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From general base to general acid catalysis in a sodium-specific DNAzyme by a guanine-to-adenine mutation

机译:通过鸟嘌呤与腺嘌呤突变将一般碱从钠特异性DNAzyme催化到一般酸催化

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摘要

Recently, a few Na+-specific RNA-cleaving DNAzymes were reported, where nucleobases are likely to play critical roles in catalysis. The NaA43 and NaH1 DNAzymes share the same 16-nt Na+-binding motif, but differ in one or two nucleotides in a small catalytic loop. Nevertheless, they display an opposite pH-dependency, implicating distinct catalytic mechanisms. In this work, rational mutation studies locate a catalytic adenine residue, A22, in NaH1, while previous studies found a guanine (G23) to be important for the catalysis of NaA43. Mutation with pK(a)-perturbed analogs, such as 2-aminopurine (similar to 3.8), 2,6-diaminopurine (similar to 5.6) and hypoxanthine (similar to 8.7) affected the overall reaction rate. Therefore, we propose that the N1 position of G23 (pK(a) similar to 6.6) in NaA43 functions as a general base, while that of A22 (pK(a) similar to 6.3) in NaH1 as a general acid. Further experiments with base analogs and a phosphorothioate-modified substrate suggest that the exocyclic amine in A22 and both of the non-bridging oxygens at the scissile phosphate are important for catalysis for NaH1. This is an interesting example where single point mutations can change the mechanism of cleavage from general base to general acid, and it can also explain this Na+-dependent DNAzyme scaffold being sensitive to a broad range of metal ions and molecules.
机译:最近,报道了几种Na +特异性的RNA切割的DNazymes,其中核碱基可能在催化中发挥关键作用。 NAA43和NaH1 DNazymes共享相同的16-NT Na + - 困难基序,但在小催化环中的一个或两个核苷酸不同。然而,它们显示相反的pH依赖性,暗示不同的催化机制。在这项工作中,理性突变研究位于NaH1中的催化腺嘌呤残基A22,而先前的研究发现鸟嘌呤(G23)对NAA43的催化很重要。具有PK(A)-perurbured的类似物的突变,例如2-氨基嘌呤(类似于3.8),2,6-二氨基嘌呤(类似于5.6)和脱氧碱(类似于8.7)影响了整体反应速率。因此,我们提出了Na43中G23(PK(A)类似于6.6)的N1位置作为一般碱,而NaH1中的A22(PK(A)的PK(a)类似于6.3)。基础类似物和硫代磷酸酯改性基质的进一步实验表明A22中的官方胺和股骨磷酸盐处的两种非桥接氧合对NaH1的催化很重要。这是一个有趣的例子,其中单点突变可以从一般碱裂解的机制改变为一般的酸,它也可以解释这个娜+依赖性DNA核酶支架是范围广泛的金属离子和分子的敏感。

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  • 来源
    《Nucleic Acids Research》 |2019年第15期|共9页
  • 作者单位

    Univ Waterloo Waterloo Inst Nanotechnol Dept Chem Waterloo ON N2L 3G1 Canada;

    Univ Waterloo Waterloo Inst Nanotechnol Dept Chem Waterloo ON N2L 3G1 Canada;

    Univ Waterloo Waterloo Inst Nanotechnol Dept Chem Waterloo ON N2L 3G1 Canada;

    Univ Waterloo Waterloo Inst Nanotechnol Dept Chem Waterloo ON N2L 3G1 Canada;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 生物化学;
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