首页> 美国卫生研究院文献>Metabolic Engineering Communications >Effect of pyruvate kinase gene deletion on the physiology of Corynebacterium glutamicum ATCC13032 under biotin-sufficient non-glutamate-producing conditions: Enhanced biomass production
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Effect of pyruvate kinase gene deletion on the physiology of Corynebacterium glutamicum ATCC13032 under biotin-sufficient non-glutamate-producing conditions: Enhanced biomass production

机译:丙酮酸激酶基因缺失对生物素 - 足够的非谷氨酸生产条件下谷氨酸谷氨酸ATCC13032的生理学的影响:增强生物质生产

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摘要

The effect of pyruvate kinase gene (pyk) deletion on the physiology of Corynebacterium glutamicum ATCC13032 was investigated under biotin-sufficient, non-glutamate-producing conditions. In a complex medium containing 100 g/L glucose, a defined pyk deletion mutant, strain D1, exhibited 35% enhancement in glucose consumption rate, 37% increased growth and a 57% reduction in respiration rate compared to the wild-type parent. Significant upregulation of phosphoenolpyruvate (PEP) carboxylase and downregulation of PEP carboxykinase activities were observed in the D1 mutant, which may have prevented over-accumulation of PEP caused by the pyk deletion. Moreover, we found a dramatic 63% reduction in the activity of malate:quinone oxidoreductase (MQO) in the D1 mutant. MQO, a TCA cycle enzyme that converts malate to oxaloacetate (OAA), constitutes a major primary gate to the respiratory chain in C. glutamicum, thus explaining the reduced respiration rate in the mutant. Additionally, pyruvate carboxylase gene expression was downregulated in the mutant. These changes seemed to prevent OAA over-accumulation caused by the activity changes of PEP carboxylase/PEP carboxykinase. Intrinsically the same alterations were observed in the cultures conducted in a minimal medium containing 20 g/L glucose. Despite these responses in the mutant, metabolic distortion caused by pyk deletion under non-glutamate-producing conditions required amelioration by increased biomass production, as metabolome analysis revealed increased intracellular concentrations of several precursor metabolites for building block formation associated with pyk deletion. These fermentation profiles and metabolic alterations observed in the mutant reverted completely to the wild-type phenotypes in the pyk-complemented strain, suggesting the observed metabolic changes were caused by the pyk deletion. These results demonstrated multilateral strategies to overcome metabolic disturbance caused by pyk deletion in this bacterium.
机译:丙酮酸激酶基因(PYK)缺失的谷氨酸棒状杆菌ATCC13032的生理的作用生物素足够的,非谷氨酸生产的条件下调查。在含有100克/升葡萄糖,复合介质的定义PYK缺失突变体,应变D1,显示出35%的增强中的葡萄糖消耗率,37%增加的生长和呼吸率的降低57%相对于野生型亲本。磷酸烯醇丙酮酸(PEP)羧化酶和PEP的下调显著上调羧在D1突变体,其可阻止过度积累PEP引起的PYK缺失观察到的活动。此外,我们发现在苹果酸的酶活性的显着的63%的减少:在D1突变体醌氧化还原酶(MQO)。 MQO,TCA循环酶,其将苹果酸以草酰乙酸(OAA),构成了一个主要主栅极到在谷氨酸棒杆菌的呼吸链,因此解释在突变体的降低的呼吸率。此外,丙酮酸羧化酶基因表达的突变体中下调。这些变化似乎防止因PEP羧化酶/ PEP羧激酶的活性变化OAA过度积累。本质上,在含有20g / L葡萄糖的基本培养基进行的培养物中观察到的相同的改变。尽管通过增加的生物量生产所需要改善非谷氨酸生产的条件下引起的pyk缺失突变体,代谢失真这些响应,代谢组分析显示增加的几个前体的代谢物的胞内浓度为建设PYK缺失相关的块形成。这些发酵概况和代谢改变在突变完全恢复了在PYK-补偿菌株的野生型表型观察,表明所观察到的代谢改变是由PYK删除引起的。这些结果表明多边战略来克服这种细菌引起PYK缺失代谢紊乱。

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