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G-quadruplex DNA cleavage preference and identification of a perylene diimide G-quadruplex photocleavage agent using a rapid fluorescent assay

机译:G-四链体DNA裂解优先选择和identification二酰亚胺G-四链体光裂解剂的快速荧光测定

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摘要

A rapid fluorescence assay for G-quadruplex DNA cleavage was used to investigate the preference of TMPyP4 photochemical and Mn·TMPyP4 oxidative cleavage. Both agents most efficiently cleave the c-Myc promoter G-quadruplex. Direct PAGE analysis of selected assay samples showed that for a given cleavage agent, different cleavage products are formed from different G-quadruplex structures. Cleavage assays carried out in the presence of excess competitor nucleic acid structures revealed the binding selectivity of cleavage agents, while comparisons with duplex cleavage efficiency employing a dual-labeled hairpin oligonucleotide revealed neither agent prefers G-quadruplex over duplex substrates. Finally, this assay was used to identify the perylene diimide Tel11 as a photocleavage agent for the c-Myc G-quadruplex.
机译:用快速荧光检测G-四链体DNA的裂解来研究TMPyP4光化学和Mn·TMPyP4氧化裂解的偏好。两种试剂最有效地裂解c-Myc启动子G-四链体。所选测定样品的直接PAGE分析表明,对于给定的裂解剂,不同的裂解产物由不同的G-四链体结构形成。在存在过量竞争者核酸结构的情况下进行的裂解分析揭示了裂解剂的结合选择性,而与使用双标记发夹寡核苷酸的双链体裂解效率的比较表明,没有一种试剂比双链体底物更喜欢G-四链体。最后,该测定法用于鉴定作为c-Myc G-四链体的光裂解剂的per二酰亚胺Tel11。

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