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酸性条件下膜结合ATP酶活性降低的乳酸乳球菌突变体的特性分析

Characterization of a mutant of Lactococcus lactis with reduced membrane-bound ATPase activity under acidic conditions.

作者信息

Amachi S, Ishikawa K, Toyoda S, Kagawa Y, Yokota A, Tomita F

机构信息

Department of Bioscience and Chemistry, Faculty of Agriculture, Hokkaido University, Sapporo, Japan.

出版信息

Biosci Biotechnol Biochem. 1998 Aug;62(8):1574-80. doi: 10.1271/bbb.62.1574.

Abstract

A mutant of Lactococcus lactis subsp. lactis C2 with reduced membrane-bound ATPase activity was characterized to clarify its acid sensitivity. The cytoplasmic pH of the mutant was measured in reference to the parental strain under various pH conditions. At low pH, the mutant could not maintain its cytoplasmic pH near neutral, and lost its viability faster than the parental strain. The ATPase activities of cells cultured under neutral and acidic conditions using pH-controlled jar fermentors were measured. The relative ATPase activity of the mutant at pH 7.0 was 42% of the parental strain. At pH 4.5, the parental strain showed an ATPase activity 2.8-fold higher than that at pH 7.0 while the level of increase in the mutant was only 1.6. Northern and Western blot analyses found that at pH 7.0 the transcriptional level and the amount of F1 beta subunit were similar in both strains, suggesting that the mutant has a defective ATPase structural gene. On the other hand, at pH 4.5 the transcriptional level and the amount of F1 beta subunit were found to be significantly higher in both strains than those at pH 7.0. From these results, it was suggested that the mutant has a normal regulation system for ATPase gene expression. It was concluded that the mutant is acid sensitive due to its inability to extrude protons out of the cell with defective ATPase under acidic conditions.

摘要

为阐明乳酸乳球菌乳酸亚种C2的一个膜结合ATP酶活性降低的突变体的酸敏感性,对其进行了特性分析。在不同pH条件下,以亲本菌株为参照,测定了该突变体的细胞质pH。在低pH条件下,该突变体无法将其细胞质pH维持在接近中性的水平,且其活力丧失速度比亲本菌株更快。使用pH控制的罐式发酵罐,测定了在中性和酸性条件下培养的细胞的ATP酶活性。该突变体在pH 7.0时的相对ATP酶活性为亲本菌株的42%。在pH 4.5时,亲本菌株的ATP酶活性比在pH 7.0时高2.8倍,而突变体的增加水平仅为1.6倍。Northern印迹和Western印迹分析发现,在pH 7.0时,两株菌中F1β亚基的转录水平和含量相似,这表明该突变体具有缺陷的ATP酶结构基因。另一方面,在pH 4.5时,发现两株菌中F1β亚基的转录水平和含量均显著高于在pH 7.0时。从这些结果推测,该突变体具有正常的ATP酶基因表达调控系统。得出的结论是,该突变体对酸敏感是因为在酸性条件下其有缺陷的ATP酶无法将质子排出细胞。

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