Fang Hongyu, Huang Yueming, Zuo Zhiyi
Department of Anesthesiology, University of Virginia Health System, One Hospital Dr., PO Box 800710, Charlottesville, VA 22908-0710, USA.
Am J Physiol Cell Physiol. 2006 May;290(5):C1334-40. doi: 10.1152/ajpcell.00443.2005.
Glutamate transporters (also called excitatory amino acid transporters, EAAT) are important in extracellular homeostasis of glutamate, a major excitatory neurotransmitter. EAAT4, a neuronally expressed EAAT in cerebellum, has a large portion (approximately 95% of the total L-aspartate-induced currents in human EAAT4) of substrate-gated Cl(-) currents, a distinct feature of this EAAT. We cloned EAAT4 from rat cerebellum. This molecule was predicted to have eight putative transmembrane domains. L-glutamate induced an inward current in oocytes expressing this EAAT4 at a holding potential -60 mV. Phorbol 12-myristate 13-acetate (PMA), a protein kinase C (PKC) activator, significantly increased the magnitude of L-glutamate-induced currents but did not affect the apparent affinity of EAAT4 for L-glutamate. This PMA-enhanced current had a reversal potential -17 mV at extracellular Cl(-) concentration (Cl(-)) 104 mM with an approximately 60-mV shift per 10-fold change in Cl(-), properties consistent with Cl(-)-selective conductance. However, PMA did not change EAAT4 transport activity as measured by [(3)H]-L-glutamate. Thus PMA-enhanced Cl(-) currents via EAAT4 were not thermodynamically coupled to substrate transport. These PMA-enhanced Cl(-) currents were partially blocked by staurosporine, chelerythrine, and calphostin C, the three PKC inhibitors. Ro-31-8425, a PKC inhibitor that inhibits conventional PKC isozymes at low concentrations (nM level), partially inhibited the PMA-enhanced Cl(-) currents only at a high concentration (1 microM). Intracellular injection of BAPTA, a Ca(2+)-chelating agent, did not affect the PMA-enhanced Cl(-) currents. 4alpha-Phorbol-12,13-didecanoate, an inactive analog of PMA, did not enhance glutamate-induced currents. These data suggest that PKC, possibly isozymes other than conventional ones, modulates the substrate-gated Cl(-) currents via rat EAAT4. Our results also suggest that substrate-gated ion channel activity and glutamate transport activity, two EAAT4 properties that could modulate neuronal excitability, can be regulated independently.
谷氨酸转运体(也称为兴奋性氨基酸转运体,EAAT)在主要兴奋性神经递质谷氨酸的细胞外稳态中起重要作用。EAAT4是一种在小脑中神经元表达的EAAT,具有很大一部分(在人EAAT4中约占L - 天冬氨酸诱导电流总量的95%)底物门控的Cl(-)电流,这是该EAAT的一个显著特征。我们从小鼠小脑中克隆了EAAT4。该分子预计有8个推定的跨膜结构域。在-60 mV的钳制电位下,L - 谷氨酸在表达该EAAT4的卵母细胞中诱导出内向电流。佛波醇12 - 肉豆蔻酸酯13 - 乙酸酯(PMA),一种蛋白激酶C(PKC)激活剂,显著增加了L - 谷氨酸诱导电流的幅度,但不影响EAAT4对L - 谷氨酸的表观亲和力。在细胞外Cl(-)浓度(Cl(-))为104 mM时,这种PMA增强的电流的反转电位为-17 mV,Cl(-)每10倍变化约有60 mV的偏移,这些特性与Cl(-)选择性电导一致。然而,PMA并没有改变通过[(3)H]-L - 谷氨酸测量的EAAT4转运活性。因此,PMA通过EAAT4增强的Cl(-)电流在热力学上与底物转运不偶联。这些PMA增强的Cl(-)电流被三种PKC抑制剂星形孢菌素、白屈菜红碱和钙泊三醇部分阻断。Ro - 31 - 8425是一种PKC抑制剂,在低浓度(nM水平)时抑制传统PKC同工酶,仅在高浓度(1 microM)时部分抑制PMA增强的Cl(-)电流。细胞内注射Ca(2+)螯合剂BAPTA不影响PMA增强的Cl(-)电流。4α - 佛波醇 - 12,13 - 十二烷酸酯,PMA的一种无活性类似物,不增强谷氨酸诱导的电流。这些数据表明PKC,可能是传统PKC同工酶以外的同工酶,通过大鼠EAAT4调节底物门控的Cl(-)电流。我们的结果还表明,底物门控离子通道活性和谷氨酸转运活性这两种可能调节神经元兴奋性的EAAT4特性可以独立调节。
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