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Stimulatory Effects of Peroxisome Proliferator-Activated Receptor-γon FcγReceptor-Mediated Phagocytosis by Alveolar Macrophages

机译:过氧化物酶体增殖物激活的受体-γ对肺泡巨噬细胞对Fcγ受体介导的吞噬作用的刺激作用。

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Alveolar macrophages abundantly express PPAR-γ, with both natural and synthetic agonists maintaining the cell in a quiescent state hyporesponsive to antigen stimulation. Conversely, agonists upregulate expression and function of the cell-surface receptor CD36, which mediates phagocytosis of lipids, apoptotic neutrophils, and other unopsonized materials. These effects led us to investigate the actions of PPAR-γagonists on the Fcγreceptor, which mediates phagocytosis of particles opsonized by binding of immunoglobulin G antibodies. We found that troglitazone, rosiglitazone, and 15-deoxy-Δ12,14-prostaglandinJ2increase the ability of alveolar, but not peritoneal, macrophages to carry out phagocytosis mediated by the Fcγreceptor. Receptor expression was not altered but activation of the downstream signaling proteins Syk, ERK-1, and ERK-2 was observed. Although it was previously known that PPAR-γligands stimulate phagocytosis of unopsonized materials, this is the first demonstration that they stimulate phagocytosis of opsonized materials as well.
机译:肺泡巨噬细胞大量表达PPAR-γ,天然和合成激动剂均使细胞保持对抗原刺激反应低的静态。相反,激动剂上调细胞表面受体CD36的表达和功能,该介质介导脂质,凋亡性中性粒细胞和其他未调理物质的吞噬作用。这些作用使我们研究了PPAR-γ激动剂对Fcγ受体的作用,该作用介导了由免疫球蛋白G抗体结合而调理的颗粒的吞噬作用。我们发现曲格列酮,罗格列酮和15-脱氧-Δ12,14-前列腺素J2增强了肺泡巨噬细胞(而非腹膜巨噬细胞)执行由Fcγ受体介导的吞噬作用的能力。受体表达未改变,但观察到下游信号蛋白Syk,ERK-1和ERK-2的激活。尽管先前已知PPAR-γ配体会刺激未调理材料的吞噬作用,但这是它们也刺激调理物的吞噬作用的第一个证明。

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