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首页> 外文期刊>Applied and Environmental Microbiology >Lack of Protective Osmolytes Limits Final Cell Density and Volumetric Productivity of Ethanologenic Escherichia coli KO11 during Xylose Fermentation
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Lack of Protective Osmolytes Limits Final Cell Density and Volumetric Productivity of Ethanologenic Escherichia coli KO11 during Xylose Fermentation

机译:缺乏保护性渗透物限制了木糖发酵过程中产乙醇的大肠杆菌KO11的最终细胞密度和体积生产率

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Limited cell growth and the resulting low volumetric productivity of ethanologenic Escherichia coli KO11 in mineral salts medium containing xylose have been attributed to inadequate partitioning of carbon skeletons into the synthesis of glutamate and other products derived from the citrate arm of the anaerobic tricarboxylic acid pathway. The results of nuclear magnetic resonance investigations of intracellular osmolytes under different growth conditions coupled with those of studies using genetically modified strains have confirmed and extended this hypothesis. During anaerobic growth in mineral salts medium containing 9% xylose (600 mM) and 1% corn steep liquor, proline was the only abundant osmolyte (71.9 nmol ml?1 optical density at 550 nm [OD550] unit?1), and growth was limited. Under aerobic conditions in the same medium, twice the cell mass was produced, and cells contained a mixture of osmolytes: glutamate (17.0 nmol ml?1 OD550 unit?1), trehalose (9.9 nmol ml?1 OD550 unit?1), and betaine (19.8 nmol ml?1 OD550 unit?1). Two independent genetic modifications of E. coli KO11 (functional expression of Bacillus subtilis citZ encoding NADH-insensitive citrate synthase; deletion of ackA encoding acetate kinase) and the addition of a metabolite, such as glutamate (11 mM) or acetate (24 mM), as a supplement each increased the intracellular glutamate pool during fermentation, doubled cell growth, and increased volumetric productivity. This apparent requirement for a larger glutamate pool for increased growth and volumetric productivity was completely eliminated by the addition of a protective osmolyte (2 mM betaine or 0.25 mM dimethylsulfoniopropionate), consistent with adaptation to osmotic stress rather than relief of a specific biosynthetic requirement.
机译:细胞生长受限以及由此产生的产乙醇的大肠杆菌KO11在含有木糖的矿物盐培养基中产生的低体积生产率,归因于碳骨架分配不足,无法合成谷氨酸和其他源自厌氧三羧酸途径柠檬酸盐的产物。在不同生长条件下对细胞内渗透物进行核磁共振研究的结果,再加上使用转基因菌株进行的研究,已经证实并扩展了这一假说。在含有9%木糖(600 mM)和1%玉米浆的无机盐培养基中进行厌氧生长时,脯氨酸是唯一的渗透渗透液(在550 nm [OD550]单位?1下光密度为71.9 nmol ml?1),以及增长是有限的。在有氧条件下,在相同培养基中产生两倍的细胞团,细胞中含有渗透压的混合物:谷氨酸盐(17.0 nmol ml?1 OD550单位?1),海藻糖(9.9 nmol ml?1 OD550单位?1)和甜菜碱(19.8 nmol ml?1 OD550单位?1)。大肠杆菌KO11的两个独立遗传修饰(编码NADH不敏感的柠檬酸合酶的枯草芽孢杆菌citZ的功能表达;编码乙酸激酶的ackA缺失)和添加代谢产物,例如谷氨酸(11 mM)或乙酸盐(24 mM)作为补充,每一种都在发酵过程中增加了细胞内谷氨酸池,使细胞生长增加了一倍,并提高了容积生产率。通过添加保护性渗透液(2 mM甜菜碱或0.25 mM二甲基磺基丙酸丙二酸酯)完全消除了对更大的谷氨酸池以增加生长和提高容积生产力的明显要求,这与对渗透压的适应一致,而不是减轻了特定的生物合成要求。

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