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培养的大鼠雪旺细胞对IV型胶原蛋白的生物合成。

Biosynthesis of type IV collagen by cultured rat Schwann cells.

作者信息

Carey D J, Eldridge C F, Cornbrooks C J, Timpl R, Bunge R P

出版信息

J Cell Biol. 1983 Aug;97(2):473-9. doi: 10.1083/jcb.97.2.473.

DOI:10.1083/jcb.97.2.473
PMID:6885907
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2112515/
Abstract

We have obtained evidence that rat Schwann cells synthesize and secrete type IV procollagen. Metabolic labeling of primary cultures of Schwann cells plus neurons and analysis by SDS PAGE revealed the presence of a closely spaced pair of polypeptides in the medium of these cultures that (a) were susceptible to digestion by purified bacterial collagenase, (b) co-migrated with type IV procollagen secreted by rat parietal endoderm cells, and (c) were specifically immunoprecipitated by antibodies against mouse type IV collagen. Limited pepsin digestion of metabolically labeled medium or cell layers produced a pepsin-resistant fragment characteristic of pro-alpha 1(IV) chains. Removal of neuronal cell bodies from the cultures immediately before labeling did not reduce the amount of type IV procollagen detected in the medium. This indicated that Schwann cells, not neurons, were responsible for synthesis of type IV procollagen. We believe type IV procollagen is a major constituent of the Schwann-cell extracellular matrix based upon (a) its presence in a detergent-insoluble matrix preparation, (b) its presence in the cell layer of the cultures in a state in which it can be removed by brief treatment with bacterial collagenase or trypsin, and (c) positive immunofluorescence of Schwann cell-neuron cultures with anti-type-IV collagen antibodies. Secretion of type IV procollagen was substantially reduced when Schwann cells were maintained in the absence of neurons. This observation may account for the previously reported finding that Schwann cells assemble a basal lamina only when co-cultured with neurons (Bunge, M. B., A. K. Williams, and P. M. Wood, 1982, Dev. Biol., 92:449).

摘要

我们已获得证据表明,大鼠雪旺细胞能合成并分泌IV型前胶原。对雪旺细胞与神经元的原代培养物进行代谢标记,并通过SDS-PAGE分析,结果显示这些培养物的培养基中存在一对紧密相邻的多肽,它们:(a)易被纯化的细菌胶原酶消化;(b)与大鼠壁内胚层细胞分泌的IV型前胶原迁移率相同;(c)能被抗小鼠IV型胶原抗体特异性免疫沉淀。对代谢标记的培养基或细胞层进行有限的胃蛋白酶消化,产生了前α1(IV)链特有的胃蛋白酶抗性片段。在标记前立即从培养物中去除神经元细胞体,并未减少培养基中检测到的IV型前胶原的量。这表明合成IV型前胶原的是雪旺细胞,而非神经元。基于以下几点,我们认为IV型前胶原是雪旺细胞细胞外基质的主要成分:(a)它存在于去污剂不溶性基质制剂中;(b)它以一种可通过用细菌胶原酶或胰蛋白酶短暂处理而去除的状态存在于培养物的细胞层中;(c)雪旺细胞-神经元培养物用抗IV型胶原抗体进行免疫荧光检测呈阳性。当雪旺细胞在无神经元的情况下培养时,IV型前胶原的分泌显著减少。这一观察结果可能解释了先前报道的发现,即雪旺细胞仅在与神经元共培养时才组装基膜(邦奇,M. B.,A. K. 威廉姆斯,和P. M. 伍德,1982年,《发育生物学》,92:449)。

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