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牛艾美耳球虫卵囊抗原诱导的抗原特异性淋巴细胞转化

Antigen-specific lymphocyte transformation induced by oocyst antigens of Eimeria bovis.

作者信息

Hughes H P, Thomas K R, Speer C A

机构信息

Veterinary Research Laboratory, Montana State University, Bozeman 59717.

出版信息

Infect Immun. 1988 Jun;56(6):1518-25. doi: 10.1128/iai.56.6.1518-1525.1988.

DOI:10.1128/iai.56.6.1518-1525.1988
PMID:2453467
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC259430/
Abstract

Lymphoproliferative responses against a preparation of Eimeria bovis antigens (EBAg) were measured in E. bovis-immune and naive animals. Optimal lymphocyte responsiveness could be measured after 7 days of culture in the presence of antigen at a cell concentration of 2 X 10(5) cells per well. The specificity of the reaction was confirmed by limiting dilution analysis. Whereas immune peripheral blood mononuclear cells responded to EBAg (f = 1/18,824), naive cells did not (f = 0). The helper function of cells proliferating in response to EBAg was investigated by raising T-cell lines and a clonal population derived from a line. The T-cell line showed an enhanced reactivity to EBAg by limiting dilution analysis (f = 1/256) and was interleukin-2 dependent. Limiting dilution analyses indicated at least two populations of cells: one that was interleukin-2 restricted and antigen dependent and another that was antigen independent. Supernatants from T-cell lines and the clone were analyzed for the production of lymphokines after antigen stimulation. Minimal amounts of interleukin-2 were produced. The T-cell line produced both gamma interferon (IFN-gamma) (750 U) and IFN-alpha (1,250 U), whereas the clone produced IFN-gamma (1,250 U) only. Short-term (4-day) stimulation of immune cells by EBAg induced the production of IFN-gamma (600 U) and a non-IFN macrophage-activating lymphokine. We conclude that this macrophage-activating lymphokine is only produced after short-term culture and that further culture of T cells results in the proliferation of other clones producing other factors (such as IFN).

摘要

在感染牛艾美耳球虫的免疫动物和未感染的动物中,检测了针对牛艾美耳球虫抗原制剂(EBAg)的淋巴细胞增殖反应。在每孔细胞浓度为2×10⁵个细胞、存在抗原的情况下培养7天后,可检测到最佳淋巴细胞反应性。通过有限稀释分析证实了反应的特异性。免疫外周血单个核细胞对EBAg有反应(f = 1/18,824),而未感染动物的细胞则无反应(f = 0)。通过培养T细胞系和从该系衍生的克隆群体,研究了对EBAg增殖的细胞的辅助功能。通过有限稀释分析,T细胞系对EBAg的反应性增强(f = 1/256),且依赖白细胞介素-2。有限稀释分析表明至少有两类细胞群体:一类是受白细胞介素-2限制且依赖抗原的细胞,另一类是不依赖抗原的细胞。对抗原刺激后T细胞系和克隆的上清液进行细胞因子产生分析。产生的白细胞介素-2量极少。T细胞系产生γ干扰素(IFN-γ)(750 U)和IFN-α(1,250 U),而克隆仅产生IFN-γ(1,250 U)。EBAg对免疫细胞进行短期(4天)刺激可诱导产生IFN-γ(600 U)和一种非IFN巨噬细胞激活细胞因子。我们得出结论,这种巨噬细胞激活细胞因子仅在短期培养后产生,T细胞的进一步培养会导致产生其他因子(如IFN)的其他克隆的增殖。

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