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使用自动化偏振显微镜进行转录因子-DNA 结合亲和力的真实平衡测量。

True equilibrium measurement of transcription factor-DNA binding affinities using automated polarization microscopy.

机构信息

Gene Center and Department of Biochemistry, Center for Integrated Protein Science Munich (CIPSM), Ludwig-Maximilians-Universität München, Feodor-Lynen-Strasse 25, 81377, München, Germany.

出版信息

Nat Commun. 2018 Apr 23;9(1):1605. doi: 10.1038/s41467-018-03977-4.

Abstract

The complex patterns of gene expression in metazoans are controlled by selective binding of transcription factors (TFs) to regulatory DNA. To improve the quantitative understanding of this process, we have developed a novel method that uses fluorescence anisotropy measurements in a controlled delivery system to determine TF-DNA binding energies in solution with high sensitivity and throughput. Owing to its large dynamic range, the method, named high performance fluorescence anisotropy (HiP-FA), allows for reliable quantification of both weak and strong binding; binding specificities are calculated on the basis of equilibrium constant measurements for mutational DNA variants. We determine the binding preference landscapes for 26 TFs and measure high absolute affinities, but mostly lower binding specificities than reported by other methods. The revised binding preferences give rise to improved predictions of in vivo TF occupancy and enhancer expression. Our approach provides a powerful new tool for the systems-biological analysis of gene regulation.

摘要

真核生物中复杂的基因表达模式受转录因子(TFs)与调控 DNA 的选择性结合控制。为了提高对这一过程的定量理解,我们开发了一种新方法,该方法使用荧光各向异性测量在受控递释系统中进行,以高灵敏度和高通量的方式在溶液中确定 TF-DNA 结合能。由于其动态范围大,该方法命名为高性能荧光各向异性(HiP-FA),允许对弱和强结合进行可靠的定量;基于对突变 DNA 变体的平衡常数测量来计算结合特异性。我们确定了 26 个 TF 的结合偏好图谱,并测量了高绝对亲和力,但与其他方法相比,主要是较低的结合特异性。经修订的结合偏好导致对体内 TF 占据和增强子表达的改进预测。我们的方法为基因调控的系统生物学分析提供了一个强大的新工具。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8fee/5913336/f32d1cc8cd99/41467_2018_3977_Fig1_HTML.jpg

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