Engineering of a Highly Efficient Escherichia coli Strain for Mevalonate Fermentation through Chromosomal Integration

Jilong Wang; Suthamat Niyompanich; Yi-Shu Tai; Jingyu Wang; Wenqin Bai; Prithviraj Mahida; Tuo Gao; Kechun Zhang

doi:10.1128/AEM.02178-16

Engineering of a Highly Efficient Escherichia coli Strain for Mevalonate Fermentation through Chromosomal Integration

Appl Environ Microbiol. 2016 Nov 21;82(24):7176-7184. doi: 10.1128/AEM.02178-16. Print 2016 Dec 15.

Authors

Jilong Wang¹, Suthamat Niyompanich², Yi-Shu Tai¹, Jingyu Wang¹, Wenqin Bai¹, Prithviraj Mahida¹, Tuo Gao¹, Kechun Zhang³

Affiliations

¹ Department of Chemical Engineering and Materials Science, University of Minnesota, Minneapolis, Minnesota, USA.
² Department of Biology, Faculty of Science, Srinakharinwirot University, Bangkok, Thailand.
³ Department of Chemical Engineering and Materials Science, University of Minnesota, Minneapolis, Minnesota, USA kzhang@umn.edu.

Abstract

Chromosomal integration of heterologous metabolic pathways is optimal for industrially relevant fermentation, as plasmid-based fermentation causes extra metabolic burden and genetic instabilities. In this work, chromosomal integration was adapted for the production of mevalonate, which can be readily converted into β-methyl-δ-valerolactone, a monomer for the production of mechanically tunable polyesters. The mevalonate pathway, driven by a constitutive promoter, was integrated into the chromosome of Escherichia coli to replace the native fermentation gene adhE or ldhA The engineered strains (CMEV-1 and CMEV-2) did not require inducer or antibiotic and showed slightly higher maximal productivities (0.38 to ∼0.43 g/liter/h) and yields (67.8 to ∼71.4% of the maximum theoretical yield) than those of the plasmid-based fermentation. Since the glycolysis pathway is the first module for mevalonate synthesis, atpFH deletion was employed to improve the glycolytic rate and the production rate of mevalonate. Shake flask fermentation results showed that the deletion of atpFH in CMEV-1 resulted in a 2.1-fold increase in the maximum productivity. Furthermore, enhancement of the downstream pathway by integrating two copies of the mevalonate pathway genes into the chromosome further improved the mevalonate yield. Finally, our fed-batch fermentation showed that, with deletion of the atpFH and sucA genes and integration of two copies of the mevalonate pathway genes into the chromosome, the engineered strain CMEV-7 exhibited both high maximal productivity (∼1.01 g/liter/h) and high yield (86.1% of the maximum theoretical yield, 30 g/liter mevalonate from 61 g/liter glucose after 48 h in a shake flask).

Importance: Metabolic engineering has succeeded in producing various chemicals. However, few of these chemicals are commercially competitive with the conventional petroleum-derived materials. In this work, chromosomal integration of the heterologous pathway and subsequent optimization strategies ensure stable and efficient (i.e., high-titer, high-yield, and high-productivity) production of mevalonate, which demonstrates the potential for scale-up fermentation. Among the optimization strategies, we demonstrated that enhancement of the glycolytic flux significantly improved the productivity. This result provides an example of how to tune the carbon flux for the optimal production of exogenous chemicals.

MeSH terms

Chromosomes, Bacterial / genetics*
Escherichia coli / genetics*
Escherichia coli / metabolism*
Fermentation
Glucose / metabolism
Metabolic Engineering
Mevalonic Acid / metabolism*
Plasmids / genetics
Plasmids / metabolism

Substances

Glucose
Mevalonic Acid