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来源于墨西哥利什曼原虫的 2'-脱氧核糖基转移酶,是一种高效的生物催化剂,可用于从难溶性嘌呤碱基一锅、一步合成核苷。

2'-Deoxyribosyltransferase from Leishmania mexicana, an efficient biocatalyst for one-pot, one-step synthesis of nucleosides from poorly soluble purine bases.

机构信息

Department of Crystallography and Structural Biology, Institute Rocasolano (CSIC), Serrano 119, E-28006, Madrid, Spain.

Applied Biotechnology Group, European University of Madrid, E-28670, Villaviciosa de Odón, Madrid, Spain.

出版信息

Appl Microbiol Biotechnol. 2017 Oct;101(19):7187-7200. doi: 10.1007/s00253-017-8450-y. Epub 2017 Aug 7.

DOI:10.1007/s00253-017-8450-y
PMID:28785897
Abstract

Processes catalyzed by enzymes offer numerous advantages over chemical methods although in many occasions the stability of the biocatalysts becomes a serious concern. Traditionally, synthesis of nucleosides using poorly water-soluble purine bases, such as guanine, xanthine, or hypoxanthine, requires alkaline pH and/or high temperatures in order to solubilize the substrate. In this work, we demonstrate that the 2'-deoxyribosyltransferase from Leishmania mexicana (LmPDT) exhibits an unusually high activity and stability under alkaline conditions (pH 8-10) across a broad range of temperatures (30-70 °C) and ionic strengths (0-500 mM NaCl). Conversely, analysis of the crystal structure of LmPDT together with comparisons with hexameric, bacterial homologues revealed the importance of the relationships between the oligomeric state and the active site architecture within this family of enzymes. Moreover, molecular dynamics and docking approaches provided structural insights into the substrate-binding mode. Biochemical characterization of LmPDT identifies the enzyme as a type I NDT (PDT), exhibiting excellent activity, with specific activity values 100- and 4000-fold higher than the ones reported for other PDTs. Interestingly, LmPDT remained stable during 36 h at different pH values at 40 °C. In order to explore the potential of LmPDT as an industrial biocatalyst, enzymatic production of several natural and non-natural therapeutic nucleosides, such as vidarabine (ara A), didanosine (ddI), ddG, or 2'-fluoro-2'-deoxyguanosine, was carried out using poorly water-soluble purines. Noteworthy, this is the first time that the enzymatic synthesis of 2'-fluoro-2'-deoxyguanosine, ara G, and ara H by a 2'-deoxyribosyltransferase is reported.

摘要

尽管酶催化的过程具有许多优势,但在许多情况下,生物催化剂的稳定性仍然是一个严重的问题。传统上,使用水溶性较差的嘌呤碱基(如鸟嘌呤、黄嘌呤或次黄嘌呤)合成核苷需要碱性 pH 值和/或高温以使底物溶解。在这项工作中,我们证明了来自墨西哥利什曼原虫(LmPDT)的 2'-脱氧核糖基转移酶在广泛的温度(30-70°C)和离子强度(0-500 mM NaCl)范围内在碱性条件(pH 8-10)下具有异常高的活性和稳定性。相反,对 LmPDT 的晶体结构进行分析,并与六聚体细菌同源物进行比较,揭示了寡聚状态与该酶家族中活性位点结构之间关系的重要性。此外,分子动力学和对接方法提供了对底物结合模式的结构见解。LmPDT 的生化特性将该酶鉴定为 I 型 NDT(PDT),表现出出色的活性,其比其他 PDT 报道的比活值高 100-4000 倍。有趣的是,LmPDT 在 40°C 时在不同 pH 值下保持稳定 36 小时。为了探索 LmPDT 作为工业生物催化剂的潜力,使用水溶性较差的嘌呤进行了几种天然和非天然治疗性核苷的酶法生产,如阿昔洛韦(ara A)、地丹诺辛(ddI)、ddG 或 2'-氟-2'-脱氧鸟苷。值得注意的是,这是首次报道由 2'-脱氧核糖基转移酶酶法合成 2'-氟-2'-脱氧鸟苷、ara G 和 ara H。

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