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Characterization and Functional Analyses of R-Specific Enoyl Coenzyme A Hydratases in Polyhydroxyalkanoate-Producing Ralstonia eutropha

机译:产生多羟基链烷酸富营养罗尔斯通体的R-特异性烯丙基辅酶A水合酶的表征和功能分析

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摘要

A genome survey of polyhydroxyalkanoate (PHA)-producing Ralstonia eutropha H16 detected the presence of 16 orthologs of R-specific enoyl coenzyme A (enoyl-CoA) hydratase, among which three proteins shared high homologies with the enzyme specific to enoyl-CoAs of medium chain length encoded by phaJ4 from Pseudomonas aeruginosa (phaJ4Pa). The recombinant forms of the three proteins, termed PhaJ4aRe to PhaJ4cRe, actually showed enoyl-CoA hydratase activity with R specificity, and the catalytic efficiencies were elevated as the substrate chain length increased from C4 to C8. PhaJ4aRe and PhaJ4bRe showed >10-fold-higher catalytic efficiency than PhaJ4cRe. The functions of the new PhaJ4 proteins were investigated using previously engineered R. eutropha strains as host strains; these strains are capable of synthesizing poly((R)-3-hydroxybutyrate-co-(R)-3-hydroxyhexanoate) [P(3HB-co-3HHx)] from soybean oil. Deletion of phaJ4aRe from the chromosome resulted in significant decrease of 3HHx composition in the accumulated copolyester, whereas no change was observed with deletion of phaJ4bRe or phaJ4cRe, indicating that only PhaJ4aRe was one of the major enzymes supplying the (R)-3HHx-CoA monomer through β-oxidation. Introduction of phaJ4aRe or phaJ4bRe into the R. eutropha strains using a broad-host-range vector enhanced the 3HHx composition of the copolyesters, but the introduction of phaJ4cRe did not. The two genes were then inserted into the pha operon on chromosome 1 of the engineered R. eutropha by homologous recombination. These modifications enabled the biosynthesis of P(3HB-co-3HHx) composed of a larger 3HHx fraction without a negative impact on cell growth and PHA production on soybean oil, especially when phaJ4aRe or phaJ4bRe was tandemly introduced with phaJAc from Aeromonas caviae.
机译:对产多羟基链烷酸(PHA)的富营养Ralstonia eutropha H16的基因组调查发现存在16个直系同源的R特异性烯酰辅酶A(enoyl-CoA)水合酶,其中三种蛋白质与培养基中烯醇式CoAs特有的酶具有高度同源性由铜绿假单胞菌的phaJ4(phaJ4Pa)编码的链长。这三种蛋白质的重组形式,分别称为PhaJ4aRe至PhaJ4cRe,实际上表现出具有R特异性的烯酰辅酶A水合酶活性,并且随着底物链长度从C4增加到C8,催化效率也有所提高。 PhaJ4aRe和PhaJ4bRe的催化效率是PhaJ4cRe的10倍以上。使用以前设计的富营养罗汉果菌株作为宿主菌株研究了新的PhaJ4蛋白的功能。这些菌株能够从大豆油中合成聚((R)-3-羟基丁酸酯-co-(R)-3-羟基己酸酯)[P(3HB-co-3HHx)]。从染色体上删除phaJ4aRe会导致积累的共聚酯中3HHx组成的显着减少,而删除phaJ4bRe或phaJ4cRe则未观察到变化,这表明只有PhaJ4aRe是提供(R)-3HHx-CoA单体的主要酶之一通过β-氧化。使用宽宿主范围的载体将phaJ4aRe或phaJ4bRe引入到富营养的R. eutropha菌株中,可以增强共聚酯的3HHx组成,但不能引入phaJ4cRe。然后通过同源重组将这两个基因插入到富营养化工程化富营养芽孢杆菌1号染色体的pha操纵子中。这些修饰使得能够由较大的3HHx组分组成的P(3HB-co-3HHx)进行生物合成,而不会对大豆油上的细胞生长和PHA产生负面影响,尤其是当phaJ4aRe或phaJ4bRe与来自气单胞菌的phaJAc串联引入时。

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