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紫外激光光解DNA中鸟苷自由基产率非均匀分布的起源。

Origin of the heterogeneous distribution of the yield of guanyl radical in UV laser photolyzed DNA.

作者信息

Angelov Dimitar, Beylot Benedicte, Spassky Annick

机构信息

UMR 8113 French National Center for Scientific Research, Institut Gustave Roussy, 94805 Villejuif, France.

出版信息

Biophys J. 2005 Apr;88(4):2766-78. doi: 10.1529/biophysj.104.049015. Epub 2004 Dec 21.

Abstract

Oxidative guanine lesions were analyzed, at the nucleotide level, within DNA exposed to nanosecond ultraviolet (266 nm) laser pulses of variable intensity (0.002-0.1 J/cm(2)). Experiments were carried out, at room temperature, in TE buffer (20 mM Tris-HCl, pH 7.5; 1 mM EDTA) containing 35 mM NaCl, on 5'-end radioactively labeled double-stranded and single-stranded oligomer DNA at a size of 33-37 nucleobases. Lesions were analyzed on polyacrylamide gel electrophoresis by taking advantage of the specific removal of 8-oxodG from DNA by the formamidopyrimidine DNA glycosylase (Fpg protein) and of the differential sensitivity of 8-oxodG and oxazolone to piperidine. The quantum yields of lesions at individual sites, determined from the normalized intensities of bands, were plotted against the irradiation energy levels. Simplified model fitting of the experimental data enabled to evaluate the spectroscopic parameters characterizing excitation and photoionization processes. Results show that the distribution of guanine residues, excited to the lowest triplet state or photoionized, is heterogeneous and depends on the primary and secondary DNA structure. These findings are generalized in terms of excitation energy and charge-migration mediated biphotonic ionization. On the basis of the changes in the yield of the guanyl radical resulting from local helical perturbations in the DNA pi-stack, it can be assessed that the distance range of migration is <6-8 bp.

摘要

在核苷酸水平上,对暴露于可变强度(0.002 - 0.1 J/cm²)的纳秒紫外(266 nm)激光脉冲的DNA中的氧化鸟嘌呤损伤进行了分析。实验在室温下于含有35 mM NaCl的TE缓冲液(20 mM Tris - HCl,pH 7.5;1 mM EDTA)中进行,使用的是大小为33 - 37个核碱基的5'端放射性标记的双链和单链寡聚体DNA。通过利用甲酰胺嘧啶DNA糖基化酶(Fpg蛋白)从DNA中特异性去除8 - 氧代脱氧鸟苷(8 - oxodG)以及8 - oxodG和恶唑酮对哌啶的不同敏感性,在聚丙烯酰胺凝胶电泳上分析损伤。根据条带的归一化强度确定各个位点损伤的量子产率,并将其与辐照能量水平作图。对实验数据进行简化模型拟合能够评估表征激发和光电离过程的光谱参数。结果表明,被激发到最低三重态或被光电离的鸟嘌呤残基的分布是不均匀的,并且取决于DNA的一级和二级结构。这些发现基于激发能量和电荷迁移介导的双光子电离进行了概括。根据DNA π堆积中局部螺旋扰动导致的鸟苷自由基产率变化,可以评估迁移的距离范围小于6 - 8个碱基对。

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本文引用的文献

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