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鉴定和功能分析黄曲霉中棒曲霉素基因簇。

Identification and functional analysis of the aspergillic acid gene cluster in Aspergillus flavus.

机构信息

Southern Regional Research Center, USDA-ARS, New Orleans, LA, USA.

Southern Regional Research Center, USDA-ARS, New Orleans, LA, USA.

出版信息

Fungal Genet Biol. 2018 Jul;116:14-23. doi: 10.1016/j.fgb.2018.04.009. Epub 2018 Apr 16.

Abstract

Aspergillus flavus can colonize important food staples and produce aflatoxins, a group of toxic and carcinogenic secondary metabolites. Previous in silico analysis of the A. flavus genome revealed 56 gene clusters predicted to be involved in the biosynthesis of secondary metabolites. A. flavus secondary metabolites produced during infection of maize seed are of particular interest, especially with respect to their roles in the biology of the fungus. A predicted nonribosomal peptide synthetase-like (NRPS-like) gene, designated asaC (AFLA_023020), present in the uncharacterized A. flavus secondary metabolite gene cluster 11 was previously shown to be expressed during the earliest stages of maize kernel infection. Cluster 11 is composed of six additional genes encoding a number of putative decorating enzymes as well as a transporter and transcription factor. We generated knock-out mutants of the seven predicted cluster 11 genes. LC-MS analysis of extracts from knockout mutants of these genes showed that they were responsible for the synthesis of the previously characterized antimicrobial mycotoxin aspergillic acid. Extracts of the asaC mutant showed no production of aspergillic acid or its precursors. Knockout of the cluster 11 P450 oxidoreductase afforded a pyrazinone metabolite, the aspergillic acid precursor deoxyaspergillic acid. The formation of hydroxyaspergillic acid was abolished in a desaturase/hydroxylase mutant. The hydroxamic acid functional group in aspergillic acid allows the molecule to bind to iron resulting in the production of a red pigment in A. flavus identified previously as ferriaspergillin. A reduction of aflatoxin B and cyclopiazonic acid that correlated with reduced fungal growth was observed in maize kernel infection assays when aspergillic acid biosynthesis in A. flavus is halted.

摘要

黄曲霉可以定植于重要的粮食作物,并产生黄曲霉毒素,这是一组有毒和致癌的次级代谢物。先前对黄曲霉基因组的计算机分析表明,有 56 个基因簇被预测参与次级代谢物的生物合成。黄曲霉在感染玉米种子时产生的次级代谢物尤其引人注目,尤其是它们在真菌生物学中的作用。先前的研究表明,在未表征的黄曲霉次级代谢物基因簇 11 中,一个被命名为 asaC(AFLA_023020)的预测非核糖体肽合酶样(NRPS-like)基因在玉米籽粒感染的早期阶段表达。簇 11 由另外六个基因组成,这些基因编码了许多假定的修饰酶以及一个转运蛋白和转录因子。我们生成了这七个预测簇 11 基因的敲除突变体。这些基因敲除突变体的提取物的 LC-MS 分析表明,它们负责合成先前表征的抗微生物真菌毒素aspergillic acid。asaC 突变体的提取物没有产生 aspergillic acid 或其前体。簇 11 P450 氧化还原酶的敲除产生了一个吡嗪酮代谢物,aspergillic acid 的前体脱氧aspergillic acid。脱饱和酶/羟化酶突变体中羟酸基团的形成被消除。aspergillic acid 中的羟肟酸官能团允许该分子与铁结合,导致先前在黄曲霉中鉴定为 ferriaspergillin 的红色色素的产生。在黄曲霉感染玉米籽粒的试验中,当黄曲霉中的 aspergillic acid 生物合成被阻断时,观察到与真菌生长减少相关的 aflatoxin B 和 cyclopiazonic acid 的减少。

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