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Development of antisense RNA-mediated quantifiable inhibition for metabolic regulation

机译:反义RNA介导的可量化抑制对代谢调节的影响

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摘要

Trans-regulating elements such as noncoding RNAs are crucial in modifying cells, and has shown broad application in synthetic biology, metabolic engineering and RNA therapies. Although effective, titration of the regulatory levels of such elements is less explored. Encouraged by the need of fine-tuning cellular functions, we studied key parameters of the antisense RNA design including oligonucleotide length, targeting region and relative dosage to achieve differentiated inhibition. We determined a 30-nucleotide configuration that renders efficient and robust inhibition. We found that by targeting the core RBS region proportionally, quantifiable inhibition levels can be rationally obtained. A mathematic model was established accordingly with refined energy terms and successfully validated by depicting the inhibition levels for genomic targets. Additionally, we applied this fine-tuning approach for 4-hydroxycoumarin biosynthesis by simultaneous and quantifiable knockdown of multiple targets, resulting in a 3.58-fold increase in titer of the engineered strain comparing to that of the non-regulated. We believe the developed tool is broadly compatible and provides an extra layer of control in modifying living systems.
机译:诸如非编码RNA的反式调节元件在改性细胞中至关重要,并且在合成生物学,代谢工程和RNA治疗中显示了广泛的应用。虽然有效,但探索了这种因素的监管水平的滴定。通过微调蜂窝功能的需要,我们研究了反义RNA设计的关键参数,包括寡核苷酸长度,靶向区域和相对剂量以实现分化的抑制作用。我们确定了一种30核苷酸配置,使抑制有效和稳健的抑制。我们发现,通过按比例地靶向核心RBS区域,可以合理地获得可量化的抑制水平。通过精细的能量术语相应地建立了数学模型,并通过描绘基因组靶标的抑制水平成功验证。此外,我们通过多种靶标同时和可量化的敲击应用于4-羟基苏马仑生物合成的微调方法,导致工程菌株的滴度增加3.58倍,比较非调控。我们认为,开发的工具广泛兼容,并在修改生活系统中提供额外的控制层。

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