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基质溶解素产生一种抑制雪旺细胞增殖的纤连蛋白片段。

Stromelysin generates a fibronectin fragment that inhibits Schwann cell proliferation.

作者信息

Muir D, Manthorpe M

机构信息

Department of Biology, University of California, San Diego, La Jolla 92093.

出版信息

J Cell Biol. 1992 Jan;116(1):177-85. doi: 10.1083/jcb.116.1.177.

DOI:10.1083/jcb.116.1.177
PMID:1730742
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2289256/
Abstract

Our previous report (Muir, D., S. Varon, and M. Manthorpe. 1990. J. Cell Biol. 109:2663-2672) described the isolation and partial characterization of a 55-kD antiproliferative protein found in Schwann cell (SC) and schwannoma cell line-conditioned media and we concluded that SC proliferation is under negative autocrine control. In the present study the 55-kD protein was found to possess metalloprotease activity and stromelysin immunoreactivity. The SC-derived metalloprotease shares many properties with stromelysin isolated from other sources including the ability to cleave fibronectin (FN). Furthermore, limited proteolysis of FN by the SC-derived protease generated a FN fragment which itself expresses a potent antiproliferative activity for SCs. The active FN fragment corresponds to the 29-kD amino-terminal region of the FN molecule which was also identified as an active component in SC CM. Additional evidence that a proteolytic fragment of FN can possess antiproliferative activity for SCs was provided by the finding that plasmin can generate an amino-terminal FN fragment which mimicked the activity of the SC metalloprotease-generated antiproliferative FN fragment. Both the 55-kD SC metalloprotease and the 29-kD FN fragment could completely and reversibly inhibit proliferation of SCs treated with various mitogens and both were largely ineffective at inhibiting proliferation by immortalized or transformed SC lines. Normal and transformed SC types do secrete the proform of stromelysin, however, transformed cultures do not produce activated stromelysin and thus cannot generate the antiproliferative fragment of FN. These results suggest that, once activated, a SC-derived protease similar to stromelysin cleaves FN and generates an antiproliferative activity which can maintain normal SC quiescence in vitro.

摘要

我们之前的报告(缪尔,D.,S. 瓦龙,和 M. 曼索普。1990 年。《细胞生物学杂志》109:2663 - 2672)描述了从雪旺细胞(SC)和雪旺瘤细胞系条件培养基中分离出一种 55kD 的抗增殖蛋白并对其进行了部分特性分析,我们得出结论,SC 的增殖受负性自分泌控制。在本研究中,发现该 55kD 蛋白具有金属蛋白酶活性和基质溶解素免疫反应性。源自 SC 的金属蛋白酶与从其他来源分离出的基质溶解素具有许多共同特性,包括切割纤连蛋白(FN)的能力。此外,源自 SC 的蛋白酶对 FN 的有限蛋白水解产生了一个 FN 片段,该片段本身对 SC 表现出强大的抗增殖活性。活性 FN 片段对应于 FN 分子的 29kD 氨基末端区域,该区域也被鉴定为 SC 条件培养基中的活性成分。纤溶酶能产生一个氨基末端 FN 片段,该片段模拟了 SC 金属蛋白酶产生的抗增殖 FN 片段的活性,这一发现提供了额外证据,表明 FN 的蛋白水解片段可对 SC 具有抗增殖活性。55kD 的 SC 金属蛋白酶和 29kD 的 FN 片段都能完全且可逆地抑制用各种有丝分裂原处理的 SC 的增殖,并且两者在抑制永生化或转化的 SC 系的增殖方面大多无效。正常和转化的 SC 类型确实会分泌基质溶解素的前体形式,然而,转化培养物不会产生活化的基质溶解素,因此无法产生 FN 的抗增殖片段。这些结果表明,一旦被激活,一种类似于基质溶解素的源自 SC 的蛋白酶会切割 FN 并产生一种抗增殖活性,这种活性可在体外维持正常 SC 的静止状态。

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