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同源结构域蛋白IPF-1/STF-1在一部分胰岛细胞中表达,并依赖完整的E1螺旋-环-螺旋因子结合位点促进大鼠胰岛素1基因的表达。

The homeodomain protein IPF-1/STF-1 is expressed in a subset of islet cells and promotes rat insulin 1 gene expression dependent on an intact E1 helix-loop-helix factor binding site.

作者信息

Serup P, Petersen H V, Pedersen E E, Edlund H, Leonard J, Petersen J S, Larsson L I, Madsen O D

机构信息

Hagedorn Research Institute, Gentofte, Denmark.

出版信息

Biochem J. 1995 Sep 15;310 ( Pt 3)(Pt 3):997-1003. doi: 10.1042/bj3100997.

DOI:10.1042/bj3100997
PMID:7575438
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1135994/
Abstract

The mouse homeodomain protein insulin promoter factor-1 (IPF-1) and the rat homologue somatostatin transactivating factor-1 (STF-1) are involved in early pancreatic development and have been implicated in the cell-specific regulation of insulin- and somatostatin-gene expression in mature islet beta- and delta-cells. The cell specificity of IPF-1/STF-1 expression in mature islets is, however, still unclear. Using antisera against recombinant IPF-1 and STF-1 in combination with antisera against islet hormones we find that all beta-cells in monolayers of newborn rat islet cells express STF-1, as do a fraction of the delta-cells. In adult rat and mouse pancreas we find a similar distribution. IPF-1/STF-1 expression was not detected in glucagon-producing alpha-cells. In islet cell tumour models we found that a glucagon/islet amyloid polypeptide (IAPP)-producing pluripotent rat islet cell line (NHI-6F-GLU) expresses STF-1 in all cells prior to insulin gene activation induced by in vivo culture. In contrast, a mouse alpha-cell line (alpha TC1) exclusively expressed IPF-1 in a small subset of insulin-producing cells while an insulin-negative subclone (alpha TC1.9) was negative for IPF-1. In transfection experiments using alpha TC1.9 cells STF-1 activated a rat insulin 1 reporter gene dependent not only on both STF-1-binding sites, but also on the E1-binding site for the helix-loop-helix factor IEF-1. However, the endogenous mouse insulin genes remained inactive in these cells. These results suggest that the insulin promoter acquires its very high, yet cell-specific, activity at least partly through the action of IPF-1/STF-1. This action is dependent on helix-loop-helix factors bound to the E1 element.

摘要

小鼠同源异型结构域蛋白胰岛素启动子因子-1(IPF-1)和大鼠同源物生长抑素反式激活因子-1(STF-1)参与胰腺早期发育,并与成熟胰岛β细胞和δ细胞中胰岛素和生长抑素基因表达的细胞特异性调控有关。然而,IPF-1/STF-1在成熟胰岛中表达的细胞特异性仍不清楚。使用针对重组IPF-1和STF-1的抗血清,结合针对胰岛激素的抗血清,我们发现新生大鼠胰岛细胞单层中的所有β细胞均表达STF-1,一部分δ细胞也表达。在成年大鼠和小鼠胰腺中我们发现了类似的分布。在产生胰高血糖素的α细胞中未检测到IPF-1/STF-1表达。在胰岛细胞瘤模型中,我们发现一个产生胰高血糖素/胰岛淀粉样多肽(IAPP)的多能大鼠胰岛细胞系(NHI-6F-GLU)在体内培养诱导胰岛素基因激活之前,所有细胞均表达STF-1。相反,一个小鼠α细胞系(αTC1)仅在一小部分产生胰岛素的细胞中表达IPF-1,而一个胰岛素阴性亚克隆(αTC1.9)对IPF-1呈阴性。在使用αTC1.9细胞的转染实验中,STF-1激活了大鼠胰岛素1报告基因,这不仅依赖于两个STF-1结合位点,还依赖于螺旋-环-螺旋因子IEF-1的E1结合位点。然而,内源性小鼠胰岛素基因在这些细胞中仍无活性。这些结果表明,胰岛素启动子至少部分通过IPF-1/STF-1的作用获得其非常高的、但具有细胞特异性的活性。这种作用依赖于与E1元件结合的螺旋-环-螺旋因子。

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Glucose modulates the binding activity of the beta-cell transcription factor IUF1 in a phosphorylation-dependent manner.葡萄糖以磷酸化依赖的方式调节β细胞转录因子IUF1的结合活性。
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一个高内涵体外胰岛β细胞复制发现平台。
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