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一种大鼠抗小鼠κ链特异性单克隆抗体187.1.10:纯化、免疫化学特性及其作为通用二抗试剂的用途。

A rat anti-mouse kappa chain specific monoclonal antibody, 187.1.10: purification, immunochemical properties and its utility as a general second-antibody reagent.

作者信息

Ware C F, Reade J L, Der L C

出版信息

J Immunol Methods. 1984 Nov 16;74(1):93-104. doi: 10.1016/0022-1759(84)90371-5.

Abstract

A rat IgG1 monoclonal antibody, produced by hybridoma 187.1.10, exhibits specificity for mouse immunoglobulins containing kappa light chains (Yelton et al., 1981). The 187.1.10 hybridoma cell line secreted upwards of 200 micrograms/ml of monoclonal antibody in tissue culture and the secreted product was purified in a single step by antigen-immunoadsorbent affinity chromatography. The homogeneity of the purified 187.1.10 protein was determined by isoelectrofocusing and SDS gel electrophoresis. Equilibrium binding analyses of the radioiodinated 187.1.10 antibody indicated a strong interaction with its antigen of KA = 2 X 10(9) l/mole. The 187.1.10 antibody did not readily bind to Staph. aureus protein A unless it was complexed with antigen. The binding of immune complexes of 187.1.10 to protein A was shown to be dependent on the Fc region of the antigen. The utility of the 187.1.10 monoclonal antibody as a general second antibody reagent for studying mouse immunoglobulins was demonstrated in a rapid solid phase immunoprecipitation assay to detect and analyze radioiodinated membrane proteins of a human cytotoxic T cell line.

摘要

由杂交瘤187.1.10产生的大鼠IgG1单克隆抗体,对含有κ轻链的小鼠免疫球蛋白具有特异性(耶尔顿等人,1981年)。187.1.10杂交瘤细胞系在组织培养中分泌超过200微克/毫升的单克隆抗体,分泌产物通过抗原免疫吸附亲和层析一步纯化。通过等电聚焦和SDS凝胶电泳确定纯化的187.1.10蛋白的同质性。对放射性碘化的187.1.10抗体的平衡结合分析表明,它与其抗原KA = 2×10⁹升/摩尔有强烈相互作用。187.1.10抗体除非与抗原复合,否则不容易与金黄色葡萄球菌蛋白A结合。已证明187.1.10免疫复合物与蛋白A的结合取决于抗原的Fc区域。在用于检测和分析人细胞毒性T细胞系放射性碘化膜蛋白的快速固相免疫沉淀试验中,证明了187.1.10单克隆抗体作为研究小鼠免疫球蛋白的通用二抗试剂的实用性。

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