巴斯德酵母繁殖过程中氧化应激的定量:定量逆转录聚合酶链反应和流式细胞术的基因表达分析

IF 2.5 Q3 BIOTECHNOLOGY & APPLIED MICROBIOLOGY Frontiers in chemical engineering Pub Date : 2022-10-19 DOI:10.3389/fceng.2022.1035348
A. Beugholt, K. Büchner, D. Geier, T. Becker
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引用次数: 1

摘要

当面临环境压力时,酵母细胞会通过改变特定基因的表达等方式做出反应。在本研究中,通过RT-qPCR分析基因表达,以量化酵母繁殖过程中对不同通气水平的氧化应激反应。确定了靶基因,并建立了参考基因系统。在摇瓶中进行发酵实验,施加不同的摇速以产生不同的曝气效率。在不同的繁殖阶段对细胞进行取样,除表达研究外,在用二氢乙锭(DHE)染色后通过流式细胞术进行分析,以量化细胞内的活性氧(ROS)。结果表明,在高氧发酵条件下,催化A基因CTA1在繁殖过程中的表达增加。此外,根据RT-qPCR测量,细胞内部ROS的测定显示在整个过程中氧化应激增加。
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Quantification of oxidative stress in Saccharomyces pastorianus propagation: Gene expression analysis using quantitative reverse transcription polymerase chain reaction and flow cytometry
When confronted with environmental stress, yeast cell reacts, among others, by modifying the expression of specific genes. In this study, gene expression was analyzed via RT-qPCR to quantify the oxidative stress of Saccharomyces pastorianus during yeast propagation as a reaction to different aeration levels. Target genes were identified, and a reference gene system was developed. Fermentation experiments were conducted in shaking flasks, applying different shaking speeds to generate various aeration efficiencies. The cells were sampled at different propagation stages and, additionally to the expression study, analyzed by flow cytometry after staining with dihydroethidium (DHE) to quantify reactive oxygen species (ROS) inside the cells. The results indicate that high oxygen fermentation conditions led to an increased expression of the catalase-A gene CTA1 during propagation. Furthermore, the determination of cell internal ROS shows increasing oxidative stress over the process in accordance with the RT-qPCR measurements.
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3.50
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审稿时长
13 weeks
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