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静息和受刺激的青蛙缝匠肌中钠离子的内向移动。

Inward movement of sodium ions in resting and stimulated frog's sartorius muscle.

作者信息

Venosa R A

出版信息

J Physiol. 1974 Aug;241(1):155-73. doi: 10.1113/jphysiol.1974.sp010646.

Abstract
  1. Paired frog sartorius muscles were exposed to Ringer solutions labelled with (22)Na(+) for about 20 min. At the end of this exposure one of them was stimulated supramaximally one hundred to two hundred times. Immediately after the stimulation both members of the pair were washed in a series of tubes filled with a Na(+)-free medium containing 3 x 10(-5)M strophanthidin.2. Under the above conditions the intracellular component of the efflux was exponential with an average time constant (tau) of 388 min, that is, approximately four times longer than in the presence of normal Ringer. On the other hand the mean tau for the washout of the interfibre space was 3.2 min.3. From the extrapolation to time zero of the intracellular component of the washout curve the initial intracellular radioactivity of both muscles was obtained and the resting and extra Na(+) influx were calculated.4. The mean surface membrane area/muscle weight ratio was found to be 552 cm(2).g(-1) and the mean fibre diameter 53.4 mum for muscles weighing on the average 60 mg.5. The average resting Na(+) influx in the presence of normal Ringer was 4.7 p-mole.cm(-2).sec(-1). As the external Na(+) concentration (Na(+)) was reduced the Na(+) influx diminished in a non-linear fashion. This non-linearity could be accounted for by the presence in the influx of a Na(+) for Na(+) exchange fraction which saturates at low Na(+).6. The mean extra Na(+) influx in the presence of normal Ringer was 27.4 p-mole.cm(-2).impulse(-1) and was not significantly affected either by halving Na(+) or by varying the frequency of stimulation. When Na(+) was reduced to 45 mM by partial replacement of Na(+) by Tris(+) the extra influx was significantly higher than when choline(+) instead of Tris(+) was used to substitute for Na(+).
摘要
  1. 将成对的青蛙缝匠肌暴露于用(22)Na(+)标记的林格氏液中约20分钟。在该暴露结束时,其中一块肌肉接受100至200次超强刺激。刺激后立即将这对肌肉的两块在一系列装有含3×10(-5)M毒毛花苷的无钠培养基的试管中冲洗。

  2. 在上述条件下,流出的细胞内成分呈指数形式,平均时间常数(τ)为388分钟,即比在正常林格氏液存在时大约长四倍。另一方面,纤维间空间洗脱的平均τ为3.2分钟。

  3. 从洗脱曲线的细胞内成分外推至时间零时,获得了两块肌肉的初始细胞内放射性,并计算了静息和额外的Na(+)流入量。

  4. 发现平均表面膜面积/肌肉重量比为552平方厘米·克(-1),对于平均重60毫克的肌肉,平均纤维直径为53.4微米。

  5. 在正常林格氏液存在下的平均静息Na(+)流入量为4.7皮摩尔·厘米(-2)·秒(-1)。随着外部Na(+)浓度([Na(+)](0))降低,Na(+)流入量以非线性方式减少。这种非线性可以由在低[Na(+)](0)时饱和的Na(+)与Na(+)交换部分的流入来解释。

  6. 在正常林格氏液存在下的平均额外Na(+)流入量为27.4皮摩尔·厘米(-2)·冲动(-1),并且通过将[Na(+)](0)减半或改变刺激频率均未受到显著影响。当通过用Tris(+)部分替代Na(+)将[Na(+)](0)降低至45 mM时,额外流入量显著高于使用胆碱(+)而非Tris(+)替代Na(+)时。

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