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A Highlights from MBoC Selection: Differential mast cell outcomes are sensitive to FcεRI-Syk binding kinetics

机译:MBoC选择的亮点:肥大细胞分化结果对FcεRI-Syk结合动力学敏感

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摘要

Cross-linking of immunoglobulin E–bound FcεRI triggers multiple cellular responses, including degranulation and cytokine production. Signaling is dependent on recruitment of Syk via docking of its dual SH2 domains to phosphorylated tyrosines within the FcεRI immunoreceptor tyrosine-based activation motifs. Using single-molecule imaging in live cells, we directly visualized and quantified the binding of individual mNeonGreen-tagged Syk molecules as they associated with the plasma membrane after FcεRI activation. We found that Syk colocalizes transiently to FcεRI and that Syk-FcεRI binding dynamics are independent of receptor aggregate size. Substitution of glutamic acid for tyrosine between the Syk SH2 domains (Syk-Y130E) led to an increased Syk-FcεRI off-rate, loss of site-specific Syk autophosphorylation, and impaired downstream signaling. Genome edited cells expressing only Syk-Y130E were deficient in antigen-stimulated calcium release, degranulation, and production of some cytokines (TNF-a, IL-3) but not others (MCP-1, IL-4). We propose that kinetic discrimination along the FcεRI signaling pathway occurs at the level of Syk-FcεRI interactions, with key outcomes dependent upon sufficiently long-lived Syk binding events.
机译:免疫球蛋白E结合的FcεRI的交联触发多种细胞反应,包括脱粒和细胞因子产生。信号传导依赖于Syk的双重SH2结构域与基于FcεRI免疫受体酪氨酸的激活基序内的磷酸化酪氨酸对接。使用活细胞中的单分子成像,我们直接可视化并量化了FcεRI激活后与细胞膜相关的单个mNeonGreen标记Syk分子的结合。我们发现Syk瞬时共定位到FcεRI,并且Syk-FcεRI结合动力学独立于受体聚集体大小。在Syk SH2结构域(Syk-Y130E)之间用谷氨酸替代酪氨酸导致Syk-FcεRI的解离速率增加,位点特异性Syk自磷酸化损失和下游信号传导受损。仅表达Syk-Y130E的基因组编辑细胞在抗原刺激的钙释放,脱粒和某些细胞因子(TNF-α,IL-3)的产生方面缺乏,而其他细胞因子(MCP-1,IL-4)则缺乏。我们建议沿着FcεRI信号通路的动力学区分发生在Syk-FcεRI相互作用的水平,其关键结果取决于足够长寿的Syk结合事件。

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