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少突胶质细胞系细胞中酸敏感离子通道表达的特征分析。

Characterization of acid-sensing ion channel expression in oligodendrocyte-lineage cells.

作者信息

Feldman Daniel H, Horiuchi Makoto, Keachie Krista, Mccauley Erica, Bannerman Peter, Itoh Aki, Itoh Takayuki, Pleasure David

机构信息

Institute for Pediatric Regenerative Medicine, Shriners Hospital for Children, Northern California, Sacramento, California 95817, USA.

出版信息

Glia. 2008 Aug 15;56(11):1238-49. doi: 10.1002/glia.20693.

Abstract

Acid-sensing ion channels (ASICs) are widely expressed in neurons, where they serve in pain and mechanical sensation, and contribute to learning and memory. Six ASIC subunit proteins form homo- or heteromeric channel complexes with distinct physiological properties. Of such complexes, only monomeric ASIC1a channels are Ca2+ permeable. Prior pharmacologic and genetic studies have shown that ASIC1a channel inactivation markedly diminishes CNS susceptibility to ischemic damage. Here, we characterize ASIC expression in oligodendrocyte lineage cells (OLC) by molecular, electrophysiological, calcium imaging, and immunofluorescence techniques. ASIC1a, ASIC2a, and ASIC4 mRNAs were expressed in cultured rat OLC, with steady-state levels of each of these mRNAs several-fold higher in oligodendroglial progenitors than in mature oligodendroglia. ASIC transcripts were also detected in brain white matter, and ASIC1a protein expression was detected in white matter oligodendroglia. Inactivating, proton-gated, amiloride-sensitive OLC currents were detected by whole-cell voltage clamp. These currents showed profound tachyphylaxis with slow recovery, and were predominantly blocked by psalmotoxin, indicating that homomeric ASIC1a comprised a large fraction of functional ASIC in the cultured OLC. ASIC activation substantially depolarized OLC plasma membrane in current clamp studies, and elicited transient elevations in intracellular Ca2+ in imaging studies. Thus, OLC ASIC1a channels provide a means by which an acid shift in CNS extracellular pH, by diminishing plasma membrane potential and increasing Ca2+ permeability, can activate OLC signaling pathways, and may contribute to OLC vulnerability to CNS ischemia.

摘要

酸敏感离子通道(ASICs)在神经元中广泛表达,它们在疼痛和机械感觉中发挥作用,并对学习和记忆有贡献。六种ASIC亚基蛋白形成具有不同生理特性的同源或异源通道复合物。在这些复合物中,只有单体ASIC1a通道对Ca2+具有通透性。先前的药理学和遗传学研究表明,ASIC1a通道失活可显著降低中枢神经系统对缺血性损伤的易感性。在这里,我们通过分子、电生理、钙成像和免疫荧光技术来表征少突胶质细胞系细胞(OLC)中ASIC的表达。ASIC1a、ASIC2a和ASIC4 mRNA在培养的大鼠OLC中表达,这些mRNA在少突胶质前体细胞中的稳态水平比在成熟少突胶质细胞中高几倍。在脑白质中也检测到了ASIC转录本,并且在白质少突胶质细胞中检测到了ASIC1a蛋白表达。通过全细胞膜片钳检测到了失活的、质子门控的、amiloride敏感的OLC电流。这些电流表现出明显的快速脱敏且恢复缓慢,并且主要被Psalmotoxin阻断,这表明同源ASIC1a在培养的OLC中构成了大部分功能性ASIC。在电流钳研究中,ASIC激活使OLC质膜显著去极化,并且在成像研究中引起细胞内Ca2+的短暂升高。因此,OLC的ASIC1a通道提供了一种途径,通过这种途径,中枢神经系统细胞外pH值的酸性变化,通过降低质膜电位和增加Ca2+通透性,可以激活OLC信号通路,并且可能导致OLC对中枢神经系统缺血的易感性。

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