Multicopper oxidases (MCOs) are a family of enzymes that use copper ions as cofactors to oxidize various substrates. Previous research has demonstrated that several MCOs such as MnxG, MofA and MoxA can act as putative Mn(II) oxidases. Meanwhile, the endospore coat protein CotA from Bacillus species has been confirmed as a typical MCO. To study the relationship between CotA and the Mn(II) oxidation, the cotA gene from a highly active Mn(II)-oxidizing strain Bacillus pumilus WH4 was cloned and overexpressed in Escherichia coli strain M15. The purified CotA contained approximately four copper atoms per molecule and showed spectroscopic properties typical of blue copper oxidases. Importantly, apart from the laccase activities, the CotA also displayed substantial Mn(II)-oxidase activities both in liquid culture system and native polyacrylamide gel electrophoresis. The optimum Mn(II) oxidase activity was obtained at 53°C in HEPES buffer (pH 8.0) supplemented with 0.8 mM CuCl2. Besides, the addition of o-phenanthroline and EDTA both led to a complete suppression of Mn(II)-oxidizing activity. The specific activity of purified CotA towards Mn(II) was 0.27 U/mg. The Km, Vmax and kcat values towards Mn(II) were 14.85±1.17 mM, 3.01×10−6±0.21 M·min−1 and 0.32±0.02 s−1, respectively. Moreover, the Mn(II)-oxidizing activity of the recombinant E. coli strain M15-pQE-cotA was significantly increased when cultured both in Mn-containing K liquid medium and on agar plates. After 7-day liquid cultivation, M15-pQE-cotA resulted in 18.2% removal of Mn(II) from the medium. Furthermore, the biogenic Mn oxides were clearly observed on the cell surfaces of M15-pQE-cotA by scanning electron microscopy. To our knowledge, this is the first report that provides the direct observation of Mn(II) oxidation with the heterologously expressed protein CotA, Therefore, this novel finding not only establishes the foundation for in-depth study of Mn(II) oxidation mechanisms, but also offers a potential biocatalyst for Mn(II) removal.
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机译:铜氧化酶(MCO)是一类酶,它们使用铜离子作为辅助因子来氧化各种底物。先前的研究表明,几种MCO(例如MnxG,MofA和MoxA)可以充当推定的Mn(II)氧化酶。同时,已经证实来自芽孢杆菌属物种的内生孢子外壳蛋白CotA是典型的MCO。为了研究CotA和Mn(II)氧化之间的关系,克隆了高活性Mn(II)氧化菌株短小芽孢杆菌WH4的cotA基因,并在大肠杆菌M15菌株中过表达。纯化的CotA每个分子包含大约四个铜原子,并显示出蓝色铜氧化酶特有的光谱性质。重要的是,除漆酶活性外,CotA在液体培养系统和天然聚丙烯酰胺凝胶电泳中均显示出大量的Mn(II)-氧化酶活性。在补充了0.8 mM CuCl2的HEPES缓冲液(pH 8.0)中,在53°C下获得了最佳的Mn(II)氧化酶活性。此外,邻菲咯啉和EDTA的加入均导致Mn(II)氧化活性的完全抑制。纯化的CotA对Mn(II)的比活性为0.27 U / mg。 Mn(II)的Km,Vmax和kcat值分别为14.85±1.17 mM,3.01×10 -6 ±0.21 M·min -1 和0.32±0.02 s < sup> -1 。此外,当在含Mn的K液体培养基和琼脂平板上培养时,重组大肠杆菌菌株M15-pQE-cotA的Mn(II)氧化活性显着增加。液体培养7天后,M15-pQE-cotA导致培养基中Mn(II)的去除率为18.2%。此外,通过扫描电子显微镜在M15-pQE-cotA的细胞表面上清楚地观察到了生物来源的Mn氧化物。据我们所知,这是第一份提供异源表达的蛋白质CotA对Mn(II)氧化的直接观察的报告,因此,这一新发现不仅为深入研究Mn(II)氧化机理奠定了基础,而且还提供了去除Mn(II)的潜在生物催化剂。
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