In one embodiment, the present invention relates to multispecific antigen-binding molecules capable of inducing phagocytosis of target cells by antigen-presenting cells through crosslinking antigen-presenting cells to target cells. For example, the present invention relates to bispecific antibodies capable of inducing phagocytosis of target cells by antigen-presenting cells through crosslinking antigen-presenting cells to target cells.
The present invention also relates to compositions for inducing an antitumor immune response and compositions for treating or preventing cancer, which comprise such multispecific antigen-binding molecules. The present invention further relates to methods for treating or preventing cancer, comprising the step of administering such multispecific antigen binding molecules.
Antibodies are proteins which specifically bind to an antigen with high affinity. It is known that various molecules ranging from low-molecular compounds to proteins can be antigens. Since the technique for producing monoclonal antibodies was developed, antibody modification techniques have advanced, making it easy to obtain antibodies that recognize a particular molecule.
Antibodies are drawing attention as pharmaceuticals because they are highly stable in blood plasma and have less side effects. Not only do antibodies bind to an antigen and exhibit agonistic or antagonistic effects, but they also induce cytotoxic activity mediated by effector cells (also referred to as effector functions) including ADCC (Antibody Dependent Cytotoxicity), ADCP (Antibody Dependent Cell Phagocytosis), and CDC (Complement Dependent Cytotoxicity). Taking advantage of these antibody functions, pharmaceuticals for cancer, immune diseases, chronic disease, infections, etc. have been developed (Nat Rev Drug Discov. 2018 March; 17(3):197-223 (NPL 1)).
For example, cancer immunotherapy has received a great deal of attention in recent years in cancer treatment, and this is especially so for checkpoint inhibitor antibodies targeting PD-1/PD-L1 and CTLA-4 that are widely used clinically (NPL 2, NPL 3, and NPL 4). Checkpoint inhibitors elicit antitumor effects by activating immune cells. However, problems with checkpoint inhibitors include the risk of side effects due to activation of autoreactive immune cells and the limited number of patients in which they are effective. Therefore, there is a strong demand for the development of agents having fewer side effects which are capable of eliciting an antitumor effect of immune cells, or agents capable of efficiently increasing the effect of checkpoint inhibitors.
Antigen-presenting cells activate antigen-reactive T cells by processing phagocytosed antigens and then presenting them on their major histocompatibility complexes (MHCs). Antigen-reactive T cells are considered to be important for the efficacy of checkpoint inhibitors (NPL 5).
Dendritic cells are a type of typical antigen-presenting cells and can efficiently activate antigen-reactive T cells. Therefore, they are considered to play a very important role also in cancer immunotherapy (NPL 6).
As one of the cancer immunotherapies targeting dendritic cells, there is a method in which dendritic cells cultured ex vivo are allowed to phagocytose a cancer antigen and then transferred into the body to activate tumor-reactive T cells. This has already been approved as a treatment for prostate cancer (NPL 7). However, in this method, there are many conditions that have to be optimized to maximize the original function of dendritic cells, such as culture conditions and activation conditions of artificially induced dendritic cells, routes for transferring dendritic cells, etc., and thus, sufficient therapeutic effects still have not been obtained. Therefore, in recent years, as another endeavor, there is an attempt, which is being clinically evaluated, to conjugate a cancer antigen with an antibody that recognizes an antigen on dendritic cells and allow dendritic cells that naturally exist in the body to phagocytose these conjugates (NPL 8). However, it is suggested that reactive T cells activated by this method are only T cells corresponding to the antigen conjugated to the antibody, and that T cells that react to other cancer antigens cannot be activated (NPL 9).
In one embodiment, the present invention has been made in view of the above circumstances, and an objective thereof is to provide a novel cancer immunotherapy using antigen-presenting cells such as dendritic cells.
As a result of dedicated research to achieve the above objective, the present inventors crosslinked antigen-presenting cells to target cells using a multispecific antigen-binding molecule that recognizes an antigen on antigen-presenting cells and an antigen on target cells, and discovered that phagocytosis of target cells by antigen-presenting cells can be enhanced.
The present invention is based on such findings, and as examples, provides the following embodiments:
The present invention also provides the following as other examples:
Further, the present invention also provides the following as other examples:
Further, the present invention also provides the following as other examples:
In one embodiment, a multispecific antigen-binding molecule of the present invention can crosslink antigen-presenting cells such as dendritic cells to target cells to promote phagocytosis of target cells by the antigen-presenting cells.
Further, in one embodiment, a multispecific antigen-binding molecule of the present invention is capable of making antigen-presenting cells phagocytose target cells as they are without subjecting target cells to disruption, so that not only cell surface antigens of the target cells but also their intracellular antigens are presented by the antigen-presenting cells, enabling the presentation of a wide variety of antigens by antigen-presenting cells.
The following definitions are provided to facilitate understanding of the present invention described herein.
As one aspect of the present invention, a multispecific antigen binding molecule comprising a first antigen-binding domain that binds to a first antigen on an antigen-presenting cell and a second antigen-binding domain that binds to a second antigen on a target cell is provided. In one embodiment, the multispecific antigen-binding molecule can crosslink antigen-presenting cells such as dendritic cells to target cells, and promote phagocytosis of target cells by the antigen-presenting cells. In one embodiment, the antigen-presenting cells are capable of presenting to T cells multiple types of antigen peptides derived from target cells that have been engulfed by phagocytosis. As a result, for example, activation of CD8+ effector T cells (cytotoxic T cells) targeting multiple types of tumor antigens derived from target cells can be induced. Therefore, in one embodiment, by using the multispecific antigen-binding molecule, it is possible to provide a cancer treatment having a higher efficacy as compared to conventional cancer immunotherapy targeting a specific (typically one type of) tumor antigen. Moreover, in a specific embodiment, an antitumor effect is induced in a subject administered with the multispecific antigen-binding molecule.
In the present invention, the term “antigen-binding molecule” is used in the broadest sense indicating a molecule comprising an antigen-binding domain; and specifically, it includes various types of molecules as long as they show antigen-binding activity. Molecules in which an antigen-binding domain is linked to an FcRn-binding domain include, for example, antibodies. Antibodies may include single monoclonal antibodies (including agonistic antibodies and antagonistic antibodies), human antibodies, humanized antibodies, chimeric antibodies, and such. Alternatively, when used as antibody fragments, they preferably include antigen-binding domains and antigen-binding fragments (for example, Fab, F(ab′)2, scFv, and Fv). Scaffold molecules where three dimensional structures, such as already-known stable α/β barrel protein structure, are used as a scaffold (base) and only some portions of the structures are made into libraries to construct antigen-binding domains are also included in antigen-binding molecules of the present invention.
Herein, an “antigen-binding domain” may be of any structure as long as it binds to an antigen of interest. Such domains preferably include, for example:
In the present invention, the “antigen-binding molecule” is not particularly limited as long as the molecule comprises an “antigen-binding domain” of the present invention. The antigen-binding molecule may further comprise a peptide or a protein having a length of approximately 5 amino acids or more. The peptide or the protein is not limited to a peptide or a protein derived from an organism, and may be, for example, a polypeptide consisting of an artificially designed sequence. Also, a natural polypeptide, a synthetic polypeptide, a recombinant polypeptide, or the like may be used.
Preferred examples of the antigen-binding molecules of the present invention can include an antigen-binding molecule comprising an FcRn-binding domain comprised in an antibody Fc region. As method for extending the blood half-life of proteins administered in vivo, methods which add an antibody FcRn-binding domain to a protein of interest to use the FcRn-mediated recycling function are well known.
FcRn-binding domains of the present invention may be in particular either those with reduced binding activity toward an Fcγ receptor, or those having increased binding activity toward an Fcγ receptor. In this context, the Fcγ receptor (also referred to as FcγR or FcgR herein) refers to a receptor capable of binding to the Fc region of IgG1, IgG2, IgG3, or IgG4 and means any member of the family of proteins substantially encoded by Fcγ receptor genes. In humans, this family includes, but is not limited to: FcγRI (CD64) including isoforms FcγRIa, FcγRIb, and FcγRIc; FcγRII (CD32) including isoforms FcγRIIa (including allotypes H131 (H type) and R131 (R type)), FcγRIIb (including FcγRIIb-1 and FcγRIIb-2), and FcγRIIc; and FcγRIII (CD16) including isoforms FcγRIIIa (including allotypes V158 and F158) and FcγRIIIb (including allotypes FcγRIIIb-NA1 and FcγRIIIb-NA2); and any yet-to-be-discovered human FcγR or FcγR isoform or allotype. The FcγR includes those derived from humans, mice, rats, rabbits, and monkeys. The FcγR is not limited to these molecules and may be derived from any organism. The mouse FcγRs include, but are not limited to, FcγRI (CD64), FcγRII (CD32), FcγRIII (CD16), and FcγRIII-2 (CD16-2), and any yet-to-be-discovered mouse FcγR or FcγR isoform or allotype. Preferred examples of such Fcγ receptors include human FcγRI (CD64), FcγRIIa (CD32), FcγRIIb (CD32), FcγRIIIa (CD16), and/or FcγRIIIb (CD16).
Reduced binding activity against an Fcγ receptor can be confirmed by a well-known method such as FACS, ELISA format, ALPHAScreen (amplified luminescent proximity homogeneous assay screen), or the BIACORE method based on a surface plasmon resonance (SPR) phenomenon (Proc. Natl. Acad. Sci. USA (2006) 103 (11), 4005-4010).
A “first antigen-binding domain that binds to a first antigen on an antigen-presenting cell” and a “second antigen-binding domain that binds to a second antigen on a target cell” (hereinafter, these binding domains are collectively referred to as antigen binding domains) contained in a multispecific antigen-binding molecule of the present invention mean a region that specifically binds to the respective antigen, which is a first antigen on an antigen presenting cell, or a second antigen on a target cell. Examples of the binding domains include a region containing an antigen-binding region of an antibody. When selecting a first antigen on the antigen-presenting cell and a second antigen on the target cell to which a multispecific antigen-binding molecule of the present invention binds, the antigens are selected to be mutually different. When the molecular weight of an antigen is large, the antigen-binding region of the antibody can only bind to a specific part of the antigen. The specific part is called an epitope. The antigen binding domains may be provided by one or more antibody variable domains. In a preferred embodiment, the antigen binding domains comprise an antibody light chain variable region (VL) and an antibody heavy chain variable region (VH).
An “antigen-binding molecule” of the present invention may be an antibody fragment that contains both heavy and light chains forming the “antibody variable regions” of the present invention within a single polypeptide chain, but lacking the constant regions. Such antibody fragments may be, for example, Fv, Fab, Fab′, Fab′-SH, F(ab′)2; diabodies; linear antibodies; single-chain antibody molecules (for example, scFv (single chain Fv), sc(Fv)2, sc(Fab′)2); and single domain antibodies (e.g., VHH, VH, VL).
A “multispecific” antigen-binding molecule refers to an antigen-binding molecule having in the same molecule two or more variable regions that specifically recognize different epitopes. A preferred example of a multispecific antigen-binding molecule of the present invention is an antigen-binding molecule having in the same molecule two variable regions that specifically recognize different epitopes.
In the present invention, “specifically binds” means binding in a state where one of the molecules involved in specific binding does not show any significant binding to molecules other than a single or a number of binding partner molecules. Furthermore, it is also used when an antigen-binding domain is specific to a particular epitope among multiple epitopes contained in an antigen. When an epitope bound by an antigen-binding domain is contained in multiple different antigens, antigen-binding molecules comprising the antigen-binding domain can bind to various antigens that have the epitope.
Depending on a “first antigen on an antigen-presenting cell” to be targeted, one skilled in the art can appropriately select a heavy chain variable region and a light chain variable region that bind to the antigen as a heavy chain variable region and a light chain variable region contained in a “first antigen-binding domain that binds to a first antigen on an antigen-presenting cell” in a multispecific antigen-binding molecule of the present invention. Similarly, depending on a “second antigen on a target cell” to be targeted, one skilled in the art can appropriately select a heavy chain variable region and a light chain variable region that bind to the antigen as a heavy chain variable region and a light chain variable region contained in a “second antigen-binding domain that binds to a second antigen on a target cell” in a multispecific antigen-binding molecule of the present invention.
As examples of a “first antigen-binding domain that binds to a first antigen on an antigen-presenting cell” in a multispecific antigen-binding molecule of the present invention, the following can be given, but are not restricted thereto:
a CLEC9A-binding domain having:
As examples of a “second antigen-binding domain that binds to a second antigen on a target cell” in a multispecific antigen-binding molecule of the present invention, the following can be given, but are not restricted thereto:
a GPC3-binding domain having:
Antibody variable regions used to produce various binding domains of antigen-binding molecules described herein are generally formed by three complementarity-determining regions (CDRs) that are separated by four framework regions (FRs). CDRs are regions that substantially determine the binding specificity of an antibody. The amino acid sequences of CDRs are highly diverse. On the other hand, the amino acid sequences constituting FRs often have high identity even among antibodies with different binding specificities. Therefore, generally, the binding specificity of a given antibody can be transplanted to another antibody by CDR grafting.
In the present specification, the “first antigen on the antigen-presenting cell” may preferably be an antigen that is specifically expressed on the cell surface of an antigen-presenting cell, for example, an antigen that is specifically expressed on dendritic cells. In one embodiment, it is an antigen that is specifically expressed on the dendritic cell subset responsible for cross-presentation. Examples of antigens on dendritic cells include CD1a, CD1c, CD11b, CD11c, FcεR1, CD141, XCR1, IgE, CD14, CD163, CD123, BDCA-2, ChemR23, Clec9a, CD206, CD207, and CD209 (Front Immunol. 2014 Apr. 1; 5:131), and of these antigens on dendritic cells, those classified as C-type lectin receptors include DEC205, Dectin-1, Dectin-2, Mincle, CD206, CD207 (Langerin), CD209 (DC-SIGN), Clec9a (DNGR1), Clec10a (CD301, MGL), and Clec12a (J Leukoc Biol. 2017 October; 102(4): 1017-1034). However, antigens on dendritic cells are not necessarily limited to these.
In the present specification, the “second antigen on the target cell” may preferably be an antigen which is specifically expressed on the surface of a target cell. In the present specification, the “target cell” is not particularly limited as long as it is a cell that is phagocytosed by an antigen-presenting cell and cross-presented, and examples thereof include cancer cells, bacteria, and cells infected with viruses and the like. “Cancer-specific antigen” as a non-limiting example of an antigen on a target cell means an antigen expressed by a cancer cell, which enables distinguishing between a cancer cell and a healthy cell; for example, it includes antigens that are expressed as cells become malignant and abnormal sugar chains that appear on the cell surface or on protein molecules when the cells become cancerous. Specific examples thereof include ALK receptor (pleiotrophin receptor), pleiotrophin, KS 1/4 pancreatic cancer antigen, ovary cancer antigen (CA125), prostatic acid phosphate, prostate-specific antigen (PSA), melanoma-associated antigen p97, melanoma antigen gp75, high-molecular-weight melanoma antigen (HMW-MAA), prostate-specific membrane antigen, carcinoembryonic antigen (CEA), polymorphic epithelial mucin antigen, human milk fat globule antigen, colorectal tumor-associated antigen (e.g., CEA, TAG-72, C017-1A, GICA 19-9, CTA-1, and LEA), Burkitt's lymphoma antigen 38.13, CD19, human B lymphoma antigen CD20, CD33, melanoma-specific antigen (e.g., ganglioside GD2, ganglioside GD3, ganglioside GM2, and ganglioside GM3), tumor-specific transplantation antigen (TSTA), T antigen, virus-induced tumor antigen (e.g., envelope antigens of DNA tumor virus and RNA tumor virus), colon CEA, oncofetal antigen α-fetoprotein (e.g., oncofetal trophoblastic glycoprotein 5T4 and oncofetal bladder tumor antigen), differentiation antigen (e.g., human lung cancer antigens L6 and L20), fibrosarcoma antigen, human T cell leukemia-associated antigen Gp37, newborn glycoprotein, sphingolipid, breast cancer antigen (e.g., EGFR (epithelial growth factor receptor)), NY-BR-16, NY-BR-16 and HER2 antigen (p185HER2), polymorphic epithelial mucin (PEM), malignant human lymphocyte antigen APO-1, differentiation antigen such as I antigen found in fetal erythrocytes, primary endoderm I antigen found in adult erythrocytes, I (Ma) found in embryos before transplantation or gastric cancer, M18, M39 found in mammary gland epithelium, SSEA-1 found in bone marrow cells, VEP8, VEP9, Myl, VIM-D5, D156-22 found in colorectal cancer, TRA-1-85 (blood group H), SCP-1 found in testis and ovary cancers, C14 found in colon cancer, F3 found in lung cancer, AH6 found in gastric cancer, Y hapten, Ley found in embryonic cancer cells, TL5 (blood group A), EGF receptor found in A431 cells, E1 series (blood group B) found in pancreatic cancer, FC10.2 found in embryonic cancer cells, gastric cancer antigen, CO-514 (blood group Lea) found in adenocarcinoma, NS-10 found in adenocarcinoma, CO-43 (blood group Leb), G49 found in A431 cell EGF receptor, MH2 (blood group ALeb/Ley) found in colon cancer, 19.9 found in colon cancer, gastric cancer mucin, T5A7 found in bone marrow cells, R24 found in melanoma, 4.2, GD3, D1.1, OFA-1, GM2, OFA-2, GD2, and M1:22:25:8 found in embryonic cancer cells, SSEA-3 and SSEA-4 found in 4-cell to 8-cell embryos, cutaneous T cell lymphoma-associated antigen, MART-1 antigen, sialyl Tn (STn) antigen, colon cancer antigen NY-CO-45, lung cancer antigen NY-LU-12 variant A, adenocarcinoma antigen ART1, paraneoplastic associated brain-testis-cancer antigen (onconeuronal antigen MA2 and paraneoplastic neuronal antigen), neuro-oncological ventral antigen 2 (NOVA2), blood cell cancer antigen gene 520, tumor-associated antigen CO-029, tumor-associated antigen MAGE-C1 (cancer/testis antigen CT7), MAGE-B1 (MAGE-XP antigen), MAGE-B2 (DAM6), MAGE-2, MAGE-4a, MAGE-4b, MAGE-X2, cancer-testis antigen (NY-EOS-1), YKL-40, and any fragment of these polypeptides, and modified structures thereof (aforementioned modified phosphate groups, sugar chains, etc.), EpCAM, EREG, CA19-9, CA15-3, sialyl SSEA-1 (SLX), HER2, PSMA, CEA, and CLEC12A. As a cancer-specific antigen which is the binding target of a second antigen-binding domain contained in a multispecific antigen-binding molecule of the present invention, one that is expressed on the cell surface is particularly preferable, and such cancer-specific antigens include, for example, GPC3, IL6R, CD19, CD20, EGFR, HER2, EpCAM and EREG.
As one of the preferable embodiments of an “antigen-binding molecule” of the present invention, an antibody containing a variable region of an antibody of the present invention can be given.
Herein, “antibody” refers to a natural immunoglobulin or an immunoglobulin produced by partial or complete synthesis. Antibodies can be isolated from natural sources such as naturally-occurring plasma and serum, or culture supernatants of antibody-producing hybridomas. Alternatively, antibodies can be partially or completely synthesized using techniques such as genetic recombination. Preferred antibodies include, for example, antibodies of an immunoglobulin isotype or subclass belonging thereto. Known human immunoglobulins include antibodies of the following nine classes (isotypes): IgG1, IgG2, IgG3, IgG4, IgA1, IgA2, IgD, IgE, and IgM. Of these isotypes, antibodies of the present invention include IgG1, IgG2, IgG3, and IgG4.
Methods for producing an antibody with desired binding activity are known to those skilled in the art, and antibodies can be obtained as polyclonal or monoclonal antibodies. Antibodies of the present invention preferably produced are monoclonal antibodies derived from mammals. Such mammal-derived monoclonal antibodies include antibodies produced by hybridomas or host cells transformed with an expression vector carrying an antibody gene by genetic engineering techniques.
As antibodies, recombinant antibodies produced by gene recombination technology can be used. Recombinant antibodies are obtained by cloning DNA encoding the same from hybridoma or antibody-producing cells such as sensitized lymphocytes that produce antibodies, incorporating it into a vector, introducing this into a host (host cell), and causing production therein.
Bispecific antibodies are not limited to the IgG type, but for example, an IgG type bispecific antibody can be secreted by a hybrid hybridoma (quadroma) produced by fusing two kinds of hybridomas that produce IgG antibodies (Milstein C et al. Nature 1983, 305: 537-540). In addition, it can be secreted by introducing into cells genes of L chains and H chains constituting two types of IgGs of interest, a total of four types of genes, and coexpressing them.
Antibodies of the present invention can be generated by methods known to those skilled in the art. Specifically, a DNA encoding an antibody of interest is integrated into an expression vector. In this case, it is integrated into an expression vector so that it is expressed under the control of expression control regions, for example, an enhancer and a promoter. Next, host cells are transformed with this expression vector and allowed to express antibodies. When doing so, an appropriate combination of hosts and expression vectors can be used.
Antibodies of the present invention thus obtained can be isolated from the inside or outside (medium etc.) of the host cells and purified as substantially pure and homogeneous antibodies. Antibodies can be isolated and purified using isolation and purification methods conventionally used for antibody purification, without limitation. For example, antibodies can be isolated and purified by appropriately selecting and combining column chromatography, filtration, ultrafiltration, salting-out, solvent precipitation, solvent extraction, distillation, immunoprecipitation, SDS-polyacrylamide gel electrophoresis, isoelectric focusing, dialysis, recrystallization, and such.
As one of the preferred embodiments of the multispecific antigen-binding molecules of the present invention, a multispecific antibody can be given. As the multispecific antibody of the present invention, a bispecific antibody is particularly preferable.
For association by which multispecific antibodies are formed, a technique that can be used is to suppress the unintended association between H chains by introducing electric charge repulsion to the interface between the second constant regions (CH2) or the third constant regions (CH3) of the antibody H chains (WO2006/106905).
An alternative technique known in the art can also be used for the association to form the multispecific antibodies of the present invention. An amino acid side chain present in the variable domain of one of the antibody H chains is substituted by a larger side chain (knob), and its partner amino acid side chain present in the variable domain of the other H chain is substituted by a smaller side chain (hole) such that the knob can be placed into the hole, which enables efficient association of polypeptides having Fc regions with different amino acids (WO1996/027011; Ridgway J B et al., Protein Engineering (1996) 9, 617-621; and Merchant A M et al. Nature Biotechnology (1998) 16, 677-681, US20130336973).
In addition to this technique, a further alternative technique known in the art may be used for forming the multispecific antibodies of the present invention. A portion of CH3 of one of the antibody H chains is converted to the corresponding IgA-derived sequence, and its complementary portion in CH3 of the other H chain is converted to the corresponding IgA-derived sequence. The resulting strand-exchange engineered domain CH3 can be used to cause efficient association between polypeptides having different sequences through complementary CH3 association (Protein Engineering Design & Selection, 23; 195-202, 2010). By use of this technique known in the art, the multispecific antibodies of interest can also be efficiently formed.
Even if the multispecific antibodies of interest cannot be formed efficiently, the multispecific antibodies of the present invention may be obtained by the separation and purification of the multispecific antibodies of interest from among produced antibodies. For example, a previously reported method involves introducing amino acid substitutions to two types of H chain variable regions to make their isoelectric points different, so that two types of homodimers and the heterodimerized antibodies of interest can be separately purified by ion-exchange chromatography (WO2007114325). A method using protein A to purify a heterodimerized antibody consisting of a mouse IgG2a H chain which binds to protein A and a rat IgG2b H chain which does not bind to protein A has been reported to date as a method for purifying the heterodimers (WO98050431 and WO95033844). Alternatively, the interaction between each H chain and protein A is modified by using H chains in which amino acid residues at EU numbering positions 435 and 436 which constitute the binding site between protein A and IgG are substituted with amino acids having different binding strength toward protein A such as Tyr and His, and only the heterodimerized antibodies can be efficiently purified by using a protein A column.
Alternatively, a common L chain that can confer binding ability to several different H chains may be obtained and used as the common L chain of the multispecific antibodies. Efficient multispecific IgG expression is possible by introducing genes of such a common L chain and multiple different H chains into cells to express IgGs (Nature Biotechnology (1998) 16, 677-681). When selecting a common H chain, it is also possible to use a method of selecting a common L chain corresponding to any different H chain and exhibiting a high binding ability thereto (WO2004/065611).
It is also possible to use a plurality of these technologies, for example, a combination of two or more. In addition, these techniques can be appropriately applied separately to the two H chains to be associated. The antigen-binding molecules of the present invention may be separately prepared to have the same amino acid sequence based on those with the aforementioned modification.
A multispecific antigen-binding molecule of the present invention comprises a first antigen-binding domain that binds to a first antigen on an antigen-presenting cell and a second antigen-binding domain that binds to a second antigen on a target cell. Because of this, the antigen-presenting cell and target cell are crosslinked via the multispecific antigen-binding molecule of the present invention. Specifically, the multispecific antigen-binding molecule of the present invention simultaneously binds to an antigen on an antigen-presenting cell and a cancer antigen on a target cell to bring the antigen-presenting cell into close proximity to the target cell (it can also be described as recruiting, attracting, or targeting the antigen presenting cell to the target cell). As a result, phagocytosis of the target cell by the antigen presenting cell can be induced. Methods for detecting/measuring phagocytosis include those that make dendritic cells phagocytose labeled cells and detect/measure the label by flow cytometry, image/measure the label with a microscope, or detect/measure the label by a reporter assay.
“Undisrupted” cells mean that the cells are not in debris. An example of cells becoming cell debris is cell death of cancer cells. Cell death is roughly classified into necrosis and apoptosis based on the morphological and biochemical characteristics. Apoptotic cells shrink, form cell fragments called apoptotic bodies, and are phagocytosed and removed by phagocytes in vivo. On the other hand, necrosis causes inflammation of peripheral cells by swelling of cells and eventual leakage of cell contents out of the cells. Apoptosis and necrosis are both considered to be mechanisms by which cancer cells disappear due to anticancer agents and radiation therapy (YAKUGAKU ZASSHI 137(11) 1315-1321 (2017)).
As a general method for disrupting cells, ultrasonic treatment, use of a surfactant, osmotic shock method, disrupting with a homogenizer, disrupting with glass beads, and such are known (these methods have been exemplified in the website: https:/www.gelifesciences.co.jp/technologies/protein_preparation/lysis.html).
In a preferred embodiment, it is desirable that, as the target cells to be phagocytosed, cells that are not disrupted and are countable are allowed to be phagocytosed by the antigen-presenting cells. By making antigen-presenting cells engulf undisrupted target cells as they are, it is possible to allow the antigen presenting cells to present a wide variety of antigens which the target cells have, including not only cell surface antigens, but also intracellular antigens.
Multiple types of antigens derived from target cells taken up into antigen presenting cells are processed, and the produced antigenic peptides are presented by the antigen presenting cells (epitope spreading). These antigen peptides are presented as a complex with MHC class II molecules to activate CD4+ T cells, and also presented as a complex with MHC class I molecules (cross-presentation) to activate CD8+ T cells. Methods for detecting/identifying/measuring antigen peptides derived from target cells presented on the MHC molecules of antigen presenting cells include: methods of evaluating whether or not an antigen presenting cell can activate T cells having a TCR responsive towards an arbitrary peptide antigen-MHC complex (for example, a system using OT-I mice (having OVA-reactive T cells) described in the Examples section of the present specification); methods of detecting/measuring by FACS an arbitrary antigen peptide-MHC complex using an antibody that specifically recognizes the complex; methods of directly detecting/measuring antigen peptides presented on MHCs by MS, and the like. Methods for detecting/measuring T cell activation include: methods of detecting or measuring by ELISA or FACS cytokines released upon activation; methods of detecting/measuring activation markers by FACS; methods of detecting/measuring increase in cell number, and the like.
T cells thus activated are T cells specific for the antigen peptide presented by the antigen presenting cell. By using a multispecific antigen-binding molecule of the present invention, multiple types of antigen peptides derived from target cells are presented on antigen-presenting cells, thus making it possible to induce the activation of T cells targeting multiple types of cancer antigen peptides. The multiple types of cancer antigen peptides also include those derived from antigens different from the second antigen on the target cell.
A suitable example of antigen-presenting cells having such a function is dendritic cells.
Dendritic cells are known to play an important role in antitumor immunity in both innate and adaptive immunity (Nature Reviews Cancer 4, 11-22 (January 2004)). In innate immunity, dendritic cells play a role in phagocytosing, engulfing, and degrading apoptotic cancer cells (phagocytosis). In adaptive immunity, dendritic cells present antigen peptides derived from cancer cells that have been taken up into the cells on major histocompatibility complexes (MHCs), activate naive T cells having T cell receptors (TCRs) that specifically bind to each, and the activated naive T cells are differentiated into cytotoxic T cells (CTLs), helper T cells and the like to induce an antitumor immune response (Nature Reviews Immunology volume 1, pages 126-134 (2001)). The antitumor immune response is an immune response consisting of innate immunity and adaptive immunity against cancer cells, and it is considered that cytotoxic T cells particularly play a central role in the antitumor immune response.
Cross-presentation refers to the presentation of a peptide (antigen peptide) resulted from incorporation and processing of an antigen derived from another cell to CD8+ cytotoxic T cells as a complex with an MHC class I protein. Methods for measuring cross-presentation include methods of recognizing the antigen peptide MHC-I on antigen-presenting cells by flow cytometry or mass cytometry, methods of measuring activation of CD8+ T cells by co-culturing an arbitrary antigen peptide MHC-I-reactive CD8+ cytotoxic T cells and antigen presenting cells presenting this antigen, and the like. Methods for measuring CD8+ T cell activation include: methods of measuring IFNg, granzyme B, perforin, and such released upon activation by ELISA, ELISpot assay, flow cytometry, and such; methods of measuring an activation marker on T cells (CD25, CD69, etc., Clin Cham Acta. 2012 Sep. 8; 413(17-18):1338-49) by flow cytometry; methods of measuring a change in T cell proliferation ability; and the like. It is known that a specific subset of dendritic cells plays the role of cross-presentation and activation (cross-priming) of T cells. CLEC9A (C-type lectin 9A), DEC205 (dendritic and epithelial cells, 205 kDa), CD207 (Cluster of Differentiation 207), XCR1 (XC-chemokine receptor 1), TLR3 (Toll-like receptor 3), and the like are known as markers of dendritic cells responsible for cross-presentation (Nat Rev Immunol. 2011, 11(9), 575-83).
It is known that CLEC9A, which is expressed on the cell surface of the dendritic cell subset responsible for cross-presentation, binds to F-actin exposed on necrotic cells and activates the intracellular signal transduction pathway through the interaction between intracellular domain containing ITAM (Immunoreceptor tyrosine-based activation motif) and Syk, and promotes cross-presentation by dendritic cells (Nat Rev Immunol. 2010 June; 10(6):387-402). Expression of DEC205 and the like is also known in the dendritic cell subset that is responsible for cross-presentation, but CLEC9A has been reported to be expressed in that subset with a specificity higher than DEC205 (Blood, 2012, vol. 119: pp. 2284-2292).
In addition, by using a multispecific antigen-binding molecule of the present invention in combination with an activator of antigen-presenting cells, or in a form conjugated with an activator of antigen-presenting cells, it is possible to enhance the phagocytosis of target cells by antigen-presenting cells induced by crosslinking of antigen-presenting cells and target cells via the multispecific antigen-binding molecule of the present invention, and thus enhance the induction of cytotoxic activity against the target cells.
Conjugates of a multispecific antigen-binding molecule of the present invention and an antigen-presenting cell activator may be made using a variety of bifunctional protein coupling agents such as N-succinimidyl-3-(2-pyridyldithio) propionate (SPDP), succinimidyl-4-(N-maleimidomethyl)cyclohexane-1-carboxylate (SMCC), iminothiolane (IT), bifunctional derivatives of imidoesters (such as dimethyl adipimidate HCl), active esters (such as disuccinimidyl suberate), aldehydes (such as glutaraldehyde), bis-azido compounds (such as bis (p-azidobenzoyl) hexanediamine), bis-diazonium derivatives (such as bis-(p-diazoniumbenzoyl)-ethylenediamine), diisocyanates (such as toluene 2,6-diisocyanate), and bis-active fluorine compounds (such as 1,5-difluoro-2,4-dinitrobenzene). A linker may be a “cleavable linker” facilitating release of the antigen-presenting cell activator in the cell. For example, an acid-labile linker, peptidase-sensitive linker, photolabile linker, dimethyl linker, or disulfide-containing linker (Chari et al., Cancer Res. 52:127-131 (1992)) may be used.
The conjugates of the present invention contemplate, but are not limited to such conjugates prepared with crosslinking reagents including, but not limited to, BMPS, EMCS, GMBS, HBVS, LC-SMCC, MBS, MPBH, SBAP, SIA, SIAB, SMCC, SMPB, SMPH, sulfo-EMCS, sulfo-GMBS, sulfo-KMUS, sulfo-MBS, sulfo-SIAB, sulfo-SMCC, and sulfo-SMPB, and SVSB (succinimidyl-(4-vinylsulfone)benzoate), which are commercially available (e.g., Thermo Fisher Scientific Inc.).
As antigen-presenting cell activators, agents that directly activate antigen-presenting cells (
In one embodiment, the addition of these activators allows undisrupted target cells to be efficiently phagocytosed by antigen-presenting cells as they are, as compared to the case where they are not added. When undisrupted target cells are presented to antigen-presenting cells, it is possible to allow the antigen-presenting cells to present the antigens possessed by the target cells, including a wide variety ranging from not only cell surface antigens, but also intracellular antigens. As a result, antigen-presenting cells can be more effectively activated.
In addition, known adjuvants that activate dendritic cells include killed mycobacteria and LPS (lipopolysaccharide), aluminum hydroxide, aluminum phosphate (Molecular and Cellular Immunology, 7th edition, Elsevier Japan, 2014), and IFNα, IFNγ, TNFα, IL-1β, IL-6, and LL37-DNA complex (N Engl J Med 2009; 361:496-509). Also, agonists for TLR (Toll-like receptor), NLR (nucleotide-binding oligomerization domain-like (NOD-like) receptor), RLR (RIG-I-like receptor), and C-type lectin receptors are also known to act as activators of dendritic cells (Front Immunol. 2014; 5: 255).
By conjugating an agent that directly activates antigen-presenting cells to a multispecific antigen-binding molecule of the present invention, the antigen-presenting cells bound by the multispecific antigen-binding molecule of the present invention can be specifically activated (
When using as a T cell activator an antigen-binding molecule having a binding site for an antigen that is specifically expressed in cells expressing a cancer-specific antigen to which a multispecific antigen-binding molecule of the present invention binds, and a binding site for a T cell surface antigen (e.g. CD3), in combination with the multispecific antigen-binding molecule of the present invention, the cancer cells to which the multispecific antigen-binding molecule of the present invention binds release inflammatory cytokines and the like upon being damaged by T cells recruited in the vicinity of the cancer cells mediated by the T cell activator, which enables specific activation of the antigen-presenting cells to which the multispecific antigen-binding molecule of the present invention binds (
In addition, by conjugating an antibody fragment or agent that activates effector cells (cytotoxic T cells) to a multispecific antigen-binding molecule of the present invention as a T cell activator, cancer cells to which the multispecific antigen-binding molecule of the present invention binds release inflammatory cytokines and the like upon being damaged by effector cells recruited in the vicinity of the cancer cells mediated by the antigen binding molecule, which enables specific activation of the antigen-presenting cells to which the multispecific antigen-binding molecule of the present invention binds (
The present invention also relates to a method for inducing an antitumor immune response, a method for activating cytotoxic T cells, a method for inducing cytotoxicity, a method for suppressing cell proliferation, a method for activating immunity against target cells or cancer tissues containing target cells, a method for preventing or treating cancer, a method for treating an individual having cancer, and a method of allowing an antigen peptide derived from a target cell to be presented on an MHC class I protein of an antigen presenting cell, which comprise a step of administering a multispecific antigen-binding molecule of the present invention to a subject (patient, subject, individual, etc.). Subjects include humans or non-human animals such as mice, rats, monkeys, rabbits, and dogs.
The present invention also relates to polynucleotides encoding an antigen-binding molecule of the present invention. A polynucleotide of the present invention can be incorporated into an arbitrary expression vector. A suitable host can be transformed with the expression vector to obtain cells expressing the antigen-binding molecule. An antigen binding molecule encoded by the polynucleotide can be obtained by culturing cells expressing the antigen-binding molecule and recovering the expression product from the culture supernatant. In other words, the present invention relates to a vector containing a polynucleotide encoding an antigen-binding molecule of the present invention, a cell carrying the vector, and a method of manufacturing the antigen-binding molecule comprising culturing the cell and recovering the antigen-binding molecule from the culture supernatant.
In another aspect, the present invention provides pharmaceutical compositions (pharmaceutical preparations) comprising a multispecific antigen-binding molecule of the present invention as an active ingredient. The present invention also relates to compositions for inducing an antitumor immune response, pharmaceutical compositions for inducing the activation of cytotoxic T cells (cytotoxic T cell activators), pharmaceutical compositions for inducing cytotoxicity (therapeutic agents for inducing cytotoxicity), cell proliferation suppressors, and anticancer agents, which comprise the antigen-binding molecule as an active ingredient. The pharmaceutical compositions of the present invention can also be used as cancer therapeutic agents or cancer preventive agents (compositions for treating cancer or compositions for preventing cancer). The compositions for inducing an anti-tumor immune response, the cytotoxic T cell activators, the cytotoxicity inducing therapeutic agents, the cell proliferation suppressors, and the anti-cancer agents of the present invention are preferably administered to a subject suffering from cancer or a subject with a potential of relapse. In the context of the compositions of the present invention, the induction of an antitumor immune response may preferably be the activation of cytotoxic T cells (cytotoxic T lymphocytes; CTLs).
Further, in the present invention, the compositions for inducing an anti-tumor immune response, the cytotoxic T cell activators, the cytotoxicity-inducing therapeutic agents, the cell proliferation suppressors or anticancer agents, which comprise a multispecific antigen-binding molecule of the present invention as an active ingredient can be expressed as a method of inducing an antitumor immune response, a method of activating cytotoxic T cells, a method of inducing cytotoxicity, a method of suppressing cell proliferation, a method of activating immunity against cancer cells or tumor tissues containing cancer cells, or a method of preventing or treating cancer, which includes a step of administering the antigen-binding molecule to a subject. Alternatively, they can be expressed as a use of the antigen-binding molecule in the manufacture of a composition for inducing an antitumor immune response, a pharmaceutical composition for inducing the activation of cytotoxic T cells, a pharmaceutical composition for inducing cytotoxicity, a cell proliferation suppressor or an anticancer agent. Alternatively, they can also be expressed as the antigen-binding molecule for use in the induction of an anti-tumor immune response, induction of the activation of cytotoxic T cells, induction of cytotoxicity, suppression of cell proliferation, activation of immunity against cancer cells or tumor tissues containing cancer cells, or treatment or prevention of cancer. The compositions or pharmaceutical preparations may include a pharmaceutically acceptable carrier, and optionally, additional therapeutic agents. Moreover, the methods may optionally include a step of administering an additional therapeutic agent.
In the present invention, “comprising an antigen-binding molecule as an active ingredient” means containing the antigen-binding molecule as the main active ingredient, and does not limit the content ratio of the antigen-binding molecule.
Furthermore, the pharmaceutical compositions of the present invention, or compositions for inducing an antitumor immune response, pharmaceutical compositions for inducing cytotoxicity, cell proliferation suppressors and anticancer agents (hereinafter, pharmaceutical compositions or the like) can be used in combination with an activator of antigen presenting cells. Use of an activator of antigen presenting cells in combination with a pharmaceutical composition or the like containing a multispecific antigen-binding molecule of the present invention enables enhancement of the phagocytosis of target cells by antigen presenting cells, and thus enables enhancement of the cytotoxic effect against target cells. Examples of activators of antigen presenting cells include interferon α (IFNα), poly I:C (poly-I:C), T cell activators, and the like. As used herein, the phrase “using an activator of antigen-presenting cells in combination” means that the activator of antigen-presenting cells may be formulated together in a pharmaceutical composition or the like containing a multispecific antigen-binding molecule of the present invention, or the activator of antigen-presenting cells may be contained in a pharmaceutical composition or the like that is different from the pharmaceutical composition or the like containing the multispecific antigen-binding molecule of the present invention. Their dosage forms may be the same or different. When a multispecific antigen-binding molecule of the present invention and an activator of antigen-presenting cells are contained in different pharmaceutical compositions or the like, these pharmaceutical compositions or the like can be administered to a subject at the same time, or separately. Furthermore, these pharmaceutical compositions and the like may be provided as a kit.
Further, a multispecific antigen-binding molecule of the present invention or a pharmaceutical composition comprising a multispecific antigen-binding molecule of the present invention as an active ingredient can be used as a pharmaceutical composition for enhancing the phagocytosis of target cells by antigen-presenting cells, enhancing induction of their cytotoxic activity, or enhancing cytotoxic activity when used in combination with an antigen presenting cell activator or a pharmaceutical composition or such comprising an antigen presenting cell activator as an active ingredient. Further, an activator of an antigen-presenting cell or a pharmaceutical composition or such comprising an activator of an antigen-presenting cell as an active ingredient can be used as a pharmaceutical composition for enhancing the phagocytosis of target cells by antigen-presenting cells, enhancing induction of their cytotoxic activity, or enhancing cytotoxic activity when used in combination with a multispecific antigen-binding molecule of the present invention or a pharmaceutical composition comprising a multispecific antigen-binding molecule of the present invention as an active ingredient.
Herein, “used in combination” includes the case where a pharmaceutical composition or such comprising a multispecific antigen-binding molecule of the present invention as an active ingredient and a pharmaceutical composition or such comprising an activator of antigen-presenting cells as an active ingredient are simultaneously administered to a subject, and the case where they are separately administered to a subject. Their dosage forms may be the same or different. Furthermore, these pharmaceutical compositions or such may be provided as a kit.
Furthermore, the present invention provides a method that utilizes the effects produced by using a multispecific antigen-binding molecule of the present invention described above or a pharmaceutical composition or such comprising the antigen-binding molecule as an active ingredient in combination with an antigen presenting cell activator or a pharmaceutical composition or such comprising the antigen presenting cell activator as an active ingredient to enhance the cytotoxic activity or antitumor effect of the multispecific antigen-binding molecule of the present invention or the pharmaceutical composition or such comprising the multispecific antigen-binding molecule of the present invention as an active ingredient by the antigen presenting cell activator or the pharmaceutical composition or such comprising the antigen presenting cell activator as an active ingredient.
The pharmaceutical compositions, compositions for inducing an antitumor immune response, cell proliferation suppressors, or anticancer agents of the present invention may be administered either orally or parenterally to patients. Preferred administration may be parental administration. Specifically, such administration methods include injection, nasal administration, transpulmonary administration, and percutaneous administration. Injections include, for example, intravenous injections, intramuscular injections, intraperitoneal injections, and subcutaneous injections. For example, pharmaceutical compositions, compositions for inducing an antitumor immune response, therapeutic agents for inducing cellular cytotoxicity, cell proliferation suppressors, or anticancer agents of the present invention can be administered locally or systemically by injection. Furthermore, appropriate administration methods can be selected according to the patient's age and symptoms. The dose can be selected, for example, from the range of 0.0001 mg to 1,000 mg per kg of body weight for each administration. Alternatively, the dose can be selected, for example, from the range of 0.001 mg/body to 100,000 mg/body per patient. However, the dose of a pharmaceutical composition of the present invention is not limited to these doses.
The pharmaceutical compositions of the present invention can be formulated according to conventional methods (for example, Remington's Pharmaceutical Science, latest edition, Mark Publishing Company, Easton, U.S.A.), and may also contain pharmaceutically acceptable carriers and additives. Examples include, but are not limited to, surfactants, excipients, coloring agents, flavoring agents, preservatives, stabilizers, buffers, suspension agents, isotonic agents, binders, disintegrants, lubricants, fluidity promoting agents, and corrigents, and other commonly used carriers can be suitably used. Specific examples of the carriers include light anhydrous silicic acid, lactose, crystalline cellulose, mannitol, starch, carmellose calcium, carmellose sodium, hydroxypropyl cellulose, hydroxypropyl methylcellulose, polyvinylacetal diethylaminoacetate, polyvinylpyrrolidone, gelatin, medium-chain triglyceride, polyoxyethylene hardened castor oil 60, saccharose, carboxymethyl cellulose, corn starch, inorganic salt, and such.
In another aspect, the present invention provides a method for allowing an antigen peptide derived from a target cell to be presented on an MHC class I protein of an antigen-presenting cell, which comprises a step of targeting the antigen-presenting cell to the target cell using a multispecific antigen-binding molecule of the present invention.
In another aspect, the present invention provides a method of screening for an antigen peptide derived from a cancer, which comprises a step of targeting an antigen-presenting cell to a target cell using a multispecific antigen-binding molecule of the present invention and a step of allowing an antigen peptide derived from the target cell to be presented on an MHC class I protein of the antigen-presenting cell. In yet another aspect, the present invention provides a method of screening for an antigen peptide derived from a target cell, which comprises a step targeting an antigen-presenting cell to a target cell using a multispecific antigen-binding molecule of the present invention and a step of detecting an antigen peptide derived from the target cell which has been presented on the MHC class I protein of the antigen presenting cell, which method may include a step of identifying the detected antigen peptide. By using the peptide obtained by the screening method, cytotoxic T cells specific to the MHC/peptide complex containing the peptide can be induced.
Examples of methods for detecting a target cell-derived antigen peptide presented on an MHC class I protein of an antigen presenting cell include a method of evaluating whether the antigen presenting cell can activate a T cell having a TCR reactive to an arbitrary peptide antigen-MHC complex (for example, a system using OT-I mice (having OVA-reactive T cells) described in the Examples section of the present specification), a method of detecting/measuring by FACS using an antibody that specifically detects an arbitrary antigen peptide-MHC complex, a method of directly detecting/measuring by MS the antigen peptide presented on MHC, and such. Methods for detecting/measuring T cell activation include a method of detecting/measuring by ELISA or FACS cytokines released upon activation, a method of detecting/measuring an activation marker by FACS, a method of detecting/measuring an increase in cell number, and the like.
As a method for identifying the detected antigen peptide, for example, the following method is mentioned as an example of a method for identifying the antigen peptide presented by human antigen-presenting cells. Meanwhile, it is also possible to identify antigen peptides presented by mouse antigen-presenting cells by performing a similar experiment using anti-mouse MHC antibody beads instead of the anti-HLA-DR beads described in the following example method.
(1) Generation of anti-HLA-DR beads
Furthermore, the present invention provides methods of inducing damage to cells expressing a certain cancer-specific antigen or to tumor tissues containing cells expressing the cancer-specific antigen and methods for suppressing proliferation of these cells or these tumor tissues, by contacting cells that express the cancer-specific antigen with a multispecific antigen-binding molecule of the present invention which binds to the cancer-specific antigen or with a multispecific antigen-binding molecule of the present invention and an antigen presenting cell activator. The cells bound by an antigen-binding molecule of the present invention that binds to the cancer-specific antigen are not particularly limited as long as they are cells that express the cancer-specific antigens. Specifically, suitable examples of the preferred cancer antigen-expressing cells of the present invention are cells of ovarian cancer, prostate cancer, breast cancer, uterine cancer, hepatic cancer, lung cancer, pancreatic cancer, gastric cancer, bladder cancer, and colorectal cancer.
“Contact” in the present invention is carried out, for example, by administering a multispecific antigen-binding molecule of the present invention that binds to a cancer antigen to a non-human animal transplanted with cells expressing the cancer-specific antigen into the body, or to an animal having cancer cells that intrinsically express the cancer-specific antigen. The method of administration may be either oral or parenteral. In a particularly preferred embodiment, the method of administration is a parenteral administration. Specific examples of the administration method include administration by injection, transnasal administration, transpulmonary administration, and transdermal administration. Examples of administration by injection include intravenous injection, intramuscular injection, intraperitoneal injection, and subcutaneous injection. A pharmaceutical composition of the present invention, a composition for inducing an antitumor immune response, a pharmaceutical composition for inducing cytotoxicity, a cell proliferation suppressor, and an anticancer agent can be administered systemically or locally, for example, through administration by injection. The method of administration can be selected appropriately according to the age and symptoms of test animals. When administered as an aqueous solution, an aqueous solution containing purely an antigen-binding molecule of the present invention alone may be used, or a solution containing surfactants, excipients, coloring agents, perfumes, preservatives, stabilizers, buffers, suspending agents, isotonization agents, binders, disintegrants, lubricants, fluidity promoting agents, flavoring agents, and such may be used. The dose can be selected, for example, from the range of 0.0001 mg to 1000 mg per kg body weight for a single administration. Alternatively, for example, the dose can be selected from the range of 0.001 mg/body to 100000 mg/body per patient. However, the dose of an antigen-binding molecule of the present invention is not limited to these doses.
The following method is suitably used as a method for evaluating or measuring cytotoxicity induced against cells expressing a cancer-specific antigen bound by a cancer specific antigen-binding domain constituting a multispecific antigen-binding molecule of the present invention, through the contact with the antigen-binding molecule. Examples of a method for evaluating or measuring the cytotoxic activity in vitro include methods for measuring cytotoxic T cell activity, and such. Whether an antigen-binding molecule of the present invention has T cell cytotoxic activity can be measured by known methods (for example, Current protocols in Immunology, Chapter 7. Immunologic studies in humans, Editor, John E. Coligan et al., John Wiley & Sons, Inc., (1993) and the like). For activity measurements, an antigen-binding molecule with an antigen-binding domain that binds to an antigen which differs from the antigen bound by that of the present invention and is not expressed in the cells used for the examination can be used as a control and in the same manner as the antigen-binding molecule of the present invention, and the activity can be determined to be present when the antigen-binding molecule of the present invention shows a stronger cytotoxic activity than that of the antigen-binding molecule used as a control.
To evaluate or measure cytotoxic activity in vivo, for example, cells expressing an antigen bound by a cancer-specific antigen-binding domain that constitutes a multispecific antigen-binding molecule of the present invention are intradermally or subcutaneously transplanted into a non-human test animal, and then a test antigen-binding molecule is intravenously or intraperitoneally administered daily or with an interval of few days, starting from the day of transplantation or the following day. Tumor size is measured daily and the difference in the change of tumor size can be defined as the cytotoxic activity. In a similar manner to the in vitro evaluation, a control antigen-binding molecule is administered, and an antigen-binding molecule of the present invention can be determined as exhibiting cytotoxic activity based on the finding that the tumor size in the group subjected to administration of an antigen-binding molecule of the present invention is significantly smaller than the tumor size in the group subjected to administration of the control antigen-binding molecule.
As a method for evaluating or measuring the suppressive effect on proliferation of cells expressing an antigen bound by a cancer-specific antigen-binding domain that constitutes a multispecific antigen-binding molecule of the present invention through the contact with the antigen-binding molecule, a method of measuring the uptake of isotope-labeled thymidine into cells, or the MTT method may be suitably used. As a method for evaluating or measuring the cell proliferation-suppressing activity in vivo, the same method as that described above for evaluating or measuring cytotoxic activity in vivo may be suitably used.
The present invention also provides kits for use in the methods of the present invention, which comprise an antigen-binding molecule of the present invention or an antigen-binding molecule produced by a production method of the present invention. Additionally, the kit may include in its package, a pharmaceutically acceptable carrier, solvent, instructions describing the method of use, and the like.
The present invention also relates to an antigen-binding molecule of the present invention or an antigen-binding molecule produced by a production method of the present invention for use in a method of the present invention.
Those skilled in the art will naturally understand that optional combinations of one or more of the embodiments described herein are included in the present invention, as long as they are not technically inconsistent based on the common technical knowledge of those skilled in the art.
All prior art references cited herein are incorporated by reference into this description.
In the following, the present disclosure will be described in more detail with reference to examples. However, the present disclosure may be embodied in various forms and should not be construed as being limited to the examples given herein.
The various therapies that target existing antigen presenting cells have the following problems.
The inventors thought it important to meet the following conditions in order to solve these problems.
The inventors devised molecules that crosslink antigen-presenting cells and target cells as pharmaceutical compositions that meet the above conditions.
For example, among dendritic cells, mature dendritic cells are said to have higher antigen presenting ability than immature dendritic cells (Front Immunol. 2013 Apr. 3; 4:82). Methods for activating antigen presenting cells include a method of directly activating antigen presenting cells, and a method of activating immune cells other than antigen presenting cells and indirectly activating antigen presenting cells through inflammatory cytokines or such released from these activated cells or damaged dead cells. Therefore, it was thought that it would be possible to increase the efficiency of antigen presentation shown in (1) by using a bispecific antibody that crosslinks antigen-presenting cells and target cells together with a factor that activates antigen-presenting cells (
CLEC9A is a cross-presenting DC-specific antigen having the function of presenting an engulfed antigen to MHC-I, and GPC3 is known to be expressed on the cell membrane of certain cancer cells (Trends Immunol. 2013 August; 34(8): 361-370, European Journal of Cancer Volume 47, Issue 3, February 2011, Pages 333-338). It was thought that, when using these antigens for crosslinking dendritic cells to cancer cells, it is possible to facilitate dendritic cells to phagocytose cancer cells and to present antigens held by cancer cells. Therefore, the present inventors produced a bispecific antibody composed of an anti-CLEC9A antibody and an anti-GPC3 antibody. Expression vectors for known anti-CLEC9A antibody 10B4 (heavy chain: 10B4H-mF18mP4dGK (SEQ ID NO: 1), light chain: 10B4L-mk1 (SEQ ID NO: 2)), and anti-GPC3 antibody GCH065 (heavy chain: GCH065-mF18mN4dGK (SEQ ID NO: 3), light chain: L0011-k0a (SEQ ID NO: 4)) were prepared by a method known to those skilled in the art, and these antibodies were expressed using Expi293 (Thermo Fisher Scientific) cells. A negative control antibody (heavy chain: NCHn (SEQ ID NO: 5), light chain: NCL (SEQ ID NO: 6)) was also used. Purification of antibodies from the culture supernatant and preparation of the bispecific antibody were carried out by methods known to those skilled in the art. Hereinafter, the bispecific antibody of the anti-CLEC9A antibody and the anti-GPC3 antibody will be referred to as 10B4/GCH065, and the bispecific antibody of the anti-CLEC9A antibody and negative control antibody will be referred to as 10B4/NC.
The antibodies prepared in Example 2 were used to evaluate whether the uptake of cancer cells by dendritic cells is promoted by crosslinking the dendritic cells and the cancer cells. The target cancer cells used were LL/2 (LLC1) (CRL-1642, ATCC) transfectant cells (hereinafter LLC1/′hGPC3/OVA) that express human GPC3 (hGPC3) and ovalbumin (OVA). The dendritic cells used for the evaluation were BMDC (bone marrow dendritic cells) induced from bone marrow of C57BL/6NCrl mice (female, 6-8 weeks old, Charles River) by the method described previously (Blood 2014 124:3081-3091). The antigen expression in the induced BMDC was stained by a method known to those skilled in the art using the fluorescence-labeled antibodies for flow cytometry shown in Table 1, and the results of CLEC9A expression level evaluation using Fortessa (BD Biosciences) are shown in
Target cell phagocytosis efficiency was evaluated using the above cells. First, the target cells LLC1/hGPC3/OVA were labeled using PKH26 Red Fluorescent Cell Linker Kit for General Cell Membrane Labeling (PKH26GL, SIGMA). Next, the labeled cells were frozen in liquid nitrogen and then thawed at 37° C. This operation was carried out twice.
Target cells treated as above, each antibody, and BMDC were added to low-adsorption flat bottom 96 well plates (Cat: 3474, Corning) at 2.0×104 cells/well, 1 μg/well and 2.0×104 cells/well, respectively, and reacted for 1 hour. The reaction was carried out under the conditions of 5% carbon dioxide gas and 37° C. After reacting for 1 hour, the fluorescence-labeled antibodies for flow cytometry shown in Table 2 were used to perform staining by a method known to those skilled in the art, and measured with Fortessa (BD Biosciences). What percentage of each of the CLEC9A-positive dendritic cell (CD103-positive dendritic cell) population and the CLEC9A-negative dendritic cell (CD103-negative dendritic cell) population phagocytosed the labeled cells was evaluated. The result is shown in
Similarly, the phagocytosis ratio was also enhanced when using the bispecific antibody NLDC145/GCH065 prepared according to the method described in Example 2 using a known antibody NLDC145 (heavy chain: NLDC145VH-mF18mP4dGK (SEQ ID NO: 7), light chain: NLDC145VL-mk1 (SEQ ID NO: 8)), which binds to another antigen DEC205 on CD103-positive dendritic cells, and GCH065 (heavy chain: GCH065-mF18mN4dGK (SEQ ID NO: 3), light chain: L0011-k0a (SEQ ID NO: 4)), which recognizes the target cell antigen GPC3, compared to the bispecific antibody NC/GCH065, which was made using a negative control antibody (heavy chain NCHp (SEQ ID NO: 9), light chain NCL (SEQ ID NO: 6)) and anti-GPC3 antibody GCH065 (heavy chain GCH065-mF18mN4dGK (SEQ ID NO: 3), light chain L0011-k0a (SEQ ID NO: 4)). Test conditions were: target cells LLC1/hGPC3/OVA 5.0×104 cells/well, BMDC 2.0×104 cells/well, and reaction time: 30 minutes. The results are shown in
From the above, it was shown that bispecific antibodies that recognize a target antigen and a dendritic cell antigen can induce phagocytosis of target cells by dendritic cells.
The bispecific antibody prepared in Example 2 was used to evaluate whether the antigen-presenting cells that phagocytosed the cells could present intrinsic antigens of the target cells and activate immune cells. As immune cells, CD8+ T cells isolated with the CD8a+T Isolation kit (Cat: 130-104-075, Miltenyi Biotec) from the spleen of OT-I mice (Stock No: 003831, The Jackson Laboratory) having CD8+ T cells recognizing the OVA peptide (257-264)-MHC class I complex were used.
To a low adsorption flat-bottom 96-well-plate (Cat: 3474, Corning) were added target cells LLC1/hGPC3/OVA at 5.0×104 cells/well, each antibody at 1 μg/well, CD8+ T cells at 1.0×105 cells/well, BMDC at 1.0×105 cells/well, and poly I:C (Cat: P1530, SIGMA) or IFNα (Cat: 752806, Biolegend) at 20 μg/well or 10000 U/well, respectively, followed by reaction for 48 hours. The reaction was carried out under the conditions of 5% carbon dioxide gas and 37° C. After the reaction was completed, the supernatant was collected, and the amount of mouse IFNγ (mIFNγ) in the supernatant was measured using Mouse IFN-gamma DuoSet ELISA (R&D, Cat: DY485). As shown in
It was evaluated whether an antitumor effect could be induced, using subcutaneous transplantation model mice and the bispecific antibody 10B4/GCH065 composed of anti-CLEC9A antibody 10B4 (heavy chain 10B4H-mF18mP4dGK (SEQ ID NO: 1), light chain 10B4L-mk1 (SEQ ID NO: 2)) and anti-GPC3 antibody GCH065 (heavy chain GCH065-mF18mN4dGK (SEQ ID NO: 3), light chain L0011-k0a (SEQ ID NO: 4)), and the bispecific antibody NC/GCH065 made using a negative control antibody (heavy chain NCHp (SEQ ID NO: 9), light chain NCL (SEQ ID NO: 6)) and anti-GPC3 antibody GCH065 (heavy chain GCH065-mF18mN4dGK (SEQ ID NO: 3), light chain L0011-k0a (SEQ ID NO: 4)) according to the method described in Example 2. First, the target cells, LLC1/hGPC3/OVA, were transplanted to C57BL/6NCrl mice (female, 8 weeks old, Charles River) at 2×106 cells each. The tumor diameter and body weight were measured 7 days after transplantation, and randomization was performed based on the results, followed by dividing the mice into 2 groups (6 animals/group). Then, in each randomized group, agents were administered on the 8th and 11th days after transplantation as described below.
Group 1: NC/GCH065 5 mg/kg+poly I:C 50 μg
Group 2: 10B4/GCH065 5 mg/kg+poly I:C 50 μg
Each antibody was administered intravenously, and poly I:C (tlrl-pic, InvivoGen) was administered intratumorally. The tumor diameter was measured twice a week. A graph of change in tumor diameter is shown in
It is thought that antigen presenting efficiency can be increased by activating antigen presenting cells as shown in Example 1 (3). There are two methods for this: a method in which antigen-presenting cells are directly activated; and a method in which immune cells other than antigen-presenting cells are activated and antigen-presenting cells are indirectly activated through inflammatory cytokines released from the activated cells or damaged dead cells. Examples thereof are shown in
In
In
The phagocytosis efficiency of hEpCAM-positive target cells was evaluated using the same system as in Example 3. As target cells, Colon 38 (MC38) (Japanese Foundation For Cancer Research) expressing human EpCAM (hEpCAM) transfectant cells (hereinafter MC38/hEpCAM) were used. The heavy chain and light chain variable regions of the known anti-hEpCAM antibody described in WO2010142990A1 were used.
First, the target cells MC38/hEpCAM were labeled using PKH26 Red Fluorescent Cell Linker Kit for General Cell Membrane Labeling (PKH26GL, SIGMA). Next, the labeled cells were frozen in liquid nitrogen and then thawed at 37° C. This operation was done twice.
To a low-adsorption flat bottom 96 well plate (Cat: 3474, Corning) were added target cells that had been subjected to the above operation at 5.0×104 cells/well, each antibody at 1 μg/well and BMDC at 5.0×104 cells/well, followed by reaction for 1 hour at 200 μl/well. The reaction was carried out under the conditions of 5% carbon dioxide gas and 37° C. After reacting for 1 hour, the fluorescence-labeled antibodies for flow cytometry shown in Table 2 were used to perform staining by a method known to those skilled in the art, and measurement was carried out using Fortessa (BD Biosciences). It was evaluated as to what percentage each of the CLEC9A-positive dendritic cell (CD103-positive dendritic cell) population and the CLEC9A-negative dendritic cell (CD103-negative dendritic cell) population phagocytosed the labeled cells. The result is shown in
The bispecific antibody NLDC145/GCH065 prepared by the method described in Example 2 using known antibody NLDC145 (heavy chain: NLDC145VH-mF18mP4dGK (SEQ ID NO: 7), light chain: NLDC145VL-mk1 (SEQ ID NO: 8)), which binds to DEC205, and GCH065 (heavy chain: GCH065-mF18mN4dGK (SEQ ID NO: 3), light chain: L0011-k0a (SEQ ID NO: 4)), which recognizes the target cell antigen GPC3, was used to evaluate whether antigen presenting cells that phagocytosed cells can present intrinsic antigens of target cells and activate immune cells. As immune cells, as in Example 4, CD8+ T cells isolated from the spleen of OT-I mice (Stock No: 003831, The Jackson Laboratory) using the CD8a+T Isolation kit (Cat: 130-104-075, Miltenyi Biotec) were used. As target cells, LLC1/hGPC3/OVA which were freeze-thawed 4 times were used.
Into a low adsorption flat-bottom 96 well plate (Cat: 3474, Corning) were added target cells LLC1/hGPC3/OVA at 5.0×104 cells/well, each antibody at 1 μg/well, CD8+ T cells at 1.0×105 cells/well, BMDC at 1.0×105 cells/well, and poly I:C (Cat: P1530, SIGMA) at 4 μg/well, followed by reaction for 48 hours at 200 μl/well. The reaction was carried out under the conditions of 5% carbon dioxide gas and 37° C. After the reaction was completed, the supernatant was collected, and the amount of mouse IFNγ (mIFNγ) in the supernatant was measured using Mouse IFN-gamma DuoSet ELISA (R&D, Cat: DY485). As shown in
The bispecific antibody 10B4/3171 prepared by the method described in Example 2 using CLEC9A antibody 10B4 (heavy chain 10B4H-mF18mP4dGK (SEQ ID NO: 1), light chain 10B4L-mk1 (SEQ ID NO: 2)) and anti-hEpCAM-binding antibody 3171 (heavy chain 3171H-mF18mN4dGK (SEQ ID NO: 54), light chain 3171L-KT0 (SEQ ID NO: 55)) was used to evaluate whether antigen presenting cells that phagocytosed cells can present intrinsic antigens of target cells and activate immune cells. As immune cells, as in Example 4, CD8+ T cells isolated from the spleen of OT-I mice (Stock No: 003831, The Jackson Laboratory) using the CD8a+T Isolation kit (Cat: 130-104-075, Miltenyi Biotec) were used. Target cells used were MC38/hEpCAM/OVA prepared by introducing the Myc-OVA plasmid into MC38/hEpCAM using FuGENE (Cat: E2321A, Promega) to transiently express OVA and freeze-thawing the cells 4 times.
Into a low adsorption flat bottom 96 well plate (Cat: 3474, Corning) were added target cells MC38/hEpCAM/OVA at 1.0×104 cells/well, each antibody at 1 μg/well, CD8+ T cells at 1.0×105 cells/well, BMDC at 1.0×105 cells/well, and poly I:C (Cat: P1530, SIGMA) at 4 μg/well. The mixture was reacted for 48 hours at 200 μl/well. The reaction was carried out under the conditions of 5% carbon dioxide gas and 37° C. After the reaction was completed, the supernatant was collected, and the amount of mouse IFNγ (mIFNγ) in the supernatant was measured using Mouse IFN-gamma DuoSet ELISA (R&D, Cat: DY485). As shown in
The multispecific antigen-binding molecules of the present invention can crosslink antigen-presenting cells such as dendritic cells and target cells, promote phagocytosis of the target cells by the antigen-presenting cells, and allow multiple types of tumor antigens derived from the phagocytosed target cells to be presented to T cells. Therefore, the multispecific antigen-binding molecules of the present invention can induce activation of CD8+ cytotoxic T cells that target multiple types of tumor antigens derived from phagocytosed target cells, and are a useful means of cancer treatment as compared to conventional cancer immunotherapies that target a single tumor antigen.
Number | Date | Country | Kind |
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2018-116978 | Jun 2018 | JP | national |
Filing Document | Filing Date | Country | Kind |
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PCT/JP2019/024479 | 6/20/2019 | WO | 00 |