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吞噬作用期间人粒细胞释放过氧化氢。与超氧阴离子形成及过氧化氢细胞分解代谢的关系:对正常细胞和经细胞松弛素B处理的细胞的研究

H2O2 release from human granulocytes during phagocytosis. Relationship to superoxide anion formation and cellular catabolism of H2O2: studies with normal and cytochalasin B-treated cells.

作者信息

Root R K, Metcalf J A

出版信息

J Clin Invest. 1977 Dec;60(6):1266-79. doi: 10.1172/JCI108886.

DOI:10.1172/JCI108886
PMID:199619
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC372483/
Abstract

Normal and cytochalasin B-treated human granulocytes have been studied to determine some of the interrelationships between phagocytosis-induced respiration and superoxide and hydrogen peroxide formation and release into the extracellular medium by intact cells. By using the scopoletin fluorescent assay to continuously monitor extracellular hydrogen peroxide concentrations during contact of cells with opsonized staphylococci, it was demonstrated that the superoxide scavengers ferricytochrome c and nitroblue tetrazolium significantly reduced the amount of H(2)O(2) released with time from normal cells but did not abolish it. This inhibitory effect was reversed by the simultaneous addition of superoxide dismutase (SOD), whereas the addition of SOD alone increased the amount of detectable H(2)O(2) in the medium. The addition of sodium azide markedly inhibited myeloperoxidase-H(2)O(2)-dependent protein iodination and more than doubled H(2)O(2) release, including the residual amount remaining after exposure of the cells to ferricytochrome c, suggesting its origin from an intracellular pool shared by several pathways for H(2)O(2) catabolism. When cells were pretreated with cytochalasin B and opsonized bacteria added, reduced oxygen consumption was observed, but this was in parallel to a reduction in specific binding of organisms to the cells when compared to normal. Under the influence of inhibited phagosome formation by cytochalasin B, the cells released an increased amount of superoxide and peroxide into the extracellular medium relative to oxygen consumption, and all detectable peroxide release could be inhibited by the addition of ferricytochrome c. Decreased H(2)O(2) production in the presence of this compound could not be ascribed to diminished bacterial binding, decreased oxidase activity, or increased H(2)O(2) catabolism and was reversed by the simultaneous addition of SOD. Furthermore, SOD and ferricytochrome c had similar effects on another H(2)O(2)-dependent reaction, protein iodination, in both normal and cytochalasin B cells. When oxygen consumption, O(2.) (-), and H(2)O(2) release were compared in the presence of azide under identical incubation conditions, the molar relationships for normal cells were 1.00:0.34:0.51 and for cytochalasin B-treated cells 1.00:0.99:0.40, respectively. Nonopsonized, or opsonized but disrupted, bacteria did not stimulate any of these metabolic functions. The results indicate that with normal cells approximately 50% of H(2)O(2) released during phagocytosis is derived directly from O(2.) (-) by dismutation, the remainder appearing from an (intra)cellular source shared by azide-inhibitable heme enzymes. With cytochalasin B treatment the evidence is consistent with the derivation of all H(2)O(2) from an O(2.) (-) precursor which is released from the cell surface. Furthermore, when activated by phagocytic particle binding, the neutrophil O(2.) (-) generating system appears to make more of this compound than can be accounted for by dismutation to H(2)O(2). This establishes conditions for the direct participation of both compounds in the microbicidal and cytocidal activity of these cells.

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c55b/372483/349a2446aaee/jcinvest00660-0052-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c55b/372483/349a2446aaee/jcinvest00660-0052-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c55b/372483/349a2446aaee/jcinvest00660-0052-a.jpg
摘要

对正常和用细胞松弛素B处理的人粒细胞进行了研究,以确定吞噬作用诱导的呼吸与超氧化物和过氧化氢形成以及完整细胞释放到细胞外介质之间的一些相互关系。通过使用 scopoletin 荧光测定法在细胞与调理过的葡萄球菌接触期间连续监测细胞外过氧化氢浓度,结果表明超氧化物清除剂高铁细胞色素c和硝基蓝四氮唑显著降低了正常细胞随时间释放的H₂O₂量,但并未将其完全消除。同时添加超氧化物歧化酶(SOD)可逆转这种抑制作用,而单独添加SOD则增加了培养基中可检测到的H₂O₂量。叠氮化钠的添加显著抑制了髓过氧化物酶-H₂O₂依赖性蛋白碘化,并使H₂O₂释放量增加了一倍多,包括细胞暴露于高铁细胞色素c后剩余的量,这表明其来源于几种H₂O₂分解代谢途径共享的细胞内池。当细胞用细胞松弛素B预处理并添加调理过的细菌时,观察到耗氧量降低,但与正常情况相比,这与生物体与细胞的特异性结合减少平行。在细胞松弛素B抑制吞噬体形成的影响下,相对于耗氧量,细胞向细胞外介质释放的超氧化物和过氧化物量增加,并且添加高铁细胞色素c可抑制所有可检测到的过氧化物释放。在这种化合物存在下H₂O₂产生的减少不能归因于细菌结合减少、氧化酶活性降低或H₂O₂分解代谢增加,并且同时添加SOD可逆转这种情况。此外,SOD和高铁细胞色素c对正常细胞和细胞松弛素B处理的细胞中的另一种H₂O₂依赖性反应蛋白碘化具有相似的作用。在相同孵育条件下,在叠氮化钠存在下比较耗氧量、O₂·(-)和H₂O₂释放时,正常细胞的摩尔关系分别为1.00:0.34:0.51,细胞松弛素B处理的细胞为1.00:0.99:0.40。未调理的或调理但已破坏的细菌不会刺激这些代谢功能中的任何一种。结果表明,对于正常细胞,吞噬过程中释放的H₂O₂约50%直接由O₂·(-)通过歧化产生,其余部分来自叠氮化钠可抑制的血红素酶共享的(细胞内)来源。用细胞松弛素B处理后,证据表明所有H₂O₂均来自从细胞表面释放的O₂·(-)前体。此外,当中性粒细胞的O₂·(-)生成系统被吞噬颗粒结合激活时,似乎产生的这种化合物比通过歧化生成H₂O₂所能解释的更多。这为这两种化合物直接参与这些细胞的杀菌和杀细胞活性创造了条件。

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