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公羊精子质膜中成熟依赖性抗原的侧向区域化和扩散

Lateral regionalization and diffusion of a maturation-dependent antigen in the ram sperm plasma membrane.

作者信息

Wolf D E, Hagopian S S, Lewis R G, Voglmayr J K, Fairbanks G

出版信息

J Cell Biol. 1986 May;102(5):1826-31. doi: 10.1083/jcb.102.5.1826.

Abstract

We have used a monoclonal antibody ESA 152 in fluorescence recovery after photobleaching (FPR) studies of a maturation-dependent surface antigen of ram sperm. The antibody is an immunoglobulin G secreted by a hybridoma derived from NS1 mouse myeloma cells. The ESA 152 antigen is not detectable in testicular sperm. It is localized on the surface of ejaculated sperm where it is present on all regions of the surface, but tends to be concentrated on the posterior region of the head. The ESA 152 antigen can be extracted by detergents or chloroform-methanol. The extracted antigen is sensitive to proteases and migrates with an apparent Mr approximately 30,000 in SDS-containing 10-20% polyacrylamide gradient gels. FPR measurements of ESA 152 lateral mobility in the membrane yield diffusion coefficients in the range 10(-9)-10(-8) cm2/s, values typical of lipids but observed for proteins only at the fluid dynamic limit where diffusion is controlled by lipid fluidity. Immobile fractions, typical of membrane proteins, are observed on all regions. When the antigen is stained by a fluoresceinated Fab fragment of the ESA 152 antibody, the diffusibility is highly regionalized, with particularly low, but rapid, recovery on the midpiece. Cross-linking of the antigen with the intact ESA 152 antibody induces a redistribution in which the antigen is excluded from the posterior head region. This cross-linking is accompanied by increases in ESA 152 diffusibility on both the anterior head and the midpiece.

摘要

我们使用单克隆抗体ESA 152对公羊精子成熟依赖性表面抗原进行光漂白后荧光恢复(FPR)研究。该抗体是由源自NS1小鼠骨髓瘤细胞的杂交瘤分泌的免疫球蛋白G。在睾丸精子中检测不到ESA 152抗原。它定位于射出精子的表面,在表面的所有区域均有存在,但倾向于集中在头部的后部区域。ESA 152抗原可用去污剂或氯仿 - 甲醇提取。提取的抗原对蛋白酶敏感,在含SDS的10 - 20%聚丙烯酰胺梯度凝胶中以约30,000的表观分子量迁移。对ESA 152在膜中的侧向流动性进行FPR测量,得到的扩散系数在10^(-9)-10^(-8) cm²/s范围内,这是脂质的典型值,但仅在扩散受脂质流动性控制的流体动力学极限时才在蛋白质中观察到。在所有区域均观察到了典型的膜蛋白固定部分。当用ESA 152抗体的荧光素化Fab片段对抗原进行染色时,扩散性高度区域化,在中段恢复特别低但很快。抗原与完整的ESA 152抗体交联会导致重新分布,其中抗原被排除在头部后部区域。这种交联伴随着ESA 152在前头部和中段的扩散性增加。

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