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松弛素调节人皮肤成纤维细胞中前胶原酶和胶原蛋白的合成与分泌。

Relaxin modulates synthesis and secretion of procollagenase and collagen by human dermal fibroblasts.

作者信息

Unemori E N, Amento E P

机构信息

Department of Developmental Biology, Genentech, Inc., South San Francisco, California 94080.

出版信息

J Biol Chem. 1990 Jun 25;265(18):10681-5.

PMID:2162358
Abstract

Relaxin is believed to play a role in connective tissue remodeling during pregnancy (Bell, R.J., Eddie, L. W., Lester, A. R., Wood, E. C., Johnston, P.D., and Niall, H. D. (1987) Obstet. Gynecol. 69, 585-589; MacLennan, A. H. (1983) Clin. Reprod. Fertil. 2, 77-95). In the present study, normal human fibroblasts exposed to concentrations of a synthetic bioactive relaxin peptide from 0.1 to 10 ng/ml synthesized and secreted the metalloproteinase procollagenase, which was immunoprecipitable as a doublet of 52 and 57 kDa by a monoclonal antibody to human collagenase. The stimulation in procollagenase protein expression was reflected in an elevation in procollagenase mRNA levels. Media conditioned for 48 h by relaxin-treated fibroblasts (0.1 ng/ml) contained 1.7 units/ml activatable collagenase compared with 0.2 units/ml by untreated fibroblasts. In addition, relaxin caused a modest decrease in the levels of tissue inhibitor of metalloproteinases, as detected by reverse zymography and Northern analysis. Relaxin was also a potent modulator of the collagen secretory phenotype of these fibroblasts. Relaxin at 100 ng/ml down-regulated collagen secretion by 40%. When fibroblasts were treated simultaneously with cytokines such as transforming growth factor beta or interleukin 1 beta, which stimulated collagen synthesis to at least 9-fold of basal levels, relaxin at 100 ng/ml was able to down-regulate collagen expression by up to 88%. This decrease was reflected by changes at the mRNA level. These results indicate that relaxin can cause significant collagen turnover both by stimulating collagenase expression and by down-modulating collagen synthesis and secretion.

摘要

人们认为松弛素在孕期结缔组织重塑过程中发挥作用(贝尔,R.J.,埃迪,L.W.,莱斯特,A.R.,伍德,E.C.,约翰斯顿,P.D.,以及尼尔,H.D.(1987年)《妇产科学》69卷,585 - 589页;麦克伦南,A.H.(1983年)《临床生殖与生育》2卷,77 - 95页)。在本研究中,暴露于浓度为0.1至10纳克/毫升的合成生物活性松弛素肽的正常人成纤维细胞合成并分泌金属蛋白酶原胶原酶,用针对人胶原酶的单克隆抗体可将其免疫沉淀为52千道尔顿和57千道尔顿的双峰。原胶原酶蛋白表达的刺激反映在原胶原酶mRNA水平的升高上。经松弛素处理的成纤维细胞(0.1纳克/毫升)培养48小时的培养基中含有1.7单位/毫升可激活的胶原酶,而未处理的成纤维细胞培养基中为0.2单位/毫升。此外,通过反向酶谱分析和Northern分析检测到,松弛素使金属蛋白酶组织抑制剂水平适度降低。松弛素也是这些成纤维细胞胶原分泌表型的有效调节剂。100纳克/毫升的松弛素使胶原分泌下调40%。当成纤维细胞同时用细胞因子如转化生长因子β或白细胞介素1β处理时,这些细胞因子可将胶原合成刺激至基础水平的至少9倍,100纳克/毫升的松弛素能够使胶原表达下调高达88%。这种降低在mRNA水平上有所体现。这些结果表明,松弛素可通过刺激胶原酶表达以及下调胶原合成与分泌,导致显著的胶原周转。

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