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小分子与DNA无碱基位点的结合:核黄素的强结合作用可改善对胸腺嘧啶相关单核苷酸多态性的识别

Small-molecule binding at an abasic site of DNA: strong binding of lumiflavin for improved recognition of thymine-related single nucleotide polymorphisms.

作者信息

Sankaran N B, Sato Yusuke, Sato Fuyuki, Rajendar Burki, Morita Kotaro, Seino Takehiro, Nishizawa Seiichi, Teramae Norio

机构信息

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

出版信息

J Phys Chem B. 2009 Feb 5;113(5):1522-9. doi: 10.1021/jp808576t.

Abstract

The binding behavior of lumiflavin, a biologically vital ligand, with DNA duplexes containing an abasic (AP) site and various target nucleobases opposite the AP site is studied. Lumiflavin binds selectively to thymine (T) opposite the AP site in a DNA duplex over other nucleobases. Using 1H NMR spectroscopy and fluorescence measurements, we show that ligand-DNA complexation takes place by hydrogen-bond formation between the ligand and the target nucleobases and by stacking interactions between the ligand and the nucleobases flanking the AP site. From isothermal titration calorimetric experiments, we find that ligand incorporation into the AP sites is primarily enthalpy-driven. Examination of ionic strength dependency of ligand binding with DNA reveals that ligand-DNA complexation is a manifestation of both electrostatic and nonelectrostatic interactions and that the contribution from the nonelectrolyte effect is fundamental for the stabilization of the ligand-DNA complex. In comparison to riboflavin, reported previously as a T-selective ligand, lumiflavin binds to the DNA much more strongly and is a more promising ligand for efficient detection of T-related single nucleotide polymorphisms.

摘要

研究了生物重要配体核黄素与含有无碱基(AP)位点以及与AP位点相对的各种目标核碱基的DNA双链体的结合行为。在DNA双链体中,核黄素相对于其他核碱基选择性地与AP位点对面的胸腺嘧啶(T)结合。通过1H NMR光谱和荧光测量,我们表明配体与DNA的络合通过配体与目标核碱基之间的氢键形成以及配体与AP位点侧翼核碱基之间的堆积相互作用发生。从等温滴定量热实验中,我们发现配体掺入AP位点主要是由焓驱动的。对配体与DNA结合的离子强度依赖性的研究表明,配体与DNA的络合是静电和非静电相互作用的表现,并且非电解质效应的贡献对于配体 - DNA复合物的稳定是至关重要的。与先前报道的作为T选择性配体的核黄素相比,核黄素与DNA的结合更强,并且是用于有效检测T相关单核苷酸多态性的更有前景的配体。

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