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作 者:崔香丽[1] 陈还珍[1] 武冬梅[1] 吴博威[1]
出 处:《生理学报》2002年第3期219-224,共6页Acta Physiologica Sinica
基 金:theNationalNaturalScienceFoundationofChina (No 30 170 346 )
摘 要:实验观察了钠氢交换或钠钙交换抑制剂 5 (N ,N 二甲基 )氨氯吡咪 (DMA)对正常和心肌肥厚大鼠分离心室肌细胞钙瞬变和细胞收缩的影响。通过负载荧光染料Fura 2 /Am ,应用离子影像分析系统 (IonImagingSystem)同步测定离体大鼠心肌细胞钙瞬变和细胞长度。结果表明 :DMA 10 μmol/L分别使钙瞬变和细胞缩短从对照组的 2 0 9.6 0± 5 4.96和 3.0 7± 0 .97μm增加到 2 38.5 0± 80 .41和 4.0 7± 1.0 2 μm (P <0 .0 5 ,n =7)。应用特异性反向钠钙交换阻断剂KB R7943可完全阻断DMA的激动作用。DMA还可使尼卡地平抑制L 型钙通道后的钙瞬变和细胞收缩增加。在肥厚心肌细胞 ,DMA表现出相同的药理作用 ,但对钙瞬变和细胞缩短的刺激作用更强。结果表明 :DMA可通过反向钠钙交换途径增加正常和肥厚大鼠心肌细胞钙瞬变和细胞收缩 ,且对肥厚心肌细胞的影响比对正常心肌细胞大。The effects of 5-(N,N-dimethyl)amiloride (DMA) (a blocker of Na +/H + exchanger or Na +/Ca 2+ exchanger) on calcium transient and cell contraction in isolated ventricular myocytes in normal rats and rats with myocardial hypertrophy were examined using ion imaging system with a charge coupled digital camera (CCD camera). Loading myocytes with Fura-2, electrically triggered Ca 2+ transients and cell shortening were measured simultaneously. The results showed that 10 μmol/L DMA increased Ca 2+ transient and cell shortening from 209.60±54.96 and 3.07±0.97 μm to 238.50±80.41 and 4.07±1.02 μm, respectively (P<0.05), which was completely abolished by application of KB-R7943, a specific reverse mode Na +/Ca 2+ exchanger blocker. After blocking L-type Ca 2+ channels by nicardipine, DMA also enhanced Ca 2+ transient and cell shortening. In rats with myocardial hypertrophy, DMA showed the common pharmacologic profile as in normal rats but more intense stimulating effects on Ca 2+ transient and cell contraction. The results suggest that DMA increase Ca 2+ transient and cell contraction via stimulating reverse mode Na +/Ca 2+ exchange, and the stimulating effect is more pronounced in rats with myocardial hypertrophy than in normal ones.
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