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High Glycolytic Flux Improves Pyruvate Production by a Metabolically Engineered Escherichia coli Strain

机译:高糖酵解通量可通过代谢工程化的大肠杆菌菌株提高丙酮酸的产生

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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 5 mM betaine as osmoprotectant and an exponential feeding rate of 0.15 h?1 achieved 90 g/liter pyruvate, with an overall productivity of 2.1 g/liter · h and yield of 0.68 g/g.
机译:我们报告丙酮酸形成在大肠杆菌菌株ALS929中包含aceEF,pfl,poxB,pps和ldhA基因中的突变,分别编码丙酮酸脱氢酶复合物,丙酮酸甲酸酯裂解酶,丙酮酸氧化酶,磷酸烯醇丙酮酸合酶和乳酸脱氢酶。用葡萄糖限制的,乙酸盐限制的,氮限制的或磷限制的化学恒温器以0.15h -1的生长速率比较了糖酵解速率和丙酮酸生产率。在这四个养分限制条件中,在乙酸盐限制条件下的生长导致最高的糖酵解通量(1.60 g / g·h),丙酮酸盐形成速率(1.11 g / g·h)和丙酮酸盐产量(0.70 g / g)。 atpFH和arcA(菌株ALS1059)中的其他突变在醋酸盐有限的恒化器中将稳态糖酵解通量进一步提高至2.38 g / g·h,异源NADH氧化酶表达仅引起适度的额外改​​善。使用具有5 mM甜菜碱作为渗透保护剂的确定培养基和0.15 h?1的指数进料速率,用菌株ALS1059进行的分批补料工艺可得到90 g /升丙酮酸,总生产率为2.1 g /升·h,产量为0.68 g /G。

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