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Effect of replacing the general energy-coupling proteins of the PEP:sugar phosphotransferase system of Salmonella typhimurium with their fructose-inducible counterparts on utilization of the PTS sugar glucitol

机译:替代PEP的一般能量偶联蛋白的疗效:糖磷霉素糖磷酸盐糖酶系统及其果糖诱导对应于Pts糖葡糖醇的利用率

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A strain of Salmonella typhimurium in which the genes encoding the general phosphoenolpyruvate:sugar phosphotransferase system (PTS) proteins HPr and Enzyme I have been deleted, the normally cryptic gene encoding the fructose-inducible Enzyme I (EI* or EIfructose) is expressed, and the fructose repressor protein is inactive (fruR or cra mutant) was studied. This strain lacks HPr and EI, but expresses FPr (DTP) and EIfructose constitutively. Since FPr and EIfructose can substitute for HPr and EI, the strain grew in minimal liquid medium supplemented with the PTS sugars glucose, fructose, N-acetylglucosamine, mannitol or mannose. However, it showed very poor to negligible growth on the PTS sugar glucitol. It also grew very poorly on the non-PTS sugars maltose, melibiose and especially glycerol. Adding cAMP to the medium allowed growth on glucitol, but did not affect growth on glycerol. We suggest that poor phosphorylation of the regulatory molecule Enzyme IIAglucose by FPr is responsible for these effects.
机译:一种菌株的沙门氏菌毛刺,其中编码一般磷酸丙酮酸的基因:糖磷酸转移酶系统(PTS)蛋白质HPR和酶I已被删除,表达了编码果糖诱导酶I(EI *或EI型)的正常隐秘基因,并且研究了果糖抑制蛋白是无活性的(Frur或CRA突变体)。这种应变缺乏HPR和EI,但表达FPR(DTP)和叶霉菌素组成型。由于FPR和eIFructose可以替代HPR和EI,因此菌株在补充有Pts糖葡萄糖,果糖,N-乙酰葡糖胺,甘露醇或甘露糖的最小液体培养基中。然而,它表明PTS糖葡糖酚的贫微增长表现出很差。它在非Pts糖麦芽糖,Melibiose和尤其是甘油中也非常差。将营地添加到中等允许生长葡萄糖醇,但不影响甘油的生长。我们表明,FPR的调节分子酶Iiaglucose的差磷酸化差是对这些作用的原因。

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