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抗人补体终末C5b-9复合物新抗原的单克隆抗体。

Monoclonal antibodies against neoantigens of the terminal C5b-9 complex of human complement.

作者信息

Hugo F, Jenne D, Bhakdi S

出版信息

Biosci Rep. 1985 Aug;5(8):649-58. doi: 10.1007/BF01116996.

DOI:10.1007/BF01116996
PMID:2415178
Abstract

Assembly of the terminal C5b-C9 complement components into the cytolytic C5b-9 complex is accompanied by exposure of characteristic neoantigens on the macromolecule. We report the production and characterization of mouse monoclonal antibodies to C9-dependent neoantigens of human C5b-9. Binding-inhibition assays with EDTA-human plasma and micro-ELISA assays with purified C9 showed that the antibodies did not react with native complement components and thus confirmed the specificity of the antibodies for the neoantigens. The monoclonal antibodies did, however, cross-react with cytolytically inactive, fluid-phase C5b-9 complexes. Thus, expression of the neoantigenic determinants was not dependent on the formation of high molecular weight C9 polymers with the complex, since these are absent in fluid-phase C5b-9. Radioiodinated antibodies could be utilized in immunoradiometric assays for the detection and quantitation of C5b-9 on cell membranes. Cross-reactivities of the antibodies with C9-dependent neoantigens of several other animal species were examined and antibody clones cross-reacting with rabbit (clones 3B1, 3D8, and 2F3), sheep (clones 3D8 and 2F3) and guinea-pig (clone 3D8) neoantigens were identified. Three of four tested clones (3D8, 2F3, 1A12) precipitated C5b-9 complexes in double-diffusion assays, probably due to their interaction with multiple and repeating C9-epitopes on the terminal complexes. The monoclonal antibodies will be of value for definitive identification and quantitation of C5b-9 on cell membranes and in tissues, and for establishing immunoassays for detection and quantitation of terminal fluid-phase C5b-9 complexes in plasma.

摘要

末端补体成分C5b - C9组装成溶细胞性C5b - 9复合物时,会伴随大分子上特征性新抗原的暴露。我们报道了针对人C5b - 9的C9依赖性新抗原的小鼠单克隆抗体的制备及特性研究。用EDTA - 人血浆进行的结合抑制试验以及用纯化的C9进行的微量ELISA试验表明,这些抗体不与天然补体成分反应,从而证实了抗体对新抗原的特异性。然而,单克隆抗体确实能与溶细胞活性缺失的液相C5b - 9复合物发生交叉反应。因此,新抗原决定簇的表达并不依赖于与该复合物形成高分子量的C9聚合物,因为在液相C5b - 9中不存在这种聚合物。放射性碘化抗体可用于免疫放射分析,以检测和定量细胞膜上的C5b - 9。检测了这些抗体与其他几种动物物种的C9依赖性新抗原的交叉反应性,并鉴定出与兔(克隆3B1、3D8和2F3)、绵羊(克隆3D8和2F3)和豚鼠(克隆3D8)新抗原发生交叉反应的抗体克隆。在双向扩散试验中,四个测试克隆中的三个(3D8、2F3、1A12)沉淀了C5b - 9复合物,这可能是由于它们与末端复合物上多个重复的C9表位相互作用所致。这些单克隆抗体对于在细胞膜和组织中明确鉴定和定量C5b - 9,以及建立用于检测和定量血浆中末端液相C5b - 9复合物的免疫测定法具有重要价值。

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1
Monoclonal antibodies against neoantigens of the terminal C5b-9 complex of human complement.抗人补体终末C5b-9复合物新抗原的单克隆抗体。
Biosci Rep. 1985 Aug;5(8):649-58. doi: 10.1007/BF01116996.
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Quantitation of activation of the human terminal complement pathway by ELISA.通过酶联免疫吸附测定法对人末端补体途径的激活进行定量分析。
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Using polymerized C9 to produce a monoclonal antibody against a neoantigen of the human terminal complement complex.使用聚合的C9制备针对人末端补体复合物新抗原的单克隆抗体。
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C5b-9 assembly: average binding of one C9 molecule to C5b-8 without poly-C9 formation generates a stable transmembrane pore.C5b-9组装:一个C9分子与C5b-8的平均结合而不形成多聚C9会产生一个稳定的跨膜孔。
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Inhibition of the lytic action of cell-bound terminal complement components by human high density lipoproteins and apoproteins.人高密度脂蛋白及载脂蛋白对细胞结合的末端补体成分溶解作用的抑制
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J Immunol. 1991 Apr 1;146(7):2345-51.

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Complement activation in septic baboons detected by neoepitope-specific assays for C3b/iC3b/C3c, C5a and the terminal C5b-9 complement complex (TCC).
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Clin Exp Immunol. 1993 Feb;91(2):295-300. doi: 10.1111/j.1365-2249.1993.tb05898.x.
4
Importance of the third thrombospondin repeat of C6 for terminal complement complex assembly.C6的第三个血小板反应蛋白重复序列对末端补体复合物组装的重要性。
Immunology. 1995 Jun;85(2):214-9.
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Use of a monoclonal antibody to determine the mode of transmembrane pore formation by streptolysin O.使用单克隆抗体确定链球菌溶血素O形成跨膜孔的方式。
Infect Immun. 1986 Dec;54(3):641-5. doi: 10.1128/iai.54.3.641-645.1986.
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