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Blue light-mediated transcriptional activation and repression of gene expression in bacteria

机译:蓝光介导的细菌转录激活和基因表达的抑制

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摘要

Light-regulated modules offer unprecedented new ways to control cellular behavior in precise spatial and temporal resolution. The availability of such tools may dramatically accelerate the progression of synthetic biology applications. Nonetheless, current optogenetic toolbox of prokaryotes has potential issues such as lack of rapid and switchable control, less portable, low dynamic expression and limited parts. To address these shortcomings, we have engineered a novel bidirectional promoter system for Escherichia coli that can be induced or repressed rapidly and reversibly using the blue light dependent DNA-binding protein EL222. We demonstrated that by modulating the dosage of light pulses or intensity we could control the level of gene expression precisely. We show that both light-inducible and repressible system can function in parallel with high spatial precision in a single cell and can be switched stably between ON-and OFF-states by repetitive pulses of blue light. In addition, the light-inducible and repressible expression kinetics were quantitatively analysed using a mathematical model. We further apply the system, for the first time, to optogenetically synchronize two receiver cells performing different logic behaviors over time using blue light as a molecular clock signal. Overall, our modular approach layers a transformative platform for next-generation light-controllable synthetic biology systems in prokaryotes.
机译:光调节模块提供了前所未有的新方法来以精确的空间和时间分辨率控制细胞行为。此类工具的可用性可能会大大加速合成生物学应用的发展。然而,当前的原核生物光遗传学工具箱具有潜在的问题,例如缺乏快速和可切换的控制,便携式性差,低动态表达和有限的零件。为了解决这些缺点,我们为大肠杆菌设计了一种新型的双向启动子系统,可以使用依赖于蓝光的DNA结合蛋白EL222快速和可逆地对其进行诱导或抑制。我们证明了通过调节光脉冲的剂量或强度,我们可以精确地控制基因表达的水平。我们表明光诱导和抑制系统都可以在单个单元格中以高空间精度并行运行,并且可以通过重复的蓝光脉冲在开和关状态之间稳定切换。此外,使用数学模型定量分析了光诱导和阻遏表达动力学。我们进一步首次将该系统应用于使用蓝光作为分子时钟信号,随着时间的流逝同步地同步执行不同逻辑行为的两个接收器单元。总体而言,我们的模块化方法为原核生物中的下一代光控合成生物学系统提供了一个可转换的平台。

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