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从培养的皮质神经元释放的γ-氨基丁酸(GABA)影响硫代磷酸丁基双环磷酯(t-[(35)S]butylbicyclophosphorothionate)在GABAA受体上结合的调节 百里酚的作用。

GABA released from cultured cortical neurons influences the modulation of t-[(35)S]butylbicyclophosphorothionate binding at the GABAA receptor Effects of thymol.

作者信息

García Daniel A, Vendrell Iolanda, Galofré Mireia, Suñol Cristina

机构信息

Department of Neurochemistry and Neuropharmacology, Institut d'Investigacions Biomèdiques de Barcelona, CSIC-IDIBAPS, Barcelona, Spain.

出版信息

Eur J Pharmacol. 2008 Dec 14;600(1-3):26-31. doi: 10.1016/j.ejphar.2008.10.013. Epub 2008 Oct 11.

DOI:10.1016/j.ejphar.2008.10.013
PMID:18938153
Abstract

Thymol is a monoterpene that specifically interacts with synaptic neural functions in neuronal GABA-operated Cl(-) channels. Here we explore the effects of thymol, and propofol as positive control, on t-[(35)S]butylbicyclophosphorothionate ([(35)S]TBPS) binding in primary cultures of cortical neurons. The study includes a meaningful analysis of the effect of various exposure buffers, and their correlation with GABA released from cells, chloride influx through the GABA(A) receptor and GABA transporter activity. Cell viability was also determined. Thymol and propofol inhibited the binding of [(35)S]TBPS to cells exposed to Tris-citrate-NaCl buffer whereas a biphasic effect was observed in HEPES solution. The different effects of the two buffers analysed are due to the higher capacity of Tris-citrate-NaCl buffer to induce the release of endogenous GABA facilitating the binding of [(35)S]TBPS to its recognition site at the GABA(A) receptor. Released GABA in the presence of this buffer was inhibited by the neuronal GABA transporter inhibitor SKF 100330-A. Tris-citrate-NaCl buffer also induced a chloride influx, which was reverted by picrotoxinin. TBPS binding in living cells is facilitated by GABA released from the cells, which in turn activates basal GABA(A) receptor activity. The results deepen on the allosteric mechanism of thymol as positive modulator of the GABA(A) receptor. Furthermore, we corroborate [(35)S]TBPS binding as an important test to verify the capacity of drugs to act on and recognize a site at the GABA(A) receptor.

摘要

百里酚是一种单萜类化合物,它能特异性地与神经元γ-氨基丁酸(GABA)操纵的氯离子通道中的突触神经功能相互作用。在此,我们研究了百里酚以及作为阳性对照的丙泊酚对皮质神经元原代培养物中t-[(35)S]丁基双环磷硫代酸盐([(35)S]TBPS)结合的影响。该研究对各种暴露缓冲液的作用及其与细胞释放的GABA、通过GABA(A)受体的氯离子内流以及GABA转运体活性的相关性进行了有意义的分析。同时还测定了细胞活力。百里酚和丙泊酚抑制了[(35)S]TBPS与暴露于柠檬酸三钠-氯化钠缓冲液中的细胞的结合,而在HEPES溶液中观察到双相效应。所分析的两种缓冲液的不同作用是由于柠檬酸三钠-氯化钠缓冲液诱导内源性GABA释放的能力更强,从而促进了[(35)S]TBPS与其在GABA(A)受体上的识别位点的结合。在这种缓冲液存在下释放的GABA被神经元GABA转运体抑制剂SKF 100330-A所抑制。柠檬酸三钠-氯化钠缓冲液还诱导了氯离子内流,这被苦味毒逆转。细胞释放的GABA促进了活细胞中TBPS的结合,而这反过来又激活了基础GABA(A)受体活性。这些结果加深了对百里酚作为GABA(A)受体正性调节剂的变构机制的理解。此外,我们证实[(35)S]TBPS结合是验证药物作用于并识别GABA(A)受体上一个位点的能力的重要试验。

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