CN104592391A - Construction method and application of bispecific antibody EpCAM*CD3 - Google Patents

Construction method and application of bispecific antibody EpCAM*CD3 Download PDF

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CN104592391A
CN104592391A CN201510029971.3A CN201510029971A CN104592391A CN 104592391 A CN104592391 A CN 104592391A CN 201510029971 A CN201510029971 A CN 201510029971A CN 104592391 A CN104592391 A CN 104592391A
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cell
epcam
specific antibody
heavy chain
antibody
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CN104592391B (en
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王涛
胡柳
马莹莹
刘敬松
陈婷
范克索
周鹏飞
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Wuhan youzhiyou biopharmaceutical Co.,Ltd.
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YZY BIOPHARMA CO Ltd
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Abstract

The invention provides a bispecific antibody. The bispecific antibody is composed of a single-chain unit and a univalent unit, wherein the univalent unit has specific binding capacity for a surface antigen CD3 of an immune cell; the single-chain unit has specific binding capacity for a surface antigen EpCAM of a tumor cell; the single-chain unit contains a single-chain variable fragment (scFv) fused with a Fc fragment; and the univalent unit contains a light and heavy chain pair. The invention also provides a preparation method of the bispecific antibody and pharmaceutical application of the bispecific antibody.

Description

The construction and application of a kind of bi-specific antibody EpCAM × CD3
Technical field
The present invention relates to immunologic technical field.Specifically, structure and the preparation method of bi-specific antibody is related to.
Background technology
Bi-specific antibody (bispecific antibody, BiAb) is the artificial antibody containing two species-specific antigen binding sites, can erect bridge between target cell and functional molecular (cell), produces the effector function of guidance quality.BiAb, in biomedicine, particularly has broad application prospects in the immunotherapy of tumour.The focus that tumour cell is current immunotherapy applied research is killed by BiAb mediated cell toxic action, its principal feature is that BiAb can simultaneously in conjunction with the target molecule on tumor associated antigen and immune effector cell, and direct triggering immune effector cell is to the specific killing of tumour cell.But in bispecific antibody drug R&D process, ubiquity and is expressed difficulty, yield poorly, many obstacles such as purifying difficulty, poor stability, therefore, build new bi-specific antibody, above-mentioned obstacle can be overcome, and set up corresponding immunologic cytotoxicity animal model, be necessary.The invention provides a kind of structure of novel pair of characteristic antibody, and the research method described its pharmacodynamics and result.Be below for studied Immune Cell Antigens and tumor-cell antigen, and some background technologies of correlation technique development are introduced.
1.CD3
CD3 molecule is made up of 4 subunits: δ, ε, γ, ζ, and its molecular mass is respectively 18.9kDa, 23.1kDa, 20.5kDa, 18.7kDa, and its length has 171,207,182,164 amino-acid residues respectively.They form 6 peptide chains together, and the normal TCR-CD3 complex body being formed and contain 8 peptide chains of combining closely with φt cell receptor (T cell receptor, TCR), structural representation is shown in Fig. 1.This complex body has T cell activation signal transduction, stablizes the function of TCR structure.CD3 kytoplasm section is containing immunoreceptor tyrosine-based activation motif (immunoreceptor tyrosine-based activation motif, ITAM), TCR identifies and combines the antigen peptide of being offered by MHC (major histo-compatibility complex) molecule, cause the tyrosine residues of the conserved sequence of the ITAM of CD3 by the tyrosine protein kinase p56lck phosphorylation in T cell, then can raise the tyrosine protein kinase (as ZAP-70) that other contain SH2 (Scr homology 2) structural domain.The phosphorylation of ITAM and be one of important biochemical reaction of T cell activation intracellular signaling process commitment with the combination of ZAP-70.Therefore, the function of CD3 molecule is that transduction TCR identifies the activation signals that antigen produces.
2.EpCAM
Epithelial cell adhesion molecule EpCAM (epithelial cell adhesion molecule, CD326), the I type transmembrane glycoprotein of to be a kind of molecular weight by GA-733-2 genes encoding be 40kDa, as homophilic calcium dependent/non-dependent epithelial cell between adhesion molecule play in carcinogenesis process and act on.EpCAM is one of tumor associated antigen of identifying of using monoclonal antibody technology the earliest, and it is with polymeric form wide expression in epithelium surface, and mediation calcium independence cell syndio form adhesive function, can be included into adhesion molecule family accordingly.EpCAM also possesses other characteristics of adhesion molecule family, participates in the various procedures such as interaction, migration, cytodifferentiation, form, Cycle Regulation, intracellular signaling, metabolism comprising cell and matrix.Meanwhile, EpCAM in process LAN, points out itself and tumour closely related in the tumour of multiple epithelial origin.Under pathologic condition, EpCAM in various degree be expressed in gland cancer, comprise colorectal cancer, adenocarcinoma of stomach, mammary cancer, ovarian cancer, adenocarcinoma of lung, prostate cancer, carcinoma of the pancreas and hepatocellular carcinoma and retinoblastoma.Multinomial research has confirmed the propagation of the expression of EpCAM and mammary cancer and colon cancer cell, period profile, transfer relevant (see table 1).Monospecific anti-EpCAM monoclonal antibody (MAB), such as 17-1A MAB (glaxowellcome, Centocor), it is the assisting therapy of first German EpCAM targeted therapy colorectal cancer of approval, but, a large amount of clinical application data presentation, this Mono-specific antibodies compares chemotherapy does not have significantly more useful effect.At present, some other EpCAM targeted therapy, comprise bi-specific antibody, developing into the direction of cancer therapy, bi-specific antibody MT110 and Catumaxomab is the therapeutic double antibody medicine for tumour antigen EpCAM, wherein Catumaxomab was ratified to be used for the treatment of pernicious cancer ascites in 2009 by European Union, and MT110 in clinical studies.Obviously, EpCAM has become one of focus target of current oncotherapy research.
Table 1EpCAM tumour distribution widely
Tumour EpCAM positive rate
Ovarian cancer 88-100%
Cancer of the stomach 98%
Colorectal carcinoma 99%
Carcinoma of the pancreas 96%
Mammary cancer 90%
Carcinoma of endometrium 91-96%
Lung cancer 87%
Prostate cancer 98%
3. bi-specific antibody technical development
Bi-specific antibody, two antigen-binding sites in an antibody molecule can respectively in conjunction with the antibody of two kinds of different epitopes.
Antibody drug is the biopharmaceutical macromolecular drug prepared based on the antibody engineering technology of cell engineering and genetic engineering technique, has that specificity is high, character is homogeneous, can for advantages such as specific target spot directional preparations.Monoclonal antibody is mainly used in following three aspects clinically: oncotherapy, immunological disease treatment and anti-infective therapy.Wherein the treatment of tumour is the field that current monoclonal antibody is most widely used, and has entered in the monoclonal antibody product of clinical trial and listing at present, and the product amount accounting for oncotherapy is probably 50%.Mab treatment tumour is combined to the special target spot of sick cell by it, thus stimulating immune system kills and wounds the immunotherapy of target cell, in order to strengthen the effector function of antibody, the particularly effect of killing tumor cell, people attempt multiple method engineered antibody molecule, bi-specific antibody is one of developing direction improving Antybody therapy effect, now becomes the focus of antibody engineering research field.
Bi-specific antibody for immunotherapy is the artificial antibody containing 2 species-specific antigen binding sites, bridge can be erected between target cell and functional molecular (cell), excite the immune response with guidance quality, have broad application prospects in the immunotherapy of tumour.
4. bi-specific antibody preparation
Bi-specific antibody obtains by number of ways, and its preparation method mainly contains: chemical coupling method, hybridization-hybridoma and genetic engineering antibody preparation method.Chemical coupling method is linked together at the mode of 2 different monoclonal antibody chemical couplings, prepares bispecific monoclonal antibody, and this is bispecific monoclonal antibody concept the earliest, and the shortcoming of this sample preparation method is apparent.Hybridization-hybridoma produces bispecific monoclonal antibody by the mode of cell hybridization method or three way cross knurl, these quadromas or three way cross knurl are the hybridoma fusion by building up, or set up hybridoma and obtain from the lymphocyte cell that mouse obtains, can only produce the bi-specific antibody in mouse source, its application is greatly limited.And developing rapidly along with Protocols in Molecular Biology, there is the multiple forming types of genetic engineering double specific antibody, and be mainly divided into dual specific miniantibody, double-chain antibody, strand bivalent antibody, multivalence bi-specific antibody four class.At present, existing Several gene engineering bispecific antibody drug enters clinical experimental stage in the world, and shows good application prospect.
5. the adoptive immunotherapy of tumour
The adoptive immunotherapy of tumour is inputted after amplification in vitro in patient body by immunologically competent cell that is autologous or allosome, direct killing tumour cell, the immunologic function of adjustment and enhancing body, mainly comprises LAK cell, til cell, the T lymphocyte of activation and the immunotherapy of CIK cell.And immunotherapy can only remove a small amount of, scattered tumour cell, the entity tumor curative effect for late period is limited.Therefore often it can be used as the ordinary method combined utilization such as a kind of adjuvant therapy and operation, chemotherapy, radiotherapy.After first cleaning a large amount of tumour cells by ordinary method, then remove remaining tumour cell by immunotherapy, to improve the effect of combined therapy of tumour.Wherein, adoptive immunotherapy, as the novel method of in combined therapy of tumour, is treated with routine operation, radiotherapy, chemotherapy and other cells and molecular therapy is extensively coordinated, illustrate application prospect widely in the treatment of kinds of tumors.But one more preferably mode should be, bi-specific antibody one end in conjunction with the surface antigen CD3 of cultured immunocyte, and can input in body thereupon together, and the other end of bi-specific antibody can well in conjunction with the surface antigen of tumour cell; Like this, bi-specific antibody just can erect the bridge between tumour cell and immunocyte in vivo, makes immunocyte concentrate near tumor cells, and then kills and wounds tumour cell.Effectively can solve the metastasis and extension of tumour cell by this method, overcome drawbacks such as " not thoroughly, easily transfers, side effect large " after operation, chemicotherapy three great tradition therapeutic modality.
Summary of the invention
Term and shortenings
BiAb: bi-specific antibody (bispecific antibody)
TA: tumour antigen (tumor antigen)
VH: variable region of heavy chain (heavy chain variable region).
VL: variable region of light chain (light chain variable region).
CL: constant region of light chain (constant region of light chain).
CDR: the abbreviation being English Complementarity determining regions (CDRs), refers to the antigen complementary determining region of antibody.
ScFv: Single chain antibody fragment (single-chain variable fragment), is also called single-chain antibody.
CLD: clone exploitation (cell line development)
FACS: fluorescence-activated cell sorting (Fluorescence-activated cell sorting), also referred to as Flow cytometry.
The present invention is directed to the weak point of conventional monoclonal antibody, the initiative of the recruit-bi-specific antibody undertaken by the method for genetically engineered and antibody engineering, at conventional monoclonal antibody mainly through CDC, ADCC and apoptosis capacity are come on the basis of killing tumor cell, add the immunotherapy of mediate T cell, substantially increase effect of immunity system killing tumor cell.
Particularly, the invention provides following technical scheme:
In one embodiment, provide a kind of bi-specific antibody, it is characterized in that, this antibody described comprises: (a) unit price unit, is light-heavy chain pair, and this light-heavy chain is to being selected from T cell, NK T cell or CIK cell for immunocyte; Preferably, this light-heavy chain has specific binding capacity to immune cell surface antigenic CD3; (b) strand unit, for fusogenic peptide, this fusogenic peptide comprises single chain variable fragment ScFv and has the Fc fragment of hinge area, CH2 structural domain and CH3 structural domain, wherein this fusogenic peptide has specific binding capacity for TCSA, preferably this TCSA is EpCAM, CD20, CD30 and CD133, and more preferably this TCSA is EpCAM.
In one embodiment, the CH2 structural domain of the strand unit of described bi-specific antibody is between ScFv fragment and CH3 structural domain.
In one embodiment, the single chain variable fragment of bi-specific antibody is made up of variable region of light chain and heavy chain variable domain, they all target in epitope EpCAM.
In one embodiment, in unit price unit, light chain is combined with heavy chain by disulfide linkage; Heavy chain is combined with described fusogenic peptide by one or more disulfide linkage.
In one embodiment, strand unit comprises the anti-EpCAM of antibody for EpCAM, and unit price unit comprises the anti-CD3 of antibody for CD3, preferably, the aminoacid sequence of described anti-CD3 heavy chain is the aminoacid sequence shown in sequence number 1, the aminoacid sequence of the light chain of anti-CD3 is the aminoacid sequence shown in sequence number 3, and the aminoacid sequence of described anti-EpCAM ScFv-Fc is the aminoacid sequence shown in sequence number 5, and the halfcystine of anti-CD3 heavy chain on 222 sites is connected with the form of disulfide linkage with the halfcystine on light chain 213 site of anti-CD3, described anti-CD3 heavy chain is connected with the form of disulfide linkage with the halfcystine on 263 and 266 sites of anti-EpCAM ScFv-Fc with the halfcystine on 231 sites respectively 228, described anti-CD3 heavy chain on 394 with 411 sites with 436 and 405 sites of anti--EpCAMScFv-Fc form salt bridge be connected, described anti-CD3 heavy chain on 368 sites with 441 sites of anti-EpCAMScFv-Fc are formed knuckle-enter-cave is connected.
In one embodiment, the heavy chain in unit price unit comprises people or humanized Fc fragment, and preferably, the Fc fragment of this heavy chain comprises human IgG Fc fragment; The Fc fragment of described fusogenic peptide comprises people or humanized Fc fragment, and preferably, the Fc fragment of this fusogenic peptide comprises human IgG Fc fragment.
In one embodiment, the human IgG Fc section of described unit price unit and the IgG Fc of described strand unit are by salt bridge and knuckle-enter-cave anatomical connectivity.
In one embodiment, provide a kind of preparation method of bi-specific antibody, described method comprises:
(1) respectively heavy, the light chain of unit price unit are building up on the first expression vector, by strand cell formation on the second expression vector respectively;
(2) by the first and second expression vectors together cotransfection in cell, cultivate and get supernatant;
(3) bi-specific antibody after obtaining purifying is separated by expressing supernatant; Preferably, described cell is CHO-S cell; Or preferably, described separating step comprises: the antibody of all band Fc structural domains caught by protein A affinity chromatography post from expressing supernatant, by being separated of SP cation-exchange chromatography realize target bi-specific antibody and by product, after Q post, finally concentrated displacement damping fluid PBS.
In one embodiment, the first expression vector is pCHO1.0; Second expression vector is pCHO1.0-Totomycin.
In one embodiment, described unit price unit is anti-CD 3 antibodies, its light chain the primer that increases is Kozak (EcoR V) F, MK-Leader (EcoRV) F, L2K-VL (MK) F1 and hIgK (PacI) R, increased by over-lap PCR, Kozak sequence, leader sequence and restriction enzyme site EcoR V and PacI are introduced light chain; Its heavy chain the primer that increases is Kozak (Avr II) F, MK-Leader (AvrII) F, L2K-VH (MK) F1 and hIgG1 (sbfI) R, increased by over-lap PCR, Kozak sequence, leader sequence and restriction enzyme site AvrII and BstZl7I are introduced heavy chain; By the LC gene fragment increased with carry out homologous recombination with the pCHO1.0 expression vector that EcoRV and PacI enzyme cuts through, acquisition loading anti-CD3 light chain expression vector; Then carry out homologous recombination with HC again after cutting with AvrII and BstZl7I enzyme, obtain the pCHO1.0 expression vector of anti-CD3, the anti-CD3-HL-LDY of plasmid called after pCHO1.0-;
Described strand unit is anti-EpCAM ScFv-Fc antibody, its the primer that increases is Kozak (Avr II) F, MK-Leader (AvrII) F, M701-VH F1 and hIgG1 (sbfI) R, by pcr amplification anti-EpCAM ScFv-Fc structural domain, by Kozak sequence, leader sequence and restriction enzyme site AvrII and BstZl7I introduce ScFv-Fc, the pCHO1.0-Totomycin expression vector gene fragment increased and enzyme cut through carries out homologous recombination, obtain the expression vector loading anti-EpCAM ScFv-Fc, plasmid called after pCHO1.0-Totomycin-anti-EpCAM-ScFv-Fc-KKW.
In one embodiment, above-mentioned arbitrary bi-specific antibody or preparing the purposes in medicine according to bi-specific antibody prepared by above-mentioned either method, described medicine be used for the treatment of EpCAM specific antigen express caused by tumour or relative disease, or express EpCAM cell for killing.
In one embodiment, above-mentioned arbitrary bi-specific antibody or preparing the purposes in medicine according to bi-specific antibody prepared by above-mentioned either method, described medicine is used for screening in human tumor cell line and is used for the treatment of the drug effect that the medicine of the tumour cell relative disease of expressing EpCAM specific antigen or evaluation be used for the treatment of the medicine of the tumour cell relative disease of expressing EpCAM specific antigen.Present invention also offers following technical scheme:
The invention provides a kind of novel method and prepare bi-specific antibody SMBODY (ScFv and monomer bispecific antibody) (as shown in Figure 2), this bi-specific antibody comprises two groups heavy light chain combination, wherein one group of a kind of antigen of specific combination, and some transformations are carried out in its heavy chain Fc district, make its versus wild type, not easily self forms dimer; And the another kind of antigen of another group specific combination, carry out other transformation equally in its heavy chain Fc district, also not easily self form dimer, and be easy between these two groups of heavy and light chains form heterozygosis dimer.And wherein the antibody structure of a group is single aggressiveness Ab, another group is ScFv-Fc, doing so avoids the possibility of respective light chain and the mispairing of the other side's heavy chain, thus forms the bi-specific antibody protein molecular of 125KD.After Fc transformation, the heavy chain of single aggressiveness Ab and strand nature different dimerization, natural dimerization between CL and CH1, finally forms SMBODY simultaneously, and each domain arrangement order of SMBODY and structural representation are shown in Fig. 2.
Utilize the above method preparing bi-specific antibody in the present invention, prepare bi-specific antibody.Be wherein the bi-specific antibody that is target spot with EpCAM and people source CD3, be named as M702, as Fig. 2, anti-CD3 is here IgG form, comprise anti-CD3 heavy chain and light chain, anti-EpCAM is here ScFv-Fc form, comprises anti-EpCAM VH, VL, Fc structural domain.Above bi-specific antibody is built by antibody genetic engineering method, single aggressiveness Ab heavy chain of bi-specific antibody SMBODY and single aggressiveness Ab light chain binary expression vector, and ScFv-Fc expression vector.According to the multiple clone site design primer in LC, HC, ScFv, Fc gene order and carrier.Wherein LC, HC, ScFv and Fc carry out pcr amplification respectively, obtain gene fragment, then cloned by homologous recombination method by PCR or Overlap extension PCR method.Enzyme cuts pCHO1.0 or pCHO1.0-hygromycin vector, then purifying reclaim PCR primer and enzyme cut after carrier, point two steps are respectively by LC fragment, and HC fragment homologous recombination is cloned on pCHO1.0 carrier, ScFv-Fc fragment homologous recombination is cloned on pCHO1.0-hygromycin vector, and checks order.The expression of recombinant protein SMBODY in mammalian cell, detection, use transfection reagent will to express the plasmid co-transfection of unit price unit heavy chain, unit price unit light chain and strand unit respectively in mammalian cell, regather the expression that supernatant carries out SDS-PAGE and western blotting detection SMBODY.By centrifugal for the nutrient solution supernatant after transfection expression, filter, with the dilution of binding buffer liquid, cross affinity column, elution buffer wash-out, SDS-PAGE detects protein purification.
The useful technique effect of technical scheme of the present invention has:
1. this application provides a kind of heterodimeric antibodies, this antibody comprises two different antigen-binding polypeptides unit.This heterodimer is different from its corresponding homodimer molecular size range, the size of molecular weight can be utilized to distinguish heterodimer and homodimer, thus more conveniently determine the purity of bi-specific antibody.One of these two antigen-binding polypeptides unit comprise the light-heavy chain pair being similar to wild-type antibodies, and in whole the application, this unit is also referred to as " unit price unit ".Another antigen-binding polypeptides unit comprises single chain variable fragment (scFv).Such scFv can merge the constant fragment (Fc) to antibody.In the application's full text, this fusogenic peptide is also referred to as " strand unit ".
2. the invention discloses foundation and the application thereof of a kind of outer effect experiment method of immunocyte contact element that novel bispecific antibodies SMBODY mediates.The present invention includes that the immunocyte mediated in bispecific antibody drug research process kills and wounds, the preparation of bi-specific antibody, and the foundation of bi-specific antibody pharmacy in vitro model and detection.Bi-specific antibody SMBODY comprises one group of unit price unit (heavy light chain combination), another group is then strand unit (ScFv connects Fc combination), the wherein tumor-cell antigen of a kind of people of strand unit specific combination, comprise a series of tumour cell film surface antigens such as EpCAM, and some transformations are carried out in its heavy chain Fc district, make its versus wild type, not easily self forms dimer; And the T cell antigen CD3 of another another kind of people of group unit price unit specific combination, carry out other transformation equally in its heavy chain Fc district, also not easily self form dimer, and be easy between these two groups of unit form heterodimer.Meanwhile, bi-specific antibody can erect bridge between target cell and functional molecular (cell), excites the immune response with guidance quality, has broad application prospects in the immunotherapy of tumour.
Surprisingly, the application proves that this asymmetrical antibody is stable and has high antigen joint efficiency.This makes us feeling surprised, even because the homodimer of verified single-chain antibody is in physiological conditions all unstable.Such as, Ahmad etc. " ScFv Antibody:Principles and Clinical Application; " Clinical and Developmental Immunology, 2012:980250 (2012), the IgG antibody-like shown based on ScFv is unstable, and needs transformation further assemble to reduce and improve stability.
In addition, because have asymmetry, heterodimer has and the homodimer difference iso-electric point be made up of wherein arbitrary antigen-binding polypeptides unit.Based on the iso-electric point difference between heterodimer and homodimer, easily the heterodimer of needs can be separated with homodimer, greatly reduce the difficulty that the ubiquitous downstream process exploitation of bi-specific antibody exists.
Accompanying drawing explanation
In order to be illustrated more clearly in the technical scheme in the embodiment of the present application, be briefly described to the accompanying drawing used required in embodiment below, apparent, the accompanying drawing that the following describes is only some embodiments recorded in the application, to those skilled in the art, under the prerequisite not paying creative work, other accompanying drawing can also be obtained according to these accompanying drawings, wherein:
Fig. 1 .CD3 schematic arrangement.
Fig. 2 .EpCAM × CD3 SMBODY bi-specific antibody molecule schematic diagram.
Fig. 3. electrophoresis detection PCR primer situation map; (A) M:DL1000 labeled nucleic acid molecule; 1. anti-cd 3 antibodies light chain; (B) M:DL2000 labeled nucleic acid molecule; 1. anti-cd 3 antibodies heavy chain; 2. anti-EpCAM antibody ScFv-Fc.
Fig. 4. the double antibody electrophoresis of purifying and purity detecting situation map; (4A) SDS-PAGE electrophoresis, M: protein markers; 1-2: irreducibility EpCAM × CD3 SMBODY double antibody; 3-4: reductibility EpCAM × CD3 SMBODY double antibody; (4B) the HPLC-SEC purity peak shape figure of EpCAM × CD3 SMBODY.
Fig. 5. the EpCAM × CD3 SMBODY double antibody measured based on flow cytometric analysis and the avidity situation map of HCT116 cell; (●) anti-EpCAM monoclonal antibody; (■) M702:EpCAM × CD3 SMBODY.
Fig. 6. the EpCAM × CD3 SMBODY double antibody measured based on flow cytometric analysis and the avidity situation map of Jurkat cell; (●) anti-CD3 monoclonal antibody L2K; (■) M702:EpCAM × CD3 SMBODY.
Fig. 7. flow cytometer detection EpCAM × CD3 SMBODY double antibody is simultaneously in conjunction with HCT116 and Jurkat cell situation map; (●) M702:EpCAM × CD3 SMBODY double antibody; (■) anti-EpCAM monoclonal antibody; (▲) anti-CD49d McAb L2K.
Fig. 8. the Tm value figure of differential scanning calorimeter sweep measurement EpCAM × CD3 SMBODY double antibody.
Fig. 9. antibody is Activity determination situation map after Overheating Treatment; 9A. and EpCAM binding activities detects, (●) anti-EpCAM monoclonal antibody; (▲) M702:EpCAM × CD3 SMBODY double antibody; 9B. and CD3 binding activities detects, (●) anti-CD3 monoclonal antibody L2K; (■) M702:EpCAM × CD3 SMBODY double antibody.
Figure 10 .CIK Phenotypic examination figure, the two positive NK class cell of the CD3 in the upper right corner, CD56.
Figure 11. under flow cytometer detection different concns antibody existence condition, effector cell CIK is to the lethal effect situation map of target cell HCT116 (Figure 11 A) and NCI-N87 (Figure 11 B); (■) M702:EpCAM × CD3 SMBODY double antibody, (▲) Anti-EpCAM monoclonal antibody, (▼) Mco101: contrast 4420X CD3 double antibody, (◆) hIgG: human IgG.
Figure 12. under flow cytometer detection different concns antibody existence condition, effector cell PBMC is to the lethal effect situation map of target cell HCT116 (Figure 12 A) and NCI-N87 (Figure 12 B); (■) M702:EpCAM × CD3 SMBODY double antibody, (▲) Mco101: contrast 4420X CD3 double antibody, (▼) Anti-EpCAM monoclonal antibody, (◆) hIgG: human IgG.
Figure 13. effect experiment result figure in double antibody body; (●) represents PBS, only tail vein is to PBS, () anti-EpCAM monoclonal antibody, (△) 4420 × CD3 unrelated control double antibody, (▼) M702-1:EpCAM × CD3 SMBODY double antibody 4mg/kg concentration group (zero) M702-2:EpCAM × CD3 SMBODY double antibody 2mg/kg concentration group.
Embodiment
Below in conjunction with specific embodiment, and in further detail the present invention is described with reference to accompanying drawing.Should be understood that the embodiment in present disclosure is in order to demonstrate the invention, but not limit the scope of the invention by any way.
Embodiment 1: the expression vector establishment (EpCAM × CD3 SMBODY, M702) of bi-specific antibody
1. bi-specific antibody sequences Design
The bi-specific antibody being target spot with EpCAM and CD3 is named as M702 (EpCAM × CD3 SMBODY), and as Fig. 2, anti-EpCAM is here ScFv-Fc form, comprises anti-EpCAM VH, VL, Fc structural domain; AntiCD3 McAb is here IgG form, comprises AntiCD3 McAb heavy chain and light chain, containing Fab and Fc structural domain.Wherein ScFv-Fc one side Fc carries out KKW transformation, IgG form on one side Fc carries out LDY transformation, and concrete Fc transformation process, see PCT/CN2012/084982, makes it not easily form homodimer separately, and be easy to be formed heterozygosis dimer, i.e. EpCAM × CD3 SMBODY bi-specific antibody., in order to dual anti-physical efficiency is expressed in Chinese hamster ovary celI, and can be secreted in substratum meanwhile, have selected the leader peptide sequences of mouse kappa as secreting signal peptide.The aminoacid sequence of each structural domain and signal peptide and nucleotide sequence are shown in following SEQ ID NO:1-8.Anti-CD3 heavy chain amino acid sequence (sequence number 1)
DIKLQQSGAELARPGASVKMSCKTSGYTFTRYTMHWVKQRPGQGLEWIGYINPSRGYTNYNQKFKDKATLTTDKSSSTAYMQLSSLTSEDSAVYYCARYYDDHYCLDYWGQGTTLTVSSASTKGPSVFPLAPSSKSTSGGTAALGCLVKDYFPEPVTVSWNSGALTSGVHTFPAVLQSSGLYSLSSVVTVPSSSLGTQTYICNVNHKPSNTKVDKKVEPKSCDKTHTCPPCPAPELLGGPSVFLFPPKPKDTLMISRTPEVTCVVVDVSHEDPEVKFNWYVDGVEVHNAKTKPREEQYNSTYRVVSVLTVLHQDWL NGKEYKCKVSNKALPAPIEKTISKAKGQPREPQVYTLPPSRDELTKNQVSLTCRVKGFYPSDIAVEWESNGQPENNYKTTPPVLKSDGSFFLASKLTVDKSRWQQGNVFSCSVMHEALHNHYTQKSLSLSPGK
Anti-CD3 heavy chain nucleic acid sequence (sequence number 2)
gatatcaaactgcagcagtcaggggctgaactggcaagacctggggcctcagtgaagatgtcctgcaagacttctggctacacctttactaggtacacgatgcactgggtaaaacagaggcctggacagggtctggaatggattggatacattaatcctagccgtggttatactaattacaatcagaagttcaaggacaaggccacattgactacagacaaatcctccagcacagcctacatgcaactgagcagcctgacatctgaggactctgcagtctattactgtgcaagatattatgatgatcattactgccttgactactggggccaaggcaccactctcacagtctcctcagcgtcgaccaagggcccatcggtcttccccctggcaccctcctccaagagcacctctgggggcacagcggccctgggctgcctggtcaaggactacttccccgaaccggtgacggtgtcgtggaactcaggcgccctgaccagcggcgtgcacaccttcccggctgtcctacagtcctcaggactctactccctcagcagcgtggtgaccgtgccctccagcagcttgggcacccagacctacatctgcaacgtgaatcacaagcccagcaacaccaaggtggacaagaaagttgagcccaaatcttgtgacaaaactcacacatgcccaccgtgcccagcacctgaactcctggggggaccgtcagtcttcctcttccccccaaaacccaaggacaccctcatgatctcccggacccctgaggtcacatgcgtggtggtggacgtgagccacgaagaccctgaggtcaagttcaactggtacgtggacggcgtggaggtgcataatgccaagacaaagccgcgggaggagcagtacaacagcacgtaccgtgtggtcagcgtcctcaccgtcctgcaccaggactggctgaatggcaaggagtacaagtgcaaggtctccaacaaagccctcccagcccccatcgagaaaaccatctccaaagccaaagggcagccccgagaaccacaggtgtacaccctgcccccatcccgggatgagctgaccaagaaccaggtcagcctgacctgccgggtcaaaggcttctatcccagcgacatcgccgtggagtgggagagcaatgggcagccggagaacaactacaagaccacgcctcccgtgctgaagtccgacggctccttcttcctcgccagcaagctcaccgtggacaagagcaggtggcagcaggggaacgtcttctcatgctccgtgatgcatgaggctctgcacaaccactacacgcagaagagcctctccctgtctccgggtaaatga
Anti-CD3 light-chain amino acid sequence (sequence number 3)
DIQLTQSPAIMSASPGEKVTMTCRASSSVSYMNWYQQKSGTSPKRWIYDTSKVASGVPYRFSGSGSGTSYSLTISSMEAEDAATYYCQQWSSNPLTFGAGTKLELKRTVAAPSVFIFPPSDEQLKSGTASVVCLLNNFYPREAKVQWKVDNALQSGNSQESVTEQDSKDSTYSLSSTLTLSKADYEKHKVYACEVTHQGLSSPVTKSFNRGEC
Anti-CD3 light chain nucleic acid sequence (sequence number 4)
gacattcagctgacccagtctccagcaatcatgtctgcatctccaggggagaaggtcaccatgacctgcagagccagttcaagtgtaagttacatgaactggtaccagcagaagtcaggcacctcccccaaaagatggatttatgacacatccaaagtggcttctggagtcccttatcgcttcagtggcagtgggtctgggacctcatactctctcacaatcagcagcatggaggctgaagatgctgccacttattactgccaacagtggagtagtaacccgctcacgttcggtgctgggaccaagctggagctgaaacgtacggtggctgcaccatctgtcttcatcttcccgccatctgatgagcagttgaaatctggaactgcctctgttgtgtgcctgctgaataacttctatcccagagaggccaaagtacagtggaaggtggataacgccctccaatcgggtaactcccaggagagtgtcacagagcaggacagcaaggacagcacctacagcctcagcagcaccctgacgctgagcaaagcagactacgagaaacacaaagtctacgcctgcgaagtcacccatcagggcctgagctcgcccgtcacaaagagcttcaacaggggagagtgttag
Anti-EpCAM ScFv-Fc aminoacid sequence (sequence number 5)
EVQLLEQSGAELVRPGTSVKISCKASGYAFTNYWLGWVKQRPGHGLEWIGDIFPGSGNIHYNEKFKGKATLTADKSSSTAYMQLSSLTFEDSAVYFCARLRNWDEPMDYWGQGTTVTVSSGGGGSGGGGSGGGGSELVMTQSPSSLTVTAGEKVTMSCKSSQSLLNSGNQKNYLTWYQQKPGQPPKLLIYWASTRESGVPDRFTGSGSGTDFTLTISSVQAEDLAVYYCQNDYSYPLTFGAGTKLEIKGAAAEPKSCDKTHTCPPCPAPELLGGPSVFLFPPKPKDTLMISRTPEVTCVVVDVSHEDPEVKFNWYVDGVEVHNAKTKPREEQYNSTYRVVSVLTVLHQDWLNGKEYKCKVSNKALPAPIEKTISKAKGQPREPQVYTLPPSRDELTKNQVSLWCLVKGFYPSDIAVEWESNGQPENNYDTTPPVLDSDGSFFLYSDLTVDKSRWQQGNVFSCSVMHEALHNHYTQKSLSLSPGK
Anti-EpCAM ScFv-Fc nucleotide sequence (sequence number 6)
gaggtgcagctgctcgagcagtctggagctgagctggtaaggcctgggacttcagtgaagatatcctgcaaggcttctggatacgccttcactaactactggctaggttgggtaaagcagaggcctggacatggacttgagtggattggagatattttccctggaagtggtaatatccactacaatgagaagttcaagggcaaagccacactgactgcagacaaatcttcgagcacagcctatatgcagctcagtagcctgacatttgaggactctgctgtctatttctgtgcaagactgaggaactgggacgagcctatggactactggggccaagggaccacggtcaccgtctcctccggaggcggcggttcaggcggaggtggaagtggtggaggaggttctgagctcgtgatgacacagtctccatcctccctgactgtgacagcaggagagaaggtcactatgagctgc aagtccagtcagagtctgttaaacagtggaaatcaaaagaactacttgacctggtaccagcagaaaccagggcagcctcctaaactgttgatctactgggcatccactagggaatctggggtccctgatcgcttcacaggcagtggatctggaacagatttcactctcaccatcagcagtgtgcaggctgaagacctggcagtttattactgtcagaatgattatagttatccgctcacgttcggtgctgggaccaagcttgagatcaaaggtgcggccgcagagcccaaatcttgtgacaaaactcacacatgcccaccgtgcccagcacctgaactcctggggggaccgtcagtcttcctcttccccccaaaacccaaggacaccctcatgatctcccggacccctgaggtcacatgcgtggtggtggacgtgagccacgaagaccctgaggtcaagttcaactggtacgtggacggcgtggaggtgcataatgccaagacaaagccgcgggaggagcagtacaacagcacgtaccgtgtggtcagcgtcctcaccgtcctgcaccaggactggctgaatggcaaggagtacaagtgcaaggtctccaacaaagccctcccagcccccatcgagaaaaccatctccaaagccaaagggcagccccgagaaccacaggtgtacaccctgcccccatcccgggatgagctgaccaagaaccaggtcagcctgtggtgcctggtcaaaggcttctatcccagcgacatcgccgtggagtgggagagcaatgggcagccggagaacaactacgataccacgcctcccgtgctggactccgacggctccttcttcctctacagcgatctcaccgtggacaagagcaggtggcagcaggggaacgtcttctcatgctccgtgatgcatgaggctctgcacaaccactacacgcagaagagcctctccctgtctccgggtaaatga
The leader peptide sequences aminoacid sequence (sequence number 7) of mouse kappa
METDTLLLWVLLLWVPGSTG
The leader peptide sequences nucleotide sequence (sequence number 8) of mouse kappa
atggagacagacacactcctgctatgggtactgctgctctgggttccaggttccactggt
2. bi-specific antibody gene clone
PCHO1.0 is selected to remove heavy chain and the light chain gene of cloning and expressing AntiCD3 McAb as expression vector, pCHO1.0-Totomycin expression vector is the tetracycline genetic modification by replacing by hygromycin gene in pCHO1.0 carrier, is selected to the ScFv-Fc fusion gene of cloning and expressing anti-EpCAM.After primer in table 2 designs according to cloning approach, be sent to Jin Weizhi bio tech ltd, Suzhou and synthesize.Pcr amplification is carried out with the primer in table 1, template is gene chemical synthesis or the gene plasmid that is subcloned on pCDNA3.1 or pUC57 in earlier trials, PCT/CN2012/084982 patent has a detailed description, then anti-CD3 is heavy, light chain is building up on the expression vector of pCHO1.0 respectively respectively, is building up to by anti-EpCAM ScFv-Fc on the expression vector of pCHO1.0-Totomycin.
The primer used in the gene clone of table 2. bi-specific antibody
The template DNA of initial PCR amplification template DNA: 35ng, e.g., the light chain of target antibody and heavy chain; 10 μMs of forward primers of 1 μ l and reverse primer; The 10x PCR Buffer damping fluid of 2.5 μ l; The 10mM dNTP of 1 μ l; 2.5 units/μ l Pyrobest archaeal dna polymerase (Takara, R005A) of 1 μ l; Softly mix in microfuge pipe to 25 μ l cumulative volumes with distilled water, and in Eppendorf centrifuge fast rotational to collect at the bottom of reaction mixture to pipe.GeneAmp PCR System 9700 (Applied Biosystem) and following setting is used to carry out PCR reaction: 95 DEG C, 5 minutes; 25 following circulations: 95 DEG C, each 30 seconds; 56 DEG C, 30 seconds; With 72 DEG C, 1 minute.
Take turns overlapping pcr amplification by several, Kozak sequence, leader sequence and restriction enzyme site EcoR V and PacI are introduced light chain (Fig. 3); And Kozak sequence, leader sequence and restriction enzyme site AvrII and BstZl7I are introduced heavy chain (see Fig. 3) by corresponding primer.First by the LC gene fragment increased with carry out homologous recombination with the pCHO1.0 expression vector that EcoR V and PacI enzyme cut through, acquisition loading anti-CD3 light chain expression vector; Then carry out homologous recombination with HC again after cutting with AvrII and BstZl7I enzyme, obtain the pCHO1.0 expression vector of anti-CD3, the anti-CD3-HL-LDY of plasmid called after pCHO1.0-.
By over-lap PCR amplification anti-EpCAM ScFv-Fc structural domain, and Kozak sequence, leader sequence and restriction enzyme site AvrII and BstZl7I are introduced ScFv-Fc, the pCHO1.0-Totomycin expression vector that the gene fragment increased (Fig. 3) and enzyme cut through is carried out homologous recombination, obtain the expression vector loading anti-EpCAM ScFv-Fc, plasmid called after pCHO1.0-Totomycin-anti-EpCAM-ScFv-Fc-KKW.
Embodiment 2: bi-specific antibody expression and purification
1. the expression of bi-specific antibody
Utilization is carried out plasmid without the large extraction reagent kit of intracellular toxin (Qiagen, 12391) and is carried greatly, and the specification sheets that concrete operations provide according to manufacturer carries out.The specification sheets that CHO-S cell cultures provides according to manufacturer, in CD CHO substratum (Gibco, 10743-029), is placed in 37 DEG C, 5%CO 2cultivate in cell culture incubator, after getting out cell, according to the specification sheets (Maxcyte) of manufacturers, use Maxcyte STX electroporation by anti-for plasmid pCHO1.0-CD3-HL-LDY and pCHO1.0-Totomycin-anti-EpCAM-ScFv-Fc-KKW together cotransfection in CHO-S cell, these two kinds of plasmids of design cotransfection are to express the bi-specific antibody to EpCAM × CD3.
The 2nd day after transfection, culture temperature was lowered to 32 DEG C, and every day adds 3.5%FeedA, cultivated after 14 days, and 800*g harvested by centrifugation expresses supernatant.
2. the purifying of bi-specific antibody
Express supernatant 0.22uM membrane filtration, utilize Mabselect SuRe affinity column (purchased from GE company, 18-1153-45,17-5438-01) from expressing supernatant the antibody of catching all band Fc structural domains, with level pad (9.5mM NaH 2pO 4+ 40.5mM Na 2hPO 4, pH7.0) balance chromatography column after, cross affinity column, with elution buffer (50mM citric acid+100mM arginine, pH3.2) wash-out.By SP cation-exchange chromatography, realize target bi-specific antibody is separated with by product, cationic exchange coloum purchased from GE company (18-1153-44,17-1087-01), with level pad A (43.8mM NaH 2pO 4+ 6.2mM Na 2hPO 4, pH 6.0) and after balance chromatography column, sample, with between two pure water dilution conductance to 3.0-3.5ms, is crossed after SP pillar combines, with elution buffer B (43.8mM NaH 2pO 4+ 6.2mM Na 2hPO 4+ 1M NaCl, pH 6.0) 20 column volume linear elutions; Finally concentrated displacement damping fluid PBS.Bi-specific antibody after purifying carries out SDS-PAGE, SEC and detects, and purity is (see Fig. 4) more than 95%.
Embodiment 3: the binding activities of bi-specific antibody and cell measures (FACS)
The target antigen of bi-specific antibody of the present invention on corresponding cell is combined.The present invention is using HCT116 (purchased from ATCC, CCL-247) as the cell of the EpCAM positive, and Jurkat (Jurkat, TIB-152) as the cell of the CD3 positive, and measures its cell-bound activity with double antibody prepared by the present invention.
1. utilize flow cytometer showed method to detect the binding activities of bi-specific antibody and HCT116 cell
Cultivate enough HCT116 cells, with 0.25% trysinization, centrifugal collecting cell.Dilute bi-specific antibody, concentration is from 500nmol, and 3 times of gradient dilutions, obtain 12 concentration gradients, for subsequent use simultaneously.The cell PBS+1%FBS of collection is washed twice, then adds PBS+1%FBS re-suspended cell to 4 × 10 6individual cell/ml, plating cells in 96 orifice plates, every hole 50ul (2 × 10 5individual cell), add the bi-specific antibody that 50ul has diluted, incubated at room 1 hour; Centrifugally remove supernatant, cell is washed twice with PBS, again with the anti-human igg FC antibody (Biolegend of the PE mark diluted, 409304) re-suspended cell, room temperature lucifuge hatches 30 minutes, and PBS washes twice, use 100ul PBS resuspended again, upper machine testing, then with average fluorescent strength, by carrying out the binding affinity KD value of analytical calculation double antibody and HCT116 with software GraphPad Prism5.0.The HCT116 cell of result display EpCAM × CD3SMBODY double antibody and the EpCAM positive has good binding activities, and see Fig. 5, its KD value is only 69.82nM, has good cell-bound activity.
2. flow cytometer showed method detects the binding activities of bi-specific antibody and Jurkat cell
Cultivate enough Jurkat suspension cells, centrifugal collecting cell.Ensuing experimentation is same as the previously described embodiments, by cell resuspended for 100ul PBS, and upper machine testing, then with average fluorescent strength, by carrying out the binding affinity KD value of analytical calculation double antibody and Jurkat cell with software GraphPad Prism5.0.The Jurkat cell of result display EpCAM × CD3 SMBODY double antibody and the CD3 positive has good binding activities, and see Fig. 6, its KD value is only 50.90nM, has good cell-bound activity.
3. the common binding activities of double antibody mediation detects
By cultured HCT116 and Jurkat cell, collected by centrifugation also washes 2 times with PBS, respectively with CFSE and PKH-26 dyeing.Dilute bi-specific antibody, concentration is from 10ug/ml, and 3 times of gradient dilutions, obtain 12 concentration gradients, for subsequent use simultaneously.By the HCT116 dyeed with Jurkat cell is centrifugal removes supernatant, wash twice with PBS+1%FBS, then add PBS+1%FBS re-suspended cell to 4 × 10 6individual cell/ml, mixes by 1:1, by plating cells in 96 orifice plates, and every hole 50ul (2 × 10 5individual cell), add the bi-specific antibody that 50ul has diluted, incubated at room 1 hour; Centrifugally removing supernatant, wash cell twice with PBS, finally use 100ul PBS resuspended, upper machine testing, analyzing the ratio of two positive cell, by carrying out analytical calculation with software GraphPad Prism5.0.Result when show there is no a M702, the ratio very low (Fig. 7) of the two fluorescence of flow cytometer detection; When adding EpCAM × CD3 double antibody M702, the ratio of the two fluorescence of flow cytometer detection reaches about 40%, show that M702 simultaneously in conjunction with the HCT116 cell of the EpCAM positive and the Jurkat cell of the CD3 positive, can promote the aggregation of two kinds of cells, form an immunologic cytotoxicity complex body.
Embodiment 4: the thermal stability determination of bi-specific antibody
1. the Tm pH-value determination pH of bi-specific antibody
The thermostability of bi-specific antibody is by differential scanning calorimeter (MicroCal VP-DSC, GE company) measure, double antibody Sample Purification on Single rear substitution is in PBS damping fluid, with PBS damping fluid in contrast, calorimetric scan data are carried out scanning with the heating rate of 60 DEG C/h from 10 DEG C to 100 DEG C and are obtained.Scanning result (Fig. 8) shows, and the Tm value of bi-specific antibody, all more than 70 DEG C, shows except good thermostability.
2. the hot challenge experiment of bi-specific antibody
Single chain antibody fragments (ScFv) is coupled together variable region of heavy chain and variable region of light chain by a connection peptides (Gly4Ser) 3 and is formed.But there is the unstable of report ScFv inherence may affect quality (the Michaelson JS1 of antibody drug, etc., Anti-tumor activity of stability-engineered IgG-like bispecific antibodies targeting TRAIL-R2 and LTbetaR.MAbs.2009Mar-Apr; 1 (2): 128-41).Therefore, antibody dilution to 0.4mg/ml, is distinguished 4 DEG C, 37 DEG C, 42 DEG C, 47 DEG C, 52 DEG C, 57 DEG C, 62 DEG C, 67 DEG C, 72 DEG C, 77 DEG C, 82 DEG C, PCR instrument process 1h, often pipe 15ul by us.Centrifuging and taking supernatant, carries out flow cytometer detection according to following steps, collects single cell suspension and adds 96 orifice plates, 3 × 10 5/ hole, adds various process antibody, and adds fluorescence two and resist, and machine testing in streaming, the results are shown in Figure 9, Fig. 9 A and determine Anti-EpCAM and EpCAM × CD3SMBODY bi-specific antibody in the thermostability in conjunction with EpCAM, its T 50value be respectively 73.28 and 58.31, Fig. 9 B determine the thermostability of L2K and EpCAM × CD3 MSBODY bi-specific antibody at the antibody in conjunction with CD3, its T 50value is respectively 69.33 and 61.30, all shows good thermostability.
Embodiment 5: the cell in vitro of double antibody mediation kills and wounds detection
The separation of 1.PBMC cell and CIK cell are cultivated
Get fresh anticoagulation, the centrifugal 5min of 400g, abandons supernatant.Add the erythrocyte cracked liquid of 10 times of cell volumes, blow and beat mixing gently, room temperature or on ice cracking 4-5 minute.Should suitably shake to promote erythrocyte splitting in cracking process.4 DEG C of centrifugal 5min of 400g, abandon red supernatant.If erythrocyte splitting is incomplete, repeating step 2 and 3 once.Wash 1-2 time.Add the PBS of 5 times of cell precipitation volumes, resuspended precipitation, 4 DEG C of centrifugal 2-3 minute of 400g, abandon supernatant.1 time can be repeated again, wash 1-2 time altogether.Experimentally need can carry out the subsequent experimental such as counting with after suitable 4 DEG C of PBS re-suspended cells precipitation.
The cultivation of CIK cell, fills 30ml with CIK cell Primary culture liquid (serum-free X-Vivo cell culture fluid+750IU/ml IFN-γ ± 2% autologous plasma) by every part of cell, is added in 75cm2 culturing bottle, is placed in saturated humidity, 37 DEG C, 5.0%CO 2incubator is cultivated.Cultivate after 24 hours, add CIK cell stimulating factor mixed solution 1ml (serum-free X-Vivo cell culture fluid+75ng/ml Anti-Human CD3 ε, 750IU/ml IL-2,0.6ng/ml IL-1 α), continue to be placed in saturated humidity, 37 DEG C, 5.0%CO 2cultivate in incubator.Following step determines the thing of fluid infusion (serum-free X-Vivo nutrient solution+750IU/ml IL-2 ± 2% autologous plasma), sub-bottle according to the growing state of CIK cell, substantially will maintain cell and grow about the concentration of 2*10^6.Finally with flow cytometer FC500, Phenotypic examination is carried out to the CIK cell of collecting, comprising: CD3, CD56, CD4, CD8, detect the expression of these cell-surface antigenss in CIK cell.Detected result is shown in Figure 10, and phenotypic results display CIK cell has the two positive of CD3 and CD56 of more than 15.9%, and cultured cells has the ratio of good NK T cell.
2. double antibody effectively mediates the detection of PBMC cell killing tumour cell
With trysinization HCT116 or NCI-N87 cell, prepare single cell suspension.With final concentration be 5uM CFSE dye HCT116 or NCI-N87, after dyeing with the 10%FBS-1640 of this cell cultures by resuspended for cell to 2 × 10 5/ ml, according to 2 × 10 4/ hole, namely 100ul/ hole adds 96 orifice plate overnight incubation.Experimental design adds the CIK cell of cultivation, and 50ul/ hole, arranges control wells, and the substratum without the need to the Kong Zeyong same volume adding CIK cell fills into.Empirically design while adding CIK cell and add corresponding antibodies, 50ul/ hole, the substratum without the need to the Kong Zeyong same volume adding antibody fills into.Taking out 96 orifice plates after 48h, is single cell suspension with each porocyte of trysinization, and all supernatants in this process and the equal correspondence of cell suspension are collected in 1.5ml EP pipe, centrifugal 500g × 5min.Abandon supernatant, each hole adds the resuspended mixing cell of 150ul 1%FBS-PBS.Each pipe in streaming before machine 10-15min to add in PI (final concentration is 1ug/ml) streaming the two positive cell of machine testing CFSE, PI and account for the mortality ratio that CFSE positive cell ratio is target cell HCT116 or NCI-N87.The results are shown in Figure 11, cell killing result display EpCAM × CD3 SMBODY Mediated by Bi-specific Antibodies CIK cell killing tumor cell shows good fragmentation effect, and its maximum killing-efficiency and EC50 are obviously better than Anti-EpCAM monoclonal antibody.
3. double antibody effectively mediates the detection of PBMC cell killing tumour cell
With trysinization HCT116 cell, prepare single cell suspension.With final concentration be 5uM CFSE dye HCT116 or NCI-N87, after dyeing with the 10%FBS-1640 of this cell cultures by resuspended for cell to 2 × 10 5/ ml, according to 2 × 10 4/ hole, namely 100ul/ hole adds 96 orifice plate overnight incubation.Experimental design adds the CIK cell of cultivation, and 50ul/ hole, arranges control wells, and the substratum without the need to the Kong Zeyong same volume adding CIK cell fills into.Empirically design while adding CIK cell and add corresponding antibodies, 50ul/ hole, the substratum without the need to the Kong Zeyong same volume adding antibody fills into.Taking out 96 orifice plates after 48h, is single cell suspension with each porocyte of trysinization, and all supernatants in this process and the equal correspondence of cell suspension are collected in 1.5ml EP pipe, centrifugal 500g × 5min.Abandon supernatant, each hole adds the resuspended mixing cell of 150ul 1%FBS-PBS.Each pipe in streaming before machine 10-15min to add in PI (final concentration is 1ug/ml) streaming the two positive cell of machine testing CFSE, PI and account for the mortality ratio that CFSE positive cell ratio is target cell HCT116.The results are shown in Figure 12, cell killing result display EpCAM × CD3 SMBODY Mediated by Bi-specific Antibodies CIK cell killing tumor cell shows good fragmentation effect, and its maximum killing-efficiency and EC50 are obviously better than Anti-EpCAM monoclonal antibody.
Embodiment 6: bi-specific antibody kills and wounds the Composition analyzed of subcutaneous transplantation knurl
The foundation of Tumor Xenograft Models is by by 5 × 10 6sW480 and 5 × 10 6cIK cell mixes, and forms (N=8 group) in female NOD/SCID mouse right dorsal subcutaneous inoculation growth.In 2 hours, mouse random packet, Antybody therapy group, starts, with 4,2mg/kg EpCAM × CD3 SMBODY, to carry out intravenous injection respectively by tail vein.Control group comprises one group of anti-EpCAM monoclonal antibody with 4mg/kg and one group of nothing to do with control SMBODY (4420 × CD3).Contrast SMBODY is that a kind of anti-fluorescein antibody (4-4-20) sequence construct forms (Kranz DM, Voss EW Jr.Partial elucidation of an anti-hapten repertoire in BALB/c mice:comparative characterization of several monoclonal antifluorescyl antibodies.Mol Immunol.1981; 18 (10): 889-898).And continue to continue the identical dosage of administration at the 2nd day with the 4th day.At corresponding control animals intravenous injection PBS.Within every three days, result calculates and adopts following formula to carry out: 1/2 × length x width x width (mm with digital vernier kind of calliper gross tumor volume 3).
Antitumous effect assessment in EpCAM × CD3SMBODY body is completed by adoptive transfer Transplanted tumor model.Gastric cancer tumor clone SW480 is used to set up Transplanted tumor model on immunodeficient mouse NOD/SCID, and people's CIK cell, by after separating peripheral blood mononuclear cells, stimulates to cultivate and gets, 1:1 ratio combined inoculation before inoculation.As Figure 13 display, PBS group, control antibodies Anti-EpCAM, 4420 × CD3 Antybody therapy all to tumor growth without obvious suppression, but EpCAM × CD3 (2mg/kg, 4mg/kg) treatment group does not find tumor growth in same experiment, therefore, the immune tumor-killing that EpCAM × CD3 SMBODY mediates can obviously Tumor suppression growth.Also as expected, even if remain with CD3 specific molecular, but lack during EpCAM specific SMBODY molecule MCO101 (4420 × CD3) tests in vivo and can not demonstrate significant anti-tumor activity.
Should be understood that the present invention of disclosure is not limited only to specific method, scheme and the material described, because these equal alterable.Will also be understood that terminology used here is only used to describe the object of specific embodiment scheme, instead of be intended to limit the scope of the invention, scope of the present invention is only limited to appended claim.
Those skilled in the art also will recognize, or can confirm that use is no more than normal experiment, in this article many Equivalents of described specific embodiment of the present invention.These Equivalents are intended to comprise in the appended claims.

Claims (12)

1. bi-specific antibody, is characterized in that, described antibody comprises: (a) unit price unit, is light-heavy chain pair, and this light-heavy chain is to being selected from T cell, NKT cell or CIK cell for immunocyte; Preferably, this light-heavy chain has specific binding capacity to immune cell surface antigenic CD3; (b) strand unit, for fusogenic peptide, this fusogenic peptide comprises single chain variable fragment ScFv and has the Fc fragment of hinge area, CH2 structural domain and CH3 structural domain, wherein this fusogenic peptide has specific binding capacity for TCSA, preferably this TCSA is EpCAM, CD20, CD30 and CD133, and more preferably this TCSA is EpCAM.
2. described bi-specific antibody according to claim 1, is characterized in that: the CH2 structural domain of strand unit is between ScFv fragment and CH3 structural domain.
3. described bi-specific antibody according to claim 1, is characterized in that: described single chain variable fragment is made up of variable region of light chain and heavy chain variable domain, they all target in epitope EpCAM.
4. described bi-specific antibody according to claim 1, is characterized in that: in described unit price unit, light chain is combined with heavy chain by disulfide linkage; Described heavy chain is combined with described fusogenic peptide by one or more disulfide linkage.
5. the described bi-specific antibody of claim 1, is characterized in that: strand unit comprises the anti-EpCAM of antibody for EpCAM, and unit price unit comprises the anti-CD3 of antibody for CD3;
Preferably, the aminoacid sequence of described anti-CD3 heavy chain is the aminoacid sequence shown in sequence number 1, the light-chain amino acid sequence of anti-CD3 is the aminoacid sequence shown in sequence number 3, and the aminoacid sequence of described anti-EpCAM ScFv-Fc is the aminoacid sequence shown in sequence number 5, and the halfcystine of anti-CD3 heavy chain on 222 sites is connected with the form of disulfide linkage with the halfcystine on light chain 213 site of anti-CD3, described anti-CD3 heavy chain is connected with the form of disulfide linkage with the halfcystine on 263 and 266 sites of anti-EpCAM ScFv-Fc with the halfcystine on 231 sites respectively 228, described anti-CD3 heavy chain on 394 with 411 sites with 436 and 405 sites of anti--EpCAM ScFv-Fc form salt bridge be connected, described anti-CD3 heavy chain on 368 sites with 441 sites of anti-EpCAM ScFv-Fc are formed knuckle-enter-cave is connected.
6. described bi-specific antibody according to claim 1, is characterized in that: the heavy chain in described unit price unit comprises people or humanized Fc fragment, and preferably, the Fc fragment of this heavy chain comprises human IgG Fc fragment; The Fc fragment of described fusogenic peptide comprises people or humanized Fc fragment, and preferably, the Fc fragment of this fusogenic peptide comprises human IgG Fc fragment.
7. described bi-specific antibody according to claim 6, is characterized in that: the human IgG Fc section of described unit price unit and the IgG Fc of described strand unit are by salt bridge and knuckle-enter-cave anatomical connectivity.
8. prepare the method for bi-specific antibody according to any one of claim 1-7, it is characterized in that, described method comprises step:
(1) respectively heavy, the light chain of unit price unit are building up on the first expression vector, by strand cell formation on the second expression vector respectively;
(2) by the first and second expression vectors together cotransfection in cell, cultivate and get supernatant;
(3) bi-specific antibody after obtaining purifying is separated by expressing supernatant; Preferably, described cell is CHO-S cell; Or preferably, described separating step comprises: the antibody of all band Fc structural domains caught by protein A affinity chromatography post from expressing supernatant, by being separated of SP cation-exchange chromatography realize target bi-specific antibody and by product, after Q post, finally concentrated displacement damping fluid PBS.
9. described method according to claim 8, described first expression vector is pCHO1.0; Described second expression vector is pCHO1.0-Totomycin.
10. described method according to claim 8, is characterized in that, in the step (1) of described method:
Described unit price unit is anti-CD 3 antibodies, its light chain the primer that increases is Kozak (EcoR V) F, MK-Leader (EcoRV) F, L2K-VL (MK) F1 and hIgK (PacI) R, increased by over-lap PCR, Kozak sequence, leader sequence and restriction enzyme site EcoR V and PacI are introduced light chain; Its heavy chain the primer that increases is Kozak (Avr II) F, MK-Leader (AvrII) F, L2K-VH (MK) F1 and hIgG1 (sbfI) R, increased by over-lap PCR, Kozak sequence, leader sequence and restriction enzyme site AvrII and BstZl7I are introduced heavy chain; By the LC gene fragment increased with carry out homologous recombination with the pCHO1.0 expression vector that EcoR V and PacI enzyme cut through, acquisition loading anti-CD3 light chain expression vector; Then carry out homologous recombination with HC again after cutting with AvrII and BstZl7I enzyme, obtain the pCHO1.0 expression vector of anti-CD3, the anti-CD3-HL-LDY of plasmid called after pCHO1.0-;
Described strand unit is anti-EpCAM ScFv-Fc antibody, its the primer that increases is Kozak (Avr II) F, MK-Leader (AvrII) F, M701-VH F1 and hIgG1 (sbfI) R, by pcr amplification anti-EpCAM ScFv-Fc structural domain, by Kozak sequence, leader sequence and restriction enzyme site AvrII and BstZl7I introduce ScFv-Fc, the pCHO1.0-Totomycin expression vector gene fragment increased and enzyme cut through carries out homologous recombination, obtain the expression vector loading anti-EpCAM ScFv-Fc, plasmid called after pCHO1.0-Totomycin-anti-EpCAM-ScFv-Fc-KKW.
Bi-specific antibody prepared by bi-specific antibody according to any one of 11. claim 1-7 or the method according to the bi-specific antibody prepared any one of claim 8-10 is preparing the purposes in medicine, described medicine be used for the treatment of EpCAM specific antigen express caused by tumour or relative disease, or express EpCAM cell for killing.
Bi-specific antibody prepared by bi-specific antibody according to any one of 12. claim 1-7 or the method according to the bi-specific antibody prepared any one of claim 8-10 is preparing the purposes in medicine, and described medicine is used for the treatment of the drug effect of the medicine of the tumour cell relative disease of expressing EpCAM specific antigen for the medicine or evaluation screening the tumour cell relative disease being used for the treatment of expression EpCAM specific antigen in tumor cell line.
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CN113527491A (en) * 2020-08-19 2021-10-22 上海易慕峰生物科技有限公司 Humanized antibody, chimeric antigen receptor, nucleic acid, vector, cell and application
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