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Quantitative analysis of bacterial gene expression by using the gusA reporter gene system

机译:使用gusa报告基因系统定量分析细菌基因表达

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摘要

An Azospirillum brasilense Sp7 strain containing a plasmid-borne translational cytN-gusA fusion was grown in a continuous culture to quantitatively evaluate the influence of extracellular signals (such as O-2) on expression of the cytNOQP operon. The dissolved oxygen concentration was shifted at regular time intervals before the steady state was reached. The measured beta -glucuronidase activity was used to monitor cytN gene expression. However, as the beta -glucuronidase activity in the experimental setup not only depended on altered transcription of the hybrid gene when the signal was varied but was also influenced by cellular accumulation, degradation, and dilution of the hybrid fusion protein, a mathematical method was developed to describe the intrinsic properties of the dynamic bioprocess. After identification and validation of the mathematical model, the apparent specific rate of expression of the fusion, which was independent of the experimental setup, could be deduced from the model and used to quantify gene expression regulated by extracellular environmental signals. In principle, this approach can be generalized to assess the effects of external signals on bacterial gene expression.
机译:在连续培养物中培养包含质粒携带的翻译性cytN-gusA融合蛋白的巴西拟螺旋体Sp7菌株,以定量评估细胞外信号(例如O-2)对cytNOQP操纵子表达的影响。在达到稳定状态之前,以固定的时间间隔移动溶解氧的浓度。所测得的β-葡萄糖醛酸苷酶活性用于监测cytN基因表达。但是,由于实验设置中的β-葡萄糖醛酸苷酶活性不仅取决于信号变化时杂合基因的转录变化,而且还受杂合融合蛋白的细胞积累,降解和稀释的影响,因此开发了一种数学方法描述动态生物过程的内在特性。在鉴定并验证了数学模型后,可以从模型中推导出与实验设置无关的融合表达的表观比速率,并用于量化受细胞外环境信号调控的基因表达。原则上,这种方法可以推广到评估外部信号对细菌基因表达的影响。

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