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Fermentative High-Level Production of 5-Hydroxyvaleric Acid by Metabolically Engineered Corynebacterium glutamicum

Title
Fermentative High-Level Production of 5-Hydroxyvaleric Acid by Metabolically Engineered Corynebacterium glutamicum
Authors
Sohn, Yu JungKang, MinsooBaritugo, Kei-AnneSon, JinaKang, Kyoung HeeRyu, Mi-HeeLee, SiseonSohn, MingiJung, Ye JeanPark, KyungmoonPark, Si JaeJoo, Jeong ChanKim, Hee Taek
Ewha Authors
박시재
SCOPUS Author ID
박시재scopus
Issue Date
2021
Journal Title
ACS SUSTAINABLE CHEMISTRY & ENGINEERING
ISSN
2168-0485JCR Link
Citation
ACS SUSTAINABLE CHEMISTRY & ENGINEERING vol. 9, no. 6, pp. 2523 - 2533
Keywords
5-hydroxyvaleric acidCorynebacterium glutamicumL-lysineglutaric acid5-aminovaleric acid
Publisher
AMER CHEMICAL SOC
Indexed
SCIE; SCOPUS WOS scopus
Document Type
Article
Abstract
We report metabolic engineering of Corynebacterium glutanucum C. glutamicum) for high-level production of 5-hydroxyvaleric acid (S-HV), an important C5 platform chemical covering a wide range of industrial applications, using glucose as a sole carbon source. To derive 5-HV, an artificial S-HV biosynthesis pathway, composed of the first three reaction steps of an L-lysine catabolic pathway via 5-aminovaleramide along with a subsequent intracellular reduction step, was constructed: L-lysine was converted to glutarate semialdehyde through an L-lysine catabolic pathway encoded by Pseudomonas putida davTBA genes, and glutarate semialdehyde was further reduced to 5-HV by a suitable aldehyde reductase. Various aldehyde reductases including CpnD from Clostridium aminovalericum, Gbd from Ralstonia eutropha, ButA from C. glutamicum, and YihU, YahK, and YqhD from Escherichia coli were examined for efficient 5-HV production through the flask and batch cultivations, and YahK was determined to be the most appropriate aldehyde reductase. Further modification to enhance 5-HV production was investigated by deletion of an endogenous gabD gene responsible for the oxidation of glutarate semialdehyde into glutaric acid in order to suppress glutaric acid by-production. Finally, 52.1 g/L S-HV with the yield of 0.33 g/g glucose was achieved by fed-batch fermentation of the engineered C. glutamicum with overexpression of davTBA genes and the yahK gene along with gabD deletion in the chromosome.
DOI
10.1021/acssuschemeng.0c08118
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공과대학 > 화공신소재공학과 > Journal papers
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