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Single-molecule visualization of ROS-induced DNA damage in large DNA molecules

机译:大分子中ROS诱导的DNA损伤的单分子可视化

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We present a single molecule visualization approach for the quantitative analysis of reactive oxygen species (ROS) induced DNA damage, such as base oxidation and single stranded breaks in large DNA molecules. We utilized the Fenton reaction to generate DNA damage with subsequent enzymatic treatment using a mixture of three types of glycosylases to remove oxidized bases, and then fluorescent labeling on damaged lesions via nick translation. This single molecule analytical platform provided the capability to count one or two damaged sites per. DNA molecule (48.5 kb), which were reliably dependent on the concentrations of hydrogen peroxide and ferrous ion at the micromolar level. More importantly, the labeled damaged sites that were visualized under a microscope provided positional information, which offered the capability of comparing DNA damaged sites with the in silico genomic map to reveal sequence specificity that GTGR is more sensitive to oxidative damage. Consequently, single DNA molecule analysis provides a sensitive analytical platform for ROS-induced DNA damage and suggests an interesting biochemical insight that the genome primarily active during the lysogenic cycle may have less probability for oxidative DNA damage.
机译:我们提出了一种单分子可视化方法,用于定量分析活性氧(ROS)诱导的DNA损伤,例如大型DNA分子中的碱基氧化和单链断裂。我们利用Fenton反应产生DNA损伤,随后使用三种类型的糖基化酶的混合物进行酶处理以去除氧化的碱基,然后通过切口平移对受损的病变进行荧光标记。这个单分子分析平台提供了每个一个或两个受损位点计数的功能。 DNA分子(48.5 kb),可靠地取决于微摩尔水平的过氧化氢和亚铁离子的浓度。更重要的是,在显微镜下可视化的标记受损位点提供了位置信息,从而提供了将DNA受损位点与计算机基因组图谱进行比较的能力,从而揭示了GTGR对氧化损伤更敏感的序列特异性。因此,单个DNA分子分析为ROS诱导的DNA损伤提供了灵敏的分析平台,并提出了有趣的生化见解,即在溶原性周期内主要活跃的基因组可能对氧化性DNA损伤的可能性较小。

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