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Kethoxal-assisted single-stranded DNA sequencing captures global transcription dynamics and enhancer activity in situ

机译:磷喹疗辅助单链DNA测序捕获全局转录动力学和原位增强剂活动

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Transcription is a highly dynamic process that generates single-stranded DNA (ssDNA) in the genome as 'transcription bubbles'. Here we describe a kethoxal-assisted single-stranded DNA sequencing (KAS-seq) approach, based on the fast and specific reaction between N-3-kethoxal and guanines in ssDNA. KAS-seq allows rapid (within 5 min), sensitive and genome-wide capture and mapping of ssDNA produced by transcriptionally active RNA polymerases or other processes in situ using as few as 1,000 cells. KAS-seq enables definition of a group of enhancers that are single-stranded and enrich unique sequence motifs. These enhancers are associated with specific transcription-factor binding and exhibit more enhancer-promoter interactions than typical enhancers do. Under conditions that inhibit protein condensation, KAS-seq uncovers a rapid release of RNA polymerase II (Pol II) from a group of promoters. KAS-seq thus facilitates fast and accurate analysis of transcription dynamics and enhancer activities simultaneously in both low-input and high-throughput manner.
机译:转录是一种高度动态的过程,在基因组中产生单链DNA(SSDNA)作为“转录泡沫”。在这里,我们描述了一种基于在SSDNA中的N-3-磷酸甲氧基和偶胆的快速和特异性反应的磷咯醛辅助的单链DNA测序(KAS-SEQ)方法。 KAS-SEQ允许通过转录活性RNA聚合酶或使用少量1,000个细胞的转录活性RNA聚合酶或其他方法产生的SSDNA的敏感和基因组覆盖和映射。 KAS-SEQ能够定义一组单股和丰富独特的序列图案的增强剂。这些增强剂与特定的转录因子结合有关,并且表现出比典型的增强剂更高的增强剂 - 启动子相互作用。在抑制蛋白质缩合的条件下,KAS-SEQ从一组启动子揭示RNA聚合酶II(POL II)的快速释放。因此,KAS-SEQ以低输入和高吞吐量的方式促进了转录动态和增强剂活动的快速准确分析。

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    《Nature methods 》 |2020年第5期| 共22页
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  • 正文语种 eng
  • 中图分类 生物科学 ;
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