首页> 美国卫生研究院文献>Molecular and Cellular Biology >Binding sites for hepatocyte nuclear factor 3 beta or 3 gamma and pancreas transcription factor 1 are required for efficient expression of the gene encoding pancreatic alpha-amylase.
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Binding sites for hepatocyte nuclear factor 3 beta or 3 gamma and pancreas transcription factor 1 are required for efficient expression of the gene encoding pancreatic alpha-amylase.

机译:肝细胞核因子3β或3γ和胰腺转录因子1的结合位点是有效表达编码胰腺α-淀粉酶的基因所必需的。

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摘要

Efficient expression of genes under the control of alpha-amylase 2 5'-flanking sequences in exocrine pancreatic cells requires, in addition to the pancreas transcription factor 1 binding site (M. Cockell, B.J. Stevenson, M. Strubin, O. Hagenbüchle, and P. K. Wellauer, Mol. Cell. Biol. 9:2464-2476, 1989), another cis-acting element at positions -60 to -86. This DNA element, which contains an AT-rich core, site for nuclear proteins present not only in the pancreas but also in other tissues and cell lines derived from the endoderm. Purification of binding activities from pancreatic cells by DNA affinity chromatography reveals several distinct proteins ranging in size from 45 to 54 kDa (p45, p47/48, and p54). All of these proteins interact with the specific DNA sequence upon renaturation in vitro. Protein sequencing, electrophoretic mobility shift assay, and immunoblot analyses identify p54 and p47/48 as members of the hepatocyte nuclear factor 3 (HNF3 [forkhead]) family of transcription factors. p54 belongs to the subfamily of HNF3 beta proteins, while p47/48 binding activity includes HNF3 gamma. The cDNAs for two HNF3 beta proteins differing only in N-terminal amino acid sequences were isolated from a pancreatic cDNA library. The mRNAs encoding the two protein species accumulate to different steady-state levels in poly(A)+ RNA of pancreatic cells. Our results support a model by which the pancreas-specific expression of the alpha-amylase gene is mediated by a combination of cell-specific and cell lineage-specific transcription factors.
机译:除了胰腺转录因子1结合位点外,在外分泌胰腺细胞中受α-淀粉酶2 5'侧翼序列控制的基因的有效表达还需要(M.Cockell,BJ Stevenson,M.Strubin,O.Hagenbüchle和PK Wellauer,分子细胞生物学(Mol.Cell.Biol。)9:2464-2476,1989),另一种在-60至-86位的顺式作用元件。这种DNA元素包含一个富含AT的核心,不仅在胰腺中而且在从内胚层衍生的其他组织和细胞系中也存在核蛋白的位点。通过DNA亲和层析从胰腺细胞中纯化结合活性,揭示了几种不同的蛋白质,大小从45至54 kDa不等(p45,p47 / 48和p54)。在体外复性后,所有这些蛋白质都与特定的DNA序列相互作用。蛋白质测序,电泳迁移率变动分析和免疫印迹分析确定p54和p47 / 48为转录因子的肝细胞核因子3(HNF3 [forkhead])家族的成员。 p54属于HNF3β蛋白的亚家族,而p47 / 48的结合活性包括HNF3γ。从胰腺cDNA文库中分离出两个仅在N末端氨基酸序列上不同的HNF3β蛋白的cDNA。编码这两种蛋白质的mRNA在胰腺细胞的poly(A)+ RNA中积累到不同的稳态水平。我们的结果支持一种模型,通过该模型,胰腺特异性表达的α-淀粉酶基因受细胞特异性和细胞谱系特异性转录因子的组合介导。

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