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利用含有 dCas9-sgRNA 的混合反馈回路对合成细菌钟进行单细胞特征分析。

Single Cell Characterization of a Synthetic Bacterial Clock with a Hybrid Feedback Loop Containing dCas9-sgRNA.

机构信息

Physics Department, TU Munich, D-85748 Garching, Germany.

出版信息

ACS Synth Biol. 2020 Dec 18;9(12):3377-3387. doi: 10.1021/acssynbio.0c00438. Epub 2020 Nov 24.

DOI:10.1021/acssynbio.0c00438
PMID:33231079
Abstract

Genetic networks that generate oscillations in gene expression activity are found in a wide range of organisms throughout all kingdoms of life. Oscillatory dynamics facilitates the temporal orchestration of metabolic and growth processes inside cells and organisms, as well as the synchronization of such processes with periodically occurring changes in the environment. Synthetic oscillator gene circuits such as the "repressilator" can perform similar functions in bacteria. Until recently, such circuits were mainly based on a relatively small set of well-characterized transcriptional repressors and activators. A promising, sequence-programmable alternative for gene regulation is given by CRISPR interference (CRISPRi), which enables transcriptional repression of nearly arbitrary gene targets directed by short guide RNA molecules. In order to demonstrate the use of CRISPRi in the context of dynamic gene circuits, we here replaced one of the nodes of a repressilator circuit by the RNA-guided dCas9 protein. Using single cell experiments in microfluidic reactors we show that this system displays robust relaxation oscillations over multiple periods and over several days. With a period of ≈14 bacterial generations, our oscillator is similar in speed as previously reported oscillators. Using an information-theoretic approach for the analysis of the single cell data, the potential of the circuit to act as a synthetic pacemaker for cellular processes is evaluated. We also observe that the oscillator appears to affect cellular growth, leading to variations in growth rate with the oscillator's frequency.

摘要

在生命的所有领域中,从广泛的生物体中都发现了产生基因表达活性振荡的遗传网络。振荡动力学有助于在细胞和生物体内部协调代谢和生长过程,以及使这些过程与环境中周期性发生的变化同步。类似于“阻遏物”的合成振荡器基因电路可以在细菌中执行类似的功能。直到最近,这种电路主要基于一组相对较小的、特征明确的转录阻遏物和激活物。CRISPR 干扰(CRISPRi)为基因调控提供了一种有前途的、序列可编程的替代方法,它可以通过短向导 RNA 分子靶向转录抑制几乎任意的基因靶标。为了在动态基因电路的背景下展示 CRISPRi 的用途,我们在这里用 RNA 指导的 dCas9 蛋白取代了阻遏物电路的一个节点。使用微流控反应器中的单细胞实验,我们表明该系统在多个周期和几天内显示出稳健的弛豫振荡。我们的振荡器的周期约为 14 个细菌世代,与之前报道的振荡器速度相似。通过对单细胞数据进行信息论分析,评估了该电路作为细胞过程合成起搏器的潜力。我们还观察到,振荡器似乎会影响细胞生长,导致振荡器频率的增长率发生变化。

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