大鼠谷氨酸能海马轴突中的Kv7/KCNQ/M通道及其在兴奋性调节和递质释放中的作用。
Kv7/KCNQ/M-channels in rat glutamatergic hippocampal axons and their role in regulation of excitability and transmitter release.
作者信息
Vervaeke K, Gu N, Agdestein C, Hu H, Storm J F
机构信息
Department of Physiology at IMB and Centre for Molecular Biology and Neuroscience, CMBN, University of Oslo, PB 1103 Blindern, N-0317 Oslo, Norway.
出版信息
J Physiol. 2006 Oct 1;576(Pt 1):235-56. doi: 10.1113/jphysiol.2006.111336. Epub 2006 Jul 13.
M-current (I(M)) plays a key role in regulating neuronal excitability. Mutations in Kv7/KCNQ subunits, the molecular correlates of I(M), are associated with a familial human epilepsy syndrome. Kv7/KCNQ subunits are widely expressed, and I(M) has been recorded in somata of several types of neurons, but the subcellular distribution of M-channels remains elusive. By combining field-potential, whole-cell and intracellular recordings from area CA1 in rat hippocampal slices, and computational modelling, we provide evidence for functional M-channels in unmyelinated axons in the brain. Our data indicate that presynaptic M-channels can regulate axonal excitability and synaptic transmission, provided the axons are depolarized into the I(M) activation range (beyond approximately -65 mV). Here, such depolarization was achieved by increasing the extracellular K(+) concentration (K(+)). Extracellular recordings in the presence of moderately elevated K(+) (7-11 mm), showed that the specific M-channel blocker XE991 reduced the amplitude of the presynaptic fibre volley and the field EPSP in a K(+)-dependent manner, both in stratum radiatum and in stratum lacknosum moleculare. The M-channel opener, retigabine, had opposite effects. The higher the K(+), the greater the effects of XE991 and retigabine. Similar pharmacological modulation of EPSPs recorded intracellularly from CA1 pyramidal neurons, while blocking postsynaptic K(+) channels with intracellular Cs(+), confirmed that active M-channels are located presynaptically. Computational analysis with an axon model showed that presynaptic I(M) can control Na(+) channel inactivation and thereby affect the presynaptic action potential amplitude and Ca(2+) influx, provided the axonal membrane potential is sufficiently depolarized. Finally, we compared the effects of blocking I(M) on the spike after-depolarization and bursting in CA3 pyramidal neuron somata versus their axons. In standard K(+) (2.5 mm), XE991 increased the ADP and promoted burst firing at the soma, but not in the axons. However, I(M) contributed to the refractory period in the axons when spikes were broadened by a low dose 4-aminopyridine (200 microm). Our results indicate that functional Kv7/KCNQ/M-channels are present in unmyelinated axons in the brain, and that these channels may have contrasting effects on excitability depending on their subcellular localization.
M电流(I(M))在调节神经元兴奋性方面起着关键作用。Kv7/KCNQ亚基作为I(M)的分子关联物,其突变与一种家族性人类癫痫综合征相关。Kv7/KCNQ亚基广泛表达,并且在几种类型神经元的胞体中记录到了I(M),但M通道的亚细胞分布仍不清楚。通过结合大鼠海马切片CA1区的场电位、全细胞和细胞内记录以及计算建模,我们为脑中无髓鞘轴突中功能性M通道提供了证据。我们的数据表明,只要轴突去极化到I(M)激活范围(超过约 -65 mV),突触前M通道就能调节轴突兴奋性和突触传递。在此,这种去极化是通过增加细胞外钾离子浓度(K⁺)来实现的。在中等升高的K⁺(7 - 11 mM)存在下进行的细胞外记录显示,特异性M通道阻滞剂XE991以K⁺依赖性方式降低了突触前纤维群峰电位和场兴奋性突触后电位(fEPSP)的幅度,在辐射层和分子层均如此。M通道开放剂瑞替加滨则有相反的作用。K⁺越高,XE991和瑞替加滨的作用越大。在CA1锥体神经元细胞内记录的fEPSP的类似药理学调节,同时用细胞内Cs⁺阻断突触后钾通道,证实了活性M通道位于突触前。用轴突模型进行的计算分析表明,只要轴突膜电位充分去极化,突触前I(M)就能控制钠离子通道失活,从而影响突触前动作电位幅度和钙离子内流。最后,我们比较了阻断I(M)对CA3锥体神经元胞体与其轴突的动作电位后去极化和爆发的影响。在标准K⁺(2.5 mM)下,XE991增加了动作电位后去极化(ADP)并促进了胞体的爆发性放电,但在轴突中没有。然而,当用低剂量4 - 氨基吡啶(200 μM)使动作电位变宽时,I(M)对轴突的不应期有贡献。我们的结果表明,功能性Kv7/KCNQ/M通道存在于脑中的无髓鞘轴突中,并且这些通道根据其亚细胞定位可能对兴奋性有不同的影响。
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