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近端顺式作用元件,包括类固醇生成因子1,介导大鼠促性腺激素释放激素受体基因启动子中远端增强子的效率。

Proximal cis-acting elements, including steroidogenic factor 1, mediate the efficiency of a distal enhancer in the promoter of the rat gonadotropin-releasing hormone receptor gene.

作者信息

Pincas H, Amoyel K, Counis R, Laverrière J N

机构信息

Endocrinologie Cellulaire et Moléculaire de la Reproduction, Université Pierre et Marie Curie, Centre National de la Recherche Scientifique, ESA 7080, Case 244, Paris cedex 05, France.

出版信息

Mol Endocrinol. 2001 Feb;15(2):319-37. doi: 10.1210/mend.15.2.0593.

DOI:10.1210/mend.15.2.0593
PMID:11158337
Abstract

The gonadotrope-specific and regulated expression of the GnRH receptor (GnRH-R) gene is dependent on multiple transcription factors that interact with the noncanonical GnRH-R activating sequence (GRAS), the activator protein-1 (AP-1) element, and the steroidogenic factor-1 (SF-1) binding site. However, these three elements are not sufficient to mediate the complete cell-specific expression of the rat GnRH-R gene. In the present study, we demonstrate, by transient transfection in gonadotrope-derived alphaT3-1 and LssT2 cell lines, the existence of a distal enhancer [GnRH-R- specific enhancer (GnSE)] that is highly active in the context of the GnRH-R gene promoter. We show that the GnSE activity (-1,135/-753) is mediated through a functional interaction with a proximal region (-275/-226) that includes the SF-1 response element. Regions of similar length containing either the AP-1 or GRAS elements are less active or inactive. Transfection assays using an artificial promoter containing two SF-1 elements fused to a minimal PRL promoter indicate that SF-1 is crucial in this interaction. In addition, by altering the promoter with deletion and block- replacement mutations, we have identified the active elements of GnSE within two distinct sequences at positions -983/-962 and -871/-862. Sequence analysis and electrophoretic mobility shift experiments suggest that GnSE response elements interact, in these two regions, with GATA- and LIM-related factors, respectively. Altogether, these data establish the importance of the GnSE in the GnRH-R gene expression and reveal a novel role for SF-1 as a mediator of enhancer activity, a mechanism that might regulate other SF-1 target genes.

摘要

促性腺激素释放激素受体(GnRH-R)基因在促性腺细胞中的特异性表达及表达调控,依赖于多个转录因子,这些转录因子可与非典型GnRH-R激活序列(GRAS)、激活蛋白-1(AP-1)元件以及类固醇生成因子-1(SF-1)结合位点相互作用。然而,这三个元件并不足以介导大鼠GnRH-R基因完整的细胞特异性表达。在本研究中,我们通过在源自促性腺细胞的αT3-1和LssT2细胞系中进行瞬时转染,证明了存在一个远端增强子[GnRH-R特异性增强子(GnSE)],该增强子在GnRH-R基因启动子的背景下具有高活性。我们发现,GnSE活性区域(-1,135/-753)是通过与包含SF-1反应元件的近端区域(-275/-226)发生功能性相互作用来介导的。含有AP-元素或GRAS元件的长度相似的区域活性较低或无活性。使用包含两个与最小PRL启动子融合的SF-1元件的人工启动子进行转染分析表明,SF-1在这种相互作用中至关重要。此外,通过缺失和阻断-置换突变改变启动子,我们在-983/-962和-871/-862位置的两个不同序列中鉴定出了GnSE的活性元件。序列分析和电泳迁移率变动实验表明,GnSE反应元件在这两个区域分别与GATA相关因子和LIM相关因子相互作用。总之,这些数据证实了GnSE在GnRH-R基因表达中的重要性,并揭示了SF-1作为增强子活性介导因子的新作用,这一机制可能调控其他SF-1靶基因。

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