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Stopped-flow fluorescence resonance energy transfer for analysis of nucleosome dynamics.

机译:停止流荧光共振能量转移,用于分析核小体动力学。

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摘要

Macromolecular assemblies and machines undergo large-scale conformational changes as essential features of their normal function. Modern stopped-flow instrumentation and biotechnology combine to provide a powerful tool for characterizing the rates and natures of these conformational changes. Standard commercially available instruments provide extraordinary sensitivity and speed, allowing analysis of millisecond or longer timescale processes, with concentrations as low as a few nanomolar and volumes of just a few hundred microliters. One can now place specific dyes anywhere desired on a nucleic acid, and often on a protein as well. This ability allows the use of fluorescence resonance energy transfer experiments for detailed conformational analyses, even as the system is evolving rapidly over time following the initiation of a reaction. This approach is ideally suited for analysis of intrinsic properties of chromatin and of the machines that control chromatin assembly, disassembly, and function.
机译:大分子组装体和机器作为其正常功能的基本特征经历了大规模的构象变化。现代的止流仪器和生物技术相结合,为表征这些构象变化的速率和性质提供了强大的工具。标准的商用仪器可提供非凡的灵敏度和速度,可分析几毫秒或更长时间的过程,其浓度低至几纳摩尔,体积仅为几百微升。现在,人们可以将特定的染料放置在核酸上所需的任何位置,通常也可以放置在蛋白质上。此功能允许使用荧光共振能量转移实验进行详细的构象分析,即使系统在反应开始后随时间而迅速发展。该方法非常适合分析染色质的内在特性以及控制染色质组装,拆卸和功能的机器。

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