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Isolation sequence and expression of a human keratin K5 gene: transcriptional regulation of keratins and insights into pairwise control.

机译:人角蛋白K5基因的分离序列和表达:角蛋白的转录调控和成对控制的见解。

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摘要

The mitotically active basal layers of most stratified squamous epithelia express 10 to 30% of their total protein as keratin. The two keratins specifically expressed in these cells are the type II keratin K5 (58 kilodaltons) and its corresponding partner, type I keratin K14 (50 kilodaltons), both of which are essential for the formation of 8-nm filaments. Dissecting the molecular mechanisms underlying the coordinate regulation of the two keratins is an important first step in understanding epidermal differentiation and in designing promoters that will enable delivery and expression of foreign gene products in stratified squamous epithelia, e.g., skin. Previously, we reported the sequence of the gene encoding human K14 (D. Marchuk, S. McCrohon, and E. Fuchs, Cell 39:491-498, 1984; Marchuk et al., Proc. Natl. Acad. Sci. USA 82:1609-1613, 1985). We have now isolated and characterized the gene encoding human K5. The sequence of the coding portion of this gene matched perfectly with that of a partial K5 cDNA sequence obtained from a cultured human epidermal library (R. Lersch and E. Fuchs, Mol. Cell. Biol. 8:486-493, 1988), and gene transfection studies indicated that the gene is functional. Nuclear runoff experiments demonstrated that the K5 and K14 genes were both transcribed at dramatically higher levels in cultured human epidermal cells than in fibroblasts, indicating that at least part of the regulation of the expression of this keratin pair is at the transcriptional level. When the K5 gene was transfected transiently into NIH 3T3 fibroblasts, foreign expression of the gene caused the appearance of endogenous mouse K14 and the subsequent formation of a keratin filament array in the cells. In this case, transcriptional changes did not appear to be involved in the regulation, suggesting that there may be multiple control mechanisms underlying the pairwise expression of keratins.
机译:最分层的鳞状上皮细胞的有丝分裂活性基底层将其总蛋白的10%至30%表示为角蛋白。在这些细胞中特异性表达的两种角蛋白是II型角蛋白K5(58道尔顿)和其对应的伴侣I型角蛋白K14(50道尔顿),这两者对于形成8 nm的细丝都是必不可少的。剖析两种角蛋白的协调调节基础的分子机制是理解表皮分化和设计启动子的重要第一步,启动子将使外源基因产物能够在分层的鳞状上皮细胞(例如皮肤)中传递和表达。以前,我们报道了编码人K14的基因的序列(D. Marchuk,S。McCrohon和E. Fuchs,Cell 39:491-498,1984; Marchuk等,美国国家科学院学报82 :1609-1613,1985)。现在我们已经分离并鉴定了编码人K5的基因。该基因的编码部分的序列与从培养的人表皮文库中获得的部分K5 cDNA序列完全匹配(R. Lersch和E. Fuchs,Mol。Cell。Biol。8:486-493,1988),基因转染研究表明该基因具有功能。核径流实验表明,在培养的人表皮细胞中,K5和K14基因的转录水平都比成纤维细胞中的转录水平高得多,这表明该角蛋白对表达的至少部分调控是在转录水平上。当将K5基因瞬时转染到NIH 3T3成纤维细胞中时,该基因的外源表达导致内源性小鼠K14的出现以及随后在细胞中形成角蛋白丝阵列。在这种情况下,转录变化似乎不参与调节,表明角蛋白的成对表达可能存在多种控制机制。

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