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CRISPR-Cas tools for simultaneous transcription translation control in bacteria

机译:CRISPR-Cas工具用于细菌中的同步转录和翻译控制

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摘要

Robust control over gene translation at arbitrary mRNA targets is an outstanding challenge in microbial synthetic biology. The development of tools that can regulate translation will greatly expand our ability to precisely control genes across the genome. In Escherichia coli, most genes are contained in multi-gene operons, which are subject to polar effects where targeting one gene for repression leads to silencing of other genes in the same operon. These effects pose a challenge for independently regulating individual genes in multi-gene operons. Here, we use CRISPR-dCas13 to address this challenge. We find dCas13-mediated repression exhibits up to 6-fold lower polar effects compared to dCas9. We then show that we can selectively activate single genes in a synthetic multi-gene operon by coupling dCas9 transcriptional activation of an operon with dCas13 translational repression of individual genes within the operon. We also show that dCas13 and dCas9 can be multiplexed for improved biosynthesis of a medically-relevant human milk oligosaccharide. Taken together, our findings suggest that combining transcriptional and translational control can access effects that are difficult to achieve with either mode independently. These combined tools for gene regulation will expand our abilities to precisely engineer bacteria for biotechnology and perform systematic genetic screens.
机译:对任意 mRNA 靶标的基因翻译的稳健控制是微生物合成生物学中的一项突出挑战。可以调节翻译的工具的开发将极大地扩展我们精确控制整个基因组基因的能力。在大肠杆菌中,大多数基因包含在多基因操纵子中,这些操纵子会受到极性效应的影响,其中靶向一个基因进行抑制会导致同一操纵子中的其他基因沉默。这些效应对独立调控多基因操纵子中的单个基因构成了挑战。在这里,我们使用 CRISPR-dCas13 来应对这一挑战。我们发现 dCas13 介导的抑制表现出比 dCas9 低 6 倍的极性效应。然后,我们表明,我们可以通过将操纵子的 dCas9 转录激活与操纵子内单个基因的 dCas13 翻译抑制耦合,选择性地激活合成多基因操纵子中的单个基因。我们还表明,dCas13 和 dCas9 可以多路复用以改善医学相关母乳低聚糖的生物合成。综上所述,我们的研究结果表明,结合转录和翻译控制可以获得任何一种模式都难以独立实现的效果。这些用于基因调控的组合工具将扩展我们的能力,以精确设计用于生物技术的细菌并进行系统的遗传筛选。

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