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DNA 酶的作用:基于密度泛函理论计算研究 9DB1 的作用机制。

DNAzymes at Work: A DFT Computational Investigation on the Mechanism of 9DB1.

机构信息

Dipartimento di Chimica "G. Ciamician" , Alma Mater Studiorum - Università di Bologna , V. F. Selmi 2, 40126 Bologna , Italy.

出版信息

J Chem Inf Model. 2019 Apr 22;59(4):1547-1553. doi: 10.1021/acs.jcim.8b00815. Epub 2019 Feb 15.

Abstract

The 9DB1 DNAzyme follows an addition-elimination (A+D) two-step mechanism, involving a phosphorane intermediate, where the 3'-hydroxyl group (nucleophile) of one RNA fragment attacks the 5'-triphosphate of another RNA fragment. This mechanism does not involve a divalent metal cation in agreement with the experimental evidence. The process is assisted by two proton transfers that activate the nucleophile (first step) and the leaving group (second step). The dA nucleotide is not directly involved in the reaction. However, it plays an important role in determining the regioselectivity of the process: since the dA phosphate forms a strong hydrogen bond with the 2'-hydroxyl, only the 3'-hydroxyl can behave as a nucleophile and form the new 3'-5' bond. In silico mutagenesis, where the dA phosphate oxygen involved in the hydrogen contact was replaced by a sulfur atom, causes a significant rearrangement of the A ribose position with an increase in the activation barrier and a consequent lower enzymatic activity in agreement with the experimental evidence. A similar effect is determined by the replacement of the 2'-hydroxyl with different groups such as F, H, and OMe.

摘要

9DB1 DNA 酶遵循加成-消除 (A+D) 两步机制,涉及膦烷中间体,其中一个 RNA 片段的 3'-羟基(亲核试剂)攻击另一个 RNA 片段的 5'-三磷酸。该机制不涉及二价金属阳离子,与实验证据一致。该过程由两个质子转移辅助,激活亲核试剂(第一步)和离去基团(第二步)。dA 核苷酸不直接参与反应。然而,它在确定反应的区域选择性方面起着重要作用:由于 dA 磷酸盐与 2'-羟基形成强氢键,只有 3'-羟基可以作为亲核试剂并形成新的 3'-5'键。在计算机模拟诱变中,参与氢键的 dA 磷酸盐氧被硫原子取代,导致 A 核糖位置发生显著重排,增加了活化势垒,从而导致酶活性降低,这与实验证据一致。类似的效果是由用不同基团(如 F、H 和 OMe)取代 2'-羟基决定的。

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