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促性腺激素释放激素受体基因的促性腺激素细胞表达是否由激活素反应元件的自分泌/旁分泌刺激介导?

Is gonadotrope expression of the gonadotropin releasing hormone receptor gene mediated by autocrine/paracrine stimulation of an activin response element?

作者信息

Duval D L, Ellsworth B S, Clay C M

机构信息

Department of Physiology, Colorado State University, Fort Collins 80523, USA.

出版信息

Endocrinology. 1999 Apr;140(4):1949-52. doi: 10.1210/endo.140.4.6780.

DOI:10.1210/endo.140.4.6780
PMID:10098536
Abstract

Expression of the FSHbeta subunit and GnRH receptor (GnRHR) genes in gonadotropes is stimulated by activin. We sought to identify the cis-acting element(s) in the murine GnRHR gene promoter which confer activin responsiveness. We established that 600 bp of 5'flanking sequence from the murine GnRHR gene were sufficient to confer activin responsiveness in the gonadotrope-derived alphaT3-1 cell line. Since alphaT3-1 cells, like gonadotropes, secrete activin, we examined the ability of follistatin, an activin binding protein, to block the activin response. Increasing concentrations of follistatin from 0 to 100 ng/ml resulted in a dose dependent decrease in activity of the -600 promoter. Contained within this region are three elements important for expression in alphaT3-1 cells: a Steroidogenic Factor-1 binding site (SF-1), an Activator Protein-1(AP-1) element, and an element termed the GnRH receptor activating sequence or GRAS. A block mutation of GRAS inhibited the ability of the promoter to respond to follistatin. A more refined analysis using a series of two-bp mutations which scan GRAS and flanking sequence revealed exact convergence of GRAS with activin/follistatin responsiveness. Finally, a construct consisting of 3 copies of GRAS placed upstream of a heterologous minimal promoter (3xGRAS-PRL-LUC) was responsive to both activin stimulation and follistatin inhibition in alphaT3-1 cells. Thus, autocrine/paracrine stimulation of gonadotropes by activin illustrates a unique mechanism for cell-specific gene expression.

摘要

促性腺激素细胞中促卵泡素β亚基和促性腺激素释放激素受体(GnRHR)基因的表达受激活素刺激。我们试图鉴定小鼠GnRHR基因启动子中赋予激活素反应性的顺式作用元件。我们确定,来自小鼠GnRHR基因的600 bp 5'侧翼序列足以在促性腺激素细胞来源的αT3-1细胞系中赋予激活素反应性。由于αT3-1细胞与促性腺激素细胞一样分泌激活素,我们检测了激活素结合蛋白卵泡抑素阻断激活素反应的能力。卵泡抑素浓度从0增加到100 ng/ml导致-600启动子活性呈剂量依赖性降低。该区域包含对αT3-1细胞表达重要的三个元件:一个类固醇生成因子-1结合位点(SF-1)、一个激活蛋白-1(AP-1)元件和一个称为GnRH受体激活序列或GRAS的元件。GRAS的阻断突变抑制了启动子对卵泡抑素反应的能力。使用一系列扫描GRAS及其侧翼序列的双碱基突变进行的更精细分析显示,GRAS与激活素/卵泡抑素反应性完全一致。最后,由3个GRAS拷贝置于异源最小启动子上游组成的构建体(3xGRAS-PRL-LUC)在αT3-1细胞中对激活素刺激和卵泡抑素抑制均有反应。因此,激活素对促性腺激素细胞的自分泌/旁分泌刺激说明了细胞特异性基因表达的独特机制。

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