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Cloning of a Novel Aldo-Keto Reductase Gene from Klebsiella sp. Strain F51-1-2 and Its Functional Expression in Escherichia coli

机译:克隆的克雷伯氏菌新的Aldo-酮还原酶基因F51-1-2菌株及其在大肠杆菌中的功能表达

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摘要

A soil bacterium capable of metabolizing organophosphorus compounds by reducing the P=S group in the molecules was taxonomically identified as Klebsiella sp. strain F51-1-2. The gene involved in the reduction of organophosphorus compounds was cloned from this strain by the shotgun technique, and the deduced protein (named AKR5F1) showed homology to members of the aldo-keto reductase (AKR) superfamily. The intact coding region for AKR5F1 was subcloned into vector pET28a and overexpressed in Escherichia coli BL21(DE3). Recombinant His6-tagged AKR5F1 was purified in one step using Ni-nitrilotriacetic acid affinity chromatography. Assays for cofactor specificity indicated that reductive transformation of organophosphorus compounds by the recombinant AKR5F1 specifically required NADH. The kinetic constants of the purified recombinant AKR5F1 toward six thion organophosphorus compounds were determined. For example, the Km and kcat values of reductive transformation of malathion by the purified recombinant AKR5F1 are 269.5 ± 47.0 μΜ and 25.7 ± 1.7 min−1, respectively. Furthermore, the reductive transformation of organophosphorus compounds can be largely explained by structural modeling.
机译:通过还原分子中的P = S基团能够代谢有机磷化合物的土壤细菌在分类学上被鉴定为克雷伯菌。菌株F51-1-2。通过the弹枪技术从该菌株中克隆了涉及有机磷化合物还原的基因,推导的蛋白质(名为AKR5F1)与醛基酮还原酶(AKR)超家族成员具有同源性。将完整的AKR5F1编码区亚克隆到载体pET28a中,并在大肠杆菌BL21(DE3)中过表达。重组的带有His6标签的AKR5F1使用Ni-三氮三乙酸亲和色谱一步纯化。辅助因子特异性的测定表明,重组AKR5F1对有机磷化合物的还原转化特别需要NADH。确定了纯化的重组AKR5F1对六种硫代有机磷化合物的动力学常数。例如,纯化的重组AKR5F1对马拉硫磷的还原转化的Km和kcat值分别为269.5±47.0μM和25.7±1.7min -1 。此外,有机磷化合物的还原转化可以通过结构模型很大程度上解释。

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