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布氏锥虫引起的免疫抑制的体外模拟

In vitro simulation of immunosuppression caused by Trypanosoma brucei.

作者信息

Sileghem M, Darji A, De Baetselier P

机构信息

Instituut voor Molekulaire Biologie, Vrije Universiteit Brussel, Belgium.

出版信息

Immunology. 1991 Jun;73(2):246-8.

Abstract

Macrophage populations derived from Trypanosoma brucei-infected mice suppress both interleukin-2 (IL-2) production and IL-2 receptor (IL-2R) expression. A prostaglandin-independent mechanism accounts for the suppression of IL-2R expression, while the suppression of IL-2 is prostaglandin-dependent. A macrophage hybridoma cell line (i.e. 2C11-12) was used to mimic the parasite-induced immunosuppression in vitro. It was found that 2C11-12 cells acquired a suppressive potential in vitro following interaction with opsonized living parasites. T. brucei-pulsed 2C11-12 cells failed to block IL-2 secretion in the presence of indomethacin but still suppressed the IL-2R expression. In contrast, addition of living T. brucei parasites to the cultures caused a complete suppression of IL-2 secretion and IL-2R expression, even in the presence of indomethacin. Hence, the addition of excess living parasites to the cultures could cause a depression which was different from the suppression associated with infection, whereas the addition of parasite-pulsed 2C11-12 cells mimicked the situation occurring during infection. This model system can be adopted as a suitable tool to unravel the mechanisms underlying the suppression of IL-2R expression during T. brucei infections.

摘要

源自感染布氏锥虫小鼠的巨噬细胞群体可抑制白细胞介素-2(IL-2)的产生及IL-2受体(IL-2R)的表达。一种不依赖前列腺素的机制可解释IL-2R表达的抑制,而IL-2的抑制则依赖前列腺素。一种巨噬细胞杂交瘤细胞系(即2C11-12)被用于在体外模拟寄生虫诱导的免疫抑制。研究发现,2C11-12细胞在与调理过的活寄生虫相互作用后在体外获得了抑制潜能。在吲哚美辛存在的情况下,用布氏锥虫刺激的2C11-12细胞无法阻断IL-2的分泌,但仍可抑制IL-2R的表达。相反,向培养物中添加活的布氏锥虫寄生虫会导致IL-2分泌和IL-2R表达完全被抑制,即使在吲哚美辛存在的情况下也是如此。因此,向培养物中添加过量的活寄生虫会导致一种不同于与感染相关的抑制作用的抑制,而添加经寄生虫刺激的2C11-12细胞则模拟了感染期间发生的情况。该模型系统可作为一种合适的工具,用于阐明布氏锥虫感染期间IL-2R表达受到抑制的潜在机制。

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Macrophage activation in murine African trypanosomiasis.
Infect Immun. 1983 Mar;39(3):1080-6. doi: 10.1128/iai.39.3.1080-1086.1983.
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Methods Enzymol. 1986;133:507-30. doi: 10.1016/0076-6879(86)33087-8.
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Parasite Immunol. 1985 Mar;7(2):95-106. doi: 10.1111/j.1365-3024.1985.tb00062.x.

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