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在体内能调节新生叙利亚仓鼠昼夜节律时钟的刺激,在体外可调节视交叉上核中转录因子CREB的磷酸化。

Stimuli which entrain the circadian clock of the neonatal Syrian hamster in vivo regulate the phosphorylation of the transcription factor CREB in the suprachiasmatic nucleus in vitro.

作者信息

McNulty S, Schurov I L, Sloper P J, Hastings M H

机构信息

Department of Anatomy, University of Cambridge, UK.

出版信息

Eur J Neurosci. 1998 Mar;10(3):1063-72. doi: 10.1046/j.1460-9568.1998.00114.x.

DOI:10.1046/j.1460-9568.1998.00114.x
PMID:9753174
Abstract

Photic resetting of the adult mammalian circadian clock in vivo is associated with phosphorylation of the Ser133 residue of the calcium/cyclic AMP response-element binding-protein (CREB) in the retinorecipient region of the suprachiasmatic nucleus (SCN). Western blotting and immunocytochemistry were used to investigate whether agonists known to reset the clock of neonatal hamsters in vivo are also able to influence the phosphorylation of CREB in the suprachiasmatic hypothalamus in vitro. Antisera raised against synthetic CREB peptide sequences were used to differentiate between total CREB and the Ser133 phosphorylated form of CREB (pCREB). Western blot analysis of proteins isolated from suprachiasmatic tissue of 1-day-old Syrian hamsters revealed bands at approximately 45 kDa corresponding to total CREB and pCREB. Treatment of the tissue with a mixture of glutamatergic agonists [N-methyl-D-aspartate (NMDA), amino-methyl proprionic acid (AMPA) and kainate, all at 1 microM], or native glutamate (1 microM) had no effect on the total CREB signal, but increased the pCREB signal, indicative of agonist-stimulated phosphorylation of CREB on Ser133. A similar effect was seen following treatment of the suprachiasmatic blocks with either dopamine (1 microM) or forskolin (1 microM). Simultaneous treatment with melatonin (1 microM) significantly attenuated stimulation by forskolin. The effect of the agonists on nuclear pCREB-immunoreactivity (-ir) was investigated in primary cultures which contained a mixture of cell types characteristic of the suprachiasmatic nuclei in vivo. Basal expression of nuclear total CREB-ir was high, whereas expression of pCREB-ir was low. Treatment with glutamate (1 microM) or dopamine (1 microM) had no effect on total CREB-ir, but increased pCREB-ir in approximately 50 and 30% of cells, respectively, whereas forskolin (1 microM) increased pCREB-ir in almost all cells (> 90%). The effects of all three agonists were rapid (< 15 min), and dose and time dependent. Melatonin reversed the effects of forskolin in mixed cultures, but not in pure astrocyte cultures. Dual-immunocytochemistry (ICC) revealed that glutamate (1 microM) increased nuclear pCREB-ir in cells immunoreactive for microtubule-associated protein II (MAP II-ir), but not other cells, indicating an effect predominantly on neurons. This occurred equally in gamma-amino butyric acid (GABA)-ir and non-GABA-ir neurons. Dopamine (1 microM) was more selective, increasing pCREB-ir only in GABA-ir neurons, whereas forskolin increased pCREB-ir in all cells. The specific stimulation of pCREB-ir in GABA-ir neurons by dopamine was reversed by melatonin, but melatonin had no effect on the increase in pCREB-ir induced in GABA-ir neurons by glutamate. These results demonstrate that agonists known to entrain the circadian clock in vivo modulate phosphorylation of CREB in GABA-ir neurons derived from the neonatal suprachiasmatic nuclei.

摘要

成年哺乳动物体内生物钟的光重置与视交叉上核(SCN)视网膜接受区中钙/环磷酸腺苷反应元件结合蛋白(CREB)的丝氨酸133残基磷酸化有关。采用蛋白质免疫印迹法和免疫细胞化学法研究已知能在体内重置新生仓鼠生物钟的激动剂是否也能在体外影响视交叉上核下丘脑CREB的磷酸化。针对合成的CREB肽序列产生的抗血清用于区分总CREB和丝氨酸133磷酸化形式的CREB(pCREB)。对1日龄叙利亚仓鼠视交叉上组织分离的蛋白质进行的蛋白质免疫印迹分析显示,在约45 kDa处有对应于总CREB和pCREB的条带。用谷氨酸能激动剂混合物[均为1 μM的N-甲基-D-天冬氨酸(NMDA)、氨基甲基丙酸(AMPA)和海人酸]或天然谷氨酸(1 μM)处理该组织对总CREB信号无影响,但增加了pCREB信号,表明激动剂刺激了CREB丝氨酸133位点的磷酸化。用多巴胺(1 μM)或福斯可林(1 μM)处理视交叉上组织块后也观察到类似效果。褪黑素(1 μM)同时处理可显著减弱福斯可林的刺激作用。在含有体内视交叉上核特征性细胞类型混合物的原代培养物中研究了激动剂对核pCREB免疫反应性(-ir)的影响。核总CREB-ir的基础表达较高,而pCREB-ir的表达较低。用谷氨酸(1 μM)或多巴胺(1 μM)处理对总CREB-ir无影响,但分别使约50%和30%的细胞中pCREB-ir增加,而福斯可林(1 μM)使几乎所有细胞(>90%)中的pCREB-ir增加。所有三种激动剂的作用迅速(<15分钟),且具有剂量和时间依赖性。褪黑素可逆转混合培养物中福斯可林的作用,但在纯星形胶质细胞培养物中则不能。双重免疫细胞化学(ICC)显示,谷氨酸(1 μM)使对微管相关蛋白II免疫反应性(MAP II-ir)的细胞中核pCREB-ir增加,但对其他细胞无此作用,表明主要作用于神经元。这在γ-氨基丁酸(GABA)-ir和非GABA-ir神经元中均同样发生。多巴胺(1 μM)更具选择性,仅使GABA-ir神经元中的pCREB-ir增加,而福斯可林使所有细胞中的pCREB-ir增加。多巴胺对GABA-ir神经元中pCREB-ir的特异性刺激作用可被褪黑素逆转,但褪黑素对谷氨酸诱导的GABA-ir神经元中pCREB-ir增加无影响。这些结果表明,已知能在体内调节生物钟的激动剂可调节源自新生视交叉上核的GABA-ir神经元中CREB的磷酸化。

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