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RNA conformation and folding studied with fluorescence resonance energy transfer.

机译:RNA构象和折叠研究与荧光共振能量转移。

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Fluorescence resonance energy transfer (FRET) results from nonradiative coupling of two fluorophores and reports on distances in the range 10-100 A. It is therefore a suitable probe to determine distances in RNA molecules and define their global structure, to follow kinetics of RNA conformational changes during folding in real time, to monitor ion binding, or to analyze conformational equilibria and assess the thermodynamic stability of tertiary structure conformers. Along with the basic principles of steady-state and time-resolved fluorescence resonance energy transfer measurements, approaches to investigate RNA conformational transitions and folding are described and illustrated with selected examples. The versatility of FRET-based techniques has recently been demonstrated by implementations of FRET in high-throughput screening of potential drugs as well as studies of energy transfer that monitor RNA conformational changes on the single-molecule level.
机译:荧光共振能量转移(FRET)是由两个荧光团的非辐射偶联产生的,并报告了10-100 A范围内的距离。因此,它是确定RNA分子中的距离并定义其整体结构以遵循RNA构象动力学的合适探针。实时折叠过程中的变化,以监测离子结合或分析构象平衡并评估三级结构构象异构体的热力学稳定性。除了稳态和时间分辨荧光共振能量转移测量的基本原理外,还介绍了一些研究RNA构象转变和折叠的方法,并通过选定的例子进行了说明。最近,通过FRET在潜在药物的高通量筛选中的应用以及在单分子水平上监测RNA构象变化的能量转移研究,已证明了基于FRET的技术的多功能性。

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