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多个核心同源异型结构域结合基序对小鼠促性腺激素释放激素受体基因启动子的转录活性有不同贡献。

Multiple core homeodomain binding motifs differentially contribute to transcriptional activity of the murine gonadotropin-releasing hormone receptor gene promoter.

作者信息

Lents Clay A, Farmerie Todd A, Cherrington Brian D, Clay Colin M

机构信息

Department of Animal and Dairy Science, College of Agricultural and Environmental Sciences, The University of Georgia, 316 Rhodes Center ADS, Athens, GA 30602, USA.

出版信息

Endocrine. 2009 Jun;35(3):356-64. doi: 10.1007/s12020-009-9167-1. Epub 2009 Mar 31.

DOI:10.1007/s12020-009-9167-1
PMID:19333792
Abstract

Multiple homeodomain (Hbox) proteins have been shown to organize expression of key markers of gonadotropes. Nine putative Hbox-binding sites, characterized by the homeospecific TAAT motif, are located within the proximal 600 bp of the murine GnRHR promoter. Homeoproteins bind separate Hbox sites within this promoter, supporting basal- and endocrine-directed transcription. The function of the most proximal sites (Hbox1 and Hbox2) in the murine GnRHR is unknown; thus, understanding of the global contribution of homeospecific TAAT sites to promoter function is incomplete. Site-directed mutagenesis revealed that loss of Hbox2 reduced promoter activity in a cell-specific manner, having no effect in alphaT3-1 cells but reducing promoter function in LbetaT2 cells, another gonadotrope-derived cell line representing a later developmental stage. In contrast, eliminating Hbox1 reduced basal activity in both lines. This region displayed specific binding to homeoprotein Oct-1. Mutagenesis of a previously identified Oct-1-binding site in concert with Hbox1 led to further reduction in activity. We suggest that the two most proximal homeodomain-binding sites in the murine GnRHR promoter may regulate the promoter in a developmentally dependent fashion and that Oct-1 acts at multiple but distinct TAAT sites to support basal transcription.

摘要

多种同源异型结构域(Hbox)蛋白已被证明可调控促性腺激素细胞关键标志物的表达。九个推定的Hbox结合位点,其特征为同源特异性TAAT基序,位于小鼠促性腺激素释放激素受体(GnRHR)启动子近端600 bp内。同源蛋白结合该启动子内不同的Hbox位点,支持基础转录和内分泌定向转录。小鼠GnRHR中最近端位点(Hbox1和Hbox2)的功能尚不清楚;因此,对同源特异性TAAT位点对启动子功能的整体贡献的理解并不完整。定点诱变显示,Hbox2缺失以细胞特异性方式降低启动子活性,对αT3-1细胞无影响,但降低LβT2细胞(另一种代表后期发育阶段的促性腺激素细胞系)中的启动子功能。相反,去除Hbox1降低了两种细胞系中的基础活性。该区域显示与同源蛋白Oct-1特异性结合。与Hbox1协同作用对先前鉴定的Oct-1结合位点进行诱变导致活性进一步降低。我们认为,小鼠GnRHR启动子中两个最近端的同源异型结构域结合位点可能以发育依赖性方式调控启动子,并且Oct-1在多个但不同的TAAT位点起作用以支持基础转录。

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本文引用的文献

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A composite element that binds basic helix loop helix and basic leucine zipper transcription factors is important for gonadotropin-releasing hormone regulation of the follicle-stimulating hormone beta gene.一种结合碱性螺旋-环-螺旋和碱性亮氨酸拉链转录因子的复合元件,对促性腺激素释放激素调节促卵泡激素β基因至关重要。
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Activity of the porcine gonadotropin-releasing hormone receptor gene promoter is partially conferred by a distal gonadotrope specific element (GSE) within an upstream enhancing region, two proximal GSEs and a retinoid X receptor binding site.
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Reprod Biol Endocrinol. 2015 May 17;13:45. doi: 10.1186/s12958-015-0033-0.
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Mechanisms underlying the tissue-specific and regulated activity of the Gnrhr promoter in mammals.哺乳动物 GnRHR 启动子组织特异性和调节活性的作用机制。
Front Endocrinol (Lausanne). 2012 Dec 13;3:162. doi: 10.3389/fendo.2012.00162. eCollection 2012.
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7
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8
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9
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Mol Endocrinol. 2004 May;18(5):1158-70. doi: 10.1210/me.2003-0442. Epub 2004 Feb 5.