«Previous Article|Table of Contents|Next Article»

《南京师大学报（自然科学版）》[ISSN:1001-4616/CN:32-1239/N]

Issue:

2017年02期

Page:

51-

Research Field:

·生命科学·

Publishing date:

Info

Title:

Bispecific Anti-CD3×Anti-CD87 Single-Chain Antibody Mediates CytolyticActivity of Mononuclear Cells Against CD87-Positive Prostate Cancer in vitro

Author(s):

Gao Wanli; Yang Li; Liu Shan; Zhao Zhihui

School of Life Sciences,Nanjing Normal University,Institute of Biochemistry and Biological Products,Jiangsu Key Laboratory for Molecular and Medical Biotechnology,Nanjing 210023,China

Keywords:

single chain bispecific antibody; cytotoxity; prostate cancer; prokaryotic expression

PACS:

Q819

DOI:

10.3969/j.issn.1001-4616.2017.02.009

Abstract:

In this study,the aim was to investigate whether anti-CD3×anti-CD87 single-chain bi-functional specific antibody(scBsAb)could mediate the cytotoxicity of peripheral blood mononuclear cells(PBMCs)against CD87-positive prostatic cancer cells. First,the prokaryotic expression vector of pET24a/scBsAb was constructed and transformed into competent cells of E.coil BL-21(DE3)by genetic engineering technique. After induction with IPTG,the bacteria were ultrasonicated,and scBsAb in the form of inclusion bodies were harvested by centrifugation. The scBsAb was further purified by affinity chromatography under denaturing conditions and refolded by dilution. Second,the antigens binding activity of scBsAb was examined by flow cytometry. Lastly,the scBsAb-mediated cytotoxicity of PBMCs against CD87-positive prostatic cancer cell line PC-3 was determined by using CCK-8 assay. Our results showed that the scBsAb with high purity was obtained. scBsAb could both specifically bind to CD87 and CD3. The scBsAb-mediated killing of PBMCs against CD87⁺ PC-3 cells was related to the concentration of used scBsAb and the ratio of effector to target(E:T). When E:T was 10:1 and the scBsAb concentration was 100 μg/mL,the killing rate was 40.86%; whereas when the E:T ratio was 40:1 and scBsAb concentration was 100 μg/mL,the killing rate was 60.9%. In addition,ELISA assay showed that IFN-γ level in the co-culture system was significantly increased during the killing process. Our data indicate that anti-CD3×anti-CD87 scBsAb could mediate PBMCs to kill CD87-positive tumor cells in vitro.

References:

[1] 方敏,赵瑞,李骅,等. 抗人卵巢癌×抗人CD3双特异性单链抗体的构建,表达及复性研究[J]. 高技术通讯,2002,12(11):47-50.
[2]ARNDT C,FELDMANN A,T?PFER K,et al. Redirection of CD4⁺ and CD8⁺ T lymphocytes via a novel antibody-based modular targeting system triggers efficient killing of PSCA⁺ prostate tumor cells[J]. The prostate,2014,74(13):1 347-1 358.
[3]WOLF E,HOFMEISTER R,KUFER P,et al. BiTEs:bispecific antibody constructs with unique anti-tumor activity[J]. Drug discovery today,2005,10(18):1 237-1 244.
[4]NIELSEN L,KELLERMAN G,BEHRENDT N,et al. A 55 000-60 000 Mr receptor protein for urokinase-type plasminogen activator. Identification in human tumor cell lines and partial purification[J]. Journal of biological chemistry,1988,263(5):2 358-2 363.
[5]GE Y,ELGHETANY M T. Urokinase plasminogen activator receptor(CD87):something old,something new[J]. Laboratory hematology,2003,9:67-72.
[6]PLESNER T,BEHRENDT N,PLOUG M. Structure,function and expression on blood and bone marrow cells of the urokinase-type plasminogen activator receptor,uPAR[J]. Stem cells,1997,15(6):398-408.
[7]GHANNADAN M,BAGHESTANIAN M,WIMAZAL F,et al. Phenotypic characterization of human skin mast cells by combined staining with toluidine blue and CD antibodies[J]. Journal of investigative dermatology,1998,111(4):689-695.
[8]EBNER S,LENZ A,REIDER D,et al. Expression of maturation-/migration-related molecules on human dendritic cells from blood and skin[J]. Immunobiology,1998,198(5):568-587.
[9]HADDOCK R C,SPELL M,BAKER C,et al. Urokinase binding and receptor identification in cultured endothelial cells[J]. Journal of biological chemistry,1991,266(32):21 466-21 473.
[10]MORITA Y,HAYASHI Y,WANG Y,et al. Expression of urokinase-type plasminogen activator receptor in hepatocellular carcinoma[J]. Hepatology,1997,25(4):856-861.
[11]赵茜,吴秋良,梁小曼,等. uPA,uPAR,nm23-HI在大肠癌中的表达及其与肿瘤侵袭和转移的关系[J]. 肿瘤防治研究,2004,31(11):695.
[12]KIPRIYANOV S M,MOLDENHAUER G,MARTIN A,et al. Two amino acid mutations in an anti-human CD3 single chain Fv antibody fragment that affect the yield on bacterial secretion but not the affinity[J]. Protein engineering,1997,10(4):445-453.
[13]LI Y,PARRY G,CHEN L,et al. An anti-urokinase plasminogen activator receptor(uPAR)antibody:crystal structure and binding epitope[J]. Journal of molecular biology,2007,365(4):1 117-1 129.
[14]范冬梅,李崴,杨铭,等. 双功能抗体抗CD3/抗CD19介导T细胞对靶细胞的杀伤作用[J]. 中国癌症杂志,2011,21(1):6-11.
[15]RATHI C,MEIBOHM B. Clinical pharmacology of bispecific antibody constructs[J]. The journal of clinical pharmacology,2015,55(S3):S21-S28.
[16]MORECKI S,LINDHOFER H,YACOVLEV E,et al. Induction of long-lasting antitumor immunity by concomitant cell therapy with allogeneic lymphocytes and trifunctional bispecific antibody[J]. Experimental hematology,2008,36(8):997-1003.
[17]XIE Z,NING G,MING Y,et al. A new format of bispecific antibody:highly efficient heterodimerization,expression and tumor cell lysis[J]. Journal of immunological methods,2005,296(1/2):95-101.
[18]GUETTINGER Y,BARBIN K,PEIPP M,et al. A recombinant bispecific single-chain fragment variable specific for HLA class II and FcαRI(CD89)recruits polymorphonuclear neutrophils for efficient lysis of malignant B lymphoid cells[J]. The journal of immunology,2010,184(3):1 210-1 217.
[19]BRUENKE J,BARBIN K,KUNERT S,et al. Effective lysis of lymphoma cells with a stabilised bispecific single-chain Fv antibody against CD19 and FcgammaRIII(CD16)[J]. British journal of haematology,2005,130(2):218.
[20]ZHANG L,HOU Y,ZHANG J,et al. Cytotoxicity of cytokine-induced killer cells targeted by a bispecific antibody to gastric cancer cells[J]. Oncology letters,2013,5(6):1 826-1 832.

Memo

Memo:

-

Common functions

Last Update: 2017-06-30