Sha Lisa K, Sha Weixiao, Kuchler Laura, Daiber Andreas, Giegerich Annika K, Weigert Andreas, Knape Tilo, Snodgrass Ryan, Schröder Katrin, Brandes Ralf P, Brüne Bernhard, von Knethen Andreas
Institute of Biochemistry I-Pathobiochemistry, Faculty of Medicine, Goethe-University Frankfurt, 60590 Frankfurt am Main, Germany.
Department of Medicine II, University Medical Center, Johannes Gutenberg-University Mainz, 55116 Mainz, Germany.
Free Radic Biol Med. 2015 Jun;83:77-88. doi: 10.1016/j.freeradbiomed.2015.02.004. Epub 2015 Feb 14.
NF-E2-related factor 2 (Nrf2), known to protect against reactive oxygen species, has recently been reported to resolve acute inflammatory responses in activated macrophages. Consequently, disruption of Nrf2 promotes a proinflammatory macrophage phenotype. In the current study, we addressed the impact of this macrophage phenotype on CD8(+) T cell activation by using an antigen-driven coculture model consisting of Nrf2(-/-) and Nrf2(+/+) bone marrow-derived macrophages (BMDMΦ) and transgenic OT-1 CD8(+) T cells. OT-1 CD8(+) T cells encode a T cell receptor that specifically recognizes MHC class I-presented ovalbumin OVA(257-264) peptide, thereby causing a downstream T cell activation. Interestingly, coculture of OVA(257-264)-pulsed Nrf2(-/-) BMDMΦ with transgenic OT-1 CD8(+) T cells attenuated CD8(+) T cell activation, proliferation, and cytotoxic function. Since the provision of low-molecular-weight thiols such as glutathione (GSH) or cysteine (Cys) by macrophages limits antigen-driven CD8(+) T cell activation, we quantified the amounts of intracellular and extracellular GSH and Cys in both cocultures. Indeed, GSH levels were strongly decreased in Nrf2(-/-) cocultures compared to wild-type counterparts. Supplementation of thiols in Nrf2(-/-) cocultures via addition of glutathione ester, N-acetylcysteine, β-mercaptoethanol, or cysteine itself restored T cell proliferation as well as cytotoxicity by increasing intracellular GSH. Mechanistically, we identified two potential Nrf2-regulated genes involved in thiol synthesis in BMDMΦ: the cystine transporter subunit xCT and the modulatory subunit of the GSH-synthesizing enzyme γ-GCS (GCLM). Pharmacological inhibition of γ-GCS-dependent GSH synthesis as well as knockdown of the cystine antiporter xCT in Nrf2(+/+) BMDMΦ mimicked the effect of Nrf2(-/-) BMDMΦ on CD8(+) T cell function. Our findings demonstrate that reduced levels of GCLM as well as xCT in Nrf2(-/-) BMDMΦ limit GSH availability, thereby inhibiting antigen-induced CD8(+) T cell function.
核因子E2相关因子2(Nrf2)已知具有抵御活性氧的作用,最近有报道称其可消除活化巨噬细胞中的急性炎症反应。因此,Nrf2的破坏会促进促炎性巨噬细胞表型的形成。在本研究中,我们通过使用由Nrf2(-/-)和Nrf2(+/+)骨髓来源的巨噬细胞(BMDMΦ)以及转基因OT-1 CD8+ T细胞组成的抗原驱动共培养模型,探讨了这种巨噬细胞表型对CD8+ T细胞活化的影响。OT-1 CD8+ T细胞编码一种特异性识别MHC I类呈递的卵清蛋白OVA(257-264)肽的T细胞受体,从而引发下游的T细胞活化。有趣的是,将OVA(257-264)脉冲处理的Nrf2(-/-)BMDMΦ与转基因OT-1 CD8+ T细胞共培养会减弱CD8+ T细胞的活化、增殖和细胞毒性功能。由于巨噬细胞提供低分子量硫醇(如谷胱甘肽(GSH)或半胱氨酸(Cys))会限制抗原驱动的CD8+ T细胞活化,我们对两种共培养体系中细胞内和细胞外GSH和Cys的含量进行了定量。事实上,与野生型对应物相比,Nrf2(-/-)共培养体系中的GSH水平显著降低。通过添加谷胱甘肽酯、N-乙酰半胱氨酸、β-巯基乙醇或半胱氨酸本身,在Nrf2(-/-)共培养体系中补充硫醇,可通过增加细胞内GSH来恢复T细胞增殖以及细胞毒性。从机制上讲,我们在BMDMΦ中鉴定出两个潜在的Nrf2调节基因,它们参与硫醇合成:胱氨酸转运体亚基xCT和谷胱甘肽合成酶γ-GCS(GCLM)的调节亚基。对Nrf2(+/+)BMDMΦ中γ-GCS依赖性GSH合成进行药理学抑制以及敲低胱氨酸反向转运体xCT,模拟了Nrf2(-/-)BMDMΦ对CD8+ T细胞功能的影响。我们的研究结果表明,Nrf2(-/-)BMDMΦ中GCLM和xCT水平的降低限制了GSH的可用性,从而抑制了抗原诱导的CD8+ T细胞功能。
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