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口腔乳酸菌分离株F-ATP酶的耐酸性及抑制剂敏感性比较

Comparative acid tolerances and inhibitor sensitivities of isolated F-ATPases of oral lactic acid bacteria.

作者信息

Sturr M G, Marquis R E

机构信息

Department of Microbiology, University of Rochester, New York 14642.

出版信息

Appl Environ Microbiol. 1992 Jul;58(7):2287-91. doi: 10.1128/aem.58.7.2287-2291.1992.

Abstract

pH activity profiles and inhibitor sensitivities were compared for membrane ATPases isolated from three oral lactic acid bacteria, Lactobacillus casei ATCC 4646, Streptococcus mutans GS-5, and Streptococcus sanguis NCTC 10904, with, respectively, high, moderate, and low levels of acid tolerance. Membranes containing F1F0 ATPases were isolated by means of salt lysis of cells treated with muralytic enzymes. Membrane-free F1F0 complexes were then isolated from membranes by detergent extraction with Triton X-100 or octylglucoside. Finally, F1 complexes free of the proton-conducting F0 sector were obtained by washing membranes with buffers of low ionic strength. The pH activity profiles of the membrane-associated enzymes reflected the general acid tolerances of the organisms from which they were isolated; for example, pH optima were approximately 5.5, 6.0, and 7.0, respectively, for enzymes from L. casei, S. mutans, and S. sanguis. Roughly similar profiles were found for membrane-free F1F0 complexes, which were stabilized by phospholipids against loss of activity during storage. However, profiles for F1 enzymes were distinctly narrower, indicating that association with F0 and possibly other membrane components enhanced tolerance to both acid and alkaline media. All of the enzymes were found to have similar sensitivities to Al-F complexes, but only F1F0 enzymes were highly sensitive to dicyclohexylcarbodiimide. The procedures described for isolation of membrane-free F1F0 forms of the enzymes from oral lactic acid bacteria will be of use in future studies of the characteristics of the enzymes, especially in studies with liposomes.

摘要

比较了从三种口腔乳酸菌中分离出的膜ATP酶的pH活性曲线和抑制剂敏感性,这三种菌分别是干酪乳杆菌ATCC 4646、变形链球菌GS-5和血链球菌NCTC 10904,它们的耐酸性水平分别为高、中、低。通过用溶菌酶处理细胞后进行盐裂解来分离含有F1F0 ATP酶的膜。然后用Triton X-100或辛基葡糖苷进行去污剂萃取,从膜中分离出无膜的F1F0复合物。最后,通过用低离子强度的缓冲液洗涤膜,获得不含质子传导F0区段的F1复合物。膜相关酶的pH活性曲线反映了它们所来源的生物体的总体耐酸性;例如,干酪乳杆菌、变形链球菌和血链球菌的酶的最适pH分别约为5.5、6.0和7.0。对于无膜的F1F0复合物也发现了大致相似的曲线,这些复合物在储存过程中通过磷脂稳定,防止活性丧失。然而,F1酶的曲线明显更窄,表明与F0以及可能的其他膜成分的结合增强了对酸性和碱性介质的耐受性。发现所有酶对铝氟复合物具有相似的敏感性,但只有F1F0酶对二环己基碳二亚胺高度敏感。所描述的从口腔乳酸菌中分离无膜F1F0形式酶的方法将用于未来对这些酶特性的研究,特别是在脂质体研究中。

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