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利用单分子荧光光谱法监测 CytR 固有无序 DNA 结合域的灵活靶标识别。

Flexible Target Recognition of the Intrinsically Disordered DNA-Binding Domain of CytR Monitored by Single-Molecule Fluorescence Spectroscopy.

机构信息

Institute of Multidisciplinary Research for Advanced Materials, Tohoku University, Sendai 980-8577, Japan.

Department of Chemistry, Graduate School of Science, Tohoku University, Sendai 980-8578, Japan.

出版信息

J Phys Chem B. 2022 Aug 25;126(33):6136-6147. doi: 10.1021/acs.jpcb.2c02791. Epub 2022 Aug 15.

Abstract

The intrinsically disordered DNA-binding domain of cytidine repressor (CytR-DBD) folds in the presence of target DNA and regulates the expression of multiple genes in . To explore the conformational rearrangements in the unbound state and the target recognition mechanisms of CytR-DBD, we carried out single-molecule Förster resonance energy transfer (smFRET) measurements. The smFRET data of CytR-DBD in the absence of DNA show one major and one minor population assignable to an expanded unfolded state and a compact folded state, respectively. The population of the folded state increases and decreases upon titration with salt and denaturant, respectively, in an apparent two-state manner. The peak FRET efficiencies of both the unfolded and folded states change continuously with denaturant concentration, demonstrating the intrinsic flexibility of the DNA-binding domain and the deviation from a strict two-state transition. Remarkably, the CytR-DBD exhibits a compact structure when bound to both the specific and nonspecific DNA; however, the peak FRET efficiencies of the two structures are slightly but consistently different. The observed conformational heterogeneity highlights the potential structural changes required for CytR to bind variably spaced operator sequences.

摘要

胞嘧啶阻遏物(CytR-DBD)的固有无序 DNA 结合域在存在靶 DNA 的情况下折叠,并调节 中多个基因的表达。为了探索未结合状态下的构象重排和 CytR-DBD 的靶识别机制,我们进行了单分子Förster 共振能量转移(smFRET)测量。在没有 DNA 的情况下,CytR-DBD 的 smFRET 数据显示出一个主要和一个次要群体,分别可分配到扩展的无规卷曲状态和紧凑的折叠状态。折叠状态的群体在盐和变性剂滴定时分别增加和减少,以明显的两态方式进行。无规卷曲和折叠状态的峰 FRET 效率均随变性剂浓度连续变化,表明 DNA 结合域的固有灵活性和偏离严格的两态转变。值得注意的是,CytR-DBD 与特异性和非特异性 DNA 结合时均呈现出紧凑的结构;然而,两种结构的峰 FRET 效率略有但一致地不同。观察到的构象异质性突出了 CytR 结合可变间隔的操纵子序列所需的潜在结构变化。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8136/9422980/12ccfbc7dcc7/jp2c02791_0001.jpg

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