92/01055; NCBI GenBank Accession No. A32111) or pAD-CMV19 (NCBI GenBank Accession No. A32110). In the second antibody BIWA 8, the light chain was coded by a gene having SEQ ED NO: 9, while the heavy chain was the same as in BEWA 4. Stably transfected cell lines were generated by electroporation as follows. CHO DUX/57ss (dhfr negative mutant of Chinese Hamster Ovary cells, adapted for serum free suspension culture) were used. After tr psinisation and inactivation of trypsin with RPMI- 10 (90% RPMI 1640, 10% heat inactivated fetal calf serum), cells were washed once with RPMI-0 (RPMI 1640 without serum), and lxlO7 cells were resuspended in 0.8 ml PJ>MI-0. After addition of the linearised DNA (20 μg per plasmid; cotransfection of vectors coding
for light and heavy chain) the cells were electroporated using a Hoefer Electroporator under the following conditions: 1080 μF, 320 V, 1000 msec, 1 pulse. Cells were allowed to stand for 5 min, and were then diluted to 12500 cells/ml and 2500 cells/ml in alfa-MEM lOd (90% MEM alfa without ribonucleosides and without desoxyribonucleosides (GEBCO BRL), 10% heat inactivated dialysed fetal calf serum). The cells were seeded into 96 well microtiter plates (200 μl/well, corresponding to 2500 and 500 cells/well respectively). Clones appeared after 10 days. Only the plates with 500 cells/well were followed up (3-6 clones/well). After 14-15 days, supematants from each well were tested in a κ/γ ELISA. 53 clones were seeded in 12 well plates in alfa-MEM lOd. After 3-6 days (depending on the confluency of the cells) supematants were tested again in the κ/γ ELISA (serial dilutions) and quantitated using a human IgGl standard. Cells were frozen and stored in liquid nitrogen. IgG contents of the 53 clones ranged from 12 - 417 ng/ml. 10 clones with the highest expression level were selected and subcloned as follows: Cells of each clone were seeded into 96 well microtiter plates with densities of 1 and 5 cells/well in lOOμl/well alfa- MEM lOd (1 plate for each clone and each density). 8 days later supematants were diluted 1 :2 and 100 μl of this dilution tested in the κ γ ELISA and quantitated using a BIWA 4 preparation as standard. 5 subclones of each clone were transferred to 12 well plates. The IgG content ranged from 1.3 - 908 ng/ml. 14 clones with the highest expression level (384 - 908 ng/ml) were used for amplification with methofrexate as follows: Clones were initially cultured in 25 cm2 flasks containing alfa-MEM lOd with 20, 50 and 100 nM methofrexate. After the outgrowth of clones the supematants were tested in the κ/γ ELISA. In subsequent rounds of amplification the methofrexate concentration was raised up to 2000 nM. Initially the highest expression level ranged from 10.5-14.8 μg/ml (clone A31/100, 100 nM methofrexate). Further amplification with a methofrexate concentration of 500 nM gave an expression of 19-20 μg/ml (A31/500).
Purification of antibody. Antibody was purified from cell culture supernatant as follows. Antibody containing tissue culture supernatant was applied onto a 5 ml protein A sepharose column with a flow rate of 80-90 ml/h at 4 °C. After washing with 50 ml binding buffer (0.1 M sodium phosphate pH 7.5), the Ig fraction was eluted with elution buffer (0.1 M glycine-HCl pH 2.7). Absorption at 280 nm was monitored.
Modification of BIWA 4 with SPP to form BIWA 4-SS-Py. BIWA 4 was supplied in liquid form at a concentration of 5 mg/mL in a PBS formulation containing Tween 20. Prior to coupling of DM1 to the MAb the Tween 20 was removed. The MAb solution (40 mL) was diluted 15-fold with 25 mM MES buffer, pH 5.6, containing 50 mM NaCl (MES buffer) and then loaded onto a column (12.5 mL) of Sepharose S equilibrated in MES buffer (flow rate: 100 cm/hr). The column was washed with 10 column volumes of MES buffer. The antibody was eluted with MES buffer containing 400 mM NaCl. The antibody solution was dialysed against 50 mM potassium phosphate buffer, pH 6.5 containing 50 mM NaCl and 2 mM EDTA (Buffer A).The BIWA 4 antibody was modified using SPP ((2-Pyridyl)-5-dithiopentanoic acid N-hydroxy succinimid ester) to introduce dithiopyridyl groups. The MAb in Buffer A (185 mg, 8 mg/mL) was modified with a 7-fold molar excess of SPP in EtOH (5% v/v of MAb solution). The reaction proceeded for 90 minutes at ambient temperature. The reaction mixture was then subjected to gel filtration chromatography through Sephadex G25F (2.6 x 31.5 cm column, 167 mL) equilibrated in Buffer A. MAb-containing fractions were pooled and the degree of modification was determined by measuring the absorbance at 280 nm and the change in absorbance at 343 nm caused by the release of 2-mercaptopyridine by the addition of DTT. The concentration of released 2-mercaptopyridine was calculated using an ε343 nm of 8080 M^cm"1, and the concentration of MAb was calculated using an ε28onrn of 224,000 M^cm"1 after the absorbance at 280 nm has been corrected for the contribution from 2-mercaptopyridine. (2- mercaptopyridine A28onm = A343 nrn x 5100/8080). Recovery of the MAb was 99.6% with 5.5 releasable 2-mercaptopyridine groups linked per MAb molecule.
Conjugation of BIWA 4-SS-Py with DM1. The above modified MAb (184 mg) in Buffer A was conjugated at 2.5 mg MAb/mL using a 1.7-fold molar excess of DM1 over releasable 2-mercaptopyridine groups. DM1 was added in DMA (3% v/v of MAb solution) and the reaction mixture was incubated at ambient temperature for 29 hours. The conjugate was then isolated by gel filtration chromatography on a column of Sephacryl S300 EIR equilibrated in PBS (5 x 50 cm column, 980 mL, flow rate of 10 cm hr). The conjugate eluted as a single peak at the position of monomeric MAb with a small amount of protein eluting earlier. Fractions were assayed for the number of DM1 molecules linked per MAb molecule. (Linked DM1 molecules were determined by measuring the absorbance at both 252 nm and 280 nm). Based on the results, fractions representing 63-77% of the
column volume were pooled. The DM1 /MAb ratio in the pooled solution was found to be 3.1 and the yield of conjugated B WA 4 was 75% based on starting MAb. The conjugate, BIWI 1, was evaluated by SDS-PAGE performed under non-reducing conditions and found to be composed primarily of a monomer species (>95%) with a minor amount (<5%) of dimeric conjugate.
Analysis of in vitro binding of BIWI 1. The binding of BIWA 4 antibody and BIWI 1 conjugate to antigen-positive FaDu cells was determined. Cells (1-2 x 10"5) were incubated in 96-well plates with varying concentrations of antibody or conjugate on ice for 1 hour. The test article was washed from the plate and FITC-labeled anti-human IgG was added and the incubation on ice was continued in the dark for 1 hour. After washing, the cells were fixed with 1% paraformaldehyde and analyzed on a fluorescence activated cell sorter (FACS). BIWA 4 antibody binds with an apparent KD of 1 x 10"9 M and BIWI 1 binds with an apparent KD of 1.8 X 10"9 M. Thus, conjugation with DM1 alters the binding affinity of the antibody only slightly if at all.
1.3. Efficacy studies in nude mice
In vivo anti-tumor efficacy of BIWI 1 was tested in two nude mouse xenograft models applying antigen-positive human tumors, which differed in tumor origin, extent and homogeneity of CD44v6 expression: A431 (ATCC # CRL 1555; epidermoid carcinoma of the vulva), FaDu (ATCC # HTB 43; squamous cell carcinoma of the pharynx). Tumor cell lines A431 and FaDu were received from ATCC and cultured in RPMI 1640 medium containing 10% fetal calf serum and supplements.
Mice were randomised into the following treatment groups (treatment initial mean tumour volume/tumour volume range/number of mice):
A431
Group 1 : Control (PBS)/ 185 ± 217 mm3 / 19 - 424 mm3 / 5 mice.
Group 2: BIWA 4 (21 mg/kg/d) / 133 ± 115 mm3 / 42 - 302 mm3 / 5 mice.
Group 3 : BIWI 1 (2.1 mg/kg/d) / 107 ± 63 mm3 / 42 - 205 mm3 / 5 mice.
Group 4: BIWI 1 (7 mg/kg/d) / 132 ± 73 mm3 / 42 - 205 mm3 / 5 mice.
Group 5: BIWI 1 (21 mg/kg/d) / 107 ± 63 mm3 / 42 - 205 mm3 / 5 mice.
FaDu
Group 1 : Control (PBS)/ 142 ± 82 mm3 / 34 - 268 mm3 / 8 mice.
Group 2: BIWA 4 (21 mg/kg/d) / 134 ± 86 mm3 / 42 - 268 mm3 / 6 mice.
Group 3: BIWI 1 (2.1 mg/kg/d) / 149 ± 96 mm3 / 50 - 268 mm3 / 6 mice.
Group 4: BIWI 1 (7 mg/kg/d) / 132 ± 97 mm3 / 42 - 268 mm3 / 6 mice.
Group 5: BIWI 1 (21 mg/kg/d) / 129 ± 74 mm3 / 50 - 231 mm3 / 6 mice.
lxlO6 tumors cells were transplanted subcutaneously into the right flank of 6 week old female NMRI-nu nu mice. Treatment started when the tumors reached an average size of 107 to 185 mm3. Treatment consisted of i.v. injections of BIWI 1 given on five consecutive days, starting at day 1. 3 different doses of BEWI 1 were tested in parallel: 2.1 mg/kg/d BIWI 1 corresponding to 30 μg/kg/d DM1, 7 mg/kg/d BIWI 1 corresponding to 100 μg/kg/d DM1, and 21 mg/kg/d BIWI 1 coπesponding to 300 μg/kg/d DM1. Control animals were either untreated (PBS) or treated with unconjugated antibody (control antibody, 21 mg/kg/d). Tumor growth was monitored by measuring tumor size. A tumor response was rated as complete response when the tumor completely disappeared at any time after start of treatment. The response was rated as partial response when the tumor volume decreased after treatment but thereafter started regrowing. The tolerability of the treatment was monitored by measuring mouse weight during the whole observation period.
2. Results and Discussion
2.1. In vitro cytotoxicity of BIWI 1
The in vitro cytotoxicity of BIWI 1 was evaluated using the antigen-positive cell lines A431 and FaDu, and the antigen-negative cell line A459. Cells were exposed to different concentrations of BIWI 1 for 4 days, then stained with MTS/ PMS and assayed on an ELISA plate reader. The surviving fractions of cells were then calculated using the GraphPad Prism® software package. The results are shown in Figure 1. BIWI 1 was
effective in killing the antigen-positive A431 cells with an IC50 of about 7.6 x 10*8 M and the second antigen-positive cell line, FaDu, with an IC50 of about 2.4 x 10" M. The antigen-negative cell line, A549, was effected by the conjugate with an IC50 of about 1.3 x 10"7 M with a surviving fraction of 50% at the highest concentration of BIWI 1 tested (5 x 10"7 M). These results show that BIWI 1 is only slightly more cytotoxic against antigen- positive cells than antigen-negative cells in vitro. For comparison, another DM1 -antibody conjugate has been shown to be at least lOOOfold more cytotoxic against antigen-positive cell as compared to antigen-negative cells (Chari et al, 1992).
2.2. Efficacy in A431 xenografted nude mice
Groups of 5 mice were treated with 2.1 mg/kg/d BIWI 1, 7 mg/kg/d BIWI 1, 21 mg/kg/d BIWE 1, and 21 mg/kg/d control antibody, respectively. The average tumor size at start of treatment was 185 +/- 217 mm3 (PBS), 133 +/- 115 mm3 (control antibody), 107 +/- 63 mm3 (21 mg/kg/d BIWI 1), 132 +/- 73 mm3 (7 mg/kg/d BEWI 1), and 107 +/- 63 mm3 (2.1 mg/kg/d BEWI 1), respectively. The average tumor volume of each group during the observation period is shown in Figure 2. Tumors treated with control antibody showed similar growth as untreated tumors, the tumor volume doubling time was approximately 5 days. En animals treated either with 7 mg/kg/d BEWI 1 or 21 mg/kg/d BIWI 1 all tumors responded completely and disappeared around day 17. No tumor regrowth was observed until the end of the observation period (day 134). Tumors treated with 2.1 mg/kg/d responded completely in 3/5 cases with no tumor regrowth until day 134. The remaining 2 tumors showed a partial response but ultimately regrew. These results show that BIWI 1 induces a dose-dependent anti-tumor response in A431 xenografted nude mice, with complete and long-lasting responses from 2.1 mg/kg/d BIWI 1 to 21 mg/kg/d BIWI 1. Unconjugated control antibody shows no anti-tumor effect.
See Figure 2.
2.2. Efficacy in FaDu xenografted nude mice
Groups of 6 mice were treated with 2.1 mg/kg/d BIWI 1, 7 mg/kg/d BIWI 1, 21 mg/kg/d BIWI 1, and 21 mg/kg/d control antibody, respectively. The average tumor size at start of treatment was 142 +/- 82 mm3 (PBS), 134 +/- 86 mm3 (control antibody), 129 +/- 74 mm3 (21 mg/kg/d BIWI 1), 132 +/- 97 mm3 (7 mg/kg/d BIWI 1), and 149 +/- 96 mm3 (2.1 mg/kg/d BIWI 1), respectively. The average tumor volume of each group during the observation period is shown in Figure 3. Tumors treated with control antibody and 2.1 mg/kg/d BIWI 1 showed similar growth as untreated tumors, the tumor volume doubling time was approximately 5 days. In animals treated with 21 mg/kg/d BIWI 1 all tumors responded completely and disappeared around day 24. No tumor regrowth was observed until the end of the observation period (day 107). 1/6 tumors treated with 7 mg/kg/d BIWI 1 responded completely, 3/6 tumors showed partial responses. The remaining 2 tumors grew similar to untreated control tumors. These results show that BIWI 1 induces a dose- dependent anti -tumor response in FaDu xenografted nude mice, with complete and long- lasting responses from 7 mg/kg/d BIWI 1 to 21 mg/kg/d BIWI 1. Unconjugated control antibody shows no anti-tumor effect.
See Figure 3.
2.4. Tolerability in nude mice
The tolerability of BIWI 1 treatment was determined by monitoring mouse weight during the whole duration of the experiment in the 2 models. The maximum observed average weight loss per group was 5% in FaDu xenografted mice treated with 21 mg/kg/d BIWI 1 (Figure 4). The weight loss started around day 3 of treatment and lasted until day 10, thereafter animals regained weight and behaved similar as control animals. En all other dose groups weight loss was similar to vehicle control (PBS). An average weight loss of 5% or less in all treatment groups indicates good tolerability of BIWI 1 treatment at the given doses in nude mice. As BIWI 1 does not cross-react with mouse CD44v6, only antigen- independent effects such as toxicity caused by free DM1 can be monitored in this experiment.
3. In vivo anti-tumor efficacy in MDA-MB 453
3.1. Material and Methods
In vivo anti-tumor efficacy of BIWI 1 was tested in a nude mouse xenograft model applying the antigen-positive human tumor MDA-MB 453 (ATCC # HTB-131; breast carcinoma). The cells were received from ATCC and cultured in RPMI1640 medium containing 10% fetal calf serum and supplements. lxlO6 tumors cells were transplanted subcutaneously into the right flank of 6 week old female NMRI-nu/nu mice. For therapy experiments tumors were maintained via passaging of tumor fragments. Treatment started when the tumors reached an average size of 188 to 246 mm3. Treatment consisted of i.v. injections of BEWI 1 given weekly for four weeks. 3 different doses of BIWI 1 were tested in parallel: 6.25 mg/kg BIWI 1 corresponding to 100 μg/kg DM1, 12.5 mg/kg BIWI 1 corresponding to 200 μg/kg DM1, and 25 mg/kg BIWI 1 corresponding to 400 μg/kg DM1. PBS treated animals served as tumor growth control. Tumor growth was monitored by measuring tumor size. A tumor response was rated as complete response when the tumor completely disappeared at any time after start of treatment.
3.2. Results and Discussion
Groups of 6 mice were treated with 6.25 mg/kg BIWI 1, 12.5 mg/kg BIWI 1, and 25 mg/kg BIWI 1, respectively, once a week for four weeks. The average tumor size at start of treatment was 246 +/- 79 mm3 (PBS), 216 +/- 85 mm3 (6.25 mg/kg BIWI 1), 188 +/- 79 mm3 (12.5 mg/kg BIWI 1), and 207 +/- 96 mm3 (25 mg/kg BIWI 1), respectively. The average tumor volume of each group during the observation period is shown in Figure 5. The initial tumor volume doubling time of the control tumors was approximately 5 days. In animals treated with 25 mg/kg BEWI 1 all tumors responded completely and disappeared around day 22 after start of treatment. No tumor regrowth was observed until the end of the observation period (day 64). Tumors treated with 12.5 mg/kg or 6.25 mg/kg responded completely in 5/6 cases in each dose group, and 4 animals of each group stayed tumor free until the end of the experiment. These results show that BIWI 1 induces excellent anti- tumor responses in MDA-MB 453 xenografted nude mice when given once a week over a
period of four weeks, with complete and long-lasting responses from 6.25 mg/kg BIWI 1 to 25 mg/kg BIWI 1.
Figures
Figure 1: in vitro cytotoxicity of BIWI 1. The antigen-positive cell lines A431 and FaDu and the antigen-negative cell line A549 were used.
Figure 2: Efficacy of BIWI 1 treatment in nude mice xenografted with A431 tumors. The average tumor volumes per group with standard deviations are shown, the treatment groups are indicated. The arrow indicates start of freatment (day 1).
Figure 3: Efficacy of BIWI 1 treatment in nude mice xenografted with FaDu tumors. The average tumor volumes per group with standard deviations are shown, the treatment groups are indicated. The arrow indicates start of treatment (day 1).
Figure 4: Tolerability of BIWI 1 treatment. The average body weight change of all treatment groups in the 2 investigated models is shown. Day 1: start of treatment.
Figure 5: Efficacy of BIWI 1 treatment in nude mice xenografted with MDA-MB 453 tumors. The average tumor volumes per group with standard deviations are shown, the treatment groups are indicated. The arrows indicate the treatment days .
Claims (37)
1. A compound of formula A(LB)n wherein
A is an antibody molecule which is specific for CD44; L is a linker moiety;
B is a compound which is toxic to cells; and n is an decimal number with n = 1 to 10.
2. The compound of claim 1 wherein said linker moiety has a chemical bond capable of being cleaved inside a cell.
3. The compound of claim 2 wherein said chemical bond is a disulfide bond.
4. The compound of claims 1 to 3, wherein the antibody molecule is specific for the exon v6 of human CD44.
5. The compound of claims 1 to 4, wherein the antibody molecule is specific for an epitope within the amino acid sequence SEQ ED NO: 3.
6. The compound of claims 1 to 5, wherein the antibody molecule is the monoclonal antibody VFF-18 (DSM ACC2174) or a recombinant antibody having the complementary determining regions (CDRs) of VFF-18.
7. The compoimd of claims 1 to 6, wherein the antibody molecule comprises light chains having the amino acid sequence SEQ ID NO: 4, or SEQ ID NO: 8, and heavy chains having the amino acid sequence SEQ ED NO: 6.
8. The compound of claims 1 to 7, wherein the toxic compound B is a maytansinoid.
9. The compound of claim 8 wherein the maytansinoid has the formula
wherein represents H or SR4, wherein R represents methyl, ethyl, linear alkyl, branched alkyl, cyclic alkyl, simple or substituted aryl, or heterocychc;
R2 represents Cl or H; R3 represents H or CH3; and m represents 1, 2, or 3.
10. The compound of claim 9, wherein R\ is H or CH3, R2 is Cl, R3 is CH3, and m = 2.
11. The compound of claims 1 to 10 of formula
(Formula III) wherein A is an antibody molecule which is specific for CD44, (L') is an optional linker moiety p is a decimal number with p = 1 to 10.
12. The compound of claims 1 to 11 wherein p is 3 to 4.
13. A conjugate of a CD44v6 specific antibody molecule and a maytansinoid.
14. The conjugate of claim 13, wherein the antibody molecule is specific for an epitope within the amino acid sequence SEQ ID NO: 3.
15. The conjugate of claim 14, wherein the antibody molecule is the monoclonal antibody VFF-18 (DSM ACC2174) or a recombinant antibody having the complementary determining regions (CDRs) of VFF-18.
16. The conjugate of any one of claims 13 to 15, wherein said antibody molecule comprises light chains having the amino acid sequence SEQ ED NO: 4, or SEQ ED NO: 8, and heavy chains having the amino acid sequence SEQ ED NO: 6.
17. The conjugate of any one of claims 13 to 16, wherein the maytansinoid is linked to the antibody molecule by a disulfide moiety.
18. The conjugate of any one of claims 13 to 17, wherein the maytansinoid has the formula
Formula (IV)
19. A conjugate of a CD44v6 specific antibody molecule and a maytansinoid, wherein the antibody comprises light chains having the amino acid sequence SEQ ID NO: 4, and heavy chains having the amino acid sequence SEQ ED NO: 6, and wherein the maytansinoid has the formula
(Formula IV)
and is linked to the antibody through a disulfide bond.
20. The conjugate of any one of claims 13 to 19, wherein one or more maytansinoid residues are linked to an antibody molecule.
21. The conjugate of claim 20, wherein 3 to 4 maytansinoid residues are linked to an antibody molecule.
22. The conjugate of any one of claims 13 to 21, wherein the maytansinoid is linked to the antibody molecule through a -S-CH2CH2-CO-, a -S-CH2CH2CH2CH2-CO-, or a -S- CH(CH3)CH2CH2-CO- group.
23. Method of production of a compound A(LB)„ according to claims 1 to 12, or a conjugate according to claims 13 to 22, comprising the steps:
(a) introducing one ore more free or protected thiol groups into an antibody molecule which is specific for CD44;
(b) reacting the antibody molecule of step (a) with a compound which is toxic to cells, said compound having one or more disulfide or thiol groups; and
(c) recovering the resulting conjugate.
24. The method of claim 23, wherein the antibody molecule is specific for CD44v6.
25. The method of claim 24, wherein the antibody molecule is specific for an epitope within SEQ ID NO: 3.
26. The method of any one of claims 23 to 25, wherein the toxic compound is a maytansinoid.
27. The method of claim 26, wherein the maytansinoid has the formula
(Formula El)
wherein
R\ represents H or SR4, wherein j represents methyl, ethyl, linear alkyl, branched alkyl, cyclic alkyl, simple or substituted aryl, or heterocychc; R2 represents Cl or H; R3 represents H or CH3; and m represents 1, 2, or 3.
28. The method of claim 27, wherein R] is H or CH3, R2 is Cl, R3 is CH3, and m = 2.
29. The method of any one of claims 23 to 28, wherein (2-pyridyl)-3-dithiopropanoic acid N-hydroxy succinimid ester, (2-pyridyl)-4-dithiopentanoic acid N-hydroxy succinimid ester, or (2-pyridyl)-5-dithiopentanoic acid N-hydroxy succinimid ester is used to introduce the free or protected thiol groups into the antibody molecule.
30. Compound obtainable by a method according to any one of claims 23 to 29.
31. Pharmaceutical composition comprising a compound A(LB)„ according to claims 1 to 12, or 30, or a conjugate according to claims 13 to 22, and a pharmaceutically acceptable carrier, diluent, or excipient.
32. Use of a compound A(LB)„ according to claims 1 to 12, or 30, or a conjugate according to claims 13 to 22, for the preparation of a pharmaceutical composition for the treatment of cancer.
33. The use of claim 32, wherein the cancer is head and neck squameous cell carcinoma, esophagus squameous cell carcinoma, lung squameous cell carcinoma, skin squameous cell carcinoma, cervix squameous cell carcinoma, breast adenocarcinoma, lung adenocarcinoma, pancreas adenocarcinoma, colon adenocarcinoma, or stomach adenocarcinoma.
34. Use of a compound A(LB)n according to claims 1 to 12, or 30, or a conjugate according to claims 13 to 22, or of a pharmaceutical composition according to claim 31, for the treatment of cancer.
35. The use according to claim 34, wherein the cancer is head and neck squameous cell carcinoma, esophagus squameous cell carcinoma, lung squameous cell carcinoma, skin squameous cell carcinoma, cervix squameous cell carcinoma, breast adenocarcinoma, lung adenocarcinoma, pancreas adenocarcinoma, colon adenocarcinoma, or stomach adenocarcinoma.
36. Method of freatment of cancer in a patient in need thereof comprising administering to the patient a therapeutically effective amount of a compound A(LB)n according to any one of claims 1 to 12, or 30, or a conjugate according to claims 13 to 22, or a pharmaceutical composition according to claim 31.
37. The method of claim 36, wherein the cancer is head and neck squameous cell carcinoma, esophagus squameous cell carcinoma, lung squameous cell carcinoma, skin squameous cell carcinoma, cervix squameous cell carcinoma, breast adenocarcinoma, lung adenocarcinoma, pancreas adenocarcinoma, colon adenocarcinoma, or stomach adenocarcinoma.
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| EP01112227.2 | 2001-05-18 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| AU2002313471A1 true AU2002313471A1 (en) | 2002-12-03 |
Family
ID=
Similar Documents
| Publication | Publication Date | Title |
|---|---|---|
| US7361347B2 (en) | Cytotoxic CD44 antibody immunoconjugates | |
| EP1395290A2 (en) | Cytotoxic cd44 antibody immunoconjugates | |
| EP1391213A1 (en) | Compositions and methods for treating cancer using maytansinoid CD44 antibody immunoconjugates and chemotherapeutic agents | |
| US20050244413A1 (en) | Compositions and methods for treating cancer using cytotoxic CD44 antibody immunoconjugates and chemotherapeutic agents | |
| EP1806365A1 (en) | Antibody molecules specific for fibroblast activation protein and immunoconjugates containing them | |
| KR101529810B1 (en) | Antibody-drug conjugates | |
| US20130280282A1 (en) | Dr5 ligand drug conjugates | |
| US20110070248A1 (en) | Dr5 ligand drug conjugates | |
| CN116528911A (en) | anti-CD 73 antibody, antibody-conjugated drug and application thereof | |
| KR20230158004A (en) | Antibody immune agent conjugates and their applications | |
| EP1045861B1 (en) | Bispecific targeting moiety comprising an antibody to carcinoembryonic antigen (cea) and the ligand-binding region of the il13 receptor alpha subunit | |
| CN111295201A (en) | anti-EGFR Antibody Drug Conjugates (ADCs) and uses thereof | |
| US20040120949A1 (en) | Compositions and methods for treating cancer using cytotoxic CD44 antibody immunoconjugates and radiotherapy | |
| JP2024517776A (en) | Antibody-drug conjugates targeting nectin-4 and methods for preparing and using same | |
| EP1417974A1 (en) | Compositions and methods for treating cancer using cytotoxic CD44 antibody immunoconjugates and radiotherapy | |
| AU2002313471A1 (en) | Cytotoxic CD44 antibody immunoconjugates | |
| JP2022552349A (en) | B-lymphocyte-specific amatoxin antibody conjugates | |
| WO2023190827A1 (en) | Ph-dependent anti-sulfated glycosaminoglycan antibody and antibody-drug conjugate | |
| WO2024193605A1 (en) | Ror1-targeting antibody, antibody-drug conjugate comprising same, preparation method therefor, and use thereof |