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H1 和 H2 组胺受体的交叉脱敏和共内化揭示了组胺信号整合的新见解。

Cross-desensitization and cointernalization of H1 and H2 histamine receptors reveal new insights into histamine signal integration.

机构信息

Laboratorio de Farmacología y Patología Molecular, Instituto de Biología y Medicina Experimental, Buenos Aires, Argentina.

出版信息

Mol Pharmacol. 2013 May;83(5):1087-98. doi: 10.1124/mol.112.083394. Epub 2013 Mar 5.

Abstract

G protein-coupled receptor signaling does not result from sequential activation of a linear pathway of proteins/enzymes, but rather from complex interactions of multiple, branched signaling routes, i.e., signaling networks. In this work we present an exhaustive study of the cross-talk between H1 and H2 histamine receptors (H1R and H2R) in U937 cells and Chinese hamster ovary-transfected cells. By desensitization assays we demonstrated the existence of a crossdesensitization between both receptors independent of protein kinase A or C. H1R-agonist stimulation inhibited cell proliferation and induced apoptosis in U937 cells following treatment of 48 hours. H1R-induced antiproliferative and apoptotic response was inhibited by an H2R agonist suggesting that the cross-talk between both receptors modifies their function. Binding and confocal microscopy studies revealed cointernalization of both receptors upon treatment with the agonists. To evaluate potential heterodimerization of the receptors, sensitized emission fluorescence resonance energy transfer experiments were performed in human embryonic kidney 293T cells using H1R-cyan fluorescent protein and H2R-yellow fluorescent protein. To our knowledge these findings may represent the first demonstration of agonist-induced heterodimerization of the H1R and H2R. In addition, we also show that the inhibition of the internalization process did not prevent receptor crossdesensitization, which was mediated by G protein-coupled receptor kinase 2. Our study provides new insights into the complex signaling network mediated by histamine and further knowledge for the rational use of its ligands.

摘要

G 蛋白偶联受体信号转导并非来自于蛋白质/酶的线性途径的顺序激活,而是来自于多个分支信号通路的复杂相互作用,即信号网络。在这项工作中,我们对 U937 细胞和中国仓鼠卵巢转染细胞中 H1 和 H2 组胺受体(H1R 和 H2R)之间的串扰进行了详尽的研究。通过脱敏实验,我们证明了两种受体之间存在无蛋白激酶 A 或 C 参与的交叉脱敏。H1R 激动剂刺激可抑制 U937 细胞增殖,并在 48 小时后诱导细胞凋亡。H1R 诱导的抗增殖和凋亡反应被 H2R 激动剂抑制,表明两种受体之间的串扰改变了它们的功能。结合和共聚焦显微镜研究表明,两种受体在激动剂处理后发生共内化。为了评估受体潜在的异二聚化,在人胚肾 293T 细胞中使用 H1R-青色荧光蛋白和 H2R-黄色荧光蛋白进行了敏化发射荧光共振能量转移实验。据我们所知,这些发现可能代表了首次证明 H1R 和 H2R 的激动剂诱导的异二聚化。此外,我们还表明,抑制内化过程并不能阻止由 G 蛋白偶联受体激酶 2 介导的受体交叉脱敏。我们的研究为组胺介导的复杂信号网络提供了新的见解,并为其配体的合理使用提供了进一步的知识。

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