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Site-specific fluorescent probing of RNA molecules by unnatural base-pair transcription for local structural conformation analysis

机译:通过非天然碱基对转录对RNA分子进行定点荧光探测,以进行局部结构构象分析

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摘要

Methods for fluorescent probing at a defined position of RNA provide powerful tools for analyzing the local structural conformation of functional RNA molecules by tracking fluorescence changes. In this article, we describe the site-specific fluorescent probing of RNA by transcription with an expanded genetic alphabet, using an extra, unnatural base pair between 2-amino-6-(2-thienyl)purine (s) and pyrrole-2-carbaldehyde (Pa). The protocol comprises template DNA preparation containing Pa, transcription involving fluorescent s incorporation and structural analysis of transcripts. The s base is strongly fluorescent, and its nucleoside 5′-triphosphate is site-specifically incorporated into RNA transcripts, opposite Pa in DNA templates, by conventional T7 transcription. The fluorescent intensity of s changes depending on its environment around the probe site, providing clues about the local structural features of RNA molecules. This is the first protocol for RNA transcript preparation with fluorescent labeling at a desired position. The procedure for s-containing RNA preparation takes about 2-3 d.
机译:在RNA的确定位置进行荧光探测的方法提供了强大的工具,可通过跟踪荧光变化来分析功能性RNA分子的局部结构构象。在本文中,我们通过使用扩展的遗传字母,使用2-氨基-6-(2-噻吩基)嘌呤和吡咯-2-之间的额外非天然碱基对,描述通过转录进行转录的RNA的位点特异性荧光探测。甲醛(Pa)。该方案包括含Pa的模板DNA制备,涉及荧光掺入的转录和转录物的结构分析。该s碱基是强荧光的,并且其核苷5'-三磷酸通过常规的T7转录被位点特异性地掺入DNA模板中与Pa相反的RNA转录物中。 s的荧光强度根据其在探针位点周围的环境而变化,从而提供了有关RNA分子局部结构特征的线索。这是在所需位置进行荧光标记的RNA转录物制备的第一个方案。含s RNA的制备过程大约需要2-3 d。

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