Visualizing carboxyl-terminal domain of RNA polymerase II recruitment by FET fusion protein condensates with DNA curtains.

Linyu Zuo, Jiawei Ding, Zhi Qi
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引用次数: 0

Abstract

Many recent references show that living cells can form some membrane-less organelles by liquid-liquid phase separation (LLPS) of biomolecules, like proteins and nucleic acids. LLPS has been confirmed to link with many important biological functions in living cells, and one of the most important functions of biomolecular condensates is in the field of RNA transcription. Many studies confirm that mammalian RNA polymerase II (Pol II) molecules containing the CTD with different phosphorylation level are purposed to shuttle between initiation condensates and elongation condensates of RNA transcription. Traditional ensemble assays often experience difficulties in quantitively and directly recording the transient recruitment of Pol II CTD. Novel single-molecule approach - DNA curtains can be used to directly visualize biomolecular condensates formation and also recruitment of RNA polymerase II (Pol II) carboxyl-terminal domain (CTD) at the target sites in solution and in real time. This method can offer the potential for new insights into the mechanism of gene transcription. Here, we highlight the detailed protocol of DNA curtains method for studying LLPS.

Abstract Image

Abstract Image

用FET融合蛋白凝聚体和DNA帷幕观察RNA聚合酶II募集的羧基末端结构域。
最近的许多文献表明,活细胞可以通过液-液相分离(LLPS)形成一些无膜细胞器,如蛋白质和核酸。LLPS已被证实与活细胞中许多重要的生物学功能有关,其中生物分子凝聚物最重要的功能之一就是RNA转录。许多研究证实,哺乳动物RNA聚合酶II (Pol II)分子含有不同磷酸化水平的CTD,其目的是在RNA转录的起始凝聚体和延伸凝聚体之间穿梭。传统的系综分析在定量和直接记录Pol II CTD的瞬态招募方面经常遇到困难。新的单分子方法- DNA幕可用于直接可视化生物分子凝聚物的形成和RNA聚合酶II (Pol II)羧基末端结构域(CTD)在溶液中靶点的实时募集。这种方法可以为基因转录的机制提供新的见解。本文重点介绍了DNA帷幕法研究LLPS的详细方案。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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CiteScore
1.30
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0.00%
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117
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