Department of Drug Design and Pharmacology, Faculty of Health and Medical Sciences, University of Copenhagen, Copenhagen, Denmark.
Department of Drug Design and Pharmacology, Faculty of Health and Medical Sciences, University of Copenhagen, Copenhagen, Denmark
Mol Pharmacol. 2019 Oct;96(4):463-474. doi: 10.1124/mol.119.116772. Epub 2019 Aug 9.
G protein-coupled receptor (GPCR) internalization is crucial for the termination of GPCR activity, and in some cases is associated with G protein-independent signaling and endosomal receptor signaling. To date, internalization has been studied in great detail for class A GPCRs; whereas it is not well established to what extent the observations can be generalized to class C GPCRs, including the extracellular calcium-sensing receptor (CaSR). The CaSR is a prototypical class C GPCR that maintains stable blood calcium (Ca) levels by sensing minute changes in extracellular free Ca It is thus necessary that the activity of the CaSR is tightly regulated, even while continuously being exposed to its endogenous agonist. Previous studies have used overexpression of intracellular proteins involved in GPCR trafficking, pathway inhibitors, and cell-surface expression or functional desensitization as indirect measures to investigate CaSR internalization. However, there is no general consensus on the processes involved, and the mechanism of CaSR internalization remains poorly understood. The current study provides new insights into the internalization mechanism of the CaSR. We have used a state-of-the-art time-resolved fluorescence resonance energy transfer-based internalization assay to directly measure CaSR internalization in real-time. We demonstrate that the CaSR displays both constitutive and concentration-dependent Ca-mediated internalization. For the first time, we conclusively show that CaSR internalization is sensitive to immediate positive and negative modulation by the CaSR-specific allosteric modulators -(3-[2-chlorophenyl]propyl)-()--methyl-3-methoxybenzylamine (NPS R-568) and 2-chloro-6-[(2)-2-hydroxy-3-[(2-methyl-1-naphthalen-2-ylpropan-2-yl)amino]propoxy]benzonitrile (NPS 2143), respectively. In addition, we provide compelling evidence that CaSR internalization is -arrestin-dependent while interestingly being largely independent of G and G protein signaling. SIGNIFICANCE STATEMENT: A novel highly efficient cell-based real-time internalization assay to show that calcium-sensing receptor (CaSR) internalization is β-arrestin-dependent and sensitive to modulation by allosteric ligands.
G 蛋白偶联受体 (GPCR) 的内化对于 GPCR 活性的终止至关重要,在某些情况下,它与 G 蛋白非依赖性信号转导和内体受体信号转导有关。迄今为止,对于 A 类 GPCR 的内化已经进行了详细的研究;然而,对于这一观察结果在何种程度上可以推广到 C 类 GPCR,包括细胞外钙敏感受体 (CaSR),还没有得到很好的确定。CaSR 是一种典型的 C 类 GPCR,通过感知细胞外游离 Ca 的微小变化来维持稳定的血液 Ca 水平。因此,CaSR 的活性必须受到严格调节,即使它一直暴露于内源性激动剂中。先前的研究使用涉及 GPCR 运输的细胞内蛋白的过表达、途径抑制剂以及细胞表面表达或功能脱敏作为间接措施来研究 CaSR 的内化。然而,对于所涉及的过程,尚未达成普遍共识,并且 CaSR 内化的机制仍知之甚少。本研究为 CaSR 的内化机制提供了新的见解。我们使用了一种基于时间分辨荧光共振能量转移的最新内化测定法,直接实时测量 CaSR 的内化。我们证明 CaSR 显示组成型和浓度依赖性的 Ca 介导的内化。我们首次明确表明,CaSR 内化对 CaSR 特异性变构调节剂 -(3-[2-氯苯基]丙基)-()--甲基-3-甲氧基苯甲胺 (NPS R-568) 和 2-氯-6-[(2)-2-羟基-3-[(2-甲基-1-萘基-2-基)丙基]-2-氨基]苯并腈 (NPS 2143) 的即刻正、负调节敏感。此外,我们提供了令人信服的证据表明,CaSR 内化是 β-arrestin 依赖性的,而有趣的是,它在很大程度上独立于 G 和 G 蛋白信号转导。意义陈述:一种新的高效细胞内实时内化测定法,用于显示钙敏感受体 (CaSR) 的内化是β-arrestin 依赖性的,并且对变构配体的调节敏感。
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