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催乳激素诱导β-酪蛋白基因调控元件之间的长距离相互作用。

Lactogenic hormonal induction of long distance interactions between beta-casein gene regulatory elements.

作者信息

Kabotyanski Elena B, Rijnkels Monique, Freeman-Zadrowski Courtneay, Buser Adam C, Edwards Dean P, Rosen Jeffrey M

机构信息

Departments of Molecular and Cellular Biology, Baylor College of Medicine, One Baylor Plaza, Mail Box BCM-130, Houston, TX 77030, USA.

出版信息

J Biol Chem. 2009 Aug 21;284(34):22815-24. doi: 10.1074/jbc.M109.032490. Epub 2009 Jun 19.

Abstract

Lactogenic hormone regulation of beta-casein gene expression in mammary epithelial cells provides an excellent model in which to study the mechanisms by which steroid and peptide hormone signaling control gene expression. Prolactin- and glucocorticoid-mediated induction of beta-casein gene expression involves two principal regulatory regions, a proximal promoter and a distal enhancer located in the mouse approximately -6 kb upstream of the transcription start site. Using a chromosome conformation capture assay and quantitative real time PCR, we demonstrate that a chromatin loop is created in conjunction with the recruitment of specific transcription factors and p300 in HC11 mammary epithelial cells. Stimulation with both prolactin and hydrocortisone is required for the induction of these long range interactions between the promoter and enhancer, and no DNA looping was observed in nontreated cells or cells treated with each of the hormones separately. The lactogenic hormone-induced interaction between the proximal promoter and distal enhancer was confirmed in hormone-treated primary three-dimensional mammary acini cultures. In addition, the developmental regulation of DNA looping between the beta-casein regulatory regions was observed in lactating but not in virgin mouse mammary glands. Furthermore, beta-casein mRNA induction and long range interactions between these regulatory regions were inhibited in a progestin-dependent manner following stimulation with prolactin and hydrocortisone in HC11 cells expressing human PR-B. Collectively, these data suggest that the communication between these regulatory regions with intervening DNA looping is a crucial step required to both create and maintain active chromatin domains and regulate transcription.

摘要

乳腺上皮细胞中β-酪蛋白基因表达的催乳激素调节提供了一个极佳的模型,用于研究类固醇和肽类激素信号传导控制基因表达的机制。催乳素和糖皮质激素介导的β-酪蛋白基因表达诱导涉及两个主要调控区域,一个近端启动子和一个位于小鼠转录起始位点上游约-6 kb处的远端增强子。使用染色体构象捕获分析和定量实时PCR,我们证明在HC11乳腺上皮细胞中,伴随着特定转录因子和p300的募集形成了一个染色质环。启动子和增强子之间这些长程相互作用的诱导需要催乳素和氢化可的松的共同刺激,在未处理的细胞或单独用每种激素处理的细胞中未观察到DNA环化。在激素处理的原代三维乳腺腺泡培养物中证实了近端启动子和远端增强子之间催乳激素诱导的相互作用。此外,在泌乳小鼠乳腺中观察到β-酪蛋白调控区域之间DNA环化的发育调控,而在处女小鼠乳腺中未观察到。此外,在表达人PR-B的HC11细胞中,用催乳素和氢化可的松刺激后,这些调控区域之间的β-酪蛋白mRNA诱导和长程相互作用以孕激素依赖的方式受到抑制。这些数据共同表明,这些调控区域之间通过中间DNA环化的通讯是创建和维持活性染色质结构域以及调节转录所需的关键步骤。

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