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作 者:魏振宇[1] 谈世进[1] 唐二虎[1] 潘敬运[1] 詹澄扬[1]
机构地区:[1]中山医科大学生理学教研室,遵义医学院生理教研室
出 处:《生理学报》1995年第2期173-178,共6页Acta Physiologica Sinica
基 金:国家教委博士点科研基金;美国中华医学基金
摘 要:本实验采用分离的SD大鼠心室肌细胞,以Fura-2AM荧光指示剂负载,检测心肌细胞内游离钙浓度([Ca2+]i)变化。探讨亮啡肽(LEK)对[Ca2+]i的作用及其机制。实验结果:LEK(60μumol/L)能升高[Ca2+]i,移去细胞外液钙此效应仍能出现,用caffeine(5mmol/L)耗竭细胞内钙池的钙,该效应消失,纳洛酮(100μmol/L),百日咳毒素(200ng/L)处理8—10h及procaine(2mmol/L)都能阻断该效应。以上结果表明:亮啡肽诱导[Ca2+]i升高是通过δ受体与百日咳毒素敏感的G蛋白耦联并诱导心肌细胞内钙释放所引起。The mechanism underlying Leu-enkephalin (LEK) induced increase of the intracellular concentration of free calcium ([Ca2+]i) in rat ventricular myocytes was investigated by using fura-2 AM as a calcium indicator. The results were as follows: LEK (60 μmol/L) elevated [Ca2+]i in ventricular myocytes no matter whether extracellular calcium was removed or not. However, the effect was no longer observed when the calcium in the intracellular pool was depleted by caffeine (5 mmol/L). The LEK effect could also be blocked by naloxone (100 μmol/L), pretreatment of the cells with PTX (200ng/L) 8- 10h or procain (2 mmol/L). The results suggest that the LEK effect is mediated by coupling of G-protein with δ-receptor that induced Ca2+ release from the intracellular pool in myocytes.
分 类 号:R331.31[医药卫生—人体生理学]
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