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长期睡眠剥夺对大鼠齿状回长时程增强和脑氧化状态的影响。

The effects of long-term sleep deprivation on the long-term potentiation in the dentate gyrus and brain oxidation status in rats.

机构信息

Physiology Department of Erciyes University Medical School, Talas str, 38039 Kayseri, Turkey.

出版信息

Neurosci Res. 2011 May;70(1):71-7. doi: 10.1016/j.neures.2011.01.008. Epub 2011 Jan 21.

DOI:10.1016/j.neures.2011.01.008
PMID:21256900
Abstract

Some evidence suggests that sleep deprivation might impair synaptic plasticity and produce oxidative stress in the hippocampus. However it is not clear whether impairment of long-term potentiation depends on the oxidative stress evoked by sleep deprivation protocol. In this study we aimed to investigate the effects of a 21-day sleep deprivation period on long-term plasticity taking into account the stressful effect of sleep deprivation. Sleep deprivation was carried out using the multiple platforms method on adult male Wistar rats. Long-term potentiation was studied in the medial perforant pathway-dentate gyrus synapses. Elevated T test was applied, and blood corticosterone levels were measured. Lipid peroxidation products in whole brain and hippocampus were determined. No significant difference was found between the sleep deprived, pedestal and cage control groups at the end of the 21-day period when corticosterone levels were compared. The results of the elevated T test indicated that sleep deprivation did not change the anxiety-like behavior of the animals. When compared with cage or pedestal control groups, sleep deprived rats displayed elevated malondialdehyde levels, and decreased superoxide dismutase and glutathione peroxidase activities together with impaired long-term potentiation maintenance. It can be argued that 21-day SD may impair the maintenance of long-term potentiation evoked in the dentate gyrus, and the balance between oxidant and antioxidant defenses of the hippocampus.

摘要

一些证据表明,睡眠剥夺可能会损害海马体的突触可塑性并产生氧化应激。然而,目前尚不清楚长时程增强的损害是否取决于睡眠剥夺方案引起的氧化应激。在这项研究中,我们旨在研究 21 天的睡眠剥夺期对长期可塑性的影响,同时考虑到睡眠剥夺的应激效应。使用多平台方法对成年雄性 Wistar 大鼠进行睡眠剥夺。在中隔侧海马通路-齿状回突触中研究长时程增强。应用升高 T 检验,并测量血液皮质酮水平。测定全脑和海马中的脂质过氧化产物。在 21 天结束时,与睡眠剥夺、基座和笼状对照组相比,比较皮质酮水平时,三组间无显著差异。升高 T 检验的结果表明,睡眠剥夺并未改变动物的焦虑样行为。与笼状或基座对照组相比,睡眠剥夺大鼠的丙二醛水平升高,超氧化物歧化酶和谷胱甘肽过氧化物酶活性降低,长时程增强维持受损。可以认为,21 天的 SD 可能会损害齿状回中诱发的长时程增强的维持,以及海马体的氧化还原防御平衡。

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