Phage-Assisted Evolution of Bacillus methanolicus Methanol Dehydrogenase 2
Author(s) -
Timothy B. Roth,
Benjamin M. Woolston,
Gregory Stephanopoulos,
David R. Liu
Publication year - 2019
Publication title -
acs synthetic biology
Language(s) - Uncategorized
Resource type - Journals
SCImago Journal Rank - 2.156
H-Index - 66
ISSN - 2161-5063
DOI - 10.1021/acssynbio.8b00481
Subject(s) - methanol dehydrogenase , biochemistry , alcohol dehydrogenase , metabolic engineering , biology , synthetic biology , methanol , active site , formaldehyde dehydrogenase , protein engineering , enzyme , flux (metallurgy) , assimilation (phonology) , chemistry , computational biology , nad+ kinase , linguistics , philosophy , organic chemistry
Synthetic methylotrophy, the modification of organisms such as E. coli to grow on methanol, is a longstanding goal of metabolic engineering and synthetic biology. The poor kinetic properties of NAD-dependent methanol dehydrogenase, the first enzyme in most methanol assimilation pathways, limit pathway flux and present a formidable challenge to synthetic methylotrophy. To address this bottleneck, we used a formaldehyde biosensor to develop a phage-assisted noncontinuous evolution (PANCE) selection for variants of Bacillus methanolicus methanol dehydrogenase 2 (Bm Mdh2). Using this selection, we evolved Mdh2 variants with up to 3.5-fold improved V max . The mutations responsible for enhanced activity map to the predicted active site region homologous to that of type III iron-dependent alcohol dehydrogenases, suggesting a new critical region for future methanol dehydrogenase engineering strategies. Evolved Mdh2 variants enable twice as much 13 C-methanol assimilation into central metabolites than previously reported state-of-the-art methanol dehydrogenases. This work provides improved Mdh2 variants and establishes a laboratory evolution approach for metabolic pathways in bacterial cells.
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