Simmons S R, Karnovsky M L
J Exp Med. 1973 Jul 1;138(1):44-63. doi: 10.1084/jem.138.1.44.
A rapid method that employs monolayers of different phagocytic cells, primarily from guinea pigs and mice, has allowed a kinetic determination of (a) ingestion by these cells of labeled particles, (b) fixation of (131)I and (c) microbicidal activity in the cells after periods as short as 5' of exposure of bacteria to phagocytes. Phagocytes so examined included polymorphonuclear leukocytes (PMN) elicited into the peritoneal cavity, elicited peritoneal mononuclear cells (monocytes) (MN), and peritoneal macrophages (MAC) obtained simply by lavage. Circulating PMN from normal human subjects and from children afflicted with chronic granulomatous disease were also studied. The potential for generation of H(2)O(2) (a key component of the iodinating system) of all the normal cells studied, gauged by their content of cyanide-insensitive NADH oxidase, seemed comparable. Peroxidase levels varied widely, and were highest in PMN and almost undetectable in MAC. Catalase was at negligible levels in all the cell types obtained from mice. The fixation of (131)I by phagocytes ingesting (14)C-labeled dead tubercle bacilli appeared to be primarily a function of the cellular peroxidase content. Thus, mouse macrophages, with virtually no peroxidase, displayed no fixation of iodide. PMN proved far more able to fix (131)I during phagocytosis than did MN. In experiments comparing PMN from normal human subjects and from children with chronic granulomatous disease (CGD), a sex-linked condition characterized by a deficiency of H(2)O(2) production during phagocytosis and low microbicidal activity, the iodination ratio of CGD cells was dramatically less than that of normal PMN (by about two orders of magnitude). Capacity for iodination was correlated with bactericidal activity toward E. coli. At low bacterial loads (ca. 5:1), phagocytes killed efficiently, and little discrepancy in ability among cell types was apparent. Under the stress of higher loads of (14)C-labeled E. coli (ca. 100:1), differences in bactericidal activity were exaggerated, and a substantial disparity between MN and PMN was observed in favor of the latter. The hierarchy for killing efficiencies therefore agreed with that for iodination, with one notable exception: mouse MAC were consistently competent in their killing activity, more so than MN, even though they virtually lack peroxidase and the ability to iodinate ingested bacteria.
一种快速方法利用了主要来自豚鼠和小鼠的不同吞噬细胞单层,能够动态测定:(a) 这些细胞对标记颗粒的摄取;(b) (131)I 的固定;以及 (c) 在细菌与吞噬细胞接触短短 5 分钟后细胞中的杀菌活性。所检测的吞噬细胞包括腹腔中引出的多形核白细胞 (PMN)、引出的腹腔单核细胞 (单核细胞) (MN) 以及通过灌洗获得的腹腔巨噬细胞 (MAC)。还研究了正常人类受试者和患有慢性肉芽肿病的儿童的循环 PMN。通过其对氰化物不敏感的 NADH 氧化酶含量来衡量,所有研究的正常细胞产生 H(2)O(2)(碘化系统的关键成分)的潜力似乎相当。过氧化物酶水平差异很大,在 PMN 中最高,在 MAC 中几乎检测不到。在从小鼠获得的所有细胞类型中,过氧化氢酶水平可忽略不计。吞噬摄取 (14)C 标记的死结核杆菌的吞噬细胞对 (131)I 的固定似乎主要取决于细胞过氧化物酶含量。因此,几乎没有过氧化物酶的小鼠巨噬细胞不显示碘化物的固定。PMN 在吞噬过程中固定 (131)I 的能力远高于 MN。在比较正常人类受试者和患有慢性肉芽肿病 (CGD) 的儿童的 PMN 的实验中,CGD 是一种性连锁疾病,其特征是吞噬过程中 H(2)O(2) 产生不足且杀菌活性低,CGD 细胞的碘化率明显低于正常 PMN(约低两个数量级)。碘化能力与对大肠杆菌的杀菌活性相关。在低细菌载量(约 5:1)下,吞噬细胞有效杀伤,细胞类型之间的能力差异不明显。在较高载量的 (14)C 标记的大肠杆菌(约 100:1)的压力下,杀菌活性差异被放大,观察到 MN 和 PMN 之间存在明显差异,PMN 更具优势。因此,杀伤效率的等级与碘化等级一致,但有一个显著例外:小鼠 MAC 的杀伤活性始终很强,甚至比 MN 更强,尽管它们几乎缺乏过氧化物酶和碘化摄取细菌的能力。
