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镁对雪貂红细胞中钾转运的影响。

The effects of magnesium on potassium transport in ferret red cells.

作者信息

Flatman P W

机构信息

Department of Physiology, University Medical School, Edinburgh.

出版信息

J Physiol. 1988 Mar;397:471-87. doi: 10.1113/jphysiol.1988.sp017013.

Abstract
  1. The magnesium dependence of net and isotopic (using 86Rb as tracer) potassium transport was measured in fed ferret red cells. Bumetanide (0.1 mM) was used to dissect total flux into two components: bumetanide sensitive and bumetanide resistant. 2. Increasing the external magnesium concentration from zero (added) to 2 mM stimulated bumetanide-sensitive uptake by 16% but inhibited the bumetanide-resistant component by about 20%. 3. Ionophore A23187 was used to control internal magnesium concentration. A23187 was usually present in the cells during measurement of isotopic fluxes but was washed away before measurement of net fluxes. The magnesium-buffering characteristics of fed ferret red cells were assessed during these experiments. The cytoplasm acts as a high-capacity, low-affinity magnesium buffer over most of the range. Some high-affinity binding was seen in the presence of A23187 and 2 mM-EDTA. 4. A23187 itself slightly inhibits bumetanide-sensitive potassium transport. 5. Bumetanide-sensitive potassium transport is strongly dependent on the concentration of internal ionized magnesium. Transport is 35% maximal at 10(-7) M and increases up to the maximal rate at 1.3 mM. Further increase in ionized magnesium concentration to 3.5 mM has no additional effect. The curve relating activity to magnesium concentration is steepest at the physiological magnesium concentration. The effects of changing magnesium concentration are fully reversible. 6. Reduction of internal ionized magnesium concentration to 10(-7) M with A23187 and EDTA approximately doubles bumetanide-resistant potassium transport. 7. Bumetanide-sensitive fluxes occur via the sodium-potassium-chloride co-transport system under the conditions used. Results described in this paper thus suggest that internal magnesium may be an important physiological controller of sodium-potassium-chloride co-transport activity.
摘要
  1. 在喂食后的雪貂红细胞中测量了净钾转运和同位素(以⁸⁶Rb为示踪剂)钾转运对镁的依赖性。使用布美他尼(0.1 mM)将总通量分为两个部分:布美他尼敏感部分和布美他尼抗性部分。2. 将外部镁浓度从零(添加)增加到2 mM,刺激布美他尼敏感摄取增加16%,但抑制布美他尼抗性部分约20%。3. 使用离子载体A23187控制细胞内镁浓度。在测量同位素通量期间,A23187通常存在于细胞中,但在测量净通量之前被冲洗掉。在这些实验中评估了喂食后的雪貂红细胞的镁缓冲特性。在大多数范围内,细胞质充当高容量、低亲和力的镁缓冲剂。在存在A23187和2 mM - EDTA的情况下观察到一些高亲和力结合。4. A23187本身略微抑制布美他尼敏感的钾转运。5. 布美他尼敏感的钾转运强烈依赖于细胞内游离镁的浓度。在10⁻⁷M时转运为最大值的35%,并在1.3 mM时增加到最大速率。游离镁浓度进一步增加到3.5 mM没有额外影响。在生理镁浓度下,活性与镁浓度的关系曲线最陡峭。镁浓度变化的影响是完全可逆的。6. 用A23187和EDTA将细胞内游离镁浓度降低到10⁻⁷M,布美他尼抗性钾转运大约增加一倍。7. 在所用条件下,布美他尼敏感通量通过钠 - 钾 - 氯共转运系统发生。本文所述结果表明,细胞内镁可能是钠 - 钾 - 氯共转运活性的重要生理调节因子。

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