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大肠杆菌延滞期的启动子活性动态

Promoter activity dynamics in the lag phase of Escherichia coli.

作者信息

Madar Daniel, Dekel Erez, Bren Anat, Zimmer Anat, Porat Ziv, Alon Uri

机构信息

Department of Molecular Cell Biology, Weizmann Institute of Science, Rehovot 76100, Israel.

出版信息

BMC Syst Biol. 2013 Dec 30;7:136. doi: 10.1186/1752-0509-7-136.

Abstract

BACKGROUND

Lag phase is a period of time with no growth that occurs when stationary phase bacteria are transferred to a fresh medium. Bacteria in lag phase seem inert: their biomass does not increase. The low number of cells and low metabolic activity make it difficult to study this phase. As a consequence, it has not been studied as thoroughly as other bacterial growth phases. However, lag phase has important implications for bacterial infections and food safety. We asked which, if any, genes are expressed in the lag phase of Escherichia coli, and what is their dynamic expression pattern.

RESULTS

We developed an assay based on imaging flow cytometry of fluorescent reporter cells that overcomes the challenges inherent in studying lag phase. We distinguish between lag1 phase- in which there is no biomass growth, and lag2 phase--in which there is biomass growth but no cell division. We find that in lag1 phase, most promoters are not active, except for the enzymes that utilize the specific carbon source in the medium. These genes show promoter activities that increase exponentially with time, despite the fact that the cells do not measurably increase in size. An oxidative stress promoter, katG, is also active. When cells enter lag2 and begin to grow in size, they switch to a full growth program of promoter activity including ribosomal and metabolic genes.

CONCLUSIONS

The observed exponential increase in enzymes for the specific carbon source followed by an abrupt switch to production of general growth genes is a solution of an optimal control model, known as bang-bang control. The present approach contributes to the understanding of lag phase, the least studied of bacterial growth phases.

摘要

背景

迟缓期是指将稳定期细菌转移至新鲜培养基时出现的一段无生长的时期。处于迟缓期的细菌看似不活跃:其生物量不增加。细胞数量少且代谢活性低使得研究此阶段变得困难。因此,它没有像其他细菌生长阶段那样得到充分研究。然而,迟缓期对细菌感染和食品安全具有重要意义。我们想知道在大肠杆菌的迟缓期是否有基因表达,以及它们的动态表达模式是怎样的。

结果

我们开发了一种基于荧光报告细胞成像流式细胞术的检测方法,克服了研究迟缓期所固有的挑战。我们区分了lag1期(在此阶段生物量无增长)和lag2期(在此阶段有生物量增长但无细胞分裂)。我们发现,在lag1期,除了利用培养基中特定碳源的酶外,大多数启动子不活跃。尽管细胞大小没有明显增加,但这些基因的启动子活性随时间呈指数增加。一个氧化应激启动子katG也处于活跃状态。当细胞进入lag2期并开始增大尺寸时,它们会切换到包括核糖体和代谢基因在内的完整生长程序的启动子活性状态。

结论

观察到的针对特定碳源的酶的指数增加,随后突然切换到产生一般生长基因,是一种最优控制模型(称为开关控制)的解决方案。目前的方法有助于对细菌生长阶段中研究最少的迟缓期的理解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0bfb/3918108/e35535d608f7/1752-0509-7-136-1.jpg

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