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肺炎支原体与小鼠腹腔巨噬细胞和L细胞的体外相互作用。

The interaction in vitro of Mycoplasma pulmonis with mouse peritoneal macrophages and L-cells.

作者信息

Jones T C, Hirsch J G

出版信息

J Exp Med. 1971 Feb 1;133(2):231-59. doi: 10.1084/jem.133.2.231.

Abstract

Methods have been devised for establishing infection in vitro of mouse macrophages and fibroblasts with Mycoplasma pulmonis. The mycoplasmas attached to the cells and under appropriate cultural conditions grew into a lawn of microorganisms covering most of the cell surface. The mycoplasmas grew abundantly on fibroblasts cultured in minimal essential medium containing 20% fetal calf serum; supplementation of this medium with heart infusion broth was necessary to obtain similar growth on macrophages. The infection of these cells appeared to be essentially an extracellular process; only rarely were partially degraded mycoplasmas seen with phagocytic vacuoles. The addition to heavily infected macrophage cultures of low concentrations of anti-mycoplasma antibody stimulated rapid, massive phagocytosis of the surface microorganisms. In sharp contrast, the same antiserum had no discernable effect on the mycoplasma-fibroblast relationship. The antibody effect in the macrophage system was apparently a direct opsonic one rather than an indirect result of microbial killing, since the mycoplasmas in macrophage or fibroblast cultures incorporated labelled thymidine into DNA after the addition of antiserum to the medium. The phagocytic event and the subsequent fate of the mycoplasmas were studied in detail after the addition of antibody to the macrophage cultures. Phase-contrast cinemicrophotography revealed membrane ruffles surrounding the surface mycoplasmas and disappearance from view of the organisms; 10-30 min later translucent grapelike clusters were seen in large phagocytic vacuoles. On electronmicroscopic study the surface mycoplasmas were surrounded by pincers-like projections of the macrophage. Numerous mycoplasmas were seen in phagocytic vacuoles; in the early minutes after the addition of antibody the intracellular mycoplasmas appeared normal, but within 2 hr they appeared partially degraded with a central electron-lucent area and electron-opaque deposits at the microbial cell margin. 24 hr after the addition of antiserum, digestion of the mycoplasmas was nearly complete; the cells appeared normal except for large residual bodies composed of amorphous moderately dense material and increased lipid deposits. Degradation of mycoplasmas within macrophages was also studied using infected cultures in which the mycoplasmas, but not the macrophages, had incorporated tritiated thymidine into DNA. The appearance of large amounts of acid-soluble radiolabel after phagocytosis stimulated by antibody confirmed the degradation of the intracellular mycoplasmas.

摘要

已设计出在体外使小鼠巨噬细胞和成纤维细胞感染肺支原体的方法。支原体附着于细胞,在适当的培养条件下生长成覆盖大部分细胞表面的微生物菌苔。支原体在含有20%胎牛血清的最低必需培养基中培养的成纤维细胞上大量生长;向该培养基中添加心浸液肉汤对于在巨噬细胞上获得类似的生长是必要的。这些细胞的感染似乎基本上是一个细胞外过程;仅偶尔可见部分降解的支原体存在于吞噬泡中。向严重感染的巨噬细胞培养物中添加低浓度的抗支原体抗体可刺激对表面微生物的快速、大量吞噬作用。与之形成鲜明对比的是,相同的抗血清对支原体 - 成纤维细胞关系没有明显影响。巨噬细胞系统中的抗体作用显然是一种直接的调理作用,而不是微生物杀伤的间接结果,因为在向培养基中添加抗血清后,巨噬细胞或成纤维细胞培养物中的支原体将标记的胸苷掺入DNA中。在向巨噬细胞培养物中添加抗体后,详细研究了吞噬事件及随后支原体的命运。相差电影显微镜摄影显示围绕表面支原体的膜皱褶以及微生物从视野中消失;10 - 30分钟后,在大的吞噬泡中可见半透明的葡萄状簇。电子显微镜研究显示表面支原体被巨噬细胞的钳状突起包围。在吞噬泡中可见大量支原体;在添加抗体后的最初几分钟内,细胞内支原体看起来正常,但在2小时内它们似乎部分降解,中央有电子透明区,微生物细胞边缘有电子不透明沉积物。添加抗血清24小时后,支原体的消化几乎完成;除了由无定形中度致密物质和增加的脂质沉积物组成的大残余体外,细胞看起来正常。还使用感染的培养物研究了巨噬细胞内支原体的降解,在这些培养物中,支原体而非巨噬细胞已将氚标记的胸苷掺入DNA中。抗体刺激吞噬后大量酸溶性放射性标记物的出现证实了细胞内支原体的降解。

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