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Hibisca P157-2 马杜拉放线菌普拉迪米星生物合成基因簇的克隆、测序及特性分析

Cloning, sequencing, and characterization of the pradimicin biosynthetic gene cluster of Actinomadura hibisca P157-2.

作者信息

Kim Byung Chul, Lee Jung Min, Ahn Jong Seog, Kim Beom Seok

机构信息

Division of Biotechnology, College of Life Sciences & Biotechnology, Korea University, Seoul 136-713, Korea.

出版信息

J Microbiol Biotechnol. 2007 May;17(5):830-9.

Abstract

Pradimicins are potent antifungal antibiotics having an unusual dihydrobenzo[alpha]naphthacenequinone aglycone substituted with D-alanine and sugars. Pradimicins are polyketide antibiotics produced by Actinomadura hibisca P157-2. The gene cluster involved in the biosynthesis of pradimicins was cloned and sequenced. The pradimicin gene cluster was localized to a 39-kb DNA segment and its involvement in the biosynthesis of pradimicin was proven by gene inactivation of prmA and prmB (ketosynthases alpha and beta). The pradimicin gene cluster consists of 28 open reading frames (ORFs), encoding a type II polyketide synthase (PKS), the enzymes involved in sugar biosynthesis and tailoring enzymes as well as two resistance proteins. The deduced proteins showed strong similarities to the previously validated gene clusters of angucyclic polyketides such as rubromycin, griseorhodin, and fredericamycin. From the pradimicin gene cluster, prmP3 encoding a component of the acetyl-CoA carboxylase complex was disrupted. The production levels of pradimicins of the resulting mutants decreased to 62% of the level produced by the wild-type strain, which indicate that the acetyl-CoA carboxylase gene would have a significant role in the production of pradimicins through supplying the extender unit precursor, malonyl-CoA.

摘要

制霉菌素是一类强效抗真菌抗生素,其具有不寻常的二氢苯并[α]萘并蒽醌苷元,该苷元被D - 丙氨酸和糖类取代。制霉菌素是由 Hibisca P157 - 2 马杜拉放线菌产生的聚酮类抗生素。参与制霉菌素生物合成的基因簇被克隆并测序。制霉菌素基因簇定位于一个39 kb的DNA片段,通过对prmA和prmB(酮合成酶α和β)进行基因失活,证明了其参与制霉菌素的生物合成。制霉菌素基因簇由28个开放阅读框(ORF)组成,编码一个II型聚酮合酶(PKS)、参与糖类生物合成的酶、修饰酶以及两种抗性蛋白。推导的蛋白质与先前已验证的安古洛环类聚酮化合物(如红霉霉素、灰紫红菌素和弗雷德里卡霉素)的基因簇有很强的相似性。从制霉菌素基因簇中,破坏了编码乙酰辅酶A羧化酶复合体一个组分的prmP3。所得突变体的制霉菌素产量水平降至野生型菌株产量水平的62%,这表明乙酰辅酶A羧化酶基因通过提供延伸单元前体丙二酰辅酶A在制霉菌素的产生中具有重要作用。

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