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白细胞介素-4通过下调颗粒酶B来抑制体外产生的适应性调节性CD4 T细胞的细胞毒性潜能。

Interleukin-4 suppresses the cytotoxic potential of in vitro generated, adaptive regulatory CD4 T cells by down-regulation of granzyme B.

作者信息

Bratke Kai, Goettsching Hilke, Kuepper Michael, Geyer Simone, Luttmann Werner, Virchow J Christian

机构信息

Department of Pneumology, University of Rostock, Rostock, Germany.

出版信息

Immunology. 2009 Jul;127(3):338-44. doi: 10.1111/j.1365-2567.2008.02993.x. Epub 2008 Dec 23.

Abstract

Regulatory CD4+ T cells (Tregs) control immune responses using secretion of anti-inflammatory cytokines and/or cytotoxic mechanisms and play a central role in the outcomes of several immune pathologies. Previous studies suggest an impaired function of Tregs in allergy, especially during allergen seasons, but the underlying mechanism is not known. Therefore, we analysed the impact of the T helper type 2 cytokine interleukin (IL)-4 on in vitro generated adaptive Tregs (aTregs), which have been reported to use the granzyme B (GrB)/perforin pathway to kill autologous immune cells. aTregs were generated by co-ligation of CD3 and CD46 on CD4+ T lymphocytes and granzyme expression was analysed using flow cytometry. To quantify GrB and perforin expression as well as IL-10 secretion in response to IL-4, specific enzyme-linked immunosorbent assays were performed in cell lysates and/or culture supernatants. Using a flow cytometry-based cytotoxicity assay the impact of IL-4 on the cytotoxic potential of aTregs was investigated. While IL-4 did not affect IL-10 secretion and perforin expression in aTregs, a significant suppression of GrB synthesis was detected in the presence of IL-4. In addition, IL-4-mediated suppression of GrB led to impaired cytotoxicity of aTregs against K562 target cells. In conclusion, our data suggest that IL-4 might play a role in impaired aTreg function in allergy.

摘要

调节性CD4+ T细胞(Tregs)通过分泌抗炎细胞因子和/或细胞毒性机制来控制免疫反应,并在多种免疫病理结果中发挥核心作用。先前的研究表明,Tregs在过敏中功能受损,尤其是在过敏原季节,但潜在机制尚不清楚。因此,我们分析了2型辅助性T细胞细胞因子白细胞介素(IL)-4对体外产生的适应性Tregs(aTregs)的影响,据报道,aTregs利用颗粒酶B(GrB)/穿孔素途径杀死自体免疫细胞。通过在CD4+ T淋巴细胞上共同连接CD3和CD46来产生aTregs,并使用流式细胞术分析颗粒酶表达。为了量化GrB和穿孔素表达以及对IL-4的反应中IL-10的分泌,在细胞裂解物和/或培养上清液中进行了特异性酶联免疫吸附测定。使用基于流式细胞术的细胞毒性测定法研究了IL-4对aTregs细胞毒性潜力的影响。虽然IL-4不影响aTregs中IL-10的分泌和穿孔素的表达,但在存在IL-4的情况下检测到GrB合成受到显著抑制。此外,IL-4介导的GrB抑制导致aTregs对K562靶细胞的细胞毒性受损。总之,我们的数据表明IL-4可能在过敏中aTreg功能受损中起作用。

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