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从鼠腹水肝癌肿瘤中提取的金属蛋白酶对间质胶原的顺序降解。

Sequential degradation of interstitial collagen by metalloproteinases extracted from tumors of murine ascites hepatomas.

作者信息

Koita H, Nabeshima K, Inoue T, Koono M

机构信息

Department of Pathology, Miyazaki Medical College, Japan.

出版信息

Clin Exp Metastasis. 1991 Sep-Oct;9(5):441-56. doi: 10.1007/BF01785530.

DOI:10.1007/BF01785530
PMID:1655324
Abstract

Gelatinolytic and collagenolytic proteinases were separately isolated by different extraction methods from the mouse ascites hepatoma MH134, and from rat ascites hepatoma AH109A. The activities of two proteinases in each extract showed no significant differences, but after trypsin activation the activities of proteinases from the highly metastatic MH134 were significantly increased compared to the enzyme activities in AH109A, which has low metastatic potential. The total activities of collagenase and gelatinase were increased 7.2- and 5.1-fold; their specific activities were increased 5.2- and 4.8-fold, respectively. Gelatinase and collagenase from MH134 were characterized on gelatin zymography. The gelatinase had a molecular weight of 99 and activation by 4-aminophenylmercuric acetate (APMA) or trypsin resulted in its conversion to 79 or 79-95 kD, respectively. The collagenase revealed a major gelatinolytic band at 89 kD, which was converted to 85 and 70 kD by APMA-activation, and a minor gelatinolytic band at 60 kD. These proteinases could degrade native type I collagen to small fragments in a cooperative manner. Trypsin inhibitor, which affects the trypsin activation of latent gelatinase, was extracted together with gelatinase. The inhibitory activity of the enzyme from AH109A showed a 4.1-fold higher specific activity and 3.7-fold greater total activity than that from MH134. The proteinase(s) capable of activating the gelatinase was also extracted from MH134.

摘要

通过不同的提取方法分别从小鼠腹水肝癌MH134和大鼠腹水肝癌AH109A中分离出明胶酶解蛋白酶和胶原酶解蛋白酶。每种提取物中两种蛋白酶的活性没有显著差异,但在胰蛋白酶激活后,高转移性的MH134中蛋白酶的活性与低转移潜能的AH109A中的酶活性相比显著增加。胶原酶和明胶酶的总活性分别增加了7.2倍和5.1倍;它们的比活性分别增加了5.2倍和4.8倍。对MH134中的明胶酶和胶原酶进行了明胶酶谱分析。明胶酶的分子量为99kD,用乙酸对氨基苯汞(APMA)或胰蛋白酶激活后分别转化为79kD或79 - 95kD。胶原酶在89kD处显示出一条主要的明胶酶解带,经APMA激活后转化为85kD和70kD,在60kD处有一条次要的明胶酶解带。这些蛋白酶可以协同将天然I型胶原降解为小片段。与明胶酶一起提取到了影响潜在明胶酶胰蛋白酶激活的胰蛋白酶抑制剂。AH109A中该酶的抑制活性比MH134中的比活性高4.1倍,总活性高3.7倍。还从MH134中提取了能够激活明胶酶的蛋白酶。

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本文引用的文献

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