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催乳素释放肽通过调节迷走神经背侧复合体中的突触传递来影响大鼠的胃运动功能。

Prolactin-releasing peptide affects gastric motor function in rat by modulating synaptic transmission in the dorsal vagal complex.

作者信息

Grabauskas Gintautas, Zhou Shi-Yi, Das Sudipto, Lu Yuanxu, Owyang Chung, Moises Hylan C

机构信息

GI Division, Department of Internal Medicine, University of Michigan Medical School, 1150 West Medical Center Drive, Ann Arbor, MI 48109-0622, USA.

出版信息

J Physiol. 2004 Dec 15;561(Pt 3):821-39. doi: 10.1113/jphysiol.2004.072736. Epub 2004 Oct 14.

DOI:10.1113/jphysiol.2004.072736
PMID:15486017
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1665377/
Abstract

Prolactin-releasing peptide (PrRP) is a recently discovered neuropeptide implicated in the central control of feeding behaviour and autonomic homeostasis. PrRP-containing neurones and PrRP receptor mRNA are found in abundance in the caudal portion of the nucleus tractus solitarius (NTS), an area which together with the dorsal motor nucleus of the vagus (DMV) comprises an integrated structure, the dorsal vagal complex (DVC) that processes visceral afferent signals from and provides parasympathetic motor innervation to the gastrointestinal tract. In this study, microinjection experiments were conducted in vivo in combination with whole-cell recording from neurones in rat medullary slices to test the hypothesis that PrRP plays a role in the central control of gastric motor function, acting within the DVC to modulate the activity of preganglionic vagal motor neurones that supply the stomach. Microinjection of PrRP (0.2 pmol (20 nl)(-1)) into the DMV at the level of the area postrema (+0.2 to +0.6 mm from the calamus scriptorius, CS) markedly stimulated gastric contractions and increased intragastric pressure (IGP). Conversely, administration of peptide into the DMV at sites caudal to the obex (0.0 to -0.3 mm from the CS) decreased IGP and reduced phasic contractions. These effects occurred without change in mean arterial pressure and were abolished by ipsilateral vagotomy, indicating mediation via a vagal-dependent mechanism(s). The pattern of gastric motor responses evoked by PrRP mimicked that produced by administration of L-glutamate at the same sites, and both the effects of L-glutamate and PrRP were abolished following local administration of NMDA and non-NMDA-type glutamate receptor antagonists. On the other hand, microinjection of PrRP into the medial or comissural nucleus of the solitary tract (mNTS and comNTS, respectively) resulted in less robust changes in IGP in a smaller percentage of animals, accompanied by marked alterations in arterial pressure. Superfusion of brain slices with PrRP (100-300 nm) produced a small depolarization and increased spontaneous firing in 10 of 30 retrogradely labelled gastric-projecting DMV neurones. The excitatory effects were blocked by administration of TTX (2 mum) or specific glutamate receptor antagonists, indicating that they resulted from interactions of PrRP at a presynaptic site. Congruent with this, PrRP increased the amplitude of excitatory postsynaptic currents (EPSCs, 154 +/- 33%, 12 of 25 neurones) evoked by electrical stimulation in mNTS or comNTS. In addition, administration of PrRP decreased the paired-pulse ratio of EPSCs evoked by two identical stimuli delivered 100 ms apart (from 0.95 +/- 0.08 to 0.71 +/- 0.11, P < 0.05), whereas it did not affect the amplitude of inward currents evoked by exogenous application of L-glutamate to the slice. The frequency, but not amplitude of spontaneous EPSCs and action potential-independent miniature EPSCs was also increased by administration of PrRP, suggesting that the peptide was acting at least in part at receptors on presynaptic nerve terminals to enhance glutamatergic transmission. In recordings obtained from a separate group of slices, we did not observe any direct effects of PrRP on spontaneous discharge or postsynaptic excitability in either mNTS or comNTS neurones (n = 31). These data indicate that PrRP may act within the DVC to regulate gastric motor function by modulating the efficacy of conventional excitatory synaptic inputs from the NTS onto gastric-projecting vagal motor neurones.

摘要

催乳素释放肽(PrRP)是一种最近发现的神经肽,与进食行为的中枢控制和自主稳态有关。在孤束核(NTS)尾部大量发现了含PrRP的神经元和PrRP受体mRNA,该区域与迷走神经背运动核(DMV)一起构成一个整合结构,即背迷走复合体(DVC),它处理来自胃肠道的内脏传入信号并为胃肠道提供副交感运动神经支配。在本研究中,进行了体内微量注射实验,并结合大鼠延髓切片中神经元的全细胞记录,以检验PrRP在胃运动功能的中枢控制中发挥作用的假说,即PrRP在DVC内起作用,调节支配胃的迷走神经节前运动神经元的活动。在最后区水平(距书写髓纹(CS)+0.2至+0.6毫米)向DMV微量注射PrRP(0.2 pmol(20 nl)⁻¹)可显著刺激胃收缩并升高胃内压(IGP)。相反,在闩尾侧部位(距CS 0.0至 -0.3毫米)向DMV注射该肽可降低IGP并减少相性收缩。这些效应在平均动脉压无变化的情况下出现,并被同侧迷走神经切断所消除,表明是通过迷走神经依赖性机制介导的。PrRP诱发的胃运动反应模式与在相同部位给予L - 谷氨酸所产生的模式相似,并且在局部给予NMDA和非NMDA型谷氨酸受体拮抗剂后,L - 谷氨酸和PrRP的效应均被消除。另一方面,将PrRP微量注射到孤束核内侧或连合核(分别为mNTS和comNTS)中,在较小比例的动物中导致IGP变化较小,同时伴有动脉压的明显改变。用PrRP(100 - 300 nM)灌流脑片在30个逆行标记的投射至胃的DMV神经元中的10个中产生了小的去极化并增加了自发放电。这些兴奋效应被给予TTX(2 μM)或特异性谷氨酸受体拮抗剂所阻断,表明它们是由PrRP在突触前位点的相互作用引起的。与此一致,PrRP增加了mNTS或comNTS中电刺激诱发的兴奋性突触后电流(EPSCs,154±33%,25个神经元中的12个)的幅度。此外,给予PrRP降低了由相隔100毫秒的两个相同刺激诱发的EPSCs的成对脉冲比率(从0.95±0.08降至0.71±0.11,P < 0.05),而它不影响向切片外源性施加L - 谷氨酸诱发的内向电流幅度。给予PrRP还增加了自发EPSCs和与动作电位无关的微小EPSCs的频率,但不影响其幅度,这表明该肽至少部分作用于突触前神经末梢上受体以增强谷氨酸能传递。在从另一组切片获得的记录中,我们未观察到PrRP对mNTS或comNTS神经元的自发放电或突触后兴奋性有任何直接影响(n = 31)。这些数据表明,PrRP可能在DVC内通过调节从NTS到投射至胃的迷走神经运动神经元的传统兴奋性突触输入的效能来调节胃运动功能。

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