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Membrane-Bound ATPase Contributes to Hop Resistance of Lactobacillus brevis

机译:膜结合ATPase促进短乳杆菌的啤酒花抗性

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The activity of the membrane-bound H+-ATPase of the beer spoilage bacterium Lactobacillus brevis ABBC45 increased upon adaptation to bacteriostatic hop compounds. The ATPase activity was optimal around pH 5.6 and increased up to fourfold when L. brevis was exposed to 666 μM hop compounds. The extent of activation depended on the concentration of hop compounds and was maximal at the highest concentration tested. The ATPase activity was strongly inhibited by N,N′-dicyclohexylcarbodiimide, a known inhibitor of FoF1-ATPase. Western blots of membrane proteins of L. brevis with antisera raised against the α- and β-subunits of FoF1-ATPase from Enterococcus hirae showed that there was increased expression of the ATPase after hop adaptation. The expression levels, as well as the ATPase activity, decreased to the initial nonadapted levels when the hop-adapted cells were cultured further without hop compounds. These observations strongly indicate that proton pumping by the membrane-bound ATPase contributes considerably to the resistance of L. brevis to hop compounds.
机译:啤酒变质细菌短乳杆菌ABBC45的膜结合H + -ATPase的活性在适应抑菌啤酒花化合物后增加。 ATP酶活性在pH 5.6附近最佳,当短乳杆菌暴露于666μM啤酒花化合物时增加至四倍。活化程度取决于啤酒花化合物的浓度,并且在测试的最高浓度下最大。已知的FoF1-ATPase抑制剂N,N'-dicyclohexylcarbodiimide强烈抑制ATPase的活性。带有抗血清的短乳杆菌膜蛋白的Western印迹显示,其来自平肠肠球菌FoF1-ATPase的α和β亚基,表明啤酒花适应后ATPase的表达增加。当在没有啤酒花化合物的情况下进一步培养啤酒花适应性细胞时,表达水平以及ATPase活性均降至初始非适应性水平。这些观察结果强烈表明,通过膜结合的ATPase进行的质子泵送大大促进了短乳杆菌对啤酒花化合物的抗性。

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