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E-钙黏蛋白通过Src 和 PI3K 信号通路依赖性刺激黏着斑处的牵引力。

E-cadherin-dependent stimulation of traction force at focal adhesions via the Src and PI3K signaling pathways.

机构信息

Unité Mixte de Recherche 144, Centre National de la Recherche Scientifique, Institut Curie, Paris, France.

出版信息

Biophys J. 2012 Jul 18;103(2):175-84. doi: 10.1016/j.bpj.2012.06.009. Epub 2012 Jul 17.

Abstract

The interplay between cadherin- and integrin-dependent signals controls cell behavior, but the precise mechanisms that regulate the strength of adhesion to the extracellular matrix remains poorly understood. We deposited cells expressing a defined repertoire of cadherins and integrins on fibronectin (FN)-coated polyacrylamide gels (FN-PAG) and on FN-coated pillars used as a micro-force sensor array (μFSA), and analyzed the functional relationship between these adhesion receptors to determine how it regulates cell traction force. We found that cadherin-mediated adhesion stimulated cell spreading on FN-PAG, and this was modulated by the substrate stiffness. We compared S180 cells with cells stably expressing different cadherins on μFSA and found that traction forces were stronger in cells expressing cadherins than in parental cells. E-cadherin-mediated contact and mechanical coupling between cells are required for this increase in cell-FN traction force, which was not observed in isolated cells, and required Src and PI3K activities. Traction forces were stronger in cells expressing type I cadherins than in cells expressing type II cadherins, which correlates with our previous observation of a higher intercellular adhesion strength developed by type I compared with type II cadherins. Our results reveal one of the mechanisms whereby molecular cross talk between cadherins and integrins upregulates traction forces at cell-FN adhesion sites, and thus provide additional insight into the molecular control of cell behavior.

摘要

钙黏蛋白和整合素依赖性信号之间的相互作用控制着细胞的行为,但调控细胞与细胞外基质黏附强度的确切机制仍知之甚少。我们将表达特定钙黏蛋白和整合素组合的细胞沉积在纤维连接蛋白(FN)包被的聚丙烯酰胺凝胶(FN-PAG)和用作微力传感器阵列(μFSA)的 FN 包被的柱子上,并分析这些黏附受体之间的功能关系,以确定其如何调节细胞牵引力。我们发现钙黏蛋白介导的黏附刺激了 FN-PAG 上的细胞铺展,并且这种铺展受底物刚度的调节。我们将 S180 细胞与稳定表达 μFSA 上不同钙黏蛋白的细胞进行了比较,发现表达钙黏蛋白的细胞的牵引力比亲本细胞更强。E-钙黏蛋白介导的细胞间接触和机械偶联对于细胞-FN 牵引力的增加是必需的,在分离的细胞中没有观察到这种情况,并且需要Src 和 PI3K 活性。表达 I 型钙黏蛋白的细胞的牵引力比表达 II 型钙黏蛋白的细胞更强,这与我们之前观察到的 I 型钙黏蛋白比 II 型钙黏蛋白具有更高的细胞间黏附强度的结果一致。我们的研究结果揭示了钙黏蛋白和整合素之间的分子串扰上调细胞-FN 黏附部位牵引力的机制之一,从而为细胞行为的分子调控提供了更多的见解。

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