Fundación Ciencia y Tecnología Para el Desarrollo (FUCITED), Santiago, Chile.
Aberdeen Fungal Group, Medical Research Council Centre for Medical Mycology, University of Aberdeen, Aberdeen, United Kingdom.
Front Immunol. 2019 May 31;10:1136. doi: 10.3389/fimmu.2019.01136. eCollection 2019.
Mollusk hemocyanins have biomedical uses as carriers/adjuvants and nonspecific immunostimulants with beneficial clinical outcomes by triggering the production of proinflammatory cytokines in antigen-presenting cells (APCs) and driving immune responses toward type 1 T helper (Th1) polarization. Significant structural features of hemocyanins as a model antigen are their glycosylation patterns. Indeed, hemocyanins have a multivalent nature as highly mannosylated antigens. We have previously shown that hemocyanins are internalized by APCs through receptor-mediated endocytosis with proteins that contain C-type lectin domains, such as mannose receptor (MR). However, the contribution of other innate immune receptors to the proinflammatory signaling pathway triggered by hemocyanins is unknown. Thus, we studied the roles of Dectin-1, Dectin-2, and Toll-like receptor 4 (TLR4) in the hemocyanin activation of murine APCs, both in dendritic cells (DCs) and macrophages, using hemocyanins from KLH), (CCH) and (FLH). The results showed that these hemocyanins bound to chimeric Dectin-1 and Dectin-2 receptors ; which significantly decreased when the glycoproteins were deglycosylated. However, hemocyanin-induced proinflammatory effects in APCs from Dectin-1 knock-out (KO) and Dectin-2 KO mice were independent of both receptors. Moreover, when wild-type APCs were cultured in the presence of hemocyanins, phosphorylation of Syk kinase was not detected. We further showed that KLH and FLH induced ERK1/2 phosphorylation, a key event involved in the TLR signaling pathway. We confirmed a glycan-dependent binding of hemocyanins to chimeric TLR4 . Moreover, DCs from mice deficient for MyD88-adapter-like (Mal), a downstream adapter molecule of TLR4, were partially activated by FLH, suggesting a role of the TLR pathway in hemocyanin recognition to activate APCs. The participation of TLR4 was confirmed through a decrease in IL-12p40 and IL-6 secretion induced by FLH when a TLR4 blocking antibody was used; a reduction was also observed in DCs from C3H/HeJ mice, a mouse strain with a nonfunctional mutation for this receptor. Moreover, IL-6 secretion induced by FLH was abolished in macrophages deficient for TLR4. Our data showed the involvement of TLR4 in the hemocyanin-mediated proinflammatory response in APCs, which could cooperate with MR in innate immune recognition of these glycoproteins.
软体动物血蓝蛋白具有生物医学用途,可作为载体/佐剂和非特异性免疫刺激剂,通过在抗原呈递细胞 (APC) 中触发促炎细胞因子的产生,并促使免疫反应向 1 型辅助性 T 细胞 (Th1) 极化,从而带来有益的临床效果。血蓝蛋白作为模型抗原的重要结构特征是其糖基化模式。事实上,血蓝蛋白作为高度甘露糖化的抗原具有多价性质。我们之前已经表明,APC 通过含有 C 型凝集素结构域的蛋白(如甘露糖受体 (MR))通过受体介导的内吞作用内化血蓝蛋白。然而,其他先天免疫受体对血蓝蛋白引发的促炎信号通路的贡献尚不清楚。因此,我们使用 KLH、CCH 和 FLH 的血蓝蛋白研究了 Dectin-1、Dectin-2 和 Toll 样受体 4 (TLR4) 在 DC 和巨噬细胞中激活小鼠 APC 时的作用。结果表明,这些血蓝蛋白与嵌合 Dectin-1 和 Dectin-2 受体结合;当糖蛋白发生糖基化缺失时,结合显著减少。然而,Dectin-1 和 Dectin-2 KO 小鼠的 APC 中,血蓝蛋白诱导的促炎作用不依赖于这两种受体。此外,当野生型 APC 在血蓝蛋白存在下培养时,未检测到 Syk 激酶的磷酸化。我们进一步表明,KLH 和 FLH 诱导 ERK1/2 磷酸化,这是 TLR 信号通路中的一个关键事件。我们证实了血蓝蛋白与嵌合 TLR4 的糖依赖性结合。此外,MyD88 衔接样 (Mal) 下游衔接分子 TLR4 缺陷的小鼠 DC 被 FLH 部分激活,这表明 TLR 途径在血蓝蛋白识别和激活 APC 中起作用。通过使用 TLR4 阻断抗体,FLH 诱导的 IL-12p40 和 IL-6 分泌减少证实了 TLR4 的参与;在 TLR4 功能缺失的 C3H/HeJ 小鼠中也观察到这种减少,这种受体的这种突变使这种小鼠缺乏功能。此外,缺乏 TLR4 的巨噬细胞中 FLH 诱导的 IL-6 分泌被消除。我们的数据表明 TLR4 参与了 APC 中的血蓝蛋白介导的促炎反应,它可以与 MR 一起在这些糖蛋白的先天免疫识别中发挥作用。
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