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Target mRNAs are repressed as efficiently by microRNA-binding sites in the 5' UTR as in the 3' UTR

机译:靶标mRNA被3'UTR中的5'UTR中的microRNA结合位点有效抑制

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In animals, microRNAs (miRNAs) bind to the 3' UTRs of their target mRNAs and interfere with translation, although the exact mechanism of inhibition of protein synthesis remains unclear. Functional miRNA-binding sites in the coding regions or 5' UTRs of endogenous mRNAs have not been identified. We studied the effect of introducing miRNA target sites into the 5' UTR of luciferase reporter mRNAs containing internal ribosome entry sites (IRESs), so that potential steric hindrance by a microribonucleoprotein complex would not interfere with the initiation of translation. In human HeLa cells, which express endogenous let-7a miRNA, the translational efficiency of these IRES-containing reporters with 5' let-7 complementary sites from the Caenorhabditis elegans lin-41 3' UTR was repressed. Similarly, the IRES-containing reporters were translationally repressed when human Ago2 was tethered to either the 5' or 3' UTR. Interestingly, the method of DNA transfection affected our ability to observe miRNA-mediated repression. Our results suggest that association with any position on a target mRNA is mechanistically sufficient for a microribonucleoprotein to exert repression of translation at some step downstream of initiation.
机译:在动物中,微RNA(miRNA)与其靶mRNA的3'UTR结合并干扰翻译,尽管抑制蛋白质合成的确切机制仍不清楚。尚未确定内源性mRNA的编码区或5'UTR中的功能性miRNA结合位点。我们研究了将miRNA靶位点引入含有内部核糖体进入位点(IRESs)的荧光素酶报道基因mRNA的5'UTR中的作用,从而使微核糖核蛋白复合物潜在的空间位阻不会干扰翻译的启动。在表达内源性let-7a miRNA的人HeLa细胞中,这些含有IRES的报告子具有来自秀丽隐杆线虫lin-41 3'UTR的5'let-7互补位点的翻译效率受到抑制。同样,当将人类Ago2拴系在5'或3'UTR上时,含有IRES的报道分子受到翻译抑制。有趣的是,DNA转染方法影响了我们观察miRNA介导的阻遏的能力。我们的结果表明,与靶mRNA上任何位置的结合在机械上足以使微核糖核蛋白在起始下游的某个步骤发挥翻译抑制作用。

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