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Multiplexed tethered particle microscopy for studies of DNA-enzyme dynamics

机译:用于研究DNA酶动力学的多重束缚粒子显微镜

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摘要

DNA is the carrier of genetic information, and as such, is at the center of most essential cellular processes. To regulate its physiological function, specific proteins and motor enzymes constantly change its conformational state with well controlled dynamics. Twenty-five years ago, Schafer, Gelles, Sheetz and Landick employed the Tethered Particle Motion (TPM) technique for the first time to study transcription by RNA polymerase at the single-molecule level. TPM has since then remained one of the simplest, most affordable and yet incisive single-molecule techniques available. It is an in vitro technique which allows investigation of DNA-protein interactions that change the effective length of a DNA tether. In this chapter, we will describe a recent strategy to multiplex TPM which substantially increases the throughput of TPM experiments, as well as a simulation to estimate the time-resolution of experiments, such as transcriptional elongation assays, in which lengthy time averaging of the signal is impossible due to continual change of the DNA tether length. These improvements allow efficient study of several DNA-protein systems, including transcriptionally active DNA-RNA polymerase I complexes and DNA-gyrase complexes.
机译:DNA是遗传信息的载体,因此,DNA是最重要的细胞过程的中心。为了调节其生理功能,特定的蛋白质和运动酶通过受控的动力学不断地改变其构象状态。 25年前,Schafer,Gilles,Sheetz和Landick首次使用束缚粒子运动(TPM)技术研究单分子水平上RNA聚合酶的转录。从那时起,TPM一直是最简单,最实惠,但仍具有启发性的单分子技术之一。这是一项体外技术,可用于研究改变DNA系链有效长度的DNA-蛋白质相互作用。在本章中,我们将介绍一种最新的TPM多路复用策略,该策略可显着提高TPM实验的通量,并提供一种模拟方法来估计实验的时间分辨率,例如转录延伸测定,其中信号的长时间平均由于DNA系链长度的持续变化,因此不可能。这些改进使得可以有效地研究几种DNA-蛋白质系统,包括转录活性DNA-RNA聚合酶I复合物和DNA回转酶复合物。

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