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利用酿酒酵母工程化线粒体生产单萜。

Engineered mitochondrial production of monoterpenes in Saccharomyces cerevisiae.

机构信息

Department of Chemical and Biomolecular Engineering, University of California, Los Angeles, CA, 90095, United States.

Department of Chemistry and Biochemistry, University of California, Los Angeles, CA, 90095, United States.

出版信息

Metab Eng. 2019 Sep;55:76-84. doi: 10.1016/j.ymben.2019.06.004. Epub 2019 Jun 19.

Abstract

Monoterpene indole alkaloids (MIAs) from plants encompass a broad class of structurally complex and medicinally valuable natural products. MIAs are biologically derived from the universal precursor strictosidine. Although the strictosidine biosynthetic pathway has been identified and reconstituted, extensive work is required to optimize production of strictosidine and its precursors in yeast. In this study, we engineered a fully integrated and plasmid-free yeast strain with enhanced production of the monoterpene precursor geraniol. The geraniol biosynthetic pathway was targeted to the mitochondria to protect the GPP pool from consumption by the cytosolic ergosterol pathway. The mitochondrial geraniol producer showed a 6-fold increase in geraniol production compared to cytosolic producing strains. We further engineered the monoterpene-producing strain to synthesize the next intermediates in the strictosidine pathway: 8-hydroxygeraniol and nepetalactol. Integration of geraniol hydroxylase (G8H) from Catharanthus roseus led to essentially quantitative conversion of geraniol to 8-hydroxygeraniol at a titer of 227 mg/L in a fed-batch fermentation. Further introduction of geraniol oxidoreductase (GOR) and iridoid synthase (ISY) from C. roseus and tuning of the relative expression levels resulted in the first de novo nepetalactol production. The strategies developed in this work can facilitate future strain engineering for yeast production of later intermediates in the strictosidine biosynthetic pathway.

摘要

植物中的单萜吲哚生物碱(MIAs)包含一大类结构复杂且具有药用价值的天然产物。MIAs 是从普遍的前体物Strictosidine 生物衍生而来的。尽管已经确定并重建了 Strictosidine 生物合成途径,但仍需要大量工作来优化酵母中 Strictosidine 及其前体的生产。在这项研究中,我们构建了一种完全整合且无质粒的酵母菌株,该菌株能够增强单萜前体香叶醇的生产。香叶醇生物合成途径被靶向到线粒体,以防止 GPP 池被细胞质中的麦角固醇途径消耗。与细胞质产生菌株相比,线粒体香叶醇产生菌的香叶醇产量增加了 6 倍。我们进一步对单萜产生菌株进行工程改造,以合成 Strictosidine 途径中的下一个中间体:8-羟基香叶醇和新穿心莲内酯。整合来自长春花的香叶醇羟化酶(G8H)可导致香叶醇在分批补料发酵中的转化率达到 99.7%,终产物为 8-羟基香叶醇,产量为 227mg/L。进一步引入长春花的香叶醇氧化还原酶(GOR)和裂环烯醚萜合酶(ISY),并调整相对表达水平,可首次从头合成新穿心莲内酯。本工作中开发的策略可以促进未来酵母生产 Strictosidine 生物合成途径中后续中间体的菌株工程改造。

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