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首页> 外文期刊>Biology of Reproduction: Offical Journal of the Society for the Study of Reproduction >Role of microRNA-136-3p on the expression of luteinizing hormone-human chorionic gonadotropin receptor mRNA in rat ovaries.
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Role of microRNA-136-3p on the expression of luteinizing hormone-human chorionic gonadotropin receptor mRNA in rat ovaries.

机译:microRNA-136-3p在大鼠卵巢中促黄体生成素-绒毛膜促性腺激素受体mRNA表达中的作用。

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摘要

MicroRNAs (miRNAs) are small noncoding RNAs that interact with mRNAs and trigger either translation repression or RNA cleavage of target genes. In this study, we investigated whether miRNA was involved in down-regulation of the luteinizing hormone receptor (LHR) in rat ovaries. An miRNA microarray was used to analyze the overall miRNA expression profile of rat ovaries in association with the down-regulation of LHR mRNA. We found that 23 miRNAs were highly expressed during this period. Combining these results with data from a bioinformatics database, clustering analysis led us to focus on miR-136-3p for further analysis. In both in vivo and in vitro studies, miR-136-3p expression levels were increased at 6 h after human chorionic gonadotropin (hCG) administration, concurrent with down-regulation of LHR mRNA. Moreover, transfection of cultured granulosa cells with miR-136-3p resulted in a significant decrease in LHR mRNA levels in comparison with those of cells transfected with negative control. In contrast, transfection with a miR-136-3p inhibitor increased LHR mRNA levels. Finally, cotransfection of granulosa cells with a miR-136-3p inhibitor and a reporter vector containing the 3'-untranslated region (UTR) of LHR mRNA and Renilla luciferase coding sequence revealed that miR-136-3p bound directly to the 3'-UTR of LHR mRNA. These data demonstrated that miR-136-3p participated in the down-regulation of LHR mRNA by binding directly to LHR mRNA.
机译:MicroRNA(miRNA)是小的非编码RNA,可与mRNA相互作用并触发目标基因的翻译抑制或RNA切割。在这项研究中,我们调查了miRNA是否参与大鼠卵巢中促黄体生成激素受体(LHR)的下调。使用miRNA芯片分析与LHR mRNA下调相关的大鼠卵巢总体miRNA表达谱。我们发现在此期间高表达23个miRNA。将这些结果与生物信息学数据库中的数据相结合,聚类分析使我们专注于miR-136-3p进行进一步分析。在体内和体外研究中,施用人绒毛膜促性腺激素(hCG)后6小时,miR-136-3p表达水平均升高,同时LHR mRNA下调。而且,与用阴性对照转染的细胞相比,用miR-136-3p转染培养的颗粒细胞可导致LHR mRNA水平显着降低。相反,用miR-136-3p抑制剂转染可增加LHR mRNA水平。最后,将颗粒细胞与miR-136-3p抑制剂和包含LHR mRNA 3'-非翻译区(UTR)和海肾荧光素酶编码序列的报道载体共转染显示,miR-136-3p直接与3'-结合LHR mRNA的UTR。这些数据表明,miR-136-3p通过直接结合LHR mRNA参与了LHR mRNA的下调。

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