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活化巨噬细胞和粒细胞引起的细胞外细胞溶解。II. 过氧化氢作为细胞毒性的介质。

Extracellular cytolysis by activated macrophages and granulocytes. II. Hydrogen peroxide as a mediator of cytotoxicity.

作者信息

Nathan C F, Silverstein S C, Brukner L H, Cohn Z A

出版信息

J Exp Med. 1979 Jan 1;149(1):100-13. doi: 10.1084/jem.149.1.100.

Abstract

When deprived of oxygen, Bacille Calmette-Guérin (BCG)-activated macrophages no longer lysed P388 lymphoma cells. Both H2O2 release and cytotoxicity by BCG-activated macrophages and by granulocytes triggered with phorbol myristate acetate (PMA) were markedly inhibited when the glucose concentration in the medium was reduced to 0.03 mM or less, or if glucose were replaced with galactose. Catalase abolished PMA-triggered cytotoxicity by both types of effector cells, whereas superoxide dismutase had no effect. Ferricytochrome C reduced the cytotoxicity of BCG-activated macrophages, an effect which was largely reversed by superoxide dismutase. 10 drugs, thought to quench singlet oxygen and/or scavenge hydroxyl radical, did not affect cytotoxicity in this system. Neither azide nor cyanide reduced cytolysis, but there was marked inhibition by lactoperoxidase and iodide. This suggested that cytotoxicity was not dependent upon myeloperoxidase, and that lactoperoxidase may have diverted H2O2 from the oxidation of target cells to oxidation of substances in serum. Mouse erythrocytes, although sensitive targets, interfered with the cytolysis of lymphoma cells, probably by competition for H2O2. Starch particles with covalently bound glucose oxidase resembled macrophages in their spatial relation to the target cells and in the flux of H2O2 they generated from their surface, but were not expected to produce any other potentially toxic products. Such particles lysed lymphoma cells, and the lysis was prevented by catalase. Neither arginase nor thymidine appeared to be involved in cytolysis by BCG-activated macrophages under the conditions used. These findings demonstrated that release of H2O2 was both necessary and sufficient for cytolysis by BCG-activated macrophages and by granulocytes when pharmacologically triggered.

摘要

当缺氧时,卡介苗(BCG)激活的巨噬细胞不再裂解P388淋巴瘤细胞。当培养基中的葡萄糖浓度降至0.03 mM或更低,或者用半乳糖替代葡萄糖时,BCG激活的巨噬细胞以及由佛波酯(PMA)触发的粒细胞释放H2O2和产生细胞毒性的能力均受到显著抑制。过氧化氢酶消除了两种效应细胞由PMA触发的细胞毒性,而超氧化物歧化酶则没有作用。高铁细胞色素C降低了BCG激活的巨噬细胞的细胞毒性,超氧化物歧化酶在很大程度上逆转了这一效应。10种被认为可淬灭单线态氧和/或清除羟基自由基的药物,在该系统中不影响细胞毒性。叠氮化物和氰化物均未降低细胞溶解作用,但乳过氧化物酶和碘化物有显著抑制作用。这表明细胞毒性不依赖于髓过氧化物酶,乳过氧化物酶可能将H2O2从靶细胞的氧化转移到血清中物质的氧化。小鼠红细胞虽然是敏感靶标,但可能通过竞争H2O2干扰淋巴瘤细胞的细胞溶解。共价结合葡萄糖氧化酶的淀粉颗粒在与靶细胞的空间关系以及从其表面产生H2O2的通量方面类似于巨噬细胞,但预计不会产生任何其他潜在有毒产物。此类颗粒可裂解淋巴瘤细胞,而过氧化氢酶可阻止这种裂解。在所使用的条件下,精氨酸酶和胸苷似乎均未参与BCG激活的巨噬细胞的细胞溶解过程。这些发现表明,当通过药理学触发时,H2O2的释放对于BCG激活的巨噬细胞和粒细胞的细胞溶解既是必要的也是充分的。

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