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多种启动子元件有助于睾丸支持细胞中促卵泡激素受体(FSHR)基因的活性。

Multiple promoter elements contribute to activity of the follicle-stimulating hormone receptor (FSHR) gene in testicular Sertoli cells.

作者信息

Heckert L L, Daggett M A, Chen J

机构信息

Department of Molecular and Integrative Physiology, The University of Kansas Medical Center, Kansas City 66160, USA.

出版信息

Mol Endocrinol. 1998 Oct;12(10):1499-512. doi: 10.1210/mend.12.10.0183.

Abstract

The FSH receptor (FSHR) is expressed only in granulosa cells of the ovary and Sertoli cells of the testis. This highly specific pattern of gene expression asserts that transcriptional events unique to these two cell types are responsible for activation of the FSHR gene. We have characterized the promoter elements required for activity of the rat FSHR gene in a Sertoli cell line MSC-1, primary cultures of rat Sertoli cells, and two non-Sertoli cell lines. Transient transfection analysis of deletion and block replacement mutants identified several elements, both 5' and 3' to the transcriptional start sites, that are essential for full promoter activity in Sertoli cells. These studies confirmed the use of an important E box element (CACGTG), which had the single greatest impact on promoter function. Bases within the core CACGTG of the E box, as well as flanking sequences, were shown to be essential for its function. Electrophoretic mobility shift assays identified both upstream stimulatory factor 1 (USF1) and USF2 as primary components of the complexes binding the E box. Sequence requirements for USF binding in vitro modestly diverged from the sequence requirements for in vivo function of the element. Comparison of the E box binding proteins in different cell types revealed that similar proteins bind the E box in Sertoli and non-Sertoli cell lines. Extracts from primary cultures of rat and mouse Sertoli cells have a second E box-binding complex that cross-reacts with USF antibodies that is not present in the cell lines.

摘要

促卵泡激素受体(FSHR)仅在卵巢的颗粒细胞和睾丸的支持细胞中表达。这种高度特异性的基因表达模式表明,这两种细胞类型特有的转录事件负责FSHR基因的激活。我们已经在支持细胞系MSC-1、大鼠支持细胞原代培养物和两种非支持细胞系中,对大鼠FSHR基因活性所需的启动子元件进行了表征。对缺失和阻断替代突变体的瞬时转染分析确定了几个元件,位于转录起始位点的5'和3'端,这些元件对于支持细胞中的完全启动子活性至关重要。这些研究证实了一个重要的E盒元件(CACGTG)的作用,它对启动子功能的影响最大。E盒核心CACGTG内的碱基以及侧翼序列对其功能至关重要。电泳迁移率变动分析确定上游刺激因子1(USF1)和USF2是与E盒结合的复合物的主要成分。体外USF结合的序列要求与该元件体内功能的序列要求略有不同。不同细胞类型中E盒结合蛋白的比较表明,支持细胞系和非支持细胞系中存在相似的蛋白与E盒结合。大鼠和小鼠支持细胞原代培养物的提取物有一种与USF抗体发生交叉反应的第二个E盒结合复合物,而细胞系中不存在这种复合物。

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