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首页> 外文期刊>Inorganica Chimica Acta >Mechanism of DNA cleavage catalyzed by Mung Bean Nuclease
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Mechanism of DNA cleavage catalyzed by Mung Bean Nuclease

机译:绿豆核酸酶催化的DNA切割机理

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The interaction of zinc with different forms of DNA (lambda phage DNA, ss-oligo, ds-oligo) and Mung Bean Nuclease was studied by voltammetric techniques in order to investigate the mechanism of DNA cleavage catalyzed by a zinc metalloenzyme. Stoichiometry, dissociation constant, zinc binding sites and functions were determined for these systems. Two zinc ions were found to be involved in stabilization of a 19 mer ds-oligodeoxyribonucleotide, which was synthesized by the phosphoramidite method and used as a DNA model in the studies. Three zinc ions (Zn1, Zn2, and Zn3), which have different roles in ds-oligo cleavage, were identified in the active site of Mung Bean Nuclease. A concerted S(N)2 mechanism, which assigns a catalytic function to Zn2 and structural functions to Zn1 and Zn3, was proposed. The hydrolysis of phosphodiester bonds proceeds with inversion of configuration at the phosphorus center, forming a pentacoordinate transition state, which is stabilized by an arginine. Zn2 supplies the nucleophile, which is oriented by an aspartic acid, and activates the ds-oligo by its coordination to the phosphate free oxygen of the phosphodiester bond. Zn1 and Zn3 ions, besides stabilizing the tertiary structure of Mung Bean Nuclease, bind to the leaving group, blocking the cleavage reverse reaction. (C) 2004 Elsevier B.V. All rights reserved.
机译:通过伏安法研究了锌与不同形式的DNA(λ噬菌体DNA,ss-oligo,ds-oligo)和绿豆核酸酶之间的相互作用,以研究锌金属酶催化DNA裂解的机理。确定了这些系统的化学计量,解离常数,锌结合位点和功能。发现两个锌离子与19 mer ds-寡聚脱氧核糖核苷酸的稳定化有关,后者通过亚磷酰胺方法合成并在研究中用作DNA模型。在绿豆核酸酶的活性位点中鉴定出在ds-寡核苷酸切割中具有不同作用的三个锌离子(Zn1,Zn2和Zn3)。提出了协调一致的S(N)2机理,该机理赋予Zn2催化功能,并赋予Zn1和Zn3结构功能。磷酸二酯键的水解随着磷中心处构型的转变而进行,形成五配位过渡态,其通过精氨酸得以稳定。 Zn2提供由天冬氨酸定向的亲核试剂,并通过其与磷酸二酯键的无磷酸盐氧配位而激活ds-oligo。 Zn1和Zn3离子除稳定绿豆核酸酶的三级结构外,还与离去基团结合,阻止了裂解逆反应。 (C)2004 Elsevier B.V.保留所有权利。

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