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用一种新的细胞化学方法对人多形核白细胞表面NADH氧化酶进行定位。

Localization of NADH oxidase on the surface of human polymorphonuclear leukocytes by a new cytochemical method.

作者信息

Briggs R T, Drath D B, Karnovsky M L, Karnovsky M J

出版信息

J Cell Biol. 1975 Dec;67(3):566-86. doi: 10.1083/jcb.67.3.566.

Abstract

The ultrastructural localization of NADH oxidase, a possible enzyme in the increased oxidative activity of polymorphonuclear leukocytes (PMN) during phagocytosis, was studied. A new cytochemical technique for the localization of H2O2, a product of NADH oxidase activity, was developed. Cerous ions, in the presence of peroxide, form an electron-dense precipitate. Resting and phagocytically stimulated PMN were exposed to cerous ions at pH 7.5 to demonstrate sites of NADH-dependent, cyanide-insensitive H2O2 production. Resting PMN exhibites slight activity on the plasma membrane; phagocytizing PMN had extensive deposits of reaction product localized within the phagosome and on the plasma membrane. Peroxide involvement was demonstrated by the inhibitory effect of catalase on cerium precipitation; the surface localization of the enzyme responsible was confirmed by using nonpenetrating inhibitors of enzymatic activity. A correlative study was performed with an NADH-dependent, tetrazolium-reduction system. As with cerium, formazan deposition on the surface of the cell was NADH dependent, cyanide insensitive, and stimulated by phagocytosis. Superoxide dismutase did not inhibit tetrazolium reduction, as observed cytochemically, indicating direct enzymatic dye reduction without superoxide interposition. These findings, combined with oxygen consumption studies on resting and stimulated PMN in the presence or absence of NADH, indicate that NADH oxidase is a surface enzyme in human PMN. It is internalized during phagocytosis and retains its peroxide-generating capacity within the phagocytic vacuole.

摘要

研究了NADH氧化酶的超微结构定位,该酶可能是吞噬作用期间多形核白细胞(PMN)氧化活性增加的一种酶。开发了一种用于定位NADH氧化酶活性产物H2O2的新细胞化学技术。在过氧化物存在下,铈离子形成电子致密沉淀。将静息和吞噬刺激的PMN在pH 7.5下暴露于铈离子,以证明NADH依赖性、氰化物不敏感的H2O2产生位点。静息的PMN在质膜上表现出轻微活性;吞噬的PMN在吞噬体和质膜内有大量反应产物沉积。过氧化氢的参与通过过氧化氢酶对铈沉淀的抑制作用得以证明;通过使用酶活性的非穿透性抑制剂证实了负责该酶的表面定位。使用NADH依赖性四唑还原系统进行了相关研究。与铈一样,细胞表面的甲臜沉积依赖于NADH,对氰化物不敏感,并受到吞噬作用的刺激。如细胞化学观察到的,超氧化物歧化酶不抑制四唑还原,表明没有超氧化物介入的直接酶促染料还原。这些发现,结合在有无NADH情况下对静息和刺激的PMN的耗氧研究,表明NADH氧化酶是人类PMN中的一种表面酶。它在吞噬作用期间被内化,并在吞噬泡内保留其产生过氧化物的能力。

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