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急性和慢性吗啡对细胞外信号调节激酶1/2(ERK1/2)磷酸化的调控——对环磷酸腺苷反应元件结合因子(CREB)依赖性和Ets样蛋白1(Elk-1)依赖性转录作用的影响;基于小干扰RNA的策略

Regulation of ERK1/2 phosphorylation by acute and chronic morphine - implications for the role of cAMP-responsive element binding factor (CREB)-dependent and Ets-like protein-1 (Elk-1)-dependent transcription; small interfering RNA-based strategy.

作者信息

Ligeza Agnieszka, Wawrzczak-Bargiela Agnieszka, Kaminska Dorota, Korostynski Michal, Przewlocki Ryszard

机构信息

Department of Molecular Neuropharmacology, Institute of Pharmacology, Polish Academy of Sciences, Krakow, Poland.

出版信息

FEBS J. 2008 Aug;275(15):3836-49. doi: 10.1111/j.1742-4658.2008.06531.x. Epub 2008 Jul 4.

DOI:10.1111/j.1742-4658.2008.06531.x
PMID:18616461
Abstract

Extracellular signal-regulated kinases (ERKs) have been shown to be activated by opioids and functionally linked to addiction. Morphine-associated changes in ERK activity seem to be the characteristic features of opioid action. In this study, we observed a rapid and severe increase in ERK1/2 activity after a 5 min morphine treatment of HEK-MOR cells (transfected with the rat mu-opioid receptor MOR1) expressing mu-opioid receptor. Cellular adaptations to chronic (72 h) morphine treatment were manifested by a slight and sustained increase in ERK1/2 activity. Withdrawal caused by an opioid receptor antagonist - naloxone - attenuated phosphorylation of ERK1/2. Little information is available on the precise mechanism of ERK activity regulation. Using RNA interference technology, we generated stably transfected cells with silenced expression of cAMP-responsive element binding factor (CREB) and Ets-like protein-1 (Elk-1) transcription factors, which are known targets for activated ERK1/2. In these cells, ERK1/2 activity regulation was altered. Silencing of CREB or Elk-1 significantly increased ERK activation observed after 5 min of morphine stimulation. The initial level of activated ERKs in these cells was also augmented. Moreover, the cellular response to withdrawal signals and chronic opioid treatment was diminished. These differences suggest that both CREB-dependent and Elk-1-dependent transcription contribute to the expression of proteins regulating morphine-induced ERK activity (particular phosphatases, upstream kinases or their activatory proteins).

摘要

细胞外信号调节激酶(ERKs)已被证明可被阿片类药物激活,并在功能上与成瘾相关。ERK活性中与吗啡相关的变化似乎是阿片类药物作用的特征。在本研究中,我们观察到在用吗啡处理表达μ-阿片受体的HEK-MOR细胞(转染大鼠μ-阿片受体MOR1)5分钟后,ERK1/2活性迅速且显著增加。细胞对慢性(72小时)吗啡处理的适应性表现为ERK1/2活性轻微且持续增加。阿片受体拮抗剂纳洛酮引起的戒断减弱了ERK1/2的磷酸化。关于ERK活性调节的确切机制,目前所知甚少。利用RNA干扰技术,我们生成了稳定转染的细胞,其环磷酸腺苷反应元件结合因子(CREB)和Ets样蛋白-1(Elk-1)转录因子的表达被沉默,而这些转录因子是已知的被激活的ERK1/2的作用靶点。在这些细胞中,ERK1/2活性调节发生了改变。沉默CREB或Elk-1显著增加了吗啡刺激5分钟后观察到的ERK激活。这些细胞中激活的ERK的初始水平也有所提高。此外,细胞对戒断信号和慢性阿片类药物处理的反应减弱。这些差异表明,CREB依赖性和Elk-1依赖性转录都有助于调节吗啡诱导的ERK活性的蛋白质(特别是磷酸酶、上游激酶或其激活蛋白)的表达。

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