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细胞表面细胞外基质受体在小鼠囊胚附着和生长中的表达及功能

Expression and function of cell surface extracellular matrix receptors in mouse blastocyst attachment and outgrowth.

作者信息

Sutherland A E, Calarco P G, Damsky C H

机构信息

Department of Anatomy, University of California, San Francisco 94143.

出版信息

J Cell Biol. 1988 Apr;106(4):1331-48. doi: 10.1083/jcb.106.4.1331.

Abstract

Mouse-hatched blastocysts cultured in vitro will attach and form outgrowths of trophoblast cells on appropriate substrates, providing a model for implantation. Immediately after hatching, the surfaces of blastocysts are quiescent and are not adhesive. Over the period 24-36 h post-hatching, blastocysts cultured in serum-free medium become adhesive and attach and spread on the extracellular matrix components fibronectin, laminin, and collagen type IV in a ligand specific manner. Attachment and trophoblast outgrowth on these substrates can be inhibited by addition to the culture medium of an antibody, anti-ECMr (anti-extracellular matrix receptor), that recognizes a group of 140-kD glycoproteins similar to those of the 140-kD extracellular matrix receptor complex (integrin) recognized in avian cells by CSAT and JG22 monoclonal antibodies. Addition to the culture medium of a synthetic peptide containing the Arg-Gly-Asp tripeptide cell recognition sequence of fibronectin inhibits trophoblast outgrowth on both laminin and fibronectin. However, the presence of the peptide does not affect attachment of the blastocysts to either ligand. Immunoprecipitation of 125I surface-labeled embryos using anti-ECMr reveals that antigens recognized by this antibody are exposed on the surfaces of embryos at a time when they are spreading on the substrate, but are not detectable immediately after hatching. Immunofluorescence experiments show that both the ECMr antigens and the cytoskeletal proteins vinculin and talin are enriched on the cell processes and ventral surfaces of trophectoderm cells in embryo outgrowths, in patterns similar to those seen in fibroblasts, and consistent with their role in adhesion of the trophoblast cells to the substratum.

摘要

体外培养的小鼠孵化囊胚会在合适的底物上附着并形成滋养层细胞的生长物,从而为着床提供一个模型。孵化后,囊胚表面静止且无黏附性。在孵化后的24至36小时内,在无血清培养基中培养的囊胚会变得具有黏附性,并以配体特异性方式附着并铺展在细胞外基质成分纤连蛋白、层粘连蛋白和IV型胶原上。向培养基中添加一种抗体——抗ECMr(抗细胞外基质受体),可抑制这些底物上的附着和滋养层生长,该抗体识别一组140-kD糖蛋白,类似于在禽类细胞中被CSAT和JG22单克隆抗体识别的140-kD细胞外基质受体复合物(整合素)。向培养基中添加含有纤连蛋白的Arg-Gly-Asp三肽细胞识别序列的合成肽,可抑制滋养层在层粘连蛋白和纤连蛋白上的生长。然而,该肽的存在并不影响囊胚与任何一种配体的附着。使用抗ECMr对125I表面标记的胚胎进行免疫沉淀显示,该抗体识别的抗原在胚胎铺展在底物上时暴露于胚胎表面,但在孵化后立即无法检测到。免疫荧光实验表明,ECMr抗原以及细胞骨架蛋白纽蛋白和踝蛋白在胚胎生长物中滋养外胚层细胞的细胞突起和腹侧表面富集,其模式类似于成纤维细胞中的模式,并且与其在滋养层细胞与基质黏附中的作用一致。

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