RAMP 和 MRAP 辅助蛋白对 CB、CB、GPR18 和 GPR55 大麻素受体的表达和信号转导具有选择性作用。
RAMP and MRAP accessory proteins have selective effects on expression and signalling of the CB, CB, GPR18 and GPR55 cannabinoid receptors.
机构信息
Department of Pharmacology and Clinical Pharmacology, School of Medical Sciences, Faculty of Medical and Health Sciences, University of Auckland, Auckland, New Zealand.
Centre for Brain Research, Faculty of Medical and Health Sciences, University of Auckland, Auckland, New Zealand.
出版信息
Br J Pharmacol. 2024 Jul;181(14):2212-2231. doi: 10.1111/bph.16095. Epub 2023 Jun 1.
BACKGROUND AND PURPOSE
Receptor activity-modifying proteins (RAMPs) and melanocortin receptor accessory proteins (MRAPs) modulate expression and signalling of calcitonin and melanocortin GPCRs. Interactions with other GPCRs have also been reported. The cannabinoid receptors, CB and CB, and two putative cannabinoid receptors, GPR18 and GPR55, exhibit substantial intracellular expression and there are discrepancies in ligand responsiveness between studies. We investigated whether interactions with RAMPs or MRAPs could explain these phenomena.
EXPERIMENTAL APPROACH
Receptors and accessory proteins were co-expressed in HEK-293 cells. Selected receptors were studied at basal expression levels and also with enhanced expression produced by incorporation of a preprolactin signal sequence/peptide (pplss). Cell surface and total expression of receptors and accessory proteins were quantified using immunocytochemistry. Signalling was measured using cAMP (CAMYEL) and G protein dissociation (TRUPATH Gα) biosensors.
KEY RESULTS
MRAP2 enhanced surface and total expression of GPR18. Pplss-GPR18 increased detection of cell surface MRAP2. MRAP1α and MRAP2 reduced GPR55 surface and total expression, correlating with reduced constitutive, but not agonist-induced, signalling. GPR55, pplss-CB and CB reduced detection of MRAP1α at the cell surface. Pplss-CB agonist potency was reduced by MRAP2 in Gα but not cAMP assays, consistent with MRAP2 reducing pplss-CB expression. Some cannabinoid receptors increased RAMP2 or RAMP3 total expression without influencing surface expression.
CONCLUSIONS AND IMPLICATIONS
Mutual influences on expression and/or function for specific accessory protein-receptor pairings raises the strong potential for physiological and disease-relevant consequences. Sequestration and/or hetero-oligomerisation of cannabinoid receptors with accessory proteins is a possible novel mechanism for receptor crosstalk.
LINKED ARTICLES
This article is part of a themed issue Therapeutic Targeting of G Protein-Coupled Receptors: hot topics from the Australasian Society of Clinical and Experimental Pharmacologists and Toxicologists 2021 Virtual Annual Scientific Meeting. To view the other articles in this section visit http://onlinelibrary.wiley.com/doi/10.1111/bph.v181.14/issuetoc.
背景和目的
受体活性修饰蛋白(RAMPs)和黑素皮质素受体辅助蛋白(MRAPs)调节降钙素和黑素皮质素 G 蛋白偶联受体(GPCR)的表达和信号转导。也有报道称它们与其他 GPCR 相互作用。大麻素受体 CB 和 CB 以及两个假定的大麻素受体 GPR18 和 GPR55 表现出大量的细胞内表达,并且不同研究之间在配体反应性方面存在差异。我们研究了这些现象是否与 RAMPs 或 MRAPs 的相互作用有关。
实验方法
将受体和辅助蛋白共表达于 HEK-293 细胞中。使用免疫细胞化学法检测选定受体在基础表达水平以及通过加入前原促乳素信号序列/肽(pplss)增强表达时的细胞表面和总表达。使用 cAMP(CAMYEL)和 G 蛋白解离(TRUPATH Gα)生物传感器测量信号转导。
主要结果
MRAP2 增强了 GPR18 的细胞表面和总表达。pplss-GPR18 增加了细胞表面 MRAP2 的检测。MRAP1α 和 MRAP2 降低了 GPR55 的细胞表面和总表达,与减少组成型但不增加激动剂诱导的信号转导相关。GPR55、pplss-CB 和 CB 减少了细胞表面的 MRAP1α 检测。MRAP2 在 Gα 但不在 cAMP 测定中降低了 pplss-CB 激动剂效力,这与 MRAP2 降低 pplss-CB 表达一致。一些大麻素受体增加了 RAMP2 或 RAMP3 的总表达,而不影响细胞表面表达。
结论和意义
特定辅助蛋白-受体配对之间的相互影响表达和/或功能增加了生理和疾病相关后果的强烈可能性。大麻素受体与辅助蛋白的隔离和/或异源寡聚化可能是受体串扰的一种新机制。
相关文章
本文是澳大利亚临床和实验药理学与毒理学学会 2021 年虚拟年会治疗性靶向 G 蛋白偶联受体热点主题特刊的一部分。要查看该部分中的其他文章,请访问 http://onlinelibrary.wiley.com/doi/10.1111/bph.v181.14/issuetoc.
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