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Validation of miRNA-mRNA interactions by electrophoretic mobility shift assays

机译:通过电泳迁移率变动分析验证miRNA-mRNA相互作用

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Background MicroRNAs are small non-coding RNAs involved in gene expression regulation by targeting specific regions in the 3′-UTR of the mRNA of their target genes. This binding leads to a decrease in the protein levels of such genes either by mRNA degradation or mRNA destabilization and translation inhibition. The interaction between a miRNA and its target mRNAs is usually studied by co-transfection of a reporter expression vector containing the 3′-UTR region of the mRNA and an inhibitory or precursor molecule for the miRNA . This approach, however, does not measure the direct and physical interaction between a miRNA and a specific mRNA . Findings RNA molecules corresponding to miR-224 and to the 3′-UTR of SLC4A4 were incubated together and their interaction studied under different binding conditions using electrophoretic mobility shift assays. A direct and specific interaction between miR-224 and SLC4A4 mRNA was observed. This interaction was abolished in the presence of competitors. Conclusions In this study, we explored a new application for the electrophoretic mobility shift assay and we demonstrated that it is a useful alternative method to assess, in a direct and specific manner, whether a miRNA binds to a specific predicted target mRNA .
机译:背景技术MicroRNA是通过靶向目标基因mRNA的3'-UTR中特定区域而参与基因表达调控的小型非编码RNA。通过mRNA降解或mRNA去稳定化和翻译抑制,这种结合导致此类基因的蛋白质水平降低。 miRNA与其靶mRNA之间的相互作用通常通过共转染包含mRNA的3'-UTR区域和miRNA的抑制或前体分子的报告基因表达载体来研究。但是,这种方法不能测量miRNA与特定mRNA之间的直接和物理相互作用。将与miR-224和SLC4A4的3'-UTR对应的发现RNA分子一起孵育,并使用电泳迁移率迁移分析在不同的结合条件下研究了它们的相互作用。观察到miR-224与SLC4A4 mRNA之间存在直接和特异性的相互作用。在竞争者在场的情况下取消了这种互动。结论在这项研究中,我们探索了电泳迁移率变动分析的新应用,并且证明了它是一种有用的替代方法,可以以直接和特异性的方式评估miRNA是否与特定的预测靶标mRNA结合。

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