重建姜黄素在酵母中的生物合成揭示了咖啡酰-莽草酸酯酶在苯丙类代谢通量中的作用

IF 6.8 1区 生物学 Q1 BIOTECHNOLOGY & APPLIED MICROBIOLOGY Metabolic engineering Pub Date : 2024-03-01 DOI:10.1016/j.ymben.2024.02.011
Joseph Christian Utomo , Hailey Brynn Barrell , Rahul Kumar , Jessica Smith , Maximilian Simon Brant , Hector De la Hoz Siegler , Dae-Kyun Ro
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引用次数: 0

摘要

姜黄素是从姜黄(Curcuma longa)根中提取的一种多酚天然产品。它在食品工业中是一种流行的着色剂和调味剂,具有已知的健康益处。众所周知,传统的苯丙氨途径是由苯丙氨酸通过对香豆酰-CoA 中间体生成的。虽然羟基肉桂酰-CoA:莽草酸羟基肉桂酰转移酶(HCT)在对香豆酸下游苯丙醇类产品的生物合成过程中起着关键的催化作用,但最近发现的咖啡酰莽草酸酯酶(CSE)表明存在另一种途径。在此,我们利用姜黄素在酵母中的生产研究了传统途径和替代途径生产阿魏酰-CoA的生物合成效率。研究人员开发了一种新型模块化多重基因组编辑(MMG)-CRISPR 平台,可在两个步骤内将多达八个基因快速整合到酵母基因组中。利用该 MMG-CRISPR 平台和代谢工程策略,在工程酵母菌株中,替代 CSE 苯丙酮途径持续显示出比传统途径更高的姜黄素生产滴度(2-19 倍)。在使用不含苯丙氨酸的合成最小培养基的摇瓶培养中,姜黄素的生产滴度高达 1.5 mg/L,比非工程基础菌株提高了三个数量级(∼4800 倍)。这是首次在酵母中展示姜黄素的新生物合成。我们的工作表明,CSE 在改善酵母中苯丙类生物合成途径的代谢通量方面发挥了关键作用。此外,我们还展示了模块化多重 CRISPR/Cas9 基因组编辑在构建酵母复杂合成途径中的便利性和可靠性。
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Reconstructing curcumin biosynthesis in yeast reveals the implication of caffeoyl-shikimate esterase in phenylpropanoid metabolic flux

Curcumin is a polyphenolic natural product from the roots of turmeric (Curcuma longa). It has been a popular coloring and flavoring agent in food industries with known health benefits. The conventional phenylpropanoid pathway is known to proceed from phenylalanine via p-coumaroyl-CoA intermediate. Although hydroxycinnamoyl-CoA: shikimate hydroxycinnamoyl transferase (HCT) plays a key catalysis in the biosynthesis of phenylpropanoid products at the downstream of p-coumaric acid, a recent discovery of caffeoyl-shikimate esterase (CSE) showed that an alternative pathway exists. Here, the biosynthetic efficiency of the conventional and the alternative pathway in producing feruloyl-CoA was examined using curcumin production in yeast. A novel modular multiplex genome-edit (MMG)-CRISPR platform was developed to facilitate rapid integrations of up to eight genes into the yeast genome in two steps. Using this MMG-CRISPR platform and metabolic engineering strategies, the alternative CSE phenylpropanoid pathway consistently showed higher titers (2–19 folds) of curcumin production than the conventional pathway in engineered yeast strains. In shake flask cultures using a synthetic minimal medium without phenylalanine, the curcumin production titer reached up to 1.5 mg/L, which is three orders of magnitude (∼4800-fold) improvement over non-engineered base strain. This is the first demonstration of de novo curcumin biosynthesis in yeast. Our work shows the critical role of CSE in improving the metabolic flux in yeast towards the phenylpropanoid biosynthetic pathway. In addition, we showcased the convenience and reliability of modular multiplex CRISPR/Cas9 genome editing in constructing complex synthetic pathways in yeast.

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来源期刊
Metabolic engineering
Metabolic engineering 工程技术-生物工程与应用微生物
CiteScore
15.60
自引率
6.00%
发文量
140
审稿时长
44 days
期刊介绍: Metabolic Engineering (MBE) is a journal that focuses on publishing original research papers on the directed modulation of metabolic pathways for metabolite overproduction or the enhancement of cellular properties. It welcomes papers that describe the engineering of native pathways and the synthesis of heterologous pathways to convert microorganisms into microbial cell factories. The journal covers experimental, computational, and modeling approaches for understanding metabolic pathways and manipulating them through genetic, media, or environmental means. Effective exploration of metabolic pathways necessitates the use of molecular biology and biochemistry methods, as well as engineering techniques for modeling and data analysis. MBE serves as a platform for interdisciplinary research in fields such as biochemistry, molecular biology, applied microbiology, cellular physiology, cellular nutrition in health and disease, and biochemical engineering. The journal publishes various types of papers, including original research papers and review papers. It is indexed and abstracted in databases such as Scopus, Embase, EMBiology, Current Contents - Life Sciences and Clinical Medicine, Science Citation Index, PubMed/Medline, CAS and Biotechnology Citation Index.
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