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LIM结构域同源框基因isl-1对胰岛淀粉样多肽基因转录的激活作用。

Activation of amylin gene transcription by LIM domain homeobox gene isl-1.

作者信息

Wang M, Drucker D J

机构信息

Departments of Medicine, Banting and Best Diabetes Centre, The Toronto Hospital, Ontario, Canada.

出版信息

Mol Endocrinol. 1996 Mar;10(3):243-51. doi: 10.1210/mend.10.3.8833653.

DOI:10.1210/mend.10.3.8833653
PMID:8833653
Abstract

The amylin (IAPP) and insulin genes are coexpressed in the pancreatic beta-cell and share related promoter elements that may bind similar islet transcription factors. The observation that these promoter elements contain AT-rich subdomains suggests that homeobox proteins may be important for the regulation of both insulin and amylin gene transcription. We show here that the LIM domain homeobox protein isl-1 activates the rat amylin promoter in both fibroblast and islet cell lines. Mutation of the rAMY promoter TAAT motifs was associated with a marked reduction in both basal and isl-1 -dependent transcriptional activity. The isl-1 homeodomain binds to the AT-rich AMY element (-156 to -137) in the human amylin (hAMY) gene promoter, and electrophoretic mobility shift assay experiments using isl-1 specific antiserum detected the formation of an hAMY-isl-1 complex using nuclear extract from InR1 -G9 islet cells. Although isl-1 binds to both the insulin and amylin gene promoter elements in vitro, these sequences display marked differences in their relative transcriptional properties when ligated adjacent to a heterologous promoter and transfected into InR1 -G9 islet cells. The insulin gene E2 sequence that binds isl-1 (-230 to -208) functions as a negative element, whereas the hAMY sequence activates the thymidine kinase promoter in islet, but not nonislet, cell lines. Transfection of isl-1-depleted isl-1 (AS)InR1 -G9 cell lines demonstrated that the E2 element continued to repress thymidine kinase promoter activity, whereas the positive transcriptional activity mediated by the AMY element was considerably reduced in isl-1 (AS)-InR1-G9 cell lines. These dat2 demonstrate that highly similar elements in islet hormone gene promoters display differential functional properties and support a role for the isl-1 homeodomain protein in the regulation of amylin, but not insulin, gene transcription.

摘要

胰淀素(胰岛淀粉样多肽,IAPP)基因和胰岛素基因在胰腺β细胞中共同表达,并共享相关的启动子元件,这些元件可能结合相似的胰岛转录因子。这些启动子元件含有富含AT的亚结构域,这一观察结果表明,同源框蛋白可能对胰岛素和胰淀素基因转录的调控很重要。我们在此表明,LIM结构域同源框蛋白Isl-1在成纤维细胞和胰岛细胞系中均能激活大鼠胰淀素启动子。大鼠胰淀素(rAMY)启动子TAAT基序的突变与基础转录活性和Isl-1依赖性转录活性的显著降低相关。Isl-1同源结构域与人胰淀素(hAMY)基因启动子中富含AT的AMY元件(-156至-137)结合,使用Isl-1特异性抗血清进行的电泳迁移率变动分析实验,利用InR1 -G9胰岛细胞的核提取物检测到了hAMY-Isl-1复合物的形成。尽管Isl-1在体外与胰岛素和胰淀素基因启动子元件都能结合,但当与异源启动子相邻连接并转染到InR1 -G9胰岛细胞中时,这些序列在其相对转录特性上显示出明显差异。与Isl-1结合的胰岛素基因E2序列(-230至-208)起负性元件的作用,而hAMY序列在胰岛细胞系而非非胰岛细胞系中激活胸苷激酶启动子。对耗尽Isl-1的Isl-1(AS)InR1 -G9细胞系进行转染表明,E2元件继续抑制胸苷激酶启动子活性,而在Isl-1(AS)-InR1-G9细胞系中,由AMY元件介导的正性转录活性显著降低。这些数据表明,胰岛激素基因启动子中高度相似的元件具有不同的功能特性,并支持Isl-1同源结构域蛋白在胰淀素而非胰岛素基因转录调控中的作用。

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