慢性乙醇暴露对非洲爪蟾卵母细胞中表达的谷氨酸转运体EAAT3的影响:蛋白激酶C参与的证据。
Effects of chronic exposure to ethanol on glutamate transporter EAAT3 expressed in Xenopus oocytes: evidence for protein kinase C involvement.
作者信息
Kim Jin-Hee, Do Sang-Hwan, Kim Yong-Lak, Zuo Zhiyi
机构信息
Department of Anesthesiology, Seoul National University College of Medicine, Seoul, Korea.
出版信息
Alcohol Clin Exp Res. 2005 Nov;29(11):2046-52. doi: 10.1097/01.alc.0000187594.92476.07.
BACKGROUND
Glutamate transporters (excitatory amino acid transporters, EAAT) regulate extracellular concentrations of glutamate, a major excitatory neurotransmitter. We reported that acute ethanol exposure increases the activity of a major neuronal EAAT, EAAT3. This effect is consistent with the general inhibitory effect of acute alcohol toxicity in the central nervous system (CNS). However, chronic ethanol exposure has CNS presentations different from acute alcohol toxicity. We hypothesize that chronic ethanol exposure will affect the EAAT3 activity differently from acute ethanol exposure.
METHODS
EAAT3 was expressed in Xenopus oocytes by injection of EAAT3 mRNA. Oocytes were incubated with diluted ethanol for 24-96 hr. Using two-electrode voltage clamp, membrane currents were recorded after the application of L-glutamate. Responses were quantified by integration of the current trace and reported as microCoulombs (microC).
RESULTS
Ethanol (10-100 mM) reduced EAAT3 activity in a time-dependent and reversible manner. After a 96 hr-incubation, the activity was significantly decreased compared to the control values at any concentrations tested in this study. Kinetic study demonstrated that a 96 hr-exposure to 50 mM ethanol significantly decreased Vmax (3.6 +/- 0.3 for control versus 2.6 +/- 0.3 microC for ethanol, n = 20, p < 0.05) but had no effect on Km (57.6 +/- 12.8 for control versus 51.8 +/- 16.3 microM for ethanol, n = 20, p > 0.05) of EAAT3 for glutamate. When ethanol (50 mM for 96 hr)-treated oocytes were incubated with phorbol-12-myrisate-13-acetate (50 or 100 nM for 10 min), ethanol-induced decrease in EAAT3 activity was abolished. Preincubation of the oocytes with 100 microM chelerythrine significantly decreased EAAT3 activity (1.00 +/- 0.08 for control versus 0.51 +/- 0.09 microC for chelerythrine group, n = 18-20, p < 0.05). However, there was no statistical difference among the chelerythrine, ethanol, or chelerythrine plus ethanol groups. Likewise, staurosporine (2 microM for 1 hr) significantly decreased EAAT3 activity and there was no statistical difference among the staurosporine, ethanol, or staurosporine plus ethanol groups.
CONCLUSIONS
Our results show that chronic ethanol exposure decreases EAAT3 activity at clinically relevant concentrations and that this effect may be protein kinase C-dependent. Such an effect could be a neuroadaptive mechanism to overcome the inhibitory effect of ethanol on the excitatory neurotransmission.
背景
谷氨酸转运体(兴奋性氨基酸转运体,EAAT)调节主要兴奋性神经递质谷氨酸的细胞外浓度。我们曾报道急性乙醇暴露会增加主要神经元EAAT即EAAT3的活性。这种效应与急性酒精中毒对中枢神经系统(CNS)的一般抑制作用一致。然而,慢性乙醇暴露具有与急性酒精中毒不同的CNS表现。我们推测慢性乙醇暴露对EAAT3活性的影响与急性乙醇暴露不同。
方法
通过注射EAAT3 mRNA在非洲爪蟾卵母细胞中表达EAAT3。将卵母细胞与稀释的乙醇孵育24 - 96小时。使用双电极电压钳,在施加L - 谷氨酸后记录膜电流。通过对电流轨迹积分对反应进行定量,并以微库仑(μC)表示。
结果
乙醇(10 - 100 mM)以时间依赖性和可逆方式降低EAAT3活性。孵育96小时后,与本研究中测试的任何浓度的对照值相比,活性显著降低。动力学研究表明,暴露于50 mM乙醇96小时显著降低Vmax(对照组为3.6±0.3,乙醇组为2.6±0.3 μC,n = 20,p < 0.05),但对EAAT3转运谷氨酸的Km值无影响(对照组为57.6±12.8,乙醇组为51.8±16.3 μM,n = 20,p > 0.05)。当用佛波醇-12-肉豆蔻酸酯-13-乙酸酯(50或100 nM,10分钟)孵育乙醇(50 mM,96小时)处理的卵母细胞时,乙醇诱导的EAAT3活性降低被消除。用100 μM白屈菜红碱预孵育卵母细胞显著降低EAAT3活性(对照组为1.00±0.08,白屈菜红碱组为0.51±0.09 μC,n = 18 - 20,p < 0.05)。然而,白屈菜红碱组、乙醇组或白屈菜红碱加乙醇组之间无统计学差异。同样,星形孢菌素(2 μM,1小时)显著降低EAAT3活性,星形孢菌素组、乙醇组或星形孢菌素加乙醇组之间无统计学差异。
结论
我们的结果表明,慢性乙醇暴露在临床相关浓度下会降低EAAT3活性,且这种效应可能依赖于蛋白激酶C。这种效应可能是一种神经适应性机制,以克服乙醇对兴奋性神经传递的抑制作用。
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