Tang T, Kiang J G, Côté T E, Cox B M
Department of Pharmacology, Uniformed Services University of the Health Sciences, Bethesda, Maryland 20814-4799, USA.
Mol Pharmacol. 1995 Aug;48(2):189-93.
In ND8-47 cells, a neuroblastoma x dorsal root ganglion hybrid cell line, activation of delta-opioid receptors induced an increase in the intracellular free calcium concentration ([Ca2+]i) through dihydropyridine-sensitive calcium channels. This effect was mediated by pertussis toxin-sensitive G proteins. The G protein alpha subunits alpha i2, alpha i3, alpha q, and alpha s were detected using Western blots, whereas alpha o and alpha i1 were not found in ND8-47 cell membranes. To identify the specific G protein alpha subunit(s) responsible for the increase in [Ca2+]i, we treated ND8-47 cells with antisense oligodeoxynucleotides (AS) complementary to the mRNA for each G protein alpha subunit (alpha i2, alpha i3, or alpha s), at a concentration of 10 microM, for up to 6 days and examined their effects on opioid-induced increases in [Ca2+]i and on the levels of G protein alpha subunits. [Ca2+]i was measured in adherent cells using the fluorescent dye fura-2. Treatment of cells with alpha i2-AS (10 microM, for 6 days) resulted in a 73% inhibition of the [D-Ser2,Leu5]-enkephalin-Thr-induced increase in [Ca2+]i. In contrast, pretreatment of cells with alpha i3-AS (10 microM, for 6 days) or alpha s-AS (10 microM, for 6 days) had no effect on the [D-Ser2,Leu5]-enkephalin-Thr-induced responses. Western blots indicated that the levels of alpha i2 were decreased when cells were exposed to alpha i2-AS (10 microM) for 6 days, whereas the levels of alpha i3, alpha s, and alpha q were not affected by this treatment. Treatment of the cells with alpha i3-AS or alpha s-AS for 6 days significantly reduced alpha i3 or alpha s levels, respectively. These results indicate that the opioid-induced increase in [Ca2+]i in ND8-47 cells is mediated by G alpha i2.
在神经母细胞瘤x背根神经节杂交细胞系ND8 - 47细胞中,δ-阿片受体的激活通过二氢吡啶敏感的钙通道诱导细胞内游离钙浓度([Ca2+]i)升高。这种效应由百日咳毒素敏感的G蛋白介导。使用蛋白质免疫印迹法检测到G蛋白α亚基αi2、αi3、αq和αs,而在ND8 - 47细胞膜中未发现αo和αi1。为了确定导致[Ca2+]i升高的特定G蛋白α亚基,我们用与每个G蛋白α亚基(αi2、αi3或αs)的mRNA互补的反义寡脱氧核苷酸(AS)以10微摩尔/升的浓度处理ND8 - 47细胞长达6天,并检测它们对阿片类药物诱导的[Ca2+]i升高以及G蛋白α亚基水平的影响。使用荧光染料fura - 2在贴壁细胞中测量[Ca2+]i。用αi2 - AS(10微摩尔/升,处理6天)处理细胞导致[D - Ser2,Leu5] - 脑啡肽 - Thr诱导的[Ca2+]i升高受到73%的抑制。相比之下,用αi3 - AS(10微摩尔/升,处理6天)或αs - AS(10微摩尔/升,处理6天)预处理细胞对[D - Ser2,Leu5] - 脑啡肽 - Thr诱导的反应没有影响。蛋白质免疫印迹表明,当细胞暴露于αi2 - AS(10微摩尔/升)6天时,αi2的水平降低,而αi3、αs和αq的水平不受此处理影响。用αi3 - AS或αs - AS处理细胞6天分别显著降低了αi3或αs的水平。这些结果表明,ND8 - 47细胞中阿片类药物诱导的[Ca2+]i升高由Gαi2介导。
