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首页> 外文期刊>Applied and Environmental Microbiology >Polyketide Synthase Gene Responsible for Citrinin Biosynthesis in Monascus purpureus
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Polyketide Synthase Gene Responsible for Citrinin Biosynthesis in Monascus purpureus

机译:紫胶合成酶基因负责紫红曲霉中柠檬素的生物合成

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Citrinin produced by Aspergillus, Penicillium, and Monascus species is a polyketide compound that has nephrotoxic activity in mammals and is bactericidal toward gram-positive bacteria. To avoid the risk of citrinin contamination in other fermentation products produced by Monascus purpureus, knowledge of the citrinin biosynthetic genes is needed so that citrinin-nonproducing strains can be generated. We cloned a polyketide synthase (PKS) gene from M. purpureus with degenerate primers designed to amplify the conserved region of a ketosynthase domain of a fungal PKS. A 13-kb genomic DNA fragment was identified that contained a full-length PKS gene (pksCT) of 7,838 bp with a single 56-bp intron. pksCT encodes a 2,593-amino-acid protein that contains putative domains for ketosynthase, acyltransferase, acyl carrier protein (ACP), and a rare methyltransferase. There was no obvious thioesterase domain, which usually is downstream of the ACP domain in multi-aromatic-ring PKSs. pksCT transcription was correlated with citrinin production, suggesting that the pksCT gene product was involved in citrinin biosynthesis. Homologous recombination between the wild-type allele and a truncated disruption construct resulted in a pksCT-disrupted strain of M. purpureus. The disruptant did not produce citrinin, but a pksCT revertant generated by successive endogenous recombination events in the pksCT disruptant restored citrinin production, indicating that pksCT encoded the PKS responsible for citrinin biosynthesis in M. purpureus.
机译:由曲霉属,青霉属和红曲霉属产生的柠檬绿素是一种聚酮化合物,在哺乳动物中具有肾毒性,并且对革兰氏阳性细菌具有杀菌作用。为了避免紫杉菌产生的其他发酵产物中的citrinin污染的风险,需要了解citrinin生物合成基因,以便产生不生产citrinin的菌株。我们用简并引物从紫癜支原体克隆了聚酮化合物合酶(PKS)基因,该引物旨在扩增真菌PKS的酮合酶结构域的保守区。鉴定出一个13kb的基因组DNA片段,其中包含一个7838 bp的全长PKS基因(pksCT)和一个56 bp的内含子。 pksCT编码一个2593个氨基酸的蛋白质,其中包含酮合成酶,酰基转移酶,酰基载体蛋白(ACP)和稀有的甲基转移酶的推定域。没有明显的硫酯酶结构域,通常在多芳香环PKS中位于ACP域的下游。 pksCT转录与柑桔素的产生相关,提示pksCT基因产物参与了柑桔素的生物合成。野生型等位基因与截短的破坏构建体之间的同源重组产生了一种由pksCT破坏的紫癜支原体菌株。破坏剂不产生柠檬素,但是由pksCT破坏剂中连续的内源重组事件产生的pksCT回复子恢复了柑桔素的生产,表明pksCT编码了负责紫癜支原体中柠檬素生物合成的PKS。

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