Combinatorial metabolic engineering of industrial Gluconobacter oxydans DSM2343 for boosting 5-keto-D-gluconic acid accumulation

Jianfeng Yuan; Mianbin Wu; Jianping Lin; Lirong Yang

doi:10.1186/s12896-016-0272-y

Combinatorial metabolic engineering of industrial Gluconobacter oxydans DSM2343 for boosting 5-keto-D-gluconic acid accumulation

BMC Biotechnol. 2016 May 17;16(1):42. doi: 10.1186/s12896-016-0272-y.

Authors

Jianfeng Yuan¹, Mianbin Wu¹, Jianping Lin², Lirong Yang¹

Affiliations

¹ Key Laboratory of Biomass Chemical Engineering of the Ministry of Education,College of Chemical and Biological Engineering, Zhejiang University, Hangzhou, 310027, China.
² Key Laboratory of Biomass Chemical Engineering of the Ministry of Education,College of Chemical and Biological Engineering, Zhejiang University, Hangzhou, 310027, China. linjp@zju.edu.cn.

Abstract

Background: L-(+)-tartaric acid (L-TA) is an important organic acid, which is produced from the cream of tartar or stereospecific hydrolysis of the cis-epoxysuccinate. The former method is limited by the availability of raw material and the latter is dependent on the petrochemical material. Thus, new processes for the economical preparation of L-TA from carbohydrate or renewable resource would be much more attractive. Production of 5-keto-D-gluconate (5-KGA) from glucose by Gluconobacter oxydans is the first step to produce L-TA. The aim of this work is to enhance 5-KGA accumulation using combinatorial metabolic engineering strategies in G. oxydans. The sldAB gene, encoding sorbitol dehydrogenase, was overexpressed in an industrial strain G. oxydans ZJU2 under a carefully selected promoter, P0169. To enhance the efficiency of the oxidation by sldAB, the coenzyme pyrroloquinoline quinone (PQQ) and respiratory chain were engineered. Besides, the role in sldAB overexpression, coenzyme and respiratory chain engineering and their subsequent effects on 5-KGA production were investigated.

Results: An efficient, stable recombinant strain was constructed, whereas the 5-KGA production could be enhanced. By self-overexpressing the sldAB gene in G. oxydans ZJU2 under the constitutive promoter P0169, the resulting strain, G. oxydans ZJU3, produced 122.48 ± 0.41 g/L of 5-KGA. Furthermore, through the coenzyme and respiratory chain engineering, the titer and productivity of 5-KGA reached 144.52 ± 2.94 g/L and 2.26 g/(L · h), respectively, in a 15 L fermenter. It could be further improved the 5-KGA titer by 12.10 % through the fed-batch fermentation under the pH shift and dissolved oxygen tension (DOT) control condition, obtained 162 ± 2.12 g/L with the productivity of 2.53 g/(L · h) within 64 h.

Conclusions: The 5-KGA production could be significantly enhanced with the combinatorial metabolic engineering strategy in Gluconobacter strain, including sldAB overexpression, coenzyme and respiratory chain engineering. Fed-batch fermentation could further enlarge the positive effect and increase the 5-KGA production. All of these demonstrated that the robust recombinant strain can efficiently produce 5-KGA in larger scale to fulfill the industrial production of L-TA from 5-KGA.

Keywords: 5-keto-D-gluconate; Fed-batch fermentation; L-(+)-tartaric acid; Pyrroloquinoline quinone; Respiratory chain.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Combinatorial Chemistry Techniques / methods
Genetic Enhancement / methods*
Gluconates / isolation & purification
Gluconates / metabolism*
Gluconobacter oxydans / classification
Gluconobacter oxydans / enzymology*
Gluconobacter oxydans / genetics*
Industrial Microbiology / methods
L-Iditol 2-Dehydrogenase / genetics*
Metabolic Engineering / methods*
Promoter Regions, Genetic / genetics
Recombinant Proteins / metabolism
Species Specificity
Up-Regulation / genetics

Substances

5-keto-d-gluconate
Gluconates
Recombinant Proteins
L-Iditol 2-Dehydrogenase