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灵长类平滑肌细胞中膜型基质金属蛋白酶-1和-3的活性

Membrane-type matrix metalloproteinase-1 and -3 activity in primate smooth muscle cells.

作者信息

Shofuda K I, Hasenstab D, Kenagy R D, Shofuda T, Li Z Y, Lieber A, Clowes A W

机构信息

Division of Vascular Surgery, Department of Surgery, University of Washington School of Medicine, 1959 NE Pacific St., Seattle, WA 98195-6410, USA.

出版信息

FASEB J. 2001 Sep;15(11):2010-2. doi: 10.1096/fj.00-0871fje. Epub 2001 Jul 9.

DOI:10.1096/fj.00-0871fje
PMID:11511522
Abstract

Membrane-type matrix metalloproteinases-1 and -3 (MT1- and MT3-MMPs) are expressed by activated smooth muscle cells (SMCs) both in vitro and in vivo (19). To define their functions in SMCs, we transduced MT1- and MT3-MMP cDNAs into baboon SMCs by using adenoviral vectors. Overexpression of MT1-MMP increased the conversion of proMMP-2 to the intermediate and active forms. In contrast, in MT3-MMP-overexpressing cells, MMP-2 was activated partially. Immunoblot analyses revealed that MT1-MMP protein was present in the SMCs and accumulated in the presence of the synthetic MMP inhibitor, BB94, or tissue inhibitor of metalloproteinase-2 (TIMP-2). However, MT3-MMP protein was detectable only when BB94, but not TIMP-2, was present. Zymographic analyses showed that MT3-MMP had much stronger casein- and gelatin-degrading activities than did MT1-MMP. Furthermore, when MT3-MMP and MT1-MMP were coexpressed, MT1-MMP degradation was enhanced; this result supports the possibility that MT3-MMP can degrade MT1-MMP. SMCs overexpressing either MT1- or MT3-MMP exhibited altered morphology, without changing their proliferation. This alteration was prevented by BB94 addition. The cells, which underwent this change, showed reduced adhesion to both collagen and fibronectin and increased migration in a Boyden chamber. The present study demonstrates that MT1- and MT3-MMPs have different enzymatic activities but may nevertheless affect SMC function in the same way.

摘要

膜型基质金属蛋白酶-1和-3(MT1-MMP和MT3-MMP)在体外和体内的活化平滑肌细胞(SMC)中均有表达(19)。为了确定它们在SMC中的功能,我们使用腺病毒载体将MT1-MMP和MT3-MMP的cDNA转导到狒狒SMC中。MT1-MMP的过表达增加了前MMP-2向中间形式和活性形式的转化。相比之下,在MT3-MMP过表达的细胞中,MMP-2仅部分被激活。免疫印迹分析显示,MT1-MMP蛋白存在于SMC中,并在合成的MMP抑制剂BB94或金属蛋白酶组织抑制剂-2(TIMP-2)存在的情况下积累。然而,仅在存在BB94而非TIMP-2时才能检测到MT3-MMP蛋白。酶谱分析表明,MT3-MMP的酪蛋白和明胶降解活性比MT1-MMP强得多。此外,当MT3-MMP和MT1-MMP共表达时,MT1-MMP的降解增强;这一结果支持了MT3-MMP可以降解MT1-MMP的可能性。过表达MT1-MMP或MT3-MMP的SMC表现出形态改变,但增殖未改变。添加BB94可防止这种改变。发生这种变化的细胞对胶原蛋白和纤连蛋白的粘附减少,在博伊登小室中的迁移增加。本研究表明,MT1-MMP和MT3-MMP具有不同的酶活性,但仍可能以相同的方式影响SMC功能。

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