首页> 美国卫生研究院文献>Journal of Virology >Nick sensing by vaccinia virus DNA ligase requires a 5 phosphate at the nick and occupancy of the adenylate binding site on the enzyme.
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Nick sensing by vaccinia virus DNA ligase requires a 5 phosphate at the nick and occupancy of the adenylate binding site on the enzyme.

机译:通过牛痘病毒DNA连接酶进行的尼克感测需要在切口处有一个5磷酸并占用该酶上腺苷酸结合位点。

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摘要

Vaccinia virus DNA ligase has an intrinsic nick-sensing function. The enzyme discriminates at the substrate binding step between a DNA containing a 5' phosphate and a DNA containing a 5' hydroxyl at the nick. Further insights into nick recognition and catalysis emerge from studies of the active-site mutant K231A, which is unable to form the covalent ligase-adenylate intermediate and hence cannot activate a nicked DNA substrate via formation of the DNA-adenylate intermediate. Nonetheless, K231A does catalyze phosphodiester bond formation at a preadenylated nick. Hence, the active-site lysine of DNA ligase is not required for the strand closure step of the ligation reaction. The K231A mutant binds tightly to nicked DNA-adenylate but has low affinity for a standard DNA nick. The wild-type vaccinia virus ligase, which is predominantly ligase-adenylate, binds tightly to a DNA nick. This result suggests that occupancy of the AMP binding pocket of DNA ligase is essential for stable binding to DNA. Sequestration of an extrahelical nucleotide by DNA-bound ligase is reminiscent of the base-flipping mechanism of target-site recognition and catalysis used by other DNA modification and repair enzymes.
机译:牛痘病毒DNA连接酶具有内在的尼克感应功能。该酶在底物结合步骤中在切口处区分含有5'磷酸的DNA和含有5'羟基的DNA。活性位点突变体K231A的研究进一步发现了切口识别和催化作用,该突变体无法形成共价连接酶-腺苷酸中间体,因此无法通过形成DNA-腺苷酸中间体来激活切口的DNA底物。但是,K231A确实催化了在预腺苷酸化的切口处形成磷酸二酯键。因此,连接反应的链闭合步骤不需要DNA连接酶的活性位点赖氨酸。 K231A突变体与有缺口的DNA-腺苷酸紧密结合,但对标准DNA缺口的亲和力低。野生型痘苗病毒连接酶主要是连接酶-腺苷酸,与DNA缺口紧密结合。该结果表明,DNA连接酶的AMP结合口袋的占据对于稳定地结合DNA是必不可少的。 DNA结合的连接酶螯合螺旋外核苷酸使人联想到其他DNA修饰和修复酶使用的靶位识别和催化的碱基翻转机制。

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