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在过表达膜型基质金属蛋白酶的血管平滑肌细胞中粘着斑激酶的裂解

Cleavage of focal adhesion kinase in vascular smooth muscle cells overexpressing membrane-type matrix metalloproteinases.

作者信息

Shofuda Tomoko, Shofuda Ken-ichi, Ferri Nicola, Kenagy Richard D, Raines Elaine W, Clowes Alexander W

机构信息

Division of Vascular Surgery, Department of Surgery, University of Washington School of Medicine, Seattle, Wash 98195-6410, USA.

出版信息

Arterioscler Thromb Vasc Biol. 2004 May;24(5):839-44. doi: 10.1161/01.ATV.0000126680.78500.4c. Epub 2004 Mar 25.

DOI:10.1161/01.ATV.0000126680.78500.4c
PMID:15044209
Abstract

BACKGROUND

Membrane-type matrix metalloproteinases (MT-MMPs) were initially identified as cell surface activators of MMP-2 (gelatinase A). We have reported that MT1-MMPs and MT3-MMPs are expressed by activated vascular smooth muscle cells (SMCs) and play a role in the regulation of cell function. Overexpression of MT-MMPs results in cell rounding, decreased adherence, and increased migration. Because integrin-mediated cell adhesion regulates these events, we have investigated the functional relationship between MT-MMPs and focal adhesion assembly.

METHODS AND RESULTS

Using adenoviral vectors we show that overexpression of MT-MMPs reduces the number of focal contacts, whereas the cell surface expression of integrin subunits remains unchanged. The 125-kDa focal adhesion kinase (FAK) is cleaved resulting in a 90-kDa fragment under these conditions, and paxillin is partially dissociated from FAK after its cleavage. Pretreatment of cells with BB94, a synthetic MMP inhibitor, rescues cell adhesion and prevents changes in focal adhesions, supporting a potential role for MT-MMP enzymatic activities.

CONCLUSIONS

This study provides the first evidence that MT-MMPs are not only important in matrix degradation but also may affect the function of focal adhesions through FAK cleavage.

摘要

背景

膜型基质金属蛋白酶(MT-MMPs)最初被鉴定为MMP-2(明胶酶A)的细胞表面激活剂。我们已报道MT1-MMPs和MT3-MMPs由活化的血管平滑肌细胞(SMC)表达,并在细胞功能调节中发挥作用。MT-MMPs的过表达导致细胞变圆、黏附减少和迁移增加。由于整合素介导的细胞黏附调节这些事件,我们研究了MT-MMPs与粘着斑组装之间的功能关系。

方法与结果

使用腺病毒载体,我们发现MT-MMPs的过表达减少了粘着斑的数量,而整合素亚基的细胞表面表达保持不变。在这些条件下,125 kDa的粘着斑激酶(FAK)被切割,产生一个90 kDa的片段,并且桩蛋白在FAK切割后部分从FAK解离。用合成的MMP抑制剂BB94预处理细胞可挽救细胞黏附并防止粘着斑的变化,支持MT-MMP酶活性的潜在作用。

结论

本研究提供了首个证据,表明MT-MMPs不仅在基质降解中起重要作用,还可能通过切割FAK影响粘着斑的功能。

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