首页> 外文期刊>Journal of applied microbiology >Temporal monitoring of the nor-1 (aflD) gene of Aspergillus flavus in relation to aflatoxin B1 production during storage of peanuts under different water activity levels
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Temporal monitoring of the nor-1 (aflD) gene of Aspergillus flavus in relation to aflatoxin B1 production during storage of peanuts under different water activity levels

机译:不同水分活度下花生贮藏过程中黄曲霉的nor-1(aflD)基因与黄曲霉毒素B1产生的时间监测

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AbstractAims: A relative quantification system (RQ-PCR) was used to monitor the correlations between the activity of the nor-1 (=aflD) gene of Aspergillus flavus using real-time PCR in relation to phenotypic aflatoxin B1 (AFB1) production and populations of A. flavus in stored peanuts at three water activity levels (aw, 0.95, 0.90 and 0.85) for 6 weeks.Methods and Results: Real-time PCR was used to amplify the nor-1 gene (target gene), and benA56 (b-tubulin gene) used as a control gene. Expression of three structural genes, nor-1 (=aflD), ver-1 (=aflM), and omtA (=aflP), and the regulatory gene aflR of the aflatoxin biosynthetic pathway were also assayed. There were significant differences between nor-1 gene expression at the three aw levels; higher expression at 0.90 aw in weeks 1-3, when compared to 0.95. In contrast, in the driest treatment (0.85 aw) none or very low nor-1 expression occurred. The populations of A. flavus colony-forming units (CFUs g-1) increased over time with the highest at 0.95 aw. Highest AFB1 production was at 0.90 and 0.95 aw from weeks 3-6. Aw had a significant effect on aflR transcription at 0.95 aw over the 6-week period, while at 0.90 aw, only in the last 2 weeks.Conclusions: Correlations between different factors showed that log AFB1 x log CFUs, log AFB1 x aw, and log CFUs x aw were statistically significant, while log CFUs x RQ-PCR and RQ-PCR x aw were not. The AflR gene may not have an important role in the regulation of nor-1 expression in food matrices (e.g. peanuts).Significance and Impact of the study: Determination of correlations between nor-1 expression and aflatoxin production by A. flavus in raw peanuts under different aw levels could be helpful to predict potential risk of aflatoxin production during storage of this hygroscopic food product and minimize contamination with the AFB1.
机译:摘要目的:采用实时定量PCR(RQ-PCR)监测黄曲霉nor-1(= aflD)基因活性与表型黄曲霉毒素B1(AFB1)产量和种群之间的相关性以三种水分活度(aw,0.95、0.90和0.85)对花生中的黄曲霉进行连续6周的检测。方法和结果:实时荧光定量PCR扩增了nor-1基因(靶基因)和benA56( b-微管蛋白基因)用作对照基因。还检测了三个结构基因的表达,即nor-1(= aflD),ver-1(= aflM)和omtA(= aflP),以及黄曲霉毒素生物合成途径的调控基因aflR。在三个aw水平,nor-1基因表达之间存在显着差异。与0.95相比,第1-3周在0.90 aw时有更高的表达。相反,在最干燥的处理中(0.85 aw),没有或只有极低的nor-1表达发生。黄曲霉菌落形成单位(CFUs g-1)的数量随时间增加,最高为0.95 aw。从第3-6周开始,AFB1的最高产量为0.90和0.95 aw。 Aw对aflR转录的影响在6周内为0.95 aw,而对AflR转录的影响仅在最近2周内。结论:不同因素之间的相关性显示log AFB1 x log CFU,log AFB1 x aw和log CFU x aw在统计学上显着,而log CFU x RQ-PCR和RQ-PCR x aw没有。 AflR基因可能在食品基质(例如花生)中nor-1表达的调节中没有重要作用。研究的意义和影响:确定裸花生中黄曲霉nor-1表达与黄曲霉毒素生产之间的相关性在不同的aw水平下,可能有助于预测这种吸湿性食品在存储过程中黄曲霉毒素生产的潜在风险,并最大程度地减少AFB1的污染。

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