Páldy Eszter, Bereczki Erika, Sántha Miklós, Wenger Tibor, Borsodi Anna, Zimmer Andreas, Benyhe Sándor
Institute of Biochemistry, Biological Research Centre, Hungarian Academy of Sciences, Temesvari krt. 62, H-6726 Szeged, Hungary.
Neurochem Int. 2008 Dec;53(6-8):309-16. doi: 10.1016/j.neuint.2008.08.005. Epub 2008 Aug 29.
Formerly considered as an exclusively peripheral receptor, it is now accepted that CB(2) cannabinoid receptor is also present in limited amounts and distinct locations in the brain of several animal species, including mice. However, the possible roles of CB(2) receptors in the brain need to be clarified. The aim of our work was to study the mu-opioid receptor (MOR) mRNA expression level and functional activity after acute in vivo and in vitro treatments with the endocannabinoid noladin ether (NE) and with the CB(2) receptor antagonist SR144528 in brainstem of mice deficient in either CB(1) or CB(2) receptors. This study is based on our previous observations that noladin ether (NE) produces decrease in the activity of MOR in forebrain and this attenuation can be antagonized by the CB(2) cannabinoid antagonist SR144528, suggesting a CB(2) receptor mediated effect. We used quantitative real-time PCR to examine the changes of MOR mRNA levels, [(35)S]GTPgammaS binding assay to analyze the capability of mu-opioid agonist DAMGO to activate G-proteins and competition binding assays to directly measure the ligand binding to MOR in mice brainstem. After acute NE administration no significant changes were observed on MOR signaling. Nevertheless pretreatment of mice with SR144528 prior to the administration of NE significantly decreased MOR signaling suggesting the involvement of SR144528 in mediating the effect of MOR. mRNA expression of MORs significantly decreased both in CB(1) wild-type and CB(1) knockout mice after a single injection of SR144528 at 0.1mg/kg when compared to the vehicle treated controls. Consequently, MOR-mediated signaling was attenuated after acute in vivo treatment with SR144528 in both CB(1) wild-type and CB(1) knockout mice. In vitro addition of 1microM SR144528 caused a decrease in the maximal stimulation of DAMGO in [(35)S]GTPgammaS binding assays in CB(2) wild-type brainstem membranes whereas no significant changes were observed in CB(2) receptor knockouts. Radioligand binding competition studies showed that the noticed effect of SR144528 on MOR signaling is not mediated through MORs. Our data demonstrate that the SR144528 caused pronounced decrease in the activity of MOR is mediated via CB(2) cannabinoid receptors.
CB(2)大麻素受体以前被认为是一种仅存在于外周的受体,现在人们已经认识到,在包括小鼠在内的几种动物的大脑中,CB(2)受体也以有限的数量存在于不同的位置。然而,CB(2)受体在大脑中的可能作用仍需阐明。我们研究的目的是,在缺乏CB(1)或CB(2)受体的小鼠脑干中,研究内源性大麻素诺拉汀醚(NE)和CB(2)受体拮抗剂SR144528进行急性体内和体外处理后,μ-阿片受体(MOR)的mRNA表达水平和功能活性。本研究基于我们之前的观察结果,即诺拉汀醚(NE)会使前脑MOR的活性降低,且这种减弱可被CB(2)大麻素拮抗剂SR144528拮抗,这表明存在CB(2)受体介导的效应。我们使用定量实时PCR来检测MOR mRNA水平的变化,用[(35)S]GTPγS结合试验分析μ-阿片激动剂DAMGO激活G蛋白的能力,并用竞争结合试验直接测量配体与小鼠脑干中MOR的结合。急性给予NE后,未观察到MOR信号有显著变化。然而,在给予NE之前用SR144528预处理小鼠,显著降低了MOR信号,这表明SR144528参与介导MOR的效应。与给予溶剂对照的小鼠相比,在CB(1)野生型和CB(1)基因敲除小鼠单次注射0.1mg/kg的SR144528后,MOR的mRNA表达均显著降低。因此,在CB(1)野生型和CB(1)基因敲除小鼠中,急性体内给予SR144528后,MOR介导的信号减弱。在体外,加入1μM的SR144528会导致CB(2)野生型脑干膜中[(35)S]GTPγS结合试验中DAMGO的最大刺激作用降低,而在CB(2)受体基因敲除小鼠中未观察到显著变化。放射性配体结合竞争研究表明,SR144528对MOR信号的显著影响不是通过MOR介导的。我们的数据表明,SR144528导致MOR活性显著降低是通过CB(2)大麻素受体介导的。
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