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High glycolytic flux improves pyruvate production by a metabolically engineered escherichia coli strain
We report pyruvate formation in Escherichia coli strain
ALS929 containing mutations in the aceEF, pfl, poxB, pps, and ldhA genes which
encode, respectively, the pyruvate dehydrogenase complex, pyruvate formate
lyase, pyruvate oxidase, phosphoenolpyruvate synthase, and lactate
dehydrogenase. The glycolytic rate and pyruvate productivity were compared
using glucose-, acetate-, nitrogen-, or phosphorus-limited chemostats at a
growth rate of 0.15 h–1. Of these four nutrient limitation conditions, growth
under acetate limitation resulted in the highest glycolytic flux (1.60 g/g ·
h), pyruvate formation rate (1.11 g/g · h), and pyruvate yield (0.70 g/g).
Additional mutations in atpFH and arcA (strain ALS1059) further elevated the
steady-state glycolytic flux to 2.38 g/g · h in an acetate-limited chemostat,
with heterologous NADH oxidase expression causing only modest additional
improvement. A fed-batch process with strain ALS1059 using defined medium with