Fine‐tuning the (2S)‐naringenin synthetic pathway using an iterative high‐throughput balancing strategy

柚皮素 代谢工程 查尔酮合酶 焊剂(冶金) 大肠杆菌 生物化学 化学 高通量筛选 代谢途径 代谢通量分析 通量平衡分析 基因 生物合成 新陈代谢 类黄酮 有机化学 抗氧化剂
作者
Shenghu Zhou,Yunbin Lyu,Huazhong Li,Mattheos A. G. Koffas,Jingwen Zhou
出处
期刊:Biotechnology and Bioengineering [Wiley]
卷期号:116 (6): 1392-1404 被引量:92
标识
DOI:10.1002/bit.26941
摘要

Abstract Metabolic engineering consistently demands to produce the maximum carbon and energy flux to target chemicals. To balance metabolic flux, gene expression levels of artificially synthesized pathways usually fine‐tuned using multimodular optimization strategy. However, forward construction is an engineering conundrum because a vast number of possible pathway combinations need to be constructed and analyzed. Here, an iterative high‐throughput balancing (IHTB) strategy was established to thoroughly fine‐tune the (2 S )‐naringenin biosynthetic pathway. A series of gradient constitutive promoters from Escherichia coli were randomly cloned upstream of pathway genes, and the resulting library was screened using an ultraviolet spectrophotometry–fluorescence spectrophotometry high‐throughput method, which was established based on the interactions between AlCl 3 and (2 S )‐naringenin. The metabolic flux of the screened high‐titer strains was analyzed and iterative rounds of screening were performed based on the analysis results. After several rounds, the metabolic flux of the (2 S )‐naringenin synthetic pathway was balanced, reaching a final titer of 191.9 mg/L with 29.2 mg/L p ‐coumaric acid accumulation. Chalcone synthase was speculated to be the rate‐limiting enzyme because its expression level was closely related to the production of both (2 S )‐naringenin and p ‐coumaric acid. The established IHTB strategy can be used to efficiently balance multigene pathways, which will accelerate the development of efficient recombinant strains.
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