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Recombinant Polycistronic Structure of Hydantoinase Process Genes in Escherichia coli for the Production of Optically Pure d-Amino Acids▿ †

机译:大肠杆菌中乙内酰脲酶过程基因的重组多顺反子结构,用于生产光学纯的d-氨基酸▿†

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摘要

Two recombinant reaction systems for the production of optically pure d-amino acids from different d,l-5-monosubstituted hydantoins were constructed. Each system contained three enzymes, two of which were d-hydantoinase and d-carbamoylase from Agrobacterium tumefaciens BQL9. The third enzyme was hydantoin racemase 1 for the first system and hydantoin racemase 2 for the second system, both from A. tumefaciens C58. Each system was formed by using a recombinant Escherichia coli strain with one plasmid harboring three genes coexpressed with one promoter in a polycistronic structure. The d-carbamoylase gene was cloned closest to the promoter in order to obtain the highest level of synthesis of the enzyme, thus avoiding intermediate accumulation, which decreases the reaction rate. Both systems were able to produce 100% conversion and 100% optically pure d-methionine, d-leucine, d-norleucine, d-norvaline, d-aminobutyric acid, d-valine, d-phenylalanine, d-tyrosine, and d-tryptophan from the corresponding hydantoin racemic mixture. For the production of almost all d-amino acids studied in this work, system 1 hydrolyzed the 5-monosubstituted hydantoins faster than system 2.
机译:构建了两个重组反应系统,用于从不同的d,l-5-单取代乙内酰脲生产光学纯的d-氨基酸。每个系统包含三种酶,其中两种是根癌土壤杆菌BQL9的d-乙内酰脲酶和d-氨基甲酰酶。第三种酶是第一个系统的乙内酰脲消旋酶1和第二个系统的乙内酰脲消旋酶2,均来自根癌农杆菌C58。通过使用重组大肠杆菌菌株形成每个系统,所述大肠杆菌菌株具有一个质粒,该质粒带有在多顺反子结构中与一个启动子共表达的三个基因。为了获得酶的最高合成水平,将d-氨基甲酰酶基因克隆到最接近启动子的位置,从而避免了中间积累,从而降低了反应速率。两种系统均能产生100%的转化率和100%的光学纯d-蛋氨酸,d-亮氨酸,d-正亮氨酸,d-正缬氨酸,d-氨基丁酸,d-缬氨酸,d-苯丙氨酸,d-酪氨酸和d-相应的乙内酰脲外消旋混合物中的色氨酸。为了生产这项工作中研究的几乎所有d-氨基酸,系统1水解5-单取代乙内酰脲的速度比系统2更快。

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