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单分子 DNA 解链揭示了转录因子与其结合位点序列和上下文的不对称调节。

Single-molecule DNA unzipping reveals asymmetric modulation of a transcription factor by its binding site sequence and context.

机构信息

Faculty of Biology, Technion-Israel Institute of Technology, Haifa 32000, Israel.

Faculty of Physics, Technion-Israel Institute of Technology, Haifa 32000, Israel.

出版信息

Nucleic Acids Res. 2018 Feb 16;46(3):1513-1524. doi: 10.1093/nar/gkx1252.

Abstract

Most functional transcription factor (TF) binding sites deviate from their 'consensus' recognition motif, although their sites and flanking sequences are often conserved across species. Here, we used single-molecule DNA unzipping with optical tweezers to study how Egr-1, a TF harboring three zinc fingers (ZF1, ZF2 and ZF3), is modulated by the sequence and context of its functional sites in the Lhb gene promoter. We find that both the core 9 bp bound to Egr-1 in each of the sites, and the base pairs flanking them, modulate the affinity and structure of the protein-DNA complex. The effect of the flanking sequences is asymmetric, with a stronger effect for the sequence flanking ZF3. Characterization of the dissociation time of Egr-1 revealed that a local, mechanical perturbation of the interactions of ZF3 destabilizes the complex more effectively than a perturbation of the ZF1 interactions. Our results reveal a novel role for ZF3 in the interaction of Egr-1 with other proteins and the DNA, providing insight on the regulation of Lhb and other genes by Egr-1. Moreover, our findings reveal the potential of small changes in DNA sequence to alter transcriptional regulation, and may shed light on the organization of regulatory elements at promoters.

摘要

大多数功能转录因子 (TF) 的结合位点偏离其“共识”识别基序,尽管它们的位点和侧翼序列在物种间通常是保守的。在这里,我们使用单分子 DNA 解拉链与光学镊子研究了 Egr-1(一种含有三个锌指 (ZF1、ZF2 和 ZF3) 的 TF)如何被其在 Lhb 基因启动子中的功能位点的序列和上下文所调节。我们发现,每个位点中与 Egr-1 结合的核心 9 个碱基,以及侧翼的碱基对,都调节了蛋白-DNA 复合物的亲和力和结构。侧翼序列的影响是不对称的,ZF3 侧翼序列的影响更强。对 Egr-1 解离时间的表征表明,ZF3 相互作用的局部机械扰动比 ZF1 相互作用的扰动更有效地破坏复合物。我们的结果揭示了 ZF3 在 Egr-1 与其他蛋白质和 DNA 相互作用中的新作用,为 Egr-1 对 Lhb 和其他基因的调控提供了见解。此外,我们的发现揭示了 DNA 序列的微小变化改变转录调控的潜力,并可能阐明启动子处调控元件的组织。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e114/5815098/6656b1a13f5e/gkx1252fig1.jpg

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