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Electrically monitoring DNA repair by photolyase.

机译:电监测光解酶对DNA的修复。

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摘要

Cyclobutane pyrimidine dimers are the major DNA photoproducts produced upon exposure to UV radiation. If left unrepaired, these lesions can lead to replication errors, mutation, and cell death. Photolyase is a light-activated flavoenzyme that binds to pyrimidine dimers in DNA and repairs them in a reaction triggered by electron transfer from the photoexcited flavin cofactor to the dimer. Using gold electrodes modified with DNA duplexes containing a cyclobutane thymine dimer (T<>T), here we probe the electrochemistry of the flavin cofactor in Escherichia coli photolyase. Cyclic and square-wave voltammograms of photolyase deposited on these electrodes show a redox signal at 40 mV versus normal hydrogen electrode, consistent with electron transfer to and from the flavin in the DNA-bound protein. This signal is dramatically attenuated on surfaces where the pi-stacking of the DNA bases is perturbed by the presence of an abasic site below the T<>T, an indication that the redox pathway is DNA-mediated. DNA repair can, moreover, be monitored electrically. Exposure of photolyase on T<>T-damaged DNA films to near-UV/blue light leads to changes in the flavin signal consistent with repair, as confirmed by parallel HPLC experiments. These results demonstrate the exquisite sensitivity of DNA electrochemistry to perturbations in base pair stacking and the applicability of this chemistry to probe reactions of proteins with DNA.
机译:环丁烷嘧啶二聚体是暴露于紫外线辐射后产生的主要DNA光产物。如果不予修复,这些病变会导致复制错误,突变和细胞死亡。光裂解酶是一种光活化的黄素酶,与DNA中的嘧啶二聚体结合,并在由光激发的黄素辅因子电子转移至二聚体引发的反应中修复它们。使用经含有环丁烷胸腺嘧啶二聚体(T T)的DNA双链体修饰的金电极,在此我们探究了大肠杆菌光裂解酶中黄素辅因子的电化学。与正常氢电极相比,沉积在这些电极上的光解酶的循环伏安图和方波伏安图在40 mV电压下显示出氧化还原信号,这与DNA结合蛋白中的黄素进出电子转移一致。该信号在DNA碱基的π-堆积被T T下方的无碱基位点干扰的表面上被显着衰减,这表明氧化还原途径是DNA介导的。此外,DNA修复可以用电监控。平行HPLC实验证实,T-T损伤的DNA膜上的光解酶暴露于近紫外线/蓝光会导致黄素信号的变化与修复相一致。这些结果证明了DNA电化学对碱基对堆积中的扰动非常敏感,并且该化学方法可用于探测蛋白质与DNA的反应。

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