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From the CoverLong-Range Electron Transfer Special Feature: Protein–DNA charge transport: Redox activation of a DNA repair protein by guanine radical

机译:来自CoverLongRange电子转移特殊功能:蛋白质-DNA电荷转移:鸟嘌呤自由基对DNA修复蛋白的氧化还原激活

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摘要

DNA charge transport (CT) chemistry provides a route to carry out oxidative DNA damage from a distance in a reaction that is sensitive to DNA mismatches and lesions. Here, DNA-mediated CT also leads to oxidation of a DNA-bound base excision repair enzyme, MutY. DNA-bound Ru(III), generated through a flash/quench technique, is found to promote oxidation of the [4Fe-4S]2+ cluster of MutY to [4Fe-4S]3+ and its decomposition product [3Fe-4S]1+. Flash/quench experiments monitored by EPR spectroscopy reveal spectra with g = 2.08, 2.06, and 2.02, characteristic of the oxidized clusters. Transient absorption spectra of poly(dGC) and [Ru(phen)2dppz]3+ (dppz = dipyridophenazine), generated in situ, show an absorption characteristic of the guanine radical that is depleted in the presence of MutY with formation instead of a long-lived species with an absorption at 405 nm; we attribute this absorption also to formation of the oxidized [4Fe-4S]3+ and [3Fe-4S]1+ clusters. In ruthenium-tethered DNA assemblies, oxidative damage to the 5′-G of a 5′-GG-3′ doublet is generated from a distance but this irreversible damage is inhibited by MutY and instead EPR experiments reveal cluster oxidation. With ruthenium-tethered assemblies containing duplex versus single-stranded regions, MutY oxidation is found to be mediated by the DNA duplex, with guanine radical as an intermediate oxidant; guanine radical formation facilitates MutY oxidation. A model is proposed for the redox activation of DNA repair proteins through DNA CT, with guanine radicals, the first product under oxidative stress, in oxidizing the DNA-bound repair proteins, providing the signal to stimulate DNA repair.
机译:DNA电荷传输(CT)化学为从远处发生的对DNA错配和损伤敏感的氧化DNA损伤提供了一种途径。在此,DNA介导的CT还导致DNA结合的碱基切除修复酶MutY氧化。发现通过快速/猝灭技术生成的与DNA结合的Ru(III)可以促进MutY的[4Fe-4S] 2 + 簇氧化为[4Fe-4S] 3 + 及其分解产物[3Fe-4S] 1 + 。通过EPR光谱监测的闪断/猝灭实验揭示了氧化簇的特征为g = 2.08、2.06和2.02的光谱。聚(dGC)和[Ru(phen)2dppz] 3 + (dppz =二吡啶并吩嗪)的瞬态吸收光谱显示原位产生的鸟嘌呤自由基的吸收特征,该鸟嘌呤自由基在存在MutY形成,而不是具有405 nm吸收的长寿命物种;我们将此吸收也归因于氧化的[4Fe-4S] 3 + 和[3Fe-4S] 1 + 团簇的形成。在固定于钌的DNA组件中,从远处产生了对5'-GG-3'双峰的5'-G的氧化损伤,但MutY抑制了这种不可逆的损伤,而EPR实验显示了簇氧化。对于包含双链区和单链区的钌链组装体,发现MutY氧化是由DNA双链体介导的,其中鸟嘌呤基为中间氧化剂。鸟嘌呤自由基的形成促进MutY氧化。提出了一种模型,用于通过DNA CT与鸟嘌呤自由基的氧化还原激活DNA修复蛋白,该蛋白在氧化应激下会氧化DNA结合的修复蛋白,从而提供刺激DNA修复的信号。

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