Oxidation of Phenolate Siderophores by the Multicopper Oxidase Encoded by the Escherichia coli yacK Gene

Chulhwan Kim; W. Walter Lorenz; J. Todd Hoopes; Jeffrey F. D. Dean

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Oxidation of Phenolate Siderophores by the Multicopper Oxidase Encoded by the Escherichia coli yacK Gene

机译：大肠杆菌yacK基因编码的多铜氧化酶氧化邻苯二甲酸酯铁。

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A gene (yacK) encoding a putative multicopper oxidase (MCO) was cloned from Escherichia coli, and the expressed enzyme was demonstrated to exhibit phenoloxidase and ferroxidase activities. The purified protein contained six copper atoms per polypeptide chain and displayed optical and electron paramagnetic resonance (EPR) spectra consistent with the presence of type 1, type 2, and type 3 copper centers. The strong opticalA ₆₁₀ (Ε₆₁₀ = 10,890 M?1 cm?1) and copper stoichiometry were taken as evidence that, similar to ceruloplasmin, the enzyme likely contains multiple type 1 copper centers. The addition of copper led to immediate and reversible changes in the optical and EPR spectra of the protein, as well as decreased thermal stability of the enzyme. Copper addition also stimulated both the phenoloxidase and ferroxidase activities of the enzyme, but the other metals tested had no effect. In the presence of added copper, the enzyme displayed significant activity against two of the phenolate siderophores utilized by E. coli for iron uptake, 2,3-dihydroxybenzoate and enterobactin, as well as 3-hydroxyanthranilate, an iron siderophore utilized bySaccharomyces cerevisiae. Oxidation of enterobactin produced a colored precipitate suggestive of the polymerization reactions that characterize microbial melanization processes. As oxidation should render the phenolate siderophores incapable of binding iron, yacK MCO activity could influence levels of free iron in the periplasm in response to copper concentration. This mechanism may explain, in part, how yacK MCO moderates the sensitivity of E. coli to copper.

机译：从大肠杆菌中克隆了一个编码假定的多铜氧化酶（MCO）的基因（ yacK ），证明了该表达的酶具有酚氧化酶和亚铁氧化酶的活性。纯化的蛋白质每个多肽链包含六个铜原子，并显示出与1型，2型和3型铜中心一致的光学和电子顺磁共振（EPR）光谱。强光学 A _{610 （Ε_{610 = 10,890 M ？1 cm ？1 ）和铜化学计量作为证据，证明与铜蓝蛋白相似，该酶可能含有多个1型铜中心。铜的添加导致蛋白质的光学和EPR光谱立即发生可逆变化，并降低了酶的热稳定性。铜的添加也刺激了该酶的酚氧化酶和亚铁氧化酶活性，但是测试的其他金属没有作用。在添加铜的情况下，该酶对 E使用的两种酚盐铁载体显示出显着的活性。大肠杆菌用于摄取铁，2，3-二羟基苯甲酸酯和肠抑素，以及3-羟基邻氨基苯甲酸，这是啤酒酵母（Saccharomyces cerevisiae）所利用的铁铁载体。肠抑菌素的氧化产生了有色沉淀，这表明了表征微生物黑色素化过程的聚合反应。由于氧化应使酚盐铁载体无法结合铁，因此 yacK MCO活性可能会响应铜浓度而影响周质中游离铁的水平。该机制可能部分解释了 yacK MCO如何缓解 E的敏感性。大肠杆菌}} 展开▼

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《Journal of bacteriology》 |2001年第16期|共10页

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Chulhwan Kim; W. Walter Lorenz; J. Todd Hoopes; Jeffrey F. D. Dean;
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5. Control of Escherichia coli O157:H7, generic Escherichia coli, and Salmonella spp. on beef trimmings prior to grinding using a controlled phase carbon dioxide (CPCO2) system. [D] . Tanus Meurehg, Carlos Arturo. 2006

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6. Oxidation of Phenolate Siderophores by the Multicopper Oxidase Encoded by the Escherichia coli yacK Gene [O] . Chulhwan Kim, W. Walter Lorenz, J. Todd Hoopes, 2001

机译：大肠杆菌yacK基因编码的多铜氧化酶氧化邻苯二甲酸酯铁载体

7. Oxidation of Phenolate Siderophores by the Multicopper Oxidase Encoded by the Escherichia coli yacK Gene [O] . Kim, Chulhwan, Lorenz, W. Walter, Hoopes, J. Todd, 2001

机译：大肠杆菌yacK基因编码的多铜氧化酶氧化邻苯二甲酸酯铁载体

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Oxidation of Phenolate Siderophores by the Multicopper Oxidase Encoded by the Escherichia coli yacK Gene

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