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MopA the Mn Oxidizing Protein From Erythrobacter sp. SD-21 Requires Heme and NAD+ for Mn(II) Oxidation

机译:MopA来自红杆菌属的Mn氧化蛋白。 SD-21需要血红素和NAD +才能氧化Mn(II)

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摘要

Bacterial manganese (Mn) oxidation is catalyzed by a diverse group of microbes and can affect the fate of other elements in the environment. Yet, we understand little about the enzymes that catalyze this reaction. The Mn oxidizing protein MopA, from Erythrobacter sp. strain SD-21, is a heme peroxidase capable of Mn(II) oxidation. Unlike Mn oxidizing multicopper oxidase enzymes, an understanding of MopA is very limited. Sequence analysis indicates that MopA contains an N-terminal heme peroxidase domain and a C-terminal calcium binding domain. Heterologous expression and nickel affinity chromatography purification of the N-terminal peroxidase domain (MopA-hp) from Erythrobacter sp. strain SD-21 led to partial purification. MopA-hp is a heme binding protein that requires heme, NAD+, and calcium (Ca2+) for activity. Mn oxidation is also stimulated by the presence of pyrroloquinoline quinone. MopA-hp has a KM for Mn(II) of 154 ± 46 μM and kcat = 1.6 min−1. Although oxygen requiring MopA-hp is homologous to peroxidases based on sequence, addition of hydrogen peroxide and hydrogen peroxide scavengers had little effect on Mn oxidation, suggesting this is not the oxidizing agent. These studies provide insight into the mechanism by which MopA oxidizes Mn.
机译:细菌(Mn)的氧化被多种微生物催化,并可能影响环境中其他元素的命运。但是,我们对催化该反应的酶知之甚少。锰氧化蛋白MopA,来自红杆菌属。 SD-21菌株是能够进行Mn(II)氧化的血红素过氧化物酶。与Mn氧化多铜氧化酶不同,对MopA的理解非常有限。序列分析表明,MopA包含一个N端血红素过氧化物酶结构域和一个C端钙结合结构域。异形表达和镍亲和层析纯化N端过氧化物酶域(MopA-hp)从红杆菌。 SD-21菌株导致部分纯化。 MopA-hp是一种血红素结合蛋白,需要血红素,NAD + 和钙(Ca 2 + )才能发挥活性。吡咯并喹啉醌的存在也刺激了Mn的氧化。 MopA-hp的Mn(II)的KM为154±46μM,kcat = 1.6 min -1 。尽管需要MopA-hp的氧气与基于序列的过氧化物酶同源,但是添加过氧化氢和过氧化氢清除剂对Mn的氧化影响很小,表明这不是氧化剂。这些研究提供了MopA氧化Mn的机理的见解。

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