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通过羟基自由基足迹法探究RNA折叠

Probing RNA folding by hydroxyl radical footprinting.

作者信息

Costa Maria, Monachello Dario

机构信息

Centre de Génétique Moléculaire du C.N.R.S., Gif-sur-Yvette, France.

出版信息

Methods Mol Biol. 2014;1086:119-42. doi: 10.1007/978-1-62703-667-2_7.

Abstract

In recent years RNA molecules have emerged as central players in the regulation of gene expression. Many of these noncoding RNAs possess well-defined, complex, three-dimensional structures which are essential for their biological function. In this context, much effort has been devoted to develop computational and experimental techniques for RNA structure determination. Among available experimental tools to investigate the higher-order folding of structured RNAs, hydroxyl radical probing stands as one of the most informative and reliable ones. Hydroxyl radicals are oxidative species that cleave the nucleic acid backbone solely according to the solvent accessibility of individual phosphodiester bonds, with no sequence or secondary structure specificity. Therefore, the cleavage pattern obtained directly reflects the degree of protection/exposure to the solvent of each section of the molecule under inspection, providing valuable information about how these different sections interact together to form the final three-dimensional architecture. In this chapter we describe a robust, accurate and very sensitive hydroxyl radical probing method that can be applied to any structured RNA molecule and is suitable to investigate RNA folding and RNA conformational changes induced by binding of a ligand.

摘要

近年来,RNA分子已成为基因表达调控的核心参与者。这些非编码RNA中的许多都具有明确、复杂的三维结构,这些结构对其生物学功能至关重要。在此背景下,人们投入了大量精力来开发用于RNA结构测定的计算和实验技术。在用于研究结构化RNA高阶折叠的现有实验工具中,羟基自由基探测是最具信息性和可靠性的工具之一。羟基自由基是氧化物种,它仅根据单个磷酸二酯键的溶剂可及性切割核酸主链,没有序列或二级结构特异性。因此,直接获得的切割模式直接反映了被检查分子各部分对溶剂的保护/暴露程度,提供了有关这些不同部分如何相互作用以形成最终三维结构的有价值信息。在本章中,我们描述了一种强大、准确且非常灵敏的羟基自由基探测方法,该方法可应用于任何结构化RNA分子,适用于研究由配体结合诱导的RNA折叠和RNA构象变化。

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