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促黄体生成素受体信使核糖核酸的下调是通过细胞外信号调节激酶依赖的RNA结合蛋白诱导介导的。

Luteinizing hormone receptor mRNA down-regulation is mediated through ERK-dependent induction of RNA binding protein.

作者信息

Menon Bindu, Franzo-Romain Megan, Damanpour Shadi, Menon K M J

机构信息

Department of Obstetrics/Gynecology, University of Michigan Medical School, Ann Arbor, Michigan 48109-0617, USA.

出版信息

Mol Endocrinol. 2011 Feb;25(2):282-90. doi: 10.1210/me.2010-0366. Epub 2010 Dec 8.

DOI:10.1210/me.2010-0366
PMID:21147848
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3386540/
Abstract

The ligand-induced down-regulation of LH receptor (LHR) expression in the ovaries, at least in part, is regulated by a posttranscriptional process mediated by a specific LH receptor mRNA binding protein (LRBP). The LH-mediated signaling pathways involved in this process were examined in primary cultures of human granulosa cells. Treatment with 10 IU human chorionic gonadotropin (hCG) for 12 h resulted in the down-regulation of LHR mRNA expression while producing an increase in LHR mRNA binding to LRBP as well as a 2-fold increase in LRBP levels. The activation of ERK1/2 pathway in LH-mediated LHR mRNA down-regulation was also established by demonstrating the translocation of ERK1/2 from the cytosol to the nucleus using confocal microcopy. Inhibition of protein kinase A using H-89 or ERK1/2 by U0126 abolished the LH-induced LHR mRNA down-regulation. These treatments also abrogated both the increases in LRBP levels as well as the LHR mRNA binding activity. The abolishment of the hCG-induced increase in LRBP levels and LHR mRNA binding activity was further confirmed by transfecting granulosa cells with ERK1/2 specific small interfering RNA. This treatment also reversed the hCG-induced down-regulation of LHR mRNA. These data show that LH-regulated ERK1/2 signaling is required for the LRBP-mediated down-regulation of LHR mRNA.

摘要

配体诱导的卵巢中促黄体生成素受体(LHR)表达下调至少部分受特定促黄体生成素受体mRNA结合蛋白(LRBP)介导的转录后过程调控。在人颗粒细胞原代培养物中研究了参与该过程的促黄体生成素介导的信号通路。用10 IU人绒毛膜促性腺激素(hCG)处理12小时导致LHR mRNA表达下调,同时LHR mRNA与LRBP的结合增加,且LRBP水平增加了2倍。通过共聚焦显微镜观察到ERK1/2从细胞质转移到细胞核,也证实了ERK1/2通路在促黄体生成素介导的LHR mRNA下调中的激活。用H-89抑制蛋白激酶A或用U0126抑制ERK1/2消除了促黄体生成素诱导的LHR mRNA下调。这些处理也消除了LRBP水平的增加以及LHR mRNA结合活性。用ERK1/2特异性小干扰RNA转染颗粒细胞进一步证实了hCG诱导的LRBP水平和LHR mRNA结合活性增加的消除。该处理还逆转了hCG诱导的LHR mRNA下调。这些数据表明,促黄体生成素调节的ERK1/2信号传导是LRBP介导的LHR mRNA下调所必需的。

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