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底物与DNA光解酶结合时会发生差异扭曲:一项2-氨基嘌呤研究。

Differential distortion of substrate occurs when it binds to DNA photolyase: a 2-aminopurine study.

作者信息

Yang Kongsheng, Stanley Robert J

机构信息

Department of Chemistry, Temple University, 201 Beury Hall, Philadelphia, Pennsylvania 19122, USA.

出版信息

Biochemistry. 2006 Sep 19;45(37):11239-45. doi: 10.1021/bi060408u.

Abstract

Cyclobutylpyrimidine dimers (CPDs) are formed between adjacent pyrimidines in DNA when it is exposed to ultraviolet light. CPDs can be directly repaired by DNA photolyase (PL) upon absorption of blue-green light. We have used the fluorescent adenine analogue 2-aminopurine (2Ap) to probe the local double-helical structure of the DNA substrate when it binds to the protein. Duplex melting temperatures and van't Hoff enthalpies were obtained by both UV-vis absorption and fluorescence spectroscopies to ascertain the effect of the probe and CPD on DNA stability. Steady-state fluorescence measurements of the single- and double-stranded oligos showed that the local region around the 5'-side of the CPD lesion was more disrupted and destacked than the 3'-side in substrate-protein complexes. These results were compared with those of a protein-substrate crystal structure, demonstrating that the crystal structure and solution-state studies are in agreement with regard to the differential distortions of the target DNA at the active site of the protein.

摘要

当DNA暴露于紫外光时,环丁烷嘧啶二聚体(CPD)在DNA中相邻的嘧啶之间形成。吸收蓝绿光后,CPD可被DNA光解酶(PL)直接修复。我们使用荧光腺嘌呤类似物2-氨基嘌呤(2Ap)来探测DNA底物与蛋白质结合时的局部双螺旋结构。通过紫外可见吸收光谱和荧光光谱获得双链解链温度和范特霍夫焓,以确定探针和CPD对DNA稳定性的影响。单链和双链寡核苷酸的稳态荧光测量表明,在底物-蛋白质复合物中,CPD损伤5'侧周围的局部区域比3'侧更易被破坏和堆积。将这些结果与蛋白质-底物晶体结构的结果进行比较,表明晶体结构和溶液状态研究在蛋白质活性位点处目标DNA的差异扭曲方面是一致的。

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