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PTGS2(前列腺素内过氧化物合酶-2)在足月人体羊膜中的表达涉及快速的 mRNA 周转、聚合酶-II 的 5'-暂停和糖皮质激素的转录阻遏。

PTGS2 (prostaglandin endoperoxide synthase-2) expression in term human amnion in vivo involves rapid mRNA turnover, polymerase-II 5'-pausing, and glucocorticoid transrepression.

机构信息

Mothers and Babies Research Centre, Hunter Medical Research Institute, Newcastle, New South Wales 2305, Australia.

出版信息

Endocrinology. 2011 May;152(5):2113-22. doi: 10.1210/en.2010-1327. Epub 2011 Mar 8.

DOI:10.1210/en.2010-1327
PMID:21385935
Abstract

The in vivo role of glucocorticoids in controlling prostaglandin endoperoxide synthase-2 (PTGS2) expression in the human amnion is unclear despite extensive studies using in vitro models. We addressed this issue by determining PTGS2 mRNA levels and gene transcriptional activity, RNA polymerase-II (pol-II) binding, pol-II C-terminal domain (CTD) phosphorylation, histone acetylation, and histone methylation at the PTGS2 gene in fresh amnion and in amnion explants incubated with dexamethasone for 24 h after delivery, when adaptation from in vivo to in vitro conditions occurred. PTGS2 mRNA turnover changed during incubation involving the initial rapid decrease and subsequent rebound of the transcription rate and stabilization of mRNA. pol-II accumulated in the 5'-region of the gene, which indicated postinitiation pausing. pol-II binding, 5'-accumulation, C-terminal domain Ser-5 and Ser-2 phosphorylation, and histone acetylation decreased rapidly and did not reverse during the transcriptional rebound, suggesting that the transcriptional mechanism altered in vitro. Dexamethasone decreased PTGS2 gene activity and mRNA levels. Glucocorticoid receptor-α (GRα) was bound to the PTGS2 promoter but did not affect pol-II recruitment, pausing, or the epigenetic marks. GRα binding, however, decreased initiating (Ser-5) and elongating (Ser-2) pol-II phosphorylation. The ability of the PTGS2 promoter to bind GRα in response to dexamethasone diminished during incubation. We conclude that PTGS2 mRNA turnover is accelerated in vivo, but the underlying mechanisms are not sustained beyond 24 h in explants. Glucocorticoids chronically transrepress PTGS2 gene activity in vivo in part by interfering with transcription initiation and elongation. Glucocorticoid transrepression of PTGS2 may be important for pregnancy maintenance and the timing of parturition.

摘要

尽管使用体外模型进行了广泛的研究,但糖皮质激素在控制人羊膜中前列腺素内过氧化物合酶-2(PTGS2)表达中的体内作用仍不清楚。我们通过测定新鲜羊膜和分娩后 24 小时用地塞米松孵育的羊膜外植体中 PTGS2 mRNA 水平和基因转录活性、RNA 聚合酶-II(pol-II)结合、pol-II C 末端结构域(CTD)磷酸化、组蛋白乙酰化和 PTGS2 基因的组蛋白甲基化来解决这个问题,此时体内条件向体外条件适应。孵育过程中 PTGS2 mRNA 的周转率发生了变化,涉及转录率的快速初始下降和随后的反弹以及 mRNA 的稳定。pol-II 在基因的 5'-区域积累,表明起始后暂停。pol-II 结合、5'-积累、CTD Ser-5 和 Ser-2 磷酸化以及组蛋白乙酰化迅速下降,在转录反弹过程中并未逆转,表明体外转录机制发生了改变。地塞米松降低了 PTGS2 基因的活性和 mRNA 水平。糖皮质激素受体-α(GRα)结合到 PTGS2 启动子上,但不影响 pol-II 的募集、暂停或表观遗传标记。然而,GRα 结合减少了起始(Ser-5)和延伸(Ser-2)pol-II 磷酸化。PTGS2 启动子在孵育过程中响应地塞米松结合 GRα 的能力减弱。我们的结论是,PTGS2 mRNA 的周转率在体内加速,但外植体中超过 24 小时后,潜在机制无法维持。糖皮质激素在体内通过干扰转录起始和延伸,慢性反式抑制 PTGS2 基因的活性。PTGS2 的糖皮质激素反式抑制可能对妊娠维持和分娩时机很重要。

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