Collagen synthesis by human fibroblasts. Regulation by transforming growth factor-β in the presence of other inflammatory mediators

A S Narayanan; J Swanson; R C Page

摘要

pWe have examined the combined effects of transforming growth factor-beta (TGF-beta), serum and gamma-interferon (gamma-IFN) on collagen synthesis by fibroblasts and compared the response of fibroblast subpopulations to TGF-beta. Human diploid fibroblasts were treated with TGF-beta alone and with serum of gamma-IFN. Cells were labelled with radioactive amino acids, and collagen production was measured as collagenase-digestible radioactivity. Collagen mRNA was determined by a solution-hybridization assay using procollagen-alpha 1[I] cDNA clone HF 677. The results showed that either serum or TGF-beta increased incorporation, collagen production and mRNA by fibroblasts approx. 2-fold; however, collagen synthesis relative to total protein synthesis and collagen mRNA relative to total polyadenylated [poly(A)+] RNA were not affected. Only serum activated cell growth. Collagen production increased approx. 4-fold in cells exposed to both TGF-beta and serum, and this increase was equal to that expected for an additive effect by both components. Treatment with gamma-IFN decreased collagen production and collagen mRNA to 44 and 40% respectively, whereas total incorporation and poly(A)+ RNA were affected only marginally. Cells exposed simultaneously to both gamma-IFN and TGF-beta produced less collagen and contained less mRNA than did those treated with TGF-beta alone. The gamma-IFN decreased collagen synthesis in control and TGF-beta-treated cultures to a similar extent, and TGF-beta increased collagen synthesis 2-fold in cells pre-treated with gamma-IFN. Fibroblast strains obtained in medium containing plasma-derived serum synthesized approximately half as much collagen as did cells derived from the same explant in the presence of fresh human serum, and TGF-beta stimulated collagen production and mRNA in both cell strains. We conclude that TGF-beta, serum and gamma-IFN regulate collagen synthesis by independent mechanisms, and that the combined action of these components plays a significant role in regulating collagen synthesis during wound healing and tissue repair./p

机译：>我们检查了转化生长因子-β（TGF-beta），血清和γ-干扰素（γ-IFN）对成纤维细胞胶原合成的综合作用，并比较了成纤维细胞亚群对TGF-β的反应。人二倍体成纤维细胞分别用TGF-β和γ-IFN血清处理。用放射性氨基酸标记细胞，并以胶原酶消化的放射性测量胶原蛋白的产生。胶原蛋白mRNA是通过溶液杂交法使用胶原蛋白α1[I] cDNA HF 677溶液测定的。结果表明，血清或TGF-β均可增加成纤维细胞的掺入，胶原蛋白生成和mRNA表达。 2倍;但是，相对于总蛋白合成的胶原蛋白合成和相对于总聚腺苷酸化的[poly（A）+] RNA的胶原蛋白mRNA不受影响。仅血清激活细胞生长。胶原蛋白产量增加约。暴露于TGF-beta和血清的细胞中的4倍，并且这种增加等于预期的两种成分的加和作用。用γ-干扰素处理可分别将胶原蛋白的产生和胶原蛋白的mRNA降低至44％和40％，而总掺入和poly（A）+ RNA仅受到很小的影响。与单独用TGF-β处理的细胞相比，同时暴露于γ-IFN和TGF-β的细胞产生的胶原蛋白更少，mRNA含量也更低。在对照和TGF-β处理的培养物中，γ-IFN减少了胶原蛋白的合成，而在用γ-IFN预处理的细胞中，TGF-β将胶原蛋白的合成增加了2倍。在含有血浆来源血清的培养基中获得的成纤维细胞菌株合成的胶原蛋白约为新鲜人血清存在时来自同一外植体的细胞的胶原蛋白含量的一半，而TGF-β刺激了两种细胞株中胶原蛋白的产生和mRNA的表达。我们得出的结论是，TGF-β，血清和γ-IFN通过独立的机制调节胶原蛋白的合成，并且这些成分的联合作用在伤口愈合和组织修复过程中对胶原蛋白的合成具有重要作用。

Collagen synthesis by human fibroblasts. Regulation by transforming growth factor-β in the presence of other inflammatory mediators

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