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首页> 外文期刊>Infection and immunity >Inhibition of Migration of Mouse Macrophages by Tuberculin-Sensitive Mouse Lymphocytes and by Mouse Migration Inhibitory Factor
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Inhibition of Migration of Mouse Macrophages by Tuberculin-Sensitive Mouse Lymphocytes and by Mouse Migration Inhibitory Factor

机译:结核菌素敏感的小鼠淋巴细胞和小鼠迁移抑制因子对小鼠巨噬细胞迁移的抑制。

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The guinea pig migration inhibition technique, an accepted in vitro correlate of delayed hypersensitivity, has been adapted to a murine system. Peritoneal exudate cells from CF-1 mice vaccinated with viable cells of the H37Ra strain of Mycobacterium tuberculosis were inhibited in vitro by purified protein derivative (PPD) or whole H37Ra microorganisms. Peritoneal exudate cells from the inbred C57Bl/6 mice immunized with H37Ra cells also were inhibited in vitro by PPD or whole H37Ra microorganisms. Migration inhibitory factor (MIF) was produced by splenic lymphocytes from the H37Ra-immunized C57Bl/6 mice when incubated with either antigen. Intravenous injection of PPD or viable H37Ra organisms into H37Ra mice resulted in MIF production in vitro by splenic lymphocytes without further antigenic stimulation. Peritoneal exudate cells from nonimmunized C57Bl/6 mice and supernatant fluids from cultures of lymphocytes from nonimmunized C57Bl/6 mice were not inhibited in the presence of antigen. The production of MIF by splenic lymphocytes from immunized C57Bl/6 mice depended upon the conditions under which the lymphocytes were cultured, the time of exposure to antigen (3 days), the use of a higher concentration of PPD for stimulation of lymphocytes than that required for guinea pig cells, and also the use of cells from a highly inbred mouse strain.
机译:豚鼠迁移抑制技术是一种公认​​的迟发型超敏反应的体外相关技术,已经适应了鼠类系统。纯化的蛋白衍生物(PPD)或完整的H37Ra微生物体外抑制了接种了结核分枝杆菌H37Ra株活细胞的CF-1小鼠的腹膜分泌液。 PPD或整个H37Ra微生物体外抑制了用H37Ra细胞免疫的近交C57Bl / 6小鼠的腹膜分泌液。当与任一种抗原孵育时,来自H37Ra免疫的C57Bl / 6小鼠的脾淋巴细胞产生迁移抑制因子(MIF)。向H37Ra小鼠静脉内注射PPD或有活力的H37Ra生物体导致脾脏淋巴细胞在体外产生MIF,而没有进一步的抗原刺激。在抗原的存在下,来自未免疫的C57Bl / 6小鼠的腹膜渗出细胞和来自未免疫的C57Bl / 6小鼠的淋巴细胞培养物的上清液不被抑制。来自免疫的C57Bl / 6小鼠的脾淋巴细胞产生MIF的条件取决于培养淋巴细胞的条件,暴露于抗原的时间(3天),使用比所需要的浓度更高的PPD刺激淋巴细胞用于豚鼠细胞,以及使用高度自交系小鼠品系的细胞。

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