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[前列腺素D2和腺苷对睡眠-觉醒的调节作用]

[Sleep-wake regulation by prostaglandin D2 and adenosine].

作者信息

Nagata Nanae, Urade Yoshihiro

机构信息

Department of Molecular Behavioral Biology, Osaka Bioscience Institute, Japan.

出版信息

Brain Nerve. 2012 Jun;64(6):621-8.

PMID:22647469
Abstract

Prostaglandin (PG) D2 and adenosine are potent endogenous somnogens that accumulate in the brain during prolonged wakefulness. Lipocalin-type PGD synthase (L-PGDS) catalyzes the isomerization of PGH2, a common precursor of various prostanoids, to produce PGD2. L-PGDS is localized in the leptomeninges, choroid plexus, and oligodendrocytes of the central nervous system. PGD2 stimulates DP1 receptors localized in the basal forebrain and increases the local extracellular concentration of adenosine, a paracrine signaling molecule, to promote sleep. Adenosine activates adenosine A2A receptor-expressing neurons in the basal forebrain and ventrolateral preoptic area (VLPO) and inhibits adenosine A1 receptor-possessing arousal neurons. Sleep-promoting neurons in the VLPO send inhibitory signals to suppress the histaminergic neurons in the tuberomammillary nucleus (TMN); the histaminergic neurons contribute to arousal through histamine H1 receptors. GABAergic inhibition of TMN is involved in the induction of non-rapid eye movement (non-REM) sleep by PGD2 and adenosine A2A agonists. The neural network between the VLPO and TMN is considered to play a key role in regulation of vigilance states. Administering an L-PGD inhibitor (SeCl4), DP1 antagonist (ONO-4127Na), or adenosine A2A receptor antagonist (caffeine) suppresses both non-REM and REM sleep, indicating that the PGD2-adenosine system is crucial for maintaining physiological sleep. Selective gene-deletion strategies based on Cre/loxP technology and focal RNA interference have been used for silencing the expression of the A2A receptor by local infection with adeno-associated virus carrying Cre-recombinase or short hairpin RNA. The results of these studies have shown that the A2Asubreceptors in the shell region of the nucleus accumbens are responsible for the effect of caffeine on wakefulness.

摘要

前列腺素(PG)D2和腺苷是强效内源性促眠物质,在长时间清醒期间会在大脑中蓄积。脂联素型PGD合成酶(L-PGDS)催化各种前列腺素的共同前体PGH2异构化,生成PGD2。L-PGDS定位于中枢神经系统的软脑膜、脉络丛和少突胶质细胞。PGD2刺激位于基底前脑的DP1受体,并增加旁分泌信号分子腺苷在局部细胞外的浓度,以促进睡眠。腺苷激活基底前脑和腹外侧视前区(VLPO)中表达腺苷A2A受体的神经元,并抑制具有腺苷A1受体的觉醒神经元。VLPO中的促睡眠神经元发送抑制信号,以抑制结节乳头体核(TMN)中的组胺能神经元;组胺能神经元通过组胺H1受体促进觉醒。PGD2和腺苷A2A激动剂对TMN的GABA能抑制参与了非快速眼动(non-REM)睡眠的诱导。VLPO和TMN之间的神经网络被认为在警觉状态的调节中起关键作用。给予L-PGD抑制剂(SeCl4)、DP1拮抗剂(ONO-4127Na)或腺苷A2A受体拮抗剂(咖啡因)会抑制非快速眼动睡眠和快速眼动睡眠,这表明PGD2-腺苷系统对维持生理睡眠至关重要。基于Cre/loxP技术的选择性基因缺失策略和局部RNA干扰已被用于通过携带Cre重组酶或短发夹RNA的腺相关病毒局部感染来沉默A2A受体的表达。这些研究结果表明,伏隔核壳区的A2A亚受体是咖啡因对觉醒产生影响的原因。

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