Gehlert Donald R, Gackenheimer Susan L, Shaw Janice L
Neuroscience Discovery Research, Lilly Research Laboratories, A Division of Eli Lilly and Company, Lilly Corporate Center, Mail Code 0510, Indianapolis, IN 46285, USA.
Neuropeptides. 2006 Apr;40(2):95-105. doi: 10.1016/j.npep.2005.11.002. Epub 2006 Jan 3.
The peptide, nociceptin, was discovered as the endogenous ligand for the opioid-like receptor, ORL1. Since its discovery, this peptide has been shown to modulate the perception of pain, modulate feeding and produce behavioral effects in rodent models of mood disorders. Recently, the non-peptide agonist {(1S,3aS)-8-(2,3,3a,4,5,6-hexahydro-1H-phenalen-1-yl)-1-phenyl-1,3,8-triaza-spiro[4,5]decan-4-one} (Ro64-6198) of the ORL1 receptor has been reported in the literature. In the present study, we compared the distribution and potency of Ro64-6198 with nociceptin for their ability to stimulate [(35)S]-GTPgammaS binding to sections of rat brain. In initial studies, Ro64-6198 inhibited (125)I-nociceptin binding to the hORL1 receptors with a K(i) of 1.75 nM compared with 0.20 nM for nociceptin. To assess agonist potency in a whole cell assay, a cell line expressing the hORL1 receptor and G(alpha15) was created and used for calcium mobilization studies. In this assay system, Ro64-6198 increased intracellular calcium with an EC(50) of 52nM compared with 24 nM for nociceptin. Having verified the agonist properties of Ro64-6198, we then assessed the potency and distribution of ORL1 receptor activation in rat brain sections. In dose-response studies, Ro64-6198 increased [(35)S]-GTPgammaS binding to a variety of brain regions with EC(50) values ranging from 84.9 to 2,143 nM depending on the brain regions evaluated. These potencies were similar to that seen for nociceptin, but substantially lower than values established using [(125)I] nociceptin binding to the cloned human ORL1 receptor. In general, the brain distribution of agonist stimulated [(35)S]-GTPgammaS binding was similar when either Ro64-6198 or nociceptin were used. Using these techniques, we have demonstrated, for the first time that Ro64-6198 activates [(35)S]-GTPgammaS binding to rat brain sections and this compound stimulates a similar population of receptors as nociceptin.
肽类物质痛敏肽被发现是阿片样受体ORL1的内源性配体。自其被发现以来,该肽已被证明可调节疼痛感知、调节进食并在情绪障碍的啮齿动物模型中产生行为效应。最近,文献报道了ORL1受体的非肽激动剂{(1S,3aS)-8-(2,3,3a,4,5,6-六氢-1H-菲-1-基)-1-苯基-1,3,8-三氮杂螺[4,5]癸-4-酮}(Ro64-6198)。在本研究中,我们比较了Ro64-6198与痛敏肽在刺激[(35)S]-GTPγS与大鼠脑切片结合能力方面的分布和效力。在初步研究中,Ro64-6198抑制(125)I-痛敏肽与hORL1受体的结合,其抑制常数K(i)为1.75 nM,而痛敏肽的K(i)为0.20 nM。为了在全细胞试验中评估激动剂效力,构建了一种表达hORL1受体和G(α15)的细胞系,并用于钙动员研究。在该试验系统中,Ro64-激活细胞内钙的半数有效浓度EC(50)为52 nM,而痛敏肽为24 nM。在验证了Ro64-激动剂特性后,我们接着评估了ORL1受体在大鼠脑切片中的激活效力和分布。在剂量反应研究中,Ro64-6198增加[(35)S]-GTPγS与多种脑区的结合,其EC(50)值根据所评估的脑区不同,范围在84.9至2143 nM之间。这些效力与痛敏肽相似,但远低于使用[(125)I]痛敏肽与克隆的人ORL1受体结合所确定的值。一般来说,当使用Ro64-6198或痛敏肽时,激动剂刺激的[(35)S]-GTPγS结合的脑分布相似。使用这些技术,我们首次证明Ro64-6198可激活[(35)S]-GTPγS与大鼠脑切片的结合,并且该化合物刺激的受体群体与痛敏肽相似。
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