Shofuda Tomoko, Shofuda Ken-ichi, Ferri Nicola, Kenagy Richard D, Raines Elaine W, Clowes Alexander W
Division of Vascular Surgery, Department of Surgery, University of Washington School of Medicine, Seattle, Wash 98195-6410, USA.
Arterioscler Thromb Vasc Biol. 2004 May;24(5):839-44. doi: 10.1161/01.ATV.0000126680.78500.4c. Epub 2004 Mar 25.
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.
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.
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.
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。
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。
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。
