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Site-Specific Fluorophore Labeling of Guanosines in RNA G-Quadruplexes

机译:RNA G四联体中鸟苷的特定位点荧光团标记

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摘要

RNA G-quadruplexes are RNA secondary structures that are implicated in many cellular processes. Although conventional biophysical techniques are widely used for their in vitro characterization, more advanced methods are needed to study complex equilibria and the kinetics of their folding. We have developed a new F?rster resonance energy-transfer-based method to detect the folding of RNA G-quadruplexes, which is enabled by labeling the 2′-positions of participating guanosines with fluorophores. Importantly, this does not interfere with the required anti conformation of the nucleobase in a quadruplex with parallel topology. Sequential click reactions on the solid phase and in solution using a stop-and-go strategy circumvented the issue of unselective cross-labeling. We exemplified the method on a series of sequences under different assay conditions. In contrast to the commonly used end-labeling approach, our internal labeling strategy would also allow the study of G-quadruplex formation in long functional RNAs.
机译:RNA G四链体是涉及许多细胞过程的RNA二级结构。尽管常规的生物物理技术已广泛用于体外表征,但仍需要更先进的方法来研究复杂的平衡及其折叠动力学。我们已经开发了一种新的基于Fsterster共振能量转移的方法来检测RNA G-四链体的折叠,该方法可通过用荧光团标记参与鸟嘌呤的2'-位来实现。重要的是,这不会干扰具有平行拓扑的四链体中所需的核碱基反构象。在固相和溶液中使用“走走停停”策略的连续点击反应避免了非选择性交叉标记的问题。我们在不同的测定条件下对一系列序列举例说明了该方法。与常用的末端标记方法相比,我们的内部标记策略还可以研究长功能RNA中G-四链体的形成。

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