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确定在大肠杆菌乳糖基因开关中产生mRNA稳态产量的转录速率。

Determining the Transcription Rates Yielding Steady-State Production of mRNA in the Lac Genetic Switch of Escherichia coli.

作者信息

Atitey Komlan, Loskot Pavel, Rees Paul

机构信息

College of Engineering, Swansea University , Swansea, United Kingdom .

出版信息

J Comput Biol. 2018 Sep;25(9):1023-1039. doi: 10.1089/cmb.2018.0055. Epub 2018 Jun 29.

Abstract

To elucidate the regulatory dynamics of the gene expression activation and inactivation, an in silico biochemical model of the lac circuit in Escherichia coli was used to evaluate the transcription rates that yield the steady-state mRNA production in active and inactive states of the lac circuit. This result can be used in synthetic biology applications to understand the limits of the genetic synthesis. Since most genetic networks involve many interconnected components with positive and negative feedback control, intuitive understanding of their dynamics is often difficult to obtain. Although the kinetic model of the lac circuit considered involves only a single positive feedback, the developed computational framework can be used to evaluate supported ranges of other reaction rates in genetic circuits with more complex regulatory networks. More specifically, the inducible lac gene switch in E. coli is regulated by unbinding and binding of the inducer-repressor complexes to or from the DNA operator to switch the gene expression on and off. The dependency of mRNA production at steady state on different transcription rates and the repressor complexes has been studied by computer simulations in the Lattice Microbe software. Provided that the lac circuit is in active state, the transcription rate is independent of the inducer-repressor complexes present in the cell. In inactive state, the transcription rate is dependent on the specific inducer-repressor complex bound to the operator that inactivates the gene expression. We found that the repressor complex with the largest affinity to the operator yields the smallest range of the feasible transcription rates to yield the steady state while the lac circuit is in inactive state. In contrast, the steady state in active state can be obtained for any value of the transcription rate.

摘要

为了阐明基因表达激活和失活的调控动力学,利用大肠杆菌中乳糖操纵子回路的计算机生化模型来评估在乳糖操纵子回路的激活和失活状态下产生稳态mRNA产量的转录速率。这一结果可用于合成生物学应用,以了解基因合成的限度。由于大多数遗传网络涉及许多具有正反馈和负反馈控制的相互连接的组件,因此往往难以直观地理解它们的动力学。虽然所考虑的乳糖操纵子回路的动力学模型仅涉及单个正反馈,但所开发的计算框架可用于评估具有更复杂调控网络的遗传回路中其他反应速率的支持范围。更具体地说,大肠杆菌中的可诱导乳糖基因开关是通过诱导剂-阻遏物复合物与DNA操纵子的解离和结合来调控基因表达的开启和关闭。通过在Lattice Microbe软件中进行计算机模拟,研究了稳态下mRNA产量对不同转录速率和阻遏物复合物的依赖性。假设乳糖操纵子回路处于激活状态,转录速率与细胞中存在的诱导剂-阻遏物复合物无关。在失活状态下,转录速率取决于与操纵子结合的特定诱导剂-阻遏物复合物,该复合物会使基因表达失活。我们发现,对操纵子亲和力最大的阻遏物复合物在乳糖操纵子回路处于失活状态时,产生稳态的可行转录速率范围最小。相比之下,在激活状态下,对于任何转录速率值都可以获得稳态。

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