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Mutation of Putative GRK Phosphorylation Sites in the Cannabinoid Receptor 1 (CB1R) Confers Resistance to Cannabinoid Tolerance and Hypersensitivity to Cannabinoids in Mice

机译：大麻素受体1（CB1R）中的假定的GRK磷酸化位点的突变赋予小鼠对大麻素耐受性和对大麻素超敏反应的抗性

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For many G-protein-coupled receptors (GPCRs), including cannabinoid receptor 1 (CB1R), desensitization has been proposed as a principal mechanism driving initial tolerance to agonists. GPCR desensitization typically requires phosphorylation by a G-protein-coupled receptor kinase (GRK) and interaction of the phosphorylated receptor with an arrestin. In simple model systems, CB1R is desensitized by GRK phosphorylation at two serine residues (S426 and S430). However, the role of these serine residues in tolerance and dependence for cannabinoids in vivo was unclear. Therefore, we generated mice where S426 and S430 were mutated to nonphosphorylatable alanines (S426A/S430A). S426A/S430A mutant mice were more sensitive to acutely administered delta-9-tetrahydrocannabinol (Δ⁹-THC), have delayed tolerance to Δ⁹-THC, and showed increased dependence for Δ⁹-THC. S426A/S430A mutants also showed increased responses to elevated levels of endogenous cannabinoids. CB1R desensitization in the periaqueductal gray and spinal cord following 7 d of treatment with Δ⁹-THC was absent in S426A/S430A mutants. Δ⁹-THC-induced downregulation of CB1R in the spinal cord was also absent in S426A/S430A mutants. Cultured autaptic hippocampal neurons from S426A/S430A mice showed enhanced endocannabinoid-mediated depolarization-induced suppression of excitation (DSE) and reduced agonist-mediated desensitization of DSE. These results indicate that S426 and S430 play major roles in the acute response to, tolerance to, and dependence on cannabinoids. Additionally, S426A/S430A mice are a novel model for studying pathophysiological processes thought to involve excessive endocannabinoid signaling such as drug addiction and metabolic disease. These mice also validate the approach of mutating GRK phosphorylation sites involved in desensitization as a general means to confer exaggerated signaling to GPCRs in vivo.

机译：对于许多G蛋白偶联受体（GPCR），包括大麻素受体1（CB1R），已提出脱敏作用是驱动对激动剂产生初始耐受的主要机制。 GPCR脱敏通常需要通过G蛋白偶联受体激酶（GRK）进行磷酸化，以及磷酸化受体与抑制蛋白的相互作用。在简单模型系统中，CB1R在两个丝氨酸残基处被GRK磷酸化脱敏（S426和S430）。然而，这些丝氨酸残基在体内对大麻素的耐受性和依赖性中的作用尚不清楚。因此，我们生成了将S426和S430突变为不可磷酸化的丙氨酸（S426A / S430A）的小鼠。 S426A / S430A突变小鼠对急性施用的delta-9-四氢大麻酚（Δ^{9 -THC）敏感，对Δ^{9 -THC的耐受性有所延迟，并显示出增加的依赖性对于Δ^{9 -THC。 S426A / S430A突变体还显示出对内源性大麻素水平升高的响应增加。在S426A / S430A突变体中，用Δ^{9 -THC处理7天后，导水管周围灰色和脊髓没有CB1R脱敏。 S426A / S430A突变体中也没有Δ^{9 -THC诱导的脊髓CB1R下调。从S426A / S430A小鼠培养的自闭性海马神经元显示出增强的内源性大麻素介导的去极化诱导的兴奋抑制（DSE）和减少的激动剂介导的DSE脱敏。这些结果表明，S426和S430在对大麻素的急性反应，耐受性和依赖性中起主要作用。另外，S426A / S430A小鼠是用于研究病理生理过程的新型模型，这些过程被认为涉及过多的内源性大麻素信号传导，例如药物成瘾和代谢性疾病。这些小鼠还验证了脱敏所涉及的突变GRK磷酸化位点的方法，作为将夸大的信号传递给体内GPCR的一般手段。}}}}}

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期刊名称 The Journal of Neuroscience
作者
Daniel J. Morgan; Brian J. Davis; Chris S. Kearn; David Marcus; Alex J. Cook; Jim Wager-Miller; Alex Straiker; Michael H. Myoga; Jeffrey Karduck; Emma Leishman; Laura J. Sim-Selley; Traci A. Czyzyk; Heather B. Bradshaw; Dana E. Selley; Ken Mackie;
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年(卷),期 2014(34),15
年度 2014
页码 5152–5163
总页数 12
原文格式 PDF
正文语种
中图分类神经科学;
关键词
cannabinoid CB1 desensitization GPCR THC tolerance;

机译：大麻素;CB1;脱敏;GPCR;THC;耐受性;

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专利

1. Mutation of putative GRK phosphorylation sites in the cannabinoid receptor 1 (CB1R) confers resistance to cannabinoid tolerance and hypersensitivity to cannabinoids in mice [J] . MorganD.J., DavisB.J., KearnC.S., The Journal of Neuroscience: The Official Journal of the Society for Neuroscience . 2014,第15期

机译：大麻素受体1（CB1R）中假定的GRK磷酸化位点的突变赋予小鼠对大麻素耐受性的抗性和对大麻素的超敏性
2. The effects of beta-arrestin1 deletion on acute cannabinoid activity, brain cannabinoid receptors and tolerance to cannabinoids in mice [J] . Breivogel Chris S., Vaghela Manan S. Journal of receptor and signal transduction research . 2015,第1a6期

机译：β-arrestin1缺失对小鼠急性大麻素活性，脑大麻素受体和对大麻素耐受性的影响
3. Pharmacological properties of cannabinoid receptors in the avian brain: similarity of rat and chicken cannabinoid1 receptor recognition sites and expression of cannabinoid2 receptor-like immunoreactivity in the embryonic chick brain. [J] . Fowler CJ, Nilsson O, Andersson M, Pharmacology and Toxicology: An International Journal . 2001,第4期

机译：禽脑中大麻素受体的药理特性：大鼠和鸡的大麻素1受体识别位点的相似性以及胚胎鸡脑中大麻素2受体样免疫反应性的表达。
4. Expression and functions of μ-opioid receptors and cannabinoid receptors type 1 in T lymphocytes [C] . Jürgen Kraus International Society for Neuroimmunomodulation . 2012

机译：μ-ApiOID受体和大麻素受体1型在T淋巴细胞中的表达和功能
5. Interactions of cannabinoids with other drugs of abuse: Insights from cannabinoid CB1 receptor knockout mice [D] . Rice, Onarae Vashun. 2003

机译：大麻素与其他滥用药物的相互作用：大麻素CB1受体敲除小鼠的见解
6. Stratification of Cannabinoid 1 Receptor (CB1R) Agonist Efficacy: Manipulation of CB1R Density through Use of Transgenic Mice Reveals Congruence between In Vivo and In Vitro Assays [O] . T. W. Grim, A. J. Morales, M. M. Gonek, -1

机译：大麻素1受体（CB1R）激动剂功效的分层：通过使用转基因小鼠对CB1R密度的操纵揭示了体内和体外试验之间的一致性
7. Mutation of Putative GRK Phosphorylation Sites in the Cannabinoid Receptor 1 (CB1R) Confers Resistance to Cannabinoid Tolerance and Hypersensitivity to Cannabinoids in Mice [O] . D. J. Morgan, B. J. Davis, C. S. Kearn, 2014

机译：大麻素受体1（CB1R）中推定的GRK磷酸化位点的突变赋予小鼠大麻素对大麻素耐受性和超敏反应的抗性

Mutation of Putative GRK Phosphorylation Sites in the Cannabinoid Receptor 1 (CB1R) Confers Resistance to Cannabinoid Tolerance and Hypersensitivity to Cannabinoids in Mice

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