Ryanodine- and thapsigargin-insensitive Ca2+-induced Ca2+ release is primed by lowering external Ca2+ in rabbit autonomic neurons

被引:0
|
作者
Mitsuo Nohmi
Shao-Ying Hua
Chen Liu
Kenji Kuba
机构
[1] First Department of Physiology,
[2] Nagoya University,undefined
[3] School of Medicine,undefined
[4] 65 Tsurumai-cho,undefined
[5] Showa-ku,undefined
[6] Nagoya 466–8550,undefined
[7] Japan,undefined
[8] Department of Physiology,undefined
[9] Saga Medical School,undefined
[10] 5-1-1 Nabeshima,undefined
[11] Saga 849–8501,undefined
[12] Japan,undefined
[13] Central Laboratories for M.S.R.E.,undefined
[14] Saga Medical School,undefined
[15] 5-1-1 Nabeshima,undefined
[16] Saga 849–8501,undefined
[17] Japan,undefined
[18] Department of Physiology,undefined
[19] University of Toronto,undefined
[20] Toronto,undefined
[21] Ontario,undefined
[22] M5S 1A8 Canada,undefined
[23] Physiological Research Department,undefined
[24] The Institute of Traditional Chinese Medicine,undefined
[25] Wahan,undefined
[26] China,undefined
来源
Pflügers Archiv | 2000年 / 440卷 / 4期
关键词
Ca2+-induced Ca2+ release Ca2+ store Capacitative Ca2+ release K+-induced depolarization Low external Ca2+ Rabbit autonomic neurons;
D O I
10.1007/s004240000326
中图分类号
学科分类号
摘要
Rises in cytosolic Ca2+ induced by a high K+ concentration (30 or 60 mM) (K+-induced Ca2+ transient) were recorded by fluorimetry of Ca2+ indicators in cultured rabbit otic ganglion cells. When external Ca2+ ([Ca2+]o) was reduced to a micromolar (10–40 µM) or nanomolar (<10 nM) level prior to high-K+ treatment, K+-induced Ca2+ transients of considerable amplitude (50% of control) were generated in most cells, although those initiated at normal [Ca2+]o were reduced markedly or abolished by reducing [Ca2+]o during exposure to a high K+ concentration. Lowering [Ca2+]o alone occasionally caused a transient rise in cytosolic Ca2+. K+-induced Ca2+ transients at micromolar [Ca2+]o were repeatedly generated and propagated inwardly at a speed slower than that at normal [Ca2+]o, while those at nanomolar [Ca2+]o occurred only once. K+-induced Ca2+ transients at micromolar [Ca2+]o were not blocked by ryanodine (10 µM), carbonyl cyanide p-(trifluoromethoxy) phenylhydrazone (FCCP, 5 µM: at 20–22°C but blocked at 31–34°C) or thapsigargin (1–2 µM), but were blocked by Ni2+ (1 mM) or nicardipine (10 µM). Thus, there is a ryanodine-insensitive Ca2+-release mechanism in FCCP- and thapsigargin-insensitive Ca2+ stores in rabbit otic ganglion cells, which is primed by lowering [Ca2+]o and then activated by depolarization-induced Ca2+ entry. This Ca2+-induced Ca2+ release may operate when [Ca2+]o is decreased by intense neuronal activity.
引用
收藏
页码:588 / 599
页数:11
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