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针对牛MP26(一种晶状体纤维质膜整合蛋白)抗血清的制备、表征及定位

Preparation, characterization, and localization of antisera against bovine MP26, an integral protein from lens fiber plasma membrane.

作者信息

Paul D L, Goodenough D A

出版信息

J Cell Biol. 1983 Mar;96(3):625-32. doi: 10.1083/jcb.96.3.625.

Abstract

Polyclonal antisera were prepared in rabbits using both native and chymotrypsin-digested bovine lens fiber plasma membranes. MP26, the principal protein of lens fiber plasma membranes, and CT20, a chymotryptic fragment of MP26, were isolated electrophoretically and used to purify anti-MP26 and anti-CT20 activity from the respective antisera by affinity chromatography. These affinity-purified antisera were characterized by immunoreplica. Immunofluorescence microscopy localized MP26 on sections of methacrylate-embedded lenses in the lens fiber plasma membranes, but not the lens epithelium. Immunocytochemistry of isolated native or chymotrypsin-digested lens fiber plasma membranes localized both the MP26 and the CT20 only in the nonjunctional plasma membranes, with no detectable activity in the lens fiber junctions themselves. Electron microscopy revealed a second set of pentalaminar profiles, thinner by 4 nm than the lens fiber junctions, which contained demonstrable anti-MP26 and anti-CT20 activity following immunocytochemistry. These results indicate either that MP26 is not a component of the lens fiber junctions, or that significant conformational changes accompany assembly of MP26 into lens fiber junctions, resulting in the masking of MP26 antigenic determinants.

摘要

使用天然的和经胰凝乳蛋白酶消化的牛晶状体纤维质膜在兔体内制备多克隆抗血清。MP26是晶状体纤维质膜的主要蛋白质,而CT20是MP26的胰凝乳蛋白酶消化片段,通过电泳分离它们,并利用亲和层析从各自的抗血清中纯化抗MP26和抗CT20活性。这些亲和纯化的抗血清通过免疫印迹法进行表征。免疫荧光显微镜检查将MP26定位在甲基丙烯酸酯包埋晶状体切片的晶状体纤维质膜上,而不是晶状体上皮细胞上。对分离的天然或经胰凝乳蛋白酶消化的晶状体纤维质膜进行免疫细胞化学分析,结果显示MP26和CT20仅存在于非连接质膜中,在晶状体纤维连接部位本身未检测到活性。电子显微镜显示出另一组五片层结构,比晶状体纤维连接部位薄4纳米,在免疫细胞化学后含有可证实的抗MP26和抗CT20活性。这些结果表明,要么MP26不是晶状体纤维连接部位的组成成分,要么在MP26组装到晶状体纤维连接部位的过程中伴随着显著的构象变化,导致MP26抗原决定簇被掩盖。

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