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Substrate specificity and reaction mechanism of murine 8-oxoguanine-DNA glycosylase.

机译:鼠8-氧鸟嘌呤-DNA糖基化酶的底物特异性和反应机理。

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Genomic DNA is prone to oxidation by reactive oxygen species. A major product of DNA oxidation is the miscoding base 8-oxoguanine (8-oxoG). The mutagenic effects of 8-oxoG in mammalian cells are prevented by a DNA repair system consisting of 8-oxoguanine-DNA glycosylase (Ogg1), adenine-DNA glycosylase, and 8-oxo-dGTPase. We have cloned, overexpressed, and characterized mOgg1, the product of the murine ogg1 gene. mOgg1 is a DNA glycosylase/AP lyase belonging to the endonuclease III family of DNA repair enzymes. The AP lyase activity of mOgg1 is significantly lower than its glycosylase activity. mOgg1 releases 8-oxoG from DNA when paired with C, T, or G, but efficient DNA strand nicking is observed only with 8-oxoG:C. Binding of mOgg1 to oligonucleotides containing 8-oxoG:C is strong (K(D) = 51.5 nm), unlike other mispairs. The average residence time for mOgg1 bound to substrate containing 8-oxoG:C is 18.3 min; the time course for accumulation of the NaBH(4)-sensitive intermediate suggests a two-step reaction mechanism. Various analogs of 8-oxoG were tested as substrates for mOgg1. An electron-withdrawing or hydrogen bond acceptor moiety at C8 is required for efficient binding of mOgg1. A substituent at C6 and a keto group at C8 are required for cleavage. The proposed mechanism of 8-oxoG excision involves protonation of O(8) or the deoxyribose oxygen moiety.
机译:基因组DNA容易被活性氧氧化。DNA氧化的主要产物是误码碱基8-氧鸟嘌呤(8-oxoG)。由8-氧鸟嘌呤-DNA糖基化酶(Ogg1)、腺嘌呤-DNA糖基化酶和8-氧代-dGTP酶组成的DNA修复系统可防止8-氧代G在哺乳动物细胞中的诱变作用。我们已经克隆、过表达和表征了小鼠 ogg1 基因的产物 mOgg1。mOgg1 是一种 DNA 糖基化酶/AP 裂解酶,属于 DNA 修复酶的核酸内切酶 III 家族。mOgg1 的 AP 裂解酶活性显著低于其糖基化酶活性。当与 C、T 或 G 配对时,mOgg1 从 DNA 中释放 8-oxoG,但仅使用 8-oxoG:C 观察到有效的 DNA 链切口。 与其他错配不同,mOgg1 与含有 8-oxoG:C 的寡核苷酸的结合很强 (K(D) = 51.5 nm)。mOgg1与含有8-氧代:C的底物结合的平均停留时间为18.3分钟;NaBH(4)敏感中间体积累的时间过程表明了两步反应机制。测试了8-氧代的各种类似物作为mOgg1的底物。C8 处的吸电子或氢键受体部分是有效结合 mOgg1 所必需的。裂解需要 C6 的取代基和 C8 的酮基。提出的 8-氧代 8-氧代切除机制涉及 O(8) 或脱氧核糖氧部分的质子化。

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