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Effect of growth conditions on levels of components of the phosphoenolpyruvate:sugar phosphotransferase system in Streptococcus mutans and Streptococcus sobrinus grown in continuous culture.

机译:生长条件对连续培养的变形链球菌和sobrinus链球菌中磷酸烯醇丙酮酸:糖磷酸转移酶系统各成分水平的影响。

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摘要

The membrane-bound, sugar-specific enzyme II (EII) component of the phosphoenolpyruvate:sugar phosphotransferase system (PTS) in Streptococcus mutans Ingbritt is repressed by growth on glucose under various conditions in continuous culture. Compared with optimal PTS conditions (i.e., glucose limitation, dilution rate [D] of 0.1 h-1, and pH 7.0), EII activity for glucose (EIIGlc) and mannose (EIIMan) in cells grown at a D of 0.4 h-1 and pH 5.5 with the same glucose concentration was reduced 24- to 27-fold. EII activity with methyl alpha-glucoside and 2-deoxyglucose was reduced 6- and 26-fold, respectively. Growth with excess glucose (i.e., nitrogen limitation) resulted in 26- to 88-fold repression of EII activity with these substrates. The above conditions of low pH, high dilution rate, and excess glucose also repressed EII activity for fructose (EIIFru), but to a lesser extent (two- to fivefold). Conversely, growth of S. mutans DR0001 at a D of 0.2 h-1 and pH 5.5 resulted in increased EIIGlc and EIIMan activity. Unlike the EII component, the HPr concentration in S. mutans Ingbritt varied only twofold (5.5 to 11.4 nmol/mg of protein) despite growth at pH 5.5 with limiting and excess glucose. The HPr concentrations in S. mutans DR0001 and the glucose-PTS-defective mutant DR0001/6 were similar. In a companion study, the soluble components of the PTS (i.e., HPr, EI, and EIIILac) in Streptococcus sobrinus grown on limiting lactose in a chemostat were not influenced significantly by growth at various pHs (7.0 and 5.0) and growth rates (D of 0.1, 0.54, and 0.8 h-1). However, growth on lactose resulted in repression of both EIIGlc and EIIFru, confirming earlier results with batch-grown cells. Thus, the glucose-PTS in some strains of S. mutans is regulated at the level of EII synthesis by certain environmental conditions.
机译:变形链球菌Ingbritt中磷酸烯醇丙酮酸:糖磷酸转移酶系统(PTS)的膜结合的糖特异性酶II(EII)成分可通过在连续条件下在各种条件下在葡萄糖上的生长来抑制。与最佳PTS条件(即葡萄糖限制,0.1 h-1的稀释率[D]和pH 7.0)相比,在D为0.4 h-1的细胞中,EII对葡萄糖(EIIGlc)和甘露糖(EIIMan)的活性在相同葡萄糖浓度下,pH 5.5降低了24到27倍。甲基α-葡萄糖苷和2-脱氧葡萄糖的EII活性分别降低了6倍和26倍。用过量的葡萄糖(即氮限制)生长会导致这些底物的EII活性降低26到88倍。上述低pH,高稀释率和过量葡萄糖的条件也抑制了果糖的EII活性(EIIFru),但程度较低(二至五倍)。相反,变形链球菌DR0001在0.2h-1的D和pH 5.5下的生长导致EIIGlc和EIIMan活性增加。与EII成分不同,尽管在pH 5.5下生长受限且葡萄糖过多,变形链球菌Ingbritt中的HPr浓度仅变化了两倍(5.5至11.4 nmol / mg蛋白质)。变形链球菌DR0001和葡萄糖-PTS缺陷型突变体DR0001 / 6中的HPr浓度相似。在一项伴随研究中,在多种pH值(7.0和5.0)下的生长和生长速度(D)下,在有限的乳糖作用下,在有限的乳糖中生长的链球菌中的PTS的可溶性成分(即HPr,EI和EIIILac)均不受显着影响。 0.1、0.54和0.8 h-1)。但是,乳糖上的生长会导致EIIGlc和EIIFru的抑制,从而证实了批量培养细胞的早期结果。因此,在某些环境条件下,某些变形链球菌菌株中的葡萄糖-PTS在EII合成水平上受到调节。

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