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首页> 外文期刊>Amino acids >Site-directed mutagenesis and computational study of the Y366 active site in Bacillus subtilis protoporphyrinogen oxidase
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Site-directed mutagenesis and computational study of the Y366 active site in Bacillus subtilis protoporphyrinogen oxidase

机译:枯草芽孢杆菌原卟啉原氧化酶中Y366活性位点的定点诱变和计算研究

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摘要

Protoporphyrinogen IX oxidase (PPO), the last common enzyme of heme and chlorophyll biosynthesis, catalyses the oxidation of protoporphyrinogen IX to protoporphyrin IX, with FAD as cofactor. Among PPO, Bacillus subtilis PPO (bsPPO) is unique because of its broad substrate specificity and resistance to inhibition by diphenylethers. Identification of the activity of bsPVO would help us to understand the catalysis and resistance mechanisms. Based on the modeling and docking studies, we found that Y366 site in bsPPO was adjacent to substrate and FAD. In order to evaluate the functional role of this site, three mutants Y366A Y366E and Y366H were cloned and kinetically characterized. The efficiency of catalysis for Y366A and Y366H reduced to 10% of the wild-type enzyme's activity, while Y366E just retained 1%. Y366E shows large resistance (K_i = 153.94 μM) to acifluorfen. Molecular docking was carried out to understand the structure and functional relationship of PPO. The experimental results from the site-directed mutagenesis are consistent with the computational studies. The residue at position 366 is seemed to be responsible for substrate binding and catalysis and involved in herbicide resistance of bsPPO.
机译:原卟啉原IX氧化酶(PPO)是血红素和叶绿素生物合成的最后一种常见酶,它以FAD为辅因子催化原卟啉原IX氧化为原卟啉IX。在PPO中,枯草芽孢杆菌PPO(bsPPO)由于其广泛的底物特异性和对二苯醚抑制的抗性而独特。鉴定bsPVO的活性将有助于我们了解其催化和耐药机制。根据建模和对接研究,我们发现bsPPO中的Y366位点与底物和FAD相邻。为了评估该位点的功能作用,克隆了三个突变体Y366A,Y366E和Y366H,并对其进行了动力学表征。 Y366A和Y366H的催化效率降低至野生型酶活性的10%,而Y366E仅保留1%。 Y366E对acifluorfen表现出较大的抗性(K_i = 153.94μM)。进行分子对接以了解PPO的结构和功能关系。定点诱变的实验结果与计算研究一致。 366位的残基似乎负责底物的结合和催化,并与bsPPO的除草剂抗性有关。

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