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使用标签报告基因芯片定量分析转录因子结合和表达。

Quantitative analysis of transcription factor binding and expression using calling cards reporter arrays.

机构信息

Department of Genetics, Washington University School of Medicine in St. Louis, St. Louis, MO 63108, USA.

The Edison Family Center for Genome Sciences & Systems Biology, Washington University School of Medicine in St. Louis, St. Louis, MO 63108, USA.

出版信息

Nucleic Acids Res. 2020 May 21;48(9):e50. doi: 10.1093/nar/gkaa141.

Abstract

We report a tool, Calling Cards Reporter Arrays (CCRA), that measures transcription factor (TF) binding and the consequences on gene expression for hundreds of synthetic promoters in yeast. Using Cbf1p and MAX, we demonstrate that the CCRA method is able to detect small changes in binding free energy with a sensitivity comparable to in vitro methods, enabling the measurement of energy landscapes in vivo. We then demonstrate the quantitative analysis of cooperative interactions by measuring Cbf1p binding at synthetic promoters with multiple sites. We find that the cooperativity between Cbf1p dimers varies sinusoidally with a period of 10.65 bp and energetic cost of 1.37 KBT for sites that are positioned 'out of phase'. Finally, we characterize the binding and expression of a group of TFs, Tye7p, Gcr1p and Gcr2p, that act together as a 'TF collective', an important but poorly characterized model of TF cooperativity. We demonstrate that Tye7p often binds promoters without its recognition site because it is recruited by other collective members, whereas these other members require their recognition sites, suggesting a hierarchy where these factors recruit Tye7p but not vice versa. Our experiments establish CCRA as a useful tool for quantitative investigations into TF binding and function.

摘要

我们报告了一种工具,即 Calling Cards Reporter Arrays(CCRA),它可以测量数百个酵母合成启动子中的转录因子(TF)结合及其对基因表达的影响。使用 Cbf1p 和 MAX,我们证明 CCRA 方法能够检测到结合自由能的微小变化,其灵敏度可与体外方法相媲美,从而能够在体内测量能量景观。然后,我们通过测量具有多个位点的合成启动子上的 Cbf1p 结合来证明对协同相互作用的定量分析。我们发现,Cbf1p 二聚体之间的协同作用以 10.65 bp 的周期和 1.37 KBT 的能量成本呈正弦变化,对于处于“异相”位置的位点。最后,我们描述了一组 TF,Tye7p、Gcr1p 和 Gcr2p 的结合和表达,它们作为一个“TF 集体”共同作用,这是 TF 协同作用的一个重要但描述不足的模型。我们证明 Tye7p 经常在没有其识别位点的情况下结合启动子,因为它被其他集体成员募集,而这些其他成员则需要它们的识别位点,这表明存在一种层次结构,其中这些因素募集 Tye7p,但反之则不然。我们的实验确立了 CCRA 作为定量研究 TF 结合和功能的有用工具。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0ad7/7229839/099d50870b4f/gkaa141fig1.jpg

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