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大鼠肝细胞的底物黏附:与胶原蛋白底物的附着机制

Substrate adhesion of rat hepatocytes: mechanism of attachment to collagen substrates.

作者信息

Rubin K, Höök M, Obrink B, Timpl R

出版信息

Cell. 1981 May;24(2):463-70. doi: 10.1016/0092-8674(81)90337-8.

DOI:10.1016/0092-8674(81)90337-8
PMID:7237556
Abstract

Attachment of rat hepatocytes to collagen, which occurs without the aid of fibronectin, was found to be a time-dependent reaction characterized by an initial lag phase of 10-20 min before stable attachment bonds began to form. Increasing the density of molecules in the collagen substrates enhanced the rate of cell attachment. The hepatocytes attached essentially equally well to all the collagen types tested (types I, II, III, IV and V). The initial rate of cell attachment was more rapid to native collagen than to denatured collagen or alpha 1(I) chains, apparently indicating different affinities of the cells for these substrates. However, if cells were incubated for 60 min or more, efficient attachment occurred to the alpha 1(I) chain and to all cyanogen-bromide-treated peptides tested (alpha 1-CB2, alpha 1-CB3, alpha 1-CB4, alpha 1-CB5, alpha 1-CB6A, alpha 1-CB7, alpha 1-CB8, alpha 2-CB2, alpha 2-CB3 and alpha 2-CB4) but not to the aminopropeptide of type I procollagen. A low but significant degree of attachment also took place to substrates made of synthetic peptides with the collagen-like structures (Gly-Ala-Pro)n, (Gly-Pro-Pro)n and (Gly-Pro-Hyp)n, whereas no attachment was observed to polyproline. We suggest that the cell-binding sites in collagen have a simple structure and occur in multiple copies along the collagen molecule. Addition of collagen in solution inhibited initial cell attachment, an effect that persisted longer on substrates made of alpha 1(I) chain than on denatured collagen. The collected data are interpreted in terms of a model for cell-to-collagen adhesion where the formation of stable attachment bonds requires the binding of several low-affinity receptors, clustered at the site of adhesion, to collagen molecules in the substrate.

摘要

已发现大鼠肝细胞在没有纤连蛋白帮助的情况下与胶原蛋白附着,这是一个时间依赖性反应,其特征是在稳定附着键开始形成之前有10 - 20分钟的初始延迟期。增加胶原蛋白底物中分子的密度可提高细胞附着速率。肝细胞对所有测试的胶原蛋白类型(I型、II型、III型、IV型和V型)的附着效果基本相同。细胞附着的初始速率对天然胶原蛋白比对变性胶原蛋白或α1(I)链更快,这显然表明细胞对这些底物具有不同的亲和力。然而,如果细胞孵育60分钟或更长时间,则能有效地附着到α1(I)链以及所有测试的溴化氰处理肽(α1-CB2、α1-CB3、α1-CB4、α1-CB5、α1-CB6A、α1-CB7、α1-CB8、α2-CB2、α2-CB3和α2-CB4)上,但不能附着到I型前胶原的氨基端肽上。对具有胶原样结构的合成肽(Gly-Ala-Pro)n、(Gly-Pro-Pro)n和(Gly-Pro-Hyp)n制成的底物也有低但显著程度的附着,而对聚脯氨酸则未观察到附着。我们认为胶原蛋白中的细胞结合位点具有简单结构,并且沿胶原蛋白分子以多个拷贝形式存在。溶液中的胶原蛋白添加会抑制细胞的初始附着,这种作用在由α1(I)链制成的底物上持续的时间比对变性胶原蛋白更长。根据细胞与胶原蛋白黏附的模型对收集到的数据进行了解释,其中稳定附着键的形成需要几个低亲和力受体聚集在黏附位点并与底物中的胶原蛋白分子结合。

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