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重组巢蛋白通过精氨酸-甘氨酸-天冬氨酸(RGD)识别序列促进小鼠原代滋养层细胞的黏附和迁移。

Recombinant entactin promotes mouse primary trophoblast cell adhesion and migration through the Arg-Gly-Asp (RGD) recognition sequence.

作者信息

Yelian F D, Edgeworth N A, Dong L J, Chung A E, Armant D R

机构信息

C. S. Mott Center for Human Growth and Development, Department of Obstetrics and Gynecology, Wayne State University School of Medicine, Detroit, MI 48201.

出版信息

J Cell Biol. 1993 May;121(4):923-9. doi: 10.1083/jcb.121.4.923.

Abstract

In vitro culture of mouse blastocysts during the period coinciding with implantation has revealed that primary trophoblast cells can adhere and migrate in serum-free medium when provided with certain extracellular matrix components, including fibronectin and laminin. Tightly associated with laminin is the glycoprotein, entactin, that may play an important role in basement membrane assembly and cell attachment. Mouse blastocysts were studied using this in vitro model to determine whether entactin was capable of mediating trophoblast invasive activity. Although entactin has never been shown to promote cell migration, we report here that recombinant entactin supported blastocyst outgrowth in a dose-dependent manner, with a maximal effect at 20-50 micrograms/ml. The ability of trophoblast cells to adhere and migrate on entactin was specifically inhibited by anti-entactin antibody, but not by antibodies raised against laminin. The synthetic peptide, Gly-Arg-Gly-Asp-Ser-Pro, that contains the Arg-Gly-Asp (RGD) integrin recognition site, reversibly inhibited entactin-mediated blastocyst outgrowth in a dose-dependent manner, but had no effect on laminin-mediated outgrowth. The synthetic peptide, Gly-Phe-Arg-Gly-Asp-Gly-Gln, that comprises the actual RGD-containing sequence within entactin, promoted trophoblast outgrowth when immobilized on the substratum. Furthermore, a mutated recombinant entactin, altered to contain a Glu in place of Asp at the RGD site, provided no trophoblast cell adhesive activity. We conclude that entactin promotes trophoblast outgrowth through a mechanism mediated by the RGD recognition site, and that it may play an important role during invasion of the endometrial basement membrane at implantation.

摘要

在与着床期相吻合的时间段对小鼠囊胚进行体外培养,结果显示,当提供某些细胞外基质成分(包括纤连蛋白和层粘连蛋白)时,原代滋养层细胞能够在无血清培养基中黏附并迁移。与层粘连蛋白紧密相关的是糖蛋白巢蛋白,它可能在基底膜组装和细胞黏附中发挥重要作用。利用这种体外模型对小鼠囊胚进行研究,以确定巢蛋白是否能够介导滋养层的侵袭活性。尽管从未有研究表明巢蛋白能促进细胞迁移,但我们在此报告,重组巢蛋白以剂量依赖的方式支持囊胚生长,在20 - 50微克/毫升时效果最佳。抗巢蛋白抗体可特异性抑制滋养层细胞在巢蛋白上的黏附与迁移能力,而抗层粘连蛋白抗体则无此作用。含有精氨酸 - 甘氨酸 - 天冬氨酸(RGD)整合素识别位点的合成肽甘氨酸 - 精氨酸 - 甘氨酸 - 天冬氨酸 - 丝氨酸 - 脯氨酸,以剂量依赖的方式可逆性抑制巢蛋白介导的囊胚生长,但对层粘连蛋白介导的生长无影响。包含巢蛋白内实际含RGD序列的合成肽甘氨酸 - 苯丙氨酸 - 精氨酸 - 甘氨酸 - 天冬氨酸 - 甘氨酸 - 谷氨酰胺,固定在基质上时可促进滋养层生长。此外,一种在RGD位点将天冬氨酸替换为谷氨酸的突变重组巢蛋白,不具备滋养层细胞黏附活性。我们得出结论,巢蛋白通过由RGD识别位点介导的机制促进滋养层生长,并且它可能在着床时侵入子宫内膜基底膜的过程中发挥重要作用。

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