Neuronal nicotinic receptor-operated Ca2+ (RAMIC) mobilization for the desensitization of muscle nicotinic receptor coexisting at the muscle endplates

Hiroshi Tsuneki*, Katsuya Dezaki, Hiroshi Nojima, Ikuko Kimura, Masayasu Kimura

*この論文の責任著者

研究成果: ジャーナルへの寄稿学術論文査読

抄録

Few functional roles of neuronal nicotinic receptors (N-nAChR) are clarified, although N-nAChR have been reported to be highly permeable to Ca2+ than the muscle nicotinic receptor (M-nAChR). We have found new regulatory Ca2+ mobilization, RAMIC (Receptor Activity Modulating Intracellular Ca2+, at the endplate region in the mouse diaphragm muscles treated with a cholinesterase inhibitor by measuring Ca2+ aequorin luminescences. RAMIC mobilization is enhanced via the activation of protein kinase-A by nerve derived calcitonin gene related peptide, and promotes the M-nAChR desensitization via the protein kinase C activation. The RAMIC mobilization is depressed by a N-nAChR antagonist methyllyeaconitine (0.1 1 μM) and by monoclonal antibody to β2 subunit of N-nAChR. Furthermore, β2 and α8-related subunits were identified at murine skeletal muscle endplates either by RT PCR or by immunohistochemical staining. In isolated single skeletal muscle cells loaded with a fluorescent Ca2+ indicator fluo-3 AM, bath applied ACh (3 μM) elicits two-phasic elevation of [Ca2+]i (fast and slow components) localized beneath the endplate membranes, by using a real time-confocal laser scanning analysis. Methyllycaconitine selectively inhibits the slow Ca2+ component at the similar concentrations (1.5 μM) used to depress RAMIC. These results demonstrate that N-nAChR coexist with M- nAChR at the muscle endplates, and operates the RAMIC mobilization to promote the M-nAChR desensitization. Thus, the neuromuscular function is regulated by dual nAChR system to avoid the overexcitation.

本文言語英語
ページ(範囲)87-92
ページ数6
ジャーナルFolia Pharmacologica Japonica
108
SUPPL. 1
DOI
出版ステータス出版済み - 1996

ASJC Scopus 主題領域

  • 薬理学

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