Improved n-butanol production via co-expression of membrane-targeted tilapia metallothionein and the clostridial metabolic pathway in Escherichia coli

Wei-Chih Chin; Kuo-Hsing Lin; Chun-Chi Liu; Kenji Tsuge; Chieh-Chen Huang

doi:10.1186/s12896-017-0356-3

BMC Biotechnology (Apr 2017)

Improved n-butanol production via co-expression of membrane-targeted tilapia metallothionein and the clostridial metabolic pathway in Escherichia coli

Wei-Chih Chin,
Kuo-Hsing Lin,
Chun-Chi Liu,
Kenji Tsuge,
Chieh-Chen Huang

Affiliations

Wei-Chih Chin: Department of Life Sciences, National Chung Hsing University
Kuo-Hsing Lin: Center of Cold Chain Logistics Certification, College of Management, National Kaohsiung First University of Science and Technology
Chun-Chi Liu: Institute of Genomics and Bioinformatics, National Chung Hsing University
Kenji Tsuge: Graduate School of Science, Technology and Innovation, Kobe University
Chieh-Chen Huang: Department of Life Sciences, National Chung Hsing University

DOI: https://doi.org/10.1186/s12896-017-0356-3
Journal volume & issue: Vol. 17, no. 1
pp. 1 – 14

Abstract

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Abstract Background N-Butanol has favorable characteristics for use as either an alternative fuel or platform chemical. Bio-based n-butanol production using microbes is an emerging technology that requires further development. Although bio-industrial microbes such as Escherichia coli have been engineered to produce n-butanol, reactive oxygen species (ROS)-mediated toxicity may limit productivity. Previously, we show that outer-membrane-targeted tilapia metallothionein (OmpC-TMT) is more effective as an ROS scavenger than human and mouse metallothioneins to reduce oxidative stress in the host cell. Results The host strain (BUT1-DE) containing the clostridial n-butanol pathway displayed a decreased growth rate and limited n-butanol productivity, likely due to ROS accumulation. The clostridial n-butanol pathway was co-engineered with inducible OmpC-TMT in E. coli (BUT3-DE) for simultaneous ROS removal, and its effect on n-butanol productivity was examined. The ROS scavenging ability of cells overexpressing OmpC-TMT was examined and showed an approximately twofold increase in capacity. The modified strain improved n-butanol productivity to 320 mg/L, whereas the control strain produced only 95.1 mg/L. Transcriptomic analysis revealed three major KEGG pathways that were significantly differentially expressed in the BUT3-DE strain compared with their expression in the BUT1-DE strain, including genes involved in oxidative phosphorylation, fructose and mannose metabolism and glycolysis/gluconeogenesis. Conclusions These results indicate that OmpC-TMT can increase n-butanol production by scavenging ROS. The transcriptomic analysis suggested that n-butanol causes quinone malfunction, resulting in oxidative-phosphorylation-related nuo operon downregulation, which would diminish the ability to convert NADH to NAD+ and generate proton motive force. However, fructose and mannose metabolism-related genes (fucA, srlE and srlA) were upregulated, and glycolysis/gluconeogenesis-related genes (pfkB, pgm) were downregulated, which further assisted in regulating NADH/NAD+ redox and preventing additional ATP depletion. These results indicated that more NADH and ATP were required in the n-butanol synthetic pathway. Our study demonstrates a potential approach to increase the robustness of microorganisms and the production of toxic chemicals through the ability to reduce oxidative stress.

Published in BMC Biotechnology

ISSN: 1472-6750 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Technology: Chemical technology: Biotechnology
Website: https://bmcbiotechnol.biomedcentral.com

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