4.7 Article

High production of triterpenoids inYarrowia lipolyticathrough manipulation of lipid components

Journal

BIOTECHNOLOGY FOR BIOFUELS
Volume 13, Issue 1, Pages -

Publisher

BMC
DOI: 10.1186/s13068-020-01773-1

Keywords

Triterpenoids; Lipid manipulation; Unsaturated fatty acids; Cell morphology; Yarrowia lipolytica

Funding

  1. Major Program of the National Natural Science Foundation of China [21621004]
  2. Natural Science Foundation of Tianjin City [19JCQNJC09200]
  3. Young Elite Scientists Sponsorship Program by Tianjin [TJSQNTJ-2018-16]

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Background Lupeol exhibits novel physiological and pharmacological activities, such as anticancer and immunity-enhancing activities. However, cytotoxicity remains a challenge for triterpenoid overproduction in microbial cell factories. As lipophilic and relatively small molecular compounds, triterpenes are generally secreted into the extracellular space. The effect of increasing triterpene efflux on the synthesis capacity remains unknown. Results In this study, we developed a strategy to enhance triterpene efflux through manipulation of lipid components inY. lipolyticaby overexpressing the enzyme Delta 9-fatty acid desaturase (OLE1) and disturbing phosphatidic acid phosphatase (PAH1) and diacylglycerol kinase (DGK1). By this strategy combined with two-phase fermentation, the highest lupeol production reported to date was achieved, where the titer in the organic phase reached 381.67 mg/L and the total production was 411.72 mg/L in shake flasks, exhibiting a 33.20-fold improvement over the initial strain. Lipid manipulation led to a twofold increase in the unsaturated fatty acid (UFA) content, up to 61-73%, and an exceptionally elongated cell morphology, which might have been caused by enhanced membrane phospholipid biosynthesis flux. Both phenotypes accelerated the export of toxic products to the extracellular space and ultimately stimulated the capacity for triterpenoid synthesis, which was proven by the 5.11-fold higher ratio of extra/intracellular lupeol concentrations, 2.79-fold higher biomass accumulation and 2.56-fold higher lupeol productivity per unit OD in the modified strains. This strategy was also highly efficient for the biosynthesis of other triterpenes and sesquiterpenes, including alpha-amyrin, beta-amyrin, longifolene, longipinene and longicyclene. Conclusions In conclusion, we successfully created a high-yield lupeol-producing strain via lipid manipulation. We demonstrated that the enhancement of lupeol efflux and synthesis capacity was induced by the increased UFA content and elongated cell morphology. Our study provides a novel strategy to promote the biosynthesis of valuable but toxic products in microbial cell factories.

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