Institute of Molecular Genetics of the Czech Academy of Sciences, Prague, Czechia.
Department of Genetics and Microbiology, Faculty of Sciences, Biocev, Charles University, Prague, Czechia.
Front Immunol. 2018 Feb 26;9:364. doi: 10.3389/fimmu.2018.00364. eCollection 2018.
Recent studies have reported that the crosslinking of regulatory receptors (RRs), such as blood dendritic cell antigen 2 (BDCA-2) (CD303) or ILT7 (CD85g), of plasmacytoid dendritic cells (pDCs) efficiently suppresses the production of type I interferons (IFN-I, α/β/ω) and other cytokines in response to toll-like receptor 7 and 9 (TLR7/9) ligands. The exact mechanism of how this B cell receptor (BCR)-like signaling blocks TLR7/9-mediated IFN-I production is unknown. Here, we stimulated BCR-like signaling by ligation of RRs with BDCA-2 and ILT7 mAbs, hepatitis C virus particles, or BST2 expressing cells. We compared BCR-like signaling in proliferating pDC cell line GEN2.2 and in primary pDCs from healthy donors, and addressed the question of whether pharmacological targeting of BCR-like signaling can antagonize RR-induced pDC inhibition. To this end, we tested the TLR9-mediated production of IFN-I and proinflammatory cytokines in pDCs exposed to a panel of inhibitors of signaling molecules involved in BCR-like, MAPK, NF-ĸB, and calcium signaling pathways. We found that MEK1/2 inhibitors, PD0325901 and U0126 potentiated TLR9-mediated production of IFN-I in GEN2.2 cells. More importantly, MEK1/2 inhibitors significantly increased the TLR9-mediated IFN-I production blocked in both GEN2.2 cells and primary pDCs upon stimulation of BCR-like or phorbol 12-myristate 13-acetate-induced protein kinase C (PKC) signaling. Triggering of BCR-like and PKC signaling in pDCs resulted in an upregulation of the expression and phoshorylation of c-FOS, a downstream gene product of the MEK1/2-ERK pathway. We found that the total level of c-FOS was higher in proliferating GEN2.2 cells than in the resting primary pDCs. The PD0325901-facilitated restoration of the TLR9-mediated IFN-I production correlated with the abrogation of MEK1/2-ERK-c-FOS signaling. These results indicate that the MEK1/2-ERK pathway inhibits TLR9-mediated type I IFN production in pDCs and that pharmacological targeting of MEK1/2-ERK signaling could be a strategy to overcome immunotolerance of pDCs and re-establish their immunogenic activity.
最近的研究报告表明,浆细胞样树突状细胞(pDCs)中调节受体(RRs)的交联,如血树突状细胞抗原 2(BDCA-2)(CD303)或白细胞免疫球蛋白样受体 7(ILT7)(CD85g),可有效抑制对 Toll 样受体 7 和 9(TLR7/9)配体的 I 型干扰素(IFN-I,α/β/ω)和其他细胞因子的产生。这种 B 细胞受体(BCR)样信号如何阻断 TLR7/9 介导的 IFN-I 产生的具体机制尚不清楚。在这里,我们通过用 BDCA-2 和 ILT7 mAb、丙型肝炎病毒颗粒或表达 BST2 的细胞交联 RR 来刺激 BCR 样信号。我们比较了增殖性 pDC 细胞系 GEN2.2 和来自健康供体的原代 pDC 中的 BCR 样信号,并提出了是否可以通过药理学靶向 BCR 样信号来拮抗 RR 诱导的 pDC 抑制的问题。为此,我们测试了暴露于一系列参与 BCR 样、MAPK、NF-ĸB 和钙信号通路的信号分子抑制剂的 pDC 中 TLR9 介导的 IFN-I 和促炎细胞因子的产生。我们发现,MEK1/2 抑制剂 PD0325901 和 U0126 增强了 GEN2.2 细胞中 TLR9 介导的 IFN-I 的产生。更重要的是,MEK1/2 抑制剂显著增加了 GEN2.2 细胞和原代 pDC 中 BCR 样或佛波醇 12-肉豆蔻酸 13-乙酸酯诱导的蛋白激酶 C (PKC)信号刺激后阻断的 TLR9 介导的 IFN-I 产生。BCR 样和 PKC 信号在 pDC 中的触发导致 MEK1/2-ERK 途径下游基因产物 c-FOS 的表达和磷酸化上调。我们发现,增殖的 GEN2.2 细胞中的 c-FOS 总水平高于静止的原代 pDC。PD0325901 促进 TLR9 介导的 IFN-I 产生的恢复与 MEK1/2-ERK-c-FOS 信号的中断相关。这些结果表明,MEK1/2-ERK 途径抑制 pDC 中 TLR9 介导的 I 型 IFN 产生,并且药理学靶向 MEK1/2-ERK 信号可能是克服 pDC 免疫耐受并重建其免疫原性活性的策略。
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