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使用不可切割的底物类似物对钼辅因子生物合成中cPMP合酶的机制研究

Mechanistic Investigation of cPMP Synthase in Molybdenum Cofactor Biosynthesis Using an Uncleavable Substrate Analogue.

作者信息

Hover Bradley M, Lilla Edward A, Yokoyama Kenichi

机构信息

Department of Biochemistry, Duke University Medical Center , Durham, North Carolina 27710, United States.

出版信息

Biochemistry. 2015 Dec 15;54(49):7229-36. doi: 10.1021/acs.biochem.5b00857. Epub 2015 Dec 1.

DOI:10.1021/acs.biochem.5b00857
PMID:26575208
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4847533/
Abstract

Molybdenum cofactor (Moco) is essential for all kingdoms of life, plays central roles in various biological processes, and must be biosynthesized de novo. During its biosynthesis, the characteristic pyranopterin ring is constructed by a complex rearrangement of guanosine 5'-triphosphate (GTP) into cyclic pyranopterin monophosphate (cPMP) through the action of two enzymes, MoaA and MoaC. Recent studies revealed that MoaC catalyzes the majority of the transformation and produces cPMP from a unique cyclic nucleotide, 3',8-cyclo-7,8-dihydro-GTP (3',8-cH2GTP). However, the mechanism by which MoaC catalyzes this complex rearrangement is largely unexplored. Here, we report the mechanistic characterization of MoaC using an uncleavable substrate analogue, 3',8-cH2GMP[CH2]PP, as a probe to investigate the timing of cyclic phosphate formation. Using partially active MoaC variants, 3',8-cH2GMP[CH2]PP was found to be accepted by MoaC as a substrate and was converted to an analogue of the previously described MoaC reaction intermediate, suggesting that the early stage of catalysis proceeds without cyclic phosphate formation. In contrast, when it was incubated with wt-MoaC, 3',8-cH2GMP[CH2]PP caused mechanism-based inhibition. Detailed characterization of the inhibited MoaC suggested that 3',8-cH2GMP[CH2]PP is mainly converted to a molecule (compound Y) with an acid-labile triaminopyrimidinone base without an established pyranopterin structure. MS analysis of MoaC treated with 3',8-cH2GMP[CH2]PP provided strong evidence that compound Y forms a tight complex with MoaC likely through a covalent linkage. These observations are consistent with a mechanism in which cyclic phosphate ring formation proceeds in concert with the pterin ring formation. This mechanism would provide a thermodynamic driving force to complete the formation of the unique tetracyclic structure of cPMP.

摘要

钼辅因子(Moco)对所有生命王国都至关重要,在各种生物过程中发挥核心作用,且必须从头生物合成。在其生物合成过程中,特征性的吡喃蝶呤环是通过鸟苷5'-三磷酸(GTP)在两种酶MoaA和MoaC的作用下复杂重排为环化吡喃蝶呤单磷酸(cPMP)而构建的。最近的研究表明,MoaC催化了大部分转化过程,并从一种独特的环核苷酸3',8-环-7,8-二氢-GTP(3',8-cH2GTP)生成cPMP。然而,MoaC催化这种复杂重排的机制在很大程度上尚未被探索。在这里,我们报告了使用一种不可切割的底物类似物3',8-cH2GMP[CH2]PP作为探针来研究环状磷酸酯形成时间的MoaC的机制特征。使用部分活性的MoaC变体,发现3',8-cH2GMP[CH2]PP被MoaC接受为底物,并被转化为先前描述的MoaC反应中间体的类似物,这表明催化的早期阶段在没有环状磷酸酯形成的情况下进行。相反,当它与野生型MoaC一起孵育时,3',8-cH2GMP[CH2]PP会导致基于机制的抑制。对受抑制的MoaC的详细表征表明,3',8-cH2GMP[CH2]PP主要转化为一种具有酸不稳定的三氨基嘧啶酮碱基且没有既定吡喃蝶呤结构的分子(化合物Y)。用3',8-cH2GMP[CH2]PP处理的MoaC的质谱分析提供了有力证据,表明化合物Y可能通过共价连接与MoaC形成紧密复合物。这些观察结果与一种机制一致,即环状磷酸酯环的形成与蝶呤环的形成协同进行。这种机制将提供一种热力学驱动力来完成cPMP独特四环结构的形成。

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本文引用的文献

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