摘要
目的观察第Ⅲ组代谢型谷氨酸受体激动剂L-SOP和(R,S)-PPG对Aβ31~35所致培养神经元胞内Ca2+浓度升高的影响。方法原代培养的大鼠额叶皮层神经元,分别加入第Ⅲ组mG luR s激动剂L-SOP或(R,S)-PPG,利用实时Ca2+荧光成像技术观察对Aβ31~35所致〔Ca2+〕i升高的影响。结果急性给予Aβ31~35可引起培养神经元的〔Ca2+〕i水平呈剂量依赖性的升高,即随着Aβ31~35浓度的增加,其〔Ca2+〕i升高的幅度逐渐增加,而潜伏期逐渐缩短;经L-SOP或(R,S)-PPG预处理后,使Aβ31~35所引起的〔Ca2+〕i的平均升高幅度降低,平均潜伏期明显延长。结论在离体培养的神经元第Ⅲ组mG luR s的激活可通过抑制Aβ31~35引起的Ca2+超载,对Aβ31-35诱导的神经毒发挥保护作用。
Objective To observe the effect of group Ⅲ mGluRs agonist L-SOP and(R,S)-PPG on the increased level of intracellular calcium((Ca2+)i) of cultured neurons induced by Aβ31~35.Methods The cultured cortical neurons were pre-treated with L-SOP(100 μmol/L) or(R,S)-PPG(100 μmol/L) for 10 min.The(Ca2+)i concentration of the cells were analyzed by real time fluorescence imaging technique.Results Aβ31~35(5,10,20,25 μmol/L) increased(Ca2+)i level and decreased the average latency in a dose-dependent.The(Ca2+)i increasing amplitude induced by Aβ31~35 was decreased after L-SOP or(R,S)-PPG pretreated,and average latency was longer.Conclusions Group Ⅲ mGluRs activation can preserve isolated culture neurons by inhibiting Ca2+ overloading induced by Aβ31~35.
出处
《中国老年学杂志》
CAS
CSCD
北大核心
2011年第9期1561-1564,共4页
Chinese Journal of Gerontology
基金
国家自然科学基金(30572085)
教育部新教师基金(200800431001)
