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用于表征核糖开关折叠机制的单分子方法

Single-Molecule Approaches for the Characterization of Riboswitch Folding Mechanisms.

作者信息

Boudreault Julien, Perez-Gonzalez D Cibran, Penedo J Carlos, Lafontaine Daniel A

机构信息

Département de Biologie, Faculté des Sciences, Université de Sherbrooke, Sherbrooke, QC, Canada, J1K 2R1.

School of Physics and Astronomy, University of St. Andrews, St. Andrews, UK.

出版信息

Methods Mol Biol. 2015;1334:101-7. doi: 10.1007/978-1-4939-2877-4_6.

Abstract

Riboswitches are highly structured RNA molecules that control genetic expression by altering their structure as a function of metabolite binding. Accumulating evidence suggests that riboswitch structures are highly dynamic and perform conformational exchange between structural states that are important for the outcome of genetic regulation. To understand how ligand binding influences the folding of riboswitches, it is important to monitor in real time the riboswitch folding pathway as a function of experimental conditions. Single-molecule FRET (sm-FRET) is unique among biophysical techniques to study riboswitch conformational changes as it allows to both monitor steady-state populations of riboswitch conformers and associated interconversion dynamics. Since FRET fluorophores can be attached to virtually any nucleotide position, FRET assays can be adapted to monitor specific conformational changes, thus enabling to deduce complex riboswitch folding pathways. Herein, we show how to employ sm-FRET to study the folding pathway of the S-adenosylmethionine (SAM) and how this can be used to understand very specific conformational changes that are at the heart of riboswitch regulation mechanism.

摘要

核糖开关是高度结构化的RNA分子,通过根据代谢物结合改变其结构来控制基因表达。越来越多的证据表明,核糖开关结构具有高度动态性,并在对基因调控结果至关重要的结构状态之间进行构象交换。为了理解配体结合如何影响核糖开关的折叠,实时监测核糖开关折叠途径作为实验条件的函数非常重要。单分子荧光共振能量转移(sm-FRET)在研究核糖开关构象变化的生物物理技术中是独一无二的,因为它既能监测核糖开关构象体的稳态群体,又能监测相关的相互转化动力学。由于FRET荧光团几乎可以连接到任何核苷酸位置,FRET分析可以用于监测特定的构象变化,从而推断复杂的核糖开关折叠途径。在此,我们展示了如何利用sm-FRET研究S-腺苷甲硫氨酸(SAM)的折叠途径,以及如何利用它来理解处于核糖开关调控机制核心的非常特定的构象变化。

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