首页> 外文OA文献 >Cellular activation of mesangial gelatinase A by cytochalasin D is accompanied by enhanced mRNA expression of both gelatinase A and its membrane-associated gelatinase A activator (MT-MMP).
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Cellular activation of mesangial gelatinase A by cytochalasin D is accompanied by enhanced mRNA expression of both gelatinase A and its membrane-associated gelatinase A activator (MT-MMP).

机译:细胞松弛素D对肾小球系膜明胶酶A的细胞活化作用伴随着明胶酶A及其膜相关明胶酶A激活剂(MT-MMP)的mRNA表达增强。

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摘要

Activation of gelatinase A represents a crucial regulatory step in the control of its enzymic activity. Rat kidney mesangial cells secrete predominantly latent gelatinase A that can be activated following treatment with cytochalasin D. In the present paper we provide new evidence, using reverse transcription-PCR, that treatment of rat mesangial cells with cytochalasin D enhances the steady-state level of mRNA of the membrane-type matrix metalloproteinase (MT-MMP), as well as of gelatinase A, with no change in the level of tissue inhibitor of metalloproteinases-2 (TIMP-2) mRNA. Since the TIMP-2 protein level is reduced in conditioned medium from cytochalasin D-treated cells, the results of the present study are consistent with a model in which the action of cytochalasin D is to cause extracellular gelatinase A and TIMP-2 to be sequestered at the plasma membrane, forming a heterotrimeric complex with MT-MMP. In this manner, TIMP-2 may assume a bifunctional role causing: (i) inhibition of gelatinase A in the extracellular compartment; and (ii) guiding gelatinase A to activation through a membrane association with MT-MMP.
机译:明胶酶A的活化是控制其酶活性的关键调节步骤。大鼠肾系膜细胞主要分泌潜在的明胶酶A,可在用细胞松弛素D处理后将其激活。在本文中,我们提供了新的证据,使用逆转录PCR技术对细胞膜松弛素D处理大鼠的肾小球系膜细胞可提高其稳态水平。膜型基质金属蛋白酶(MT-MMP)以及明胶酶A的mRNA,金属蛋白酶2(TIMP-2)mRNA的组织抑制剂水平无变化。由于在经细胞松弛素D处理的细胞中,条件培养基中的TIMP-2蛋白水平降低,因此本研究的结果与其中细胞松弛素D的作用是使细胞外明胶酶A和TIMP-2被隔离的模型相一致。在质膜上,与MT-MMP形成异源三聚体复合物。以这种方式,TIMP-2可能起双功能作用,引起:(i)细胞外区隔明胶酶A的抑制; (ii)通过与MT-MMP的膜结合引导明胶酶A活化。

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  • 作者

    Ailenberg, M; Silverman, M;

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  • 年度 1996
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  • 正文语种 en
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