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DNA 与人类无嘌呤/无嘧啶内切核酸酶 1 复合物:脉冲双共振电子顺磁共振与正交自旋标记揭示的结构见解。

DNA complexes with human apurinic/apyrimidinic endonuclease 1: structural insights revealed by pulsed dipolar EPR with orthogonal spin labeling.

机构信息

N. N. Vorozhtsov Novosibirsk Institute of Organic Chemistry SB RAS, 9 Lavrentiev ave, Novosibirsk 630090, Russia.

Novosibirsk State University, Pirogova Str. 2, Novosibirsk 630090, Russia.

出版信息

Nucleic Acids Res. 2019 Sep 5;47(15):7767-7780. doi: 10.1093/nar/gkz620.

Abstract

A DNA molecule is under continuous influence of endogenous and exogenous damaging factors, which produce a variety of DNA lesions. Apurinic/apyrimidinic sites (abasic or AP sites) are among the most common DNA lesions. In this work, we applied pulse dipolar electron paramagnetic resonance (EPR) spectroscopy in combination with molecular dynamics (MD) simulations to investigate in-depth conformational changes in DNA containing an AP site and in a complex of this DNA with AP endonuclease 1 (APE1). For this purpose, triarylmethyl (TAM)-based spin labels were attached to the 5' ends of an oligonucleotide duplex, and nitroxide spin labels were introduced into APE1. In this way, we created a system that enabled monitoring the conformational changes of the main APE1 substrate by EPR. In addition, we were able to trace substrate-to-product transformation in this system. The use of different (orthogonal) spin labels in the enzyme and in the DNA substrate has a crucial advantage allowing for detailed investigation of local damage and conformational changes in AP-DNA alone and in its complex with APE1.

摘要

DNA 分子不断受到内源性和外源性损伤因素的影响,这些因素会产生各种 DNA 损伤。无碱基/嘧啶部位(脱碱基或 AP 部位)是最常见的 DNA 损伤之一。在这项工作中,我们应用脉冲双共振电子顺磁共振(EPR)光谱结合分子动力学(MD)模拟深入研究了含有 AP 部位的 DNA 以及该 DNA 与 AP 内切酶 1(APE1)复合物的构象变化。为此,我们将基于三芳基甲基(TAM)的自旋标记物连接到寡核苷酸双链的 5'端,并将氮氧自由基自旋标记物引入 APE1。通过这种方式,我们创建了一个系统,通过 EPR 监测主要 APE1 底物的构象变化。此外,我们能够在该系统中追踪底物到产物的转化。在酶和 DNA 底物中使用不同的(正交)自旋标记物具有至关重要的优势,允许单独研究 AP-DNA 及其与 APE1 复合物中的局部损伤和构象变化。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fc55/6735896/b13fba189eaf/gkz620fig1.jpg

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