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DNA Repair by DNA: The UV1C DNAzyme Catalyzes Photoreactivation of Cyclobutane Thymine Dimers in DNA More Effectively than Their de Novo Formation

机译:用DNA修复DNA:UV1C DNAzyme比其从头形成更有效地催化DNA中环丁烷胸腺嘧啶二聚体的光活化。

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摘要

UV1C, a 42-nt DNA oligonucleotide, is a deoxyribozyme (DNAzyme) that optimally uses 305 nm wavelength light to catalyze photoreactivation of a cyclobutane thymine dimer placed within a gapped, unnatural DNA substrate, TDP. Herein we show that UV1C is also capable of photoreactivating thymine dimers within an authentic single-stranded DNA substrate, LDP. This bona fide UV1C substrate enables, for the first time, investigation of whether UV1C catalyzes only photoreactivation or also the de novo formation of thymine dimers. Single-turnover experiments carried out with LDP and UV1C, relative to control experiments with LDP alone in single-stranded and double-stranded contexts, show that while UV1C does modestly promote thymine dimer formation, its major activity is indeed photoreactivation. Distinct photostationary states are reached for LDP in its three contexts: as a single strand, as a constituent of a double-helix, and as a 1:1 complex with UV1C. The above results on the cofactor-independent photoreactivation capabilities of a catalytic DNA reinforce a series of recent, unexpected reports that purely nucleotide-based photoreactivation is also operational within conventional double-helical DNA.
机译:UV1C是一种42 nt DNA寡核苷酸,是一种脱氧核酶(DNA酶),可以最佳地使用305 nm波长的光催化放置在有间隙的非天然DNA底物TDP中的环丁烷胸腺嘧啶二聚体的光活化。本文中,我们显示UV1C还能够在真实的单链DNA底物LDP中光活化胸腺嘧啶二聚体。这种真正的UV1C底物首次使人们能够研究UV1C是否仅催化光活化或胸腺嘧啶二聚体的从头形成。相对于在单链和双链环境中单独使用LDP的对照实验,用LDP和UV1C进行的单周转实验表明,尽管UV1C确实适度促进了胸腺嘧啶二聚体的形成,但其主要活性确实是光活化。在以下三种情况下,LDP达到了不同的光平稳状态:单链,双螺旋的组成以及与UV1C的1:1络合物。以上关于催化DNA的不依赖辅因子的光再活化能力的结果加强了一系列最近的,出乎意料的报道,即纯核苷酸基光再活化在常规双螺旋DNA中也可操作。

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