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En masse nascent transcription analysis to elucidate regulatory transcription factors

机译:大规模新生转录分析以阐明调节转录因子

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摘要

Despite exhaustively informing about steady-state mRNA abundance, DNA microarrays have been used with limited success to identify regulatory transcription factors (TFs). The main limitation of this approach is that altered mRNA stability also strongly governs the patterns of expressed genes. Here, we used nuclear run-on assays and microarrays to systematically interrogate changes in nascent transcription in cells treated with the topoisomerase inhibitor camptothecin (CPT). Analysis of the promoters of coordinately transcribed genes after CPT treatment suggested the involvement of TFs c-Myb and Rfx1. The predicted CPT-dependent associations were subsequently confirmed by chromatin immunoprecipitation assays. Importantly, after RNAi-mediated knockdown of each TF, the CPT-elicited induction of c-Myb- and/or Rfx1-regulated mRNAs was diminished and the overall cellular response was impaired. The strategies described here permit the successful identification of the TFs responsible for implementing adaptive gene expression programs in response to cellular stimulation.
机译:尽管详尽地告知了稳态mRNA的丰度,但DNA微阵列已被成功地用于鉴定调节转录因子(TF)。这种方法的主要局限性是,改变的mRNA稳定性也强烈控制着表达基因的模式。在这里,我们使用了核试验方法和微阵列系统地研究了拓扑异构酶抑制剂喜树碱(CPT)处理的细胞中新生转录的变化。 CPT处理后协调转录的基因启动子的分析表明,TFs c-Myb和Rfx1参与其中。随后通过染色质免疫沉淀测定法确认了预测的CPT依赖性关联。重要的是,在RNAi介导的每个TF的敲低后,CPT诱导的c-Myb和/或Rfx1调控的mRNA的诱导减弱,并且总体细胞反应受到损害。此处描述的策略可以成功识别负责响应细胞刺激而实施适应性基因表达程序的TF。

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