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[真养产碱杆菌B5786菌株聚羟基脂肪酸合酶基因(phaC)的克隆与分子结构]

[Cloning and molecular organization of the polyhydroxyalkanoic acid synthase gene (phaC) of Ralstonia eutropha strain B5786].

作者信息

Kozhevnikov I V, Volova T G, Hai T, Steinbuchel A

出版信息

Prikl Biokhim Mikrobiol. 2010 Mar-Apr;46(2):153-60.

Abstract

Class I polyhydroxyalkanoic acid (PHA) synthase gene (phaC) of Ralstonia eutropha strain B5786 was cloned and characterized. R. eutropha B5786 features the ability to synthesize multicomponent PHAs with short- and medium-chain-length monomers from simple carbohydrate substrate. A correlation was made between the molecular structure of PHA synthase and substrate specificity and the ability of strain-producers to accumulate PHAs of this or that structure. A strong similarity of PHA synthase of R. eutropha strain B5786 with PHA synthase of R. eutropha strain H16, which, as opposed to strain B5786, enables to incorporate medium chain length PHAs if hexanoate is used as carbon source, exhibited 99%. A correlation between the structure of PHA synthase of B5786 strain with synthases of microorganisms which synthesize short and medium chain length PHAs similarly to B5786 strain, showed an identity level from 26 to 41% (homology with synthase of Rhodospirillum rubrum makes 41%, Ectothiorhodospira shaposhnikovii makes 26%, Aeromonas punctata makes 40%, Thiococcus pfennigii makes 28%, Rhodococcus ruber makes 38%, and with PhaCl and PhaC2 synthases of Pseudomonas sp. 61-3 makes 34 and 37%, respectively). This allows for speaking about the absence of a direct connection between the molecular organization of PHA synthases and their functional abilities, namely, the ability to synthesize PHAs of a particular composition.

摘要

克隆并表征了真养产碱杆菌B5786菌株的I类聚羟基脂肪酸酯(PHA)合酶基因(phaC)。真养产碱杆菌B5786具有从简单碳水化合物底物合成含短链和中链长度单体的多组分PHA的能力。PHA合酶的分子结构与底物特异性以及菌株生产者积累这种或那种结构PHA的能力之间建立了相关性。真养产碱杆菌B5786菌株的PHA合酶与真养产碱杆菌H16菌株的PHA合酶有很强的相似性,与B5786菌株不同的是,如果使用己酸作为碳源,H16菌株能够掺入中链长度的PHA,相似性为99%。B5786菌株的PHA合酶结构与类似B5786菌株合成短链和中链长度PHA的微生物合酶之间的相关性表明,同一性水平为26%至41%(与红螺菌合酶的同源性为41%,沙氏外硫红螺菌为26%,点状气单胞菌为40%,芬氏硫球菌为28%,红球菌为38%,与假单胞菌61 - 3的PhaCl和PhaC2合酶的同源性分别为34%和37%)。这使得我们可以说PHA合酶的分子组织与其功能能力之间不存在直接联系,即合成特定组成PHA的能力。

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