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细胞色素P450 17α-羟化酶和类固醇生成急性调节蛋白基因启动子在正常和多囊卵巢综合征卵泡膜细胞中的差异活性

Differential activity of the cytochrome P450 17alpha-hydroxylase and steroidogenic acute regulatory protein gene promoters in normal and polycystic ovary syndrome theca cells.

作者信息

Wickenheisser J K, Quinn P G, Nelson V L, Legro R S, Strauss J F, McAllister J M

机构信息

Department of Cellular and Molecular Physiology, Pennsylvania State University College of Medicine, Hershey 17033, USA.

出版信息

J Clin Endocrinol Metab. 2000 Jun;85(6):2304-11. doi: 10.1210/jcem.85.6.6631.

Abstract

17alpha-Hydroxylase (CYP17) expression in propagated theca cells isolated from the ovaries of women with polycystic ovary syndrome (PCOS) is persistently elevated, compared with theca cells isolated from normal ovaries. To investigate the mechanism for increased CYP17 messenger RNA accumulation in PCOS theca cells, we examined CYP17 and steroidogenic acute regulatory protein (StAR) promoter activities in normal and PCOS theca cells. Conditions were established to transiently transfect human theca cells with reporter gene constructs containing 5' truncations of the human CYP17 and StAR promoters. Cotransfection of a steroidogenic factor-1 expression plasmid was found to be required for detection of basal and forskolin-stimulated CYP17 promoter activity but not for StAR promoter activity. However, cotransfection with a steroidogenic factor-1 expression plasmid augmented both basal and forskolin-stimulated StAR promoter activity. CYP17 reporter activity was compared in theca cells isolated from normal and PCOS patients. Basal and forskolin-stimulated CYP17 promoter activity was 4-fold greater in PCOS cells than in theca cells isolated from normal ovaries. In contrast, StAR promoter activity, and the activity of a reporter construct containing three copies of a cAMP response element (3xCRE), were similar in normal and PCOS theca cells. The results of these studies document: 1) that basal and cAMP-dependent CYP17 gene transcription is increased in PCOS theca cells; 2) that there is differential regulation of promoters of genes required for steroidogenesis in PCOS theca cells; and 3) that passaged normal and PCOS theca cells provide a model system for studying tissue-specific regulation of genes encoding steroidogenic enzymes and identifying the molecular mechanisms involved in increased androgen production in PCOS.

摘要

与从正常卵巢分离的卵泡膜细胞相比,从多囊卵巢综合征(PCOS)女性卵巢分离的传代卵泡膜细胞中17α-羟化酶(CYP17)的表达持续升高。为了研究PCOS卵泡膜细胞中CYP17信使核糖核酸积累增加的机制,我们检测了正常和PCOS卵泡膜细胞中CYP17和类固醇生成急性调节蛋白(StAR)的启动子活性。建立了用含有人类CYP17和StAR启动子5'端截短的报告基因构建体瞬时转染人类卵泡膜细胞的条件。发现检测基础和福斯可林刺激的CYP17启动子活性需要共转染类固醇生成因子-1表达质粒,但检测StAR启动子活性则不需要。然而,与类固醇生成因子-1表达质粒共转染可增强基础和福斯可林刺激的StAR启动子活性。比较了从正常和PCOS患者分离的卵泡膜细胞中的CYP17报告基因活性。PCOS细胞中基础和福斯可林刺激的CYP17启动子活性比从正常卵巢分离的卵泡膜细胞高4倍。相比之下,正常和PCOS卵泡膜细胞中的StAR启动子活性以及含有三个环磷酸腺苷反应元件(3xCRE)拷贝的报告构建体的活性相似。这些研究结果表明:1)PCOS卵泡膜细胞中基础和环磷酸腺苷依赖性CYP17基因转录增加;2)PCOS卵泡膜细胞中类固醇生成所需基因的启动子存在差异调节;3)传代的正常和PCOS卵泡膜细胞为研究编码类固醇生成酶的基因的组织特异性调节以及确定PCOS中雄激素产生增加所涉及的分子机制提供了一个模型系统。

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