Broad-Spectrum Gene Repression Using Scaffold Engineering of Synthetic sRNAs

心理压抑 基因表达 基因 合成生物学 突变体 生物 基因表达调控 转移RNA 计算生物学 遗传学 细胞生物学 核糖核酸
作者
Minho Noh,Seung Min Yoo,Dongsoo Yang,Sang Yup Lee
出处
期刊:ACS Synthetic Biology [American Chemical Society]
卷期号:8 (6): 1452-1461 被引量:35
标识
DOI:10.1021/acssynbio.9b00165
摘要

Gene expression regulation in broad-spectrum range is critical for constructing cell factories and genetic circuits to balance and control system-wide fluxes. Synthetic small regulatory RNAs (sRNAs) effectively regulate gene expression at the translational level by modulating an mRNA-binding chance and sRNA abundance; however, it can control target gene expression only within the limit of the intrinsic repression ability of sRNAs. Here, we systematically mutated a SgrS scaffold as a model sRNA by dividing the Hfq-binding module of the sRNA into the three regions: the A/U-rich sequence, the stem, and the hairpin loop, and examined how efficiently the mutants suppressed DsRed2 expression. By doing this, we found that a scaffold with an altered A/U-rich sequence (CUUU) and stem length and that with altered A/U-rich sequence (GCAC) showed a 3-fold stronger and a 3-fold weaker repression than the original scaffold, respectively. For practical application of altered scaffolds, proof-of-concept experiments were performed by constructing a library of 67 synthetic sRNAs with the strongest scaffold, each one targeting a different rationally selected gene, and using this library to enhance cadaverine production in Escherichia coli, yielding in 27% increase (1.67 g/L in flask cultivation, 13.7 g/L in fed-batch cultivation). Synthetic sRNAs with engineered sRNA scaffolds could be useful in modulating gene expression for strain improvement.
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