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豚鼠精子顶体周质膜中两种抗原相关的整合膜蛋白的特性分析。

Characterization of two antigenically related integral membrane proteins of the guinea pig sperm periacrosomal plasma membrane.

作者信息

Westbrook-Case V A, Winfrey V P, Olson G E

机构信息

Department of Cell Biology, Vanderbilt University, Nashville, Tennessee 37232.

出版信息

Mol Reprod Dev. 1994 Nov;39(3):309-21. doi: 10.1002/mrd.1080390308.

Abstract

The periacrosomal plasma membrane of mammalian spermatozoa functions both in recognition and in binding of the egg's zona pellucida and in the acrosome reaction. This study characterizes two antigenically related proteins with molecular weights of 35 kD (PM35) and 52 kD (PM52) of the guinea pig sperm periacrosomal plasma membrane. Polyclonal antisera were prepared against electrophoretically purified PM35 or PM52. Each antiserum recognized both the 35-kD and 52-kD polypeptides on Western blots, indicating that they are structurally related. This conclusion was supported by peptide mapping experiments demonstrating comparably sized fragments of both PM35 and PM52. Both PM35 and PM52 behave as integral membrane proteins during phase-separation analysis with Triton X-114. Electron microscopic immunocytochemistry and differential fractionation of sperm membranes established that both PM35 and PM52 are exclusively localized to the periacrosomal plasma membrane. Three different antisera were used for ultrastructural studies, and each specifically bound the cytoplasmic but not the extracellular membrane surface. The electrophoretic mobilities of the PM35 and PM52 polypeptides were unchanged during sperm maturation and during the ionophore-induced acrosome reaction. The localization of PM35 and PM52 suggests a potential role for these integral plasma membrane proteins in signal transduction or membrane fusion events of the acrosome reaction.

摘要

哺乳动物精子顶体周围的质膜在识别和结合卵子透明带以及顶体反应中发挥作用。本研究对豚鼠精子顶体周围质膜中两种分子量分别为35kD(PM35)和52kD(PM52)且抗原相关的蛋白质进行了表征。制备了针对经电泳纯化的PM35或PM52的多克隆抗血清。每种抗血清在蛋白质免疫印迹法中都识别35kD和52kD的多肽,这表明它们在结构上相关。肽图谱实验证明了PM35和PM52具有大小相当的片段,支持了这一结论。在用Triton X - 114进行相分离分析时,PM35和PM52均表现为整合膜蛋白。电子显微镜免疫细胞化学和精子膜的差速分级分离表明,PM35和PM52都仅定位于顶体周围的质膜。三种不同的抗血清用于超微结构研究,每种都特异性地结合细胞质膜表面而非细胞外膜表面。在精子成熟过程以及离子载体诱导的顶体反应过程中,PM35和PM52多肽的电泳迁移率没有变化。PM35和PM52的定位表明这些整合质膜蛋白在顶体反应的信号转导或膜融合事件中可能发挥作用。

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