ANESTHETICS AFFECT THE UPTAKE BUT NOT THE DEPOLARIZATION-EVOKED RELEASE OF GABA IN RAT STRIATAL SYNAPTOSOMES

被引:70
作者
MANTZ, J [1 ]
LECHARNY, JB [1 ]
LAUDENBACH, V [1 ]
HENZEL, D [1 ]
PEYTAVIN, G [1 ]
DESMONTS, JM [1 ]
机构
[1] UNIV PARIS 07,INSERM,U408,PARIS,FRANCE
关键词
ANESTHETICS; INTRAVENOUS; ETOMIDATE KETAMINE PROPOFOL THIOPENTAL; VOLATILE; ENFLURANE HALOTHANE ISOFLURANE; BRAIN; STRIATUM SYNAPTOSOMES; NEUROTRANSMITTERS; AMINO ACIDS; GAMMA-AMINOBUTYRIC ACID; SYMPATHETIC NERVOUS SYSTEM; ADRENERGIC RECEPTORS; ALPHA(2); AGONISTS; CLONIDINE;
D O I
10.1097/00000542-199502000-00020
中图分类号
R614 [麻醉学];
学科分类号
100217 ;
摘要
Background: Numerous classes of anesthetic agents have been shown to enhance the effects mediated by the postsynaptic gamma-aminobutyric acid A (GABA(A)) receptor-coupled chloride channel in the mammalian central nervous system. However, presynaptic actions of anesthetics potentially relevant to clinical anesthesia remain to be clarified. Therefore, in this study, the effects of intravenous and volatile anesthetics on both the uptake and the depolarization-evoked release of GABA in the rat striatum were investigated. Methods: Assay for specific GABA uptake was performed by measuring the radioactivity incorporated in purified striatal synaptosomes incubated with H-3-GABA (20 nbi, 5 min, 37 degrees C) and increasing concentrations of anesthetics in either the presence or the absence of nipecotic acid (1 mar, a specific GABA uptake inhibitor), Assay for GABA release consisted of superfusing H-3-GABA preloaded synaptosomes with artificial cerebrospinal fluid (0.5 ml.min(-1), 37 degrees C) and measuring the radioactivity obtained from 0.5 mi fractions over 18 min, first in the absence of any treatment (spontaneous release, 8 min), then in the presence of either KCI alone (9 mM, 15 mar) or with various concentrations of anesthetics (5 min), and finally, with no pharmacologic stimulation (5 min). The following anesthetic agents were tested: propofol, etomidate, thiopental, ketamine, halothane, enflurane, isoflurane, and clonidine. Results: More than 95% of H-3-GABA uptake was blocked by a 10(-3)-hr concentration of nipecotic acid, Propofol, etomidate, thiopental, and ketamine induced a dose-related, reversible, noncompetitive, inhibition of H-3-GABA uptake: IC50 = 4.6+/-0.3 X 10(-5) al, 5.8+/-0.3 X 10(-5) M, 2.1+/-0.4 X 10(-3) M, and 4.9+/-0.5 X 10(-4) al for propofol, etomidate, thiopental, and ketamine, respectively. Volatile agents and clonidine had no significant effect, even when used at concentrations greater than those used clinically. KCI application induced a significant, calcium-dependent, concentration-related, increase from basal H-3-GABA release, +34+/-10% (P<0.01) and +61+/-13% (P<0.001), respectively, for 9 mar and 15 mM KCl. The release of H-3-GABA elicited by KCI was not affected by any of the anesthetic agents tested. Conclusions: These results indicate that most of the intravenous but not the volatile anesthetics inhibit the specific high-affinity H-3-GABA uptake process in vitro in striatal nerve terminals. However, this action was observed at clinically relevant concentrations only for propofol and etomidate. In contrast, the depolarization-evoked H-3-GABA release was not affected by anesthetics. Together, these data suggest that inhibition of GABA uptake, which results in synaptic GABA accumulation, might contribute to propofol and etomidate anesthesia.
引用
收藏
页码:502 / 511
页数:10
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