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体外暴露于胞壁酰二肽或脂多糖的巨噬细胞中超氧阴离子生成增加。

Increased production of superoxide anion by macrophages exposed in vitro to muramyl dipeptide or lipopolysaccharide.

作者信息

Pabst M J, Johnston R B

出版信息

J Exp Med. 1980 Jan 1;151(1):101-14. doi: 10.1084/jem.151.1.101.

Abstract

After in vitro exposure to lipopolysaccharide (LPS) or muramyl dipeptide (MDP), cultured resident mouse peritoneal macrophages were primed to display enhanced generation of superoxide anion (O2-) in response to stimulation by phorbol myristate acetate (PMA) or opsonized zymosan. Priming with LPS (1 microgram/ml) produced a sevenfold enhancement of PMA-stimulated O2- generation; priming was detected within 30 min and persisted for at least 4 d. Exposure to MDP (1 muM) primed the macrophages to double their O2- release; the response was first observed after 4 h and persisted for at least 3 d. The priming response was not observed with stereoisomers of MDP, which are inactive as adjuvants. LPS and MDP appeared to work directly on the macrophages rather than indirectly by interacting with adherent lymphocytes: (a) Addition of nonadherent cell populations that contained lymphocytes had no effect on the response. (b) The response was normal with cells from nude mice, which lack mature T lymphocytes. (c) Macrophages from C3H/HeJ mice, whose B lymphocytes fail to respond to LPS, were weak in their response to priming LPS; the addition of normal (C3Heb/FeJ) nonadherent cells had no effect on this weak response. (d) The macrophage-like cell line J774.1 also showed enhanced O2--generating capacity after a 4-h exposure to LPS or MDP. The O2--generating capacity of macrophages primed with LPS in vitro was equivalent to that previously observed with cells elicited in vivo by injection of LPS or activated by infection with Bacille Calmette-Guérin. The data suggest that previous exposure to bacterial products could prime macrophages to respond with increased production of toxic oxygen metabolites on contact with invading microorganisms or tumor cells.

摘要

体外暴露于脂多糖(LPS)或胞壁酰二肽(MDP)后,培养的小鼠腹膜常驻巨噬细胞被致敏,以使其在受到佛波酯(PMA)或调理酵母聚糖刺激时,超氧阴离子(O2-)的生成增强。用LPS(1微克/毫升)致敏可使PMA刺激的O2-生成增强7倍;致敏在30分钟内即可检测到,并持续至少4天。暴露于MDP(1微摩尔)可使巨噬细胞的O2-释放量加倍;该反应在4小时后首次观察到,并持续至少3天。MDP的立体异构体作为佐剂无活性,未观察到致敏反应。LPS和MDP似乎直接作用于巨噬细胞,而非通过与黏附淋巴细胞相互作用间接发挥作用:(a)添加含有淋巴细胞的非黏附细胞群体对反应无影响。(b)来自缺乏成熟T淋巴细胞的裸鼠的细胞反应正常。(c)C3H/HeJ小鼠的B淋巴细胞对LPS无反应,其巨噬细胞对LPS致敏的反应较弱;添加正常(C3Heb/FeJ)非黏附细胞对这种弱反应无影响。(d)巨噬细胞样细胞系J774.1在暴露于LPS或MDP 4小时后,也显示出增强的O2-生成能力。体外经LPS致敏的巨噬细胞的O2-生成能力与先前在体内通过注射LPS诱导或经卡介苗感染激活的细胞所观察到的相当。数据表明,先前暴露于细菌产物可使巨噬细胞致敏,使其在接触入侵微生物或肿瘤细胞时,产生更多有毒氧代谢产物。

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