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分析与非洲爪蟾卵黄膜成分结合的精子表面分子。

Analysis of a sperm surface molecule that binds to a vitelline envelope component of Xenopus laevis eggs.

机构信息

Department of Medical Biology, Tokyo Metropolitan Institute of Medical Science, Setagaya-ku, Tokyo, Japan.

出版信息

Mol Reprod Dev. 2010 Aug;77(8):728-35. doi: 10.1002/mrd.21211.

Abstract

To analyze sperm surface molecules involved in sperm-egg envelope binding in Xenopus laevis, heat-solubilized vitelline envelope (VE) dot blotted onto a polyvinylidene difluoride (PVDF) sheet was incubated with a detergent extract of sperm plasma membrane (SP-ML). The membrane components bound to the VE were detected using an antibody library against sperm plasma membrane components, and a hybridoma clone producing a monoclonal antibody (mAb) 16A2A7 was identified. This mAb was used in a Far Western blotting experiment in which VE was separated by electrophoresis, and then transferred to a PVDF strip that was incubated with SP-ML. It was found that SP-ML binds to the VE component gp37 (Xenopus homolog of mammalian ZP1). The antigens reactive to mAb 16A2A7 showed apparent molecular weights of 65-130 and 20-30 kDa, and were distributed relatively evenly over the entire sperm surface. Periodate oxidation revealed that both the pertinent epitope on the sperm surface and the ligands of VE gp37 were sugar moieties. VE gp37 was exposed on the VE surface, and the mAb 16A2A7 dose-dependently inhibited sperm binding to VE. The sperm membrane molecules reactive with mAb 16A2A7 also reacted with mAb 2A3D9, which is known to recognize the glycoprotein SGP in the sperm plasma membrane and is involved in interactions with the egg plasma membrane, indicating that the sperm membrane glycoprotein has a bifunctional role in Xenopus fertilization.

摘要

为了分析参与非洲爪蟾卵母细胞透明带结合的精子表面分子,将热溶解的卵黄膜(VE)斑点印迹到聚偏二氟乙烯(PVDF)片上,然后与精子质膜(SP-ML)的去污剂提取物一起孵育。使用针对精子质膜成分的抗体文库检测与 VE 结合的膜成分,并鉴定出产生单克隆抗体(mAb)16A2A7 的杂交瘤克隆。该 mAb 用于 Far Western 印迹实验,其中 VE 通过电泳分离,然后转移到与 SP-ML 孵育的 PVDF 条上。结果发现 SP-ML 与 VE 成分 gp37(哺乳动物 ZP1 的非洲爪蟾同源物)结合。与 mAb 16A2A7 反应的抗原显示出明显的 65-130 kDa 和 20-30 kDa 的分子量,并且在整个精子表面分布相对均匀。过碘酸钠氧化表明,精子表面上的相关表位和 VE gp37 的配体都是糖基。VE gp37 暴露在 VE 表面上,mAb 16A2A7 剂量依赖性地抑制精子与 VE 的结合。与 mAb 16A2A7 反应的精子膜分子也与 mAb 2A3D9 反应,后者已知识别精子质膜中的糖蛋白 SGP,并且参与与卵质膜的相互作用,表明精子膜糖蛋白在非洲爪蟾受精中具有双重功能。

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