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激活素对促卵泡激素β亚基基因的调控涉及Smads以及TALE同源结构域蛋白Pbx1和Prep1。

Activin regulation of the follicle-stimulating hormone beta-subunit gene involves Smads and the TALE homeodomain proteins Pbx1 and Prep1.

作者信息

Bailey Janice S, Rave-Harel Naama, McGillivray Shauna M, Coss Djurdjica, Mellon Pamela L

机构信息

Department of Reproductive Medicine, University of California, San Diego, 9500 Gilman Drive, La Jolla, California 92093-0674, USA.

出版信息

Mol Endocrinol. 2004 May;18(5):1158-70. doi: 10.1210/me.2003-0442. Epub 2004 Feb 5.

Abstract

FSH is critical for normal reproductive function in both males and females. Activin, a member of the TGFbeta family of growth factors, is an important regulator of FSH expression, but little is known about the molecular mechanisms through which it acts. We used transient transfections into the immortalized gonadotrope cell line LbetaT2 to identify three regions (at -973/-962, -167, and -134) of the ovine FSH beta-subunit gene that are required for full activin response. All three regions contain homology to consensus binding sites for Smad proteins, the intracellular mediators of TGFbeta family signaling. Mutation of the distal site reduces activin responsiveness, whereas mutation of either proximal site profoundly disrupts activin regulation of the FSHbeta gene. These sites specifically bind LbetaT2 nuclear proteins in EMSAs, and the -973/-962 site binds Smad4 protein. Interestingly, the protein complex binding to the -134 site contains Smad4 in association with the homeodomain proteins Pbx1 and Prep1. Using glutathione S-transferase interaction assays, we demonstrate that Pbx1 and Prep1 interact with Smads 2 and 3 as well. The two proximal activin response elements are well conserved across species, and Pbx1 and Prep1 proteins bind to the mouse gene in vivo. Furthermore, mutation of either proximal site abrogates activin responsiveness of a mouse FSHbeta reporter gene as well, confirming their functional conservation. Our studies provide a basis for understanding activin regulation of FSHbeta gene expression and identify Pbx1 and Prep1 as Smad partners and novel mediators of activin action.

摘要

促卵泡激素(FSH)对男性和女性的正常生殖功能至关重要。激活素是转化生长因子β(TGFβ)家族生长因子的成员,是FSH表达的重要调节因子,但对其作用的分子机制了解甚少。我们通过瞬时转染永生化促性腺激素细胞系LbetaT2,确定了绵羊FSHβ亚基基因的三个区域(-973 / -962、-167和-134),这些区域是激活素充分应答所必需的。所有这三个区域都与Smad蛋白(TGFβ家族信号传导的细胞内介质)的共有结合位点具有同源性。远端位点的突变会降低激活素的反应性,而近端任何一个位点的突变都会严重破坏激活素对FSHβ基因的调节。这些位点在电泳迁移率变动分析(EMSA)中特异性结合LbetaT2核蛋白,并且-973 / -962位点结合Smad4蛋白。有趣的是,与-134位点结合的蛋白质复合物包含与同源结构域蛋白Pbx1和Prep1结合的Smad4。使用谷胱甘肽S-转移酶相互作用分析,我们证明Pbx1和Prep1也与Smad2和Smad3相互作用。两个近端激活素反应元件在物种间高度保守,并且Pbx1和Prep1蛋白在体内与小鼠基因结合。此外,任一近端位点的突变也会消除小鼠FSHβ报告基因的激活素反应性,证实了它们的功能保守性。我们的研究为理解激活素对FSHβ基因表达的调节提供了基础,并确定Pbx1和Prep1为Smad蛋白的伙伴以及激活素作用的新型介质。

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