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甲酰胺嘧啶核苷三磷酸的合成、DNA聚合酶掺入及酶促磷酸水解

Synthesis, DNA polymerase incorporation, and enzymatic phosphate hydrolysis of formamidopyrimidine nucleoside triphosphates.

作者信息

Imoto Shuhei, Patro Jennifer N, Jiang Yu Lin, Oka Natsuhisa, Greenberg Marc M

机构信息

Department of Chemistry, Johns Hopkins University, 3400 North Charles Street, Baltimore, Maryland 21218, USA.

出版信息

J Am Chem Soc. 2006 Nov 15;128(45):14606-11. doi: 10.1021/ja065525r.

Abstract

The nucleoside triphosphates of N6-(2-deoxy-alpha,beta-d-erythro-pentofuranosyl)-2,6-diamino-4-hydroxy-5-formamidopyrimidine (Fapy.dGTP) and its C-nucleoside analogue (beta-C-Fapy.dGTP) were synthesized. The lability of the formamide group required that nucleoside triphosphate formation be carried out using an umpolung strategy in which pyrophosphate was activated toward nucleophilic attack. The Klenow fragment of DNA polymerase I from Escherichia coli accepted Fapy.dGTP and beta-C-Fapy.dGTP as substrates much less efficiently than it did dGTP. Subsequent extension of a primer containing either modified nucleotide was less affected compared to when the native nucleotide is present at the 3'-terminus. The specificity constants are sufficiently large that nucleoside triphosphate incorporation could account for the level of Fapy.dG observed in cells if 1% of the dGTP pool is converted to Fapy.dGTP. Similarly, polymerase-mediated introduction of beta-C-Fapy.dG could be useful for incorporating useful amounts of this nonhydrolyzable analogue for use as an inhibitor of base excision repair. The kinetic viability of these processes is enhanced by inefficient hydrolysis of Fapy.dGTP and beta-C-Fapy.dGTP by MutT, the E. coli enzyme that releases pyrophosphate and the corresponding nucleoside monophosphate upon reaction with structurally related nucleoside triphosphates.

摘要

合成了N6-(2-脱氧-α,β-D-赤藓糖基)-2,6-二氨基-4-羟基-5-甲酰胺基嘧啶(Fapy.dGTP)及其C-核苷类似物(β-C-Fapy.dGTP)的三磷酸核苷。甲酰胺基团的不稳定性要求使用极性翻转策略进行三磷酸核苷的合成,其中焦磷酸被激活以进行亲核攻击。来自大肠杆菌的DNA聚合酶I的Klenow片段接受Fapy.dGTP和β-C-Fapy.dGTP作为底物的效率比接受dGTP的效率低得多。与天然核苷酸存在于3'-末端时相比,含有任何一种修饰核苷酸的引物的后续延伸受到的影响较小。特异性常数足够大,如果dGTP池的1%转化为Fapy.dGTP,那么三磷酸核苷的掺入可以解释在细胞中观察到的Fapy.dG的水平。同样,聚合酶介导的β-C-Fapy.dG的引入可能有助于掺入有用量的这种不可水解类似物,用作碱基切除修复的抑制剂。MutT(一种大肠杆菌酶,与结构相关的三磷酸核苷反应时会释放焦磷酸和相应的核苷单磷酸)对Fapy.dGTP和β-C-Fapy.dGTP的低效水解增强了这些过程的动力学可行性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e140/1780028/028ca94030a4/nihms-15934-0001.jpg

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