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Live-Cell Imaging of Endogenous mRNAs with a Small Molecule

机译:小分子内源性mRNA的活细胞成像

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摘要

Determination of subcellular localization and dynamics of mRNA is increasingly important to understanding gene expression. A new convenient and versatile method is reported that permits spatiotemporal imaging of specific non-engineered RNAs in living cells. The method uses transfection of a plasmid encoding a gene-specific RNA aptamer, combined with a cell-permeable synthetic small molecule, the fluorescence of which is restored only when the RNA aptamer hybridizes with its cognitive mRNA. The method was validated by live-cell imaging of the endogenous mRNA of -actin. Application of the technology to mRNAs of a total of 84 human cytoskeletal genes allowed us to observe cellular dynamics of several endogenous mRNAs including arfaptin-2, cortactin, and cytoplasmic FMR1-interacting protein2. The RNA-imaging technology and its further optimization might permit live-cell imaging of any RNA molecules.
机译:确定亚细胞定位和mRNA的动力学对于理解基因表达越来越重要。据报道,一种新的方便且通用的方法允许对活细胞中特定的非工程RNA进行时空成像。该方法使用编码基因特异性RNA适体的质粒转染,并与细胞可渗透的合成小分子结合,仅当RNA适体与其认知mRNA杂交时,其荧光才能恢复。该方法已通过活细胞成像内-肌动蛋白的mRNA验证。该技术对总共84个人类细胞骨架基因的mRNA的应用使我们能够观察到几种内源性mRNA的细胞动力学,包括afaptin-2,cortactin和胞质FMR1相互作用蛋白2。 RNA成像技术及其进一步优化可能允许对任何RNA分子进行活细胞成像。

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