Rational engineering of a malate dehydrogenase for microbial production of 2,4-dihydroxybutyric acid via homoserine pathway

被引:14
|
作者
Frazao, Claudio J. R. [1 ]
Topham, Christopher M. [2 ]
Malbert, Yoann [3 ]
Francois, Jean Marie [1 ,3 ]
Walther, Thomas [1 ,4 ]
机构
[1] Univ Toulouse, CNRS, INRA, INSA,LISBP, 135 Ave Rangueil, F-31077 Toulouse, France
[2] Mol Forces Consulting, 40 Rue Boyssonne, F-31400 Toulouse, France
[3] TWB, 3 Rue Satellites,Canal Biotech Bldg 2, F-31400 Toulouse, France
[4] Tech Univ Dresden, Inst Nat Mat Technol, D-01062 Dresden, Germany
关键词
SYNTHETIC METABOLIC PATHWAY; L-LACTATE DEHYDROGENASE; ESCHERICHIA-COLI; SUBSTRATE-SPECIFICITY; CONSTRUCTION; MUTATIONS; EVOLUTION; NADH;
D O I
10.1042/BCJ20180765
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
A synthetic pathway for the production of 2,4-dihydroxybutyric acid from homoserine (HMS), composed of two consecutive enzymatic reaction steps has been recently reported. An important step in this pathway consists in the reduction in 2-keto-4-hydroxybutyrate (OHB) into (L)-dihydroxybutyrate (DHB), by an enzyme with OHB reductase activity. In the present study, we used a rational approach to engineer an OHB reductase by using the cytosolic (L)-malate dehydrogenase from Escherichia coli (Ec-Mdh) as the template enzyme. Structural analysis of (L)-malate dehydrogenase and (L)-lactate dehydrogenase enzymes acting on sterically cognate substrates revealed key residues in the substrate and co-substrate-binding sites responsible for substrate discrimination. Accordingly, amino acid changes were introduced in a stepwise manner into these regions of the protein. This rational engineering led to the production of an Ec-Mdh-5E variant (I12V/R81A/M85E/G179D/D86S) with a turnover number (k(cat)) on OHB that was increased by more than 2000-fold (from 0.03 up to 65.0 s(-1)), which turned out to be 7-fold higher than that on its natural substrate oxaloacetate. Further kinetic analysis revealed the engineered enzyme to possess comparable catalytic efficiencies (k(cat)/K-m) between natural and synthetic OHB substrates (84 and 31 s(-1) mM(-1), respectively). Shake-flask cultivation of a HMS-overproducing E. coli strain expressing this improved OHB reductase together with a transaminase encoded by aspC able to convert HMS to OHB resulted in 89% increased DHB production as compared with our previous report using a E. coli host strain expressing an OHB reductase derived from the lactate dehydrogenase A of Lactococcus lactis.
引用
收藏
页码:3887 / 3901
页数:15
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