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雄蜂视网膜中光感受器、神经胶质细胞和细胞外空间的钾离子活性:光刺激期间的变化

Potassium activity in photoreceptors, glial cells and extracellular space in the drone retina: changes during photostimulation.

作者信息

Coles J A, Tsacopoulos M

出版信息

J Physiol. 1979 May;290(2):525-49. doi: 10.1113/jphysiol.1979.sp012788.

Abstract
  1. A double-barrelled potassium-sensitive micro-electrode was developed that was fine enough to record intracellular electrical potentials and potassium activities (aK) in the drone retina. 2. aK was measured in the photoreceptor cells, in the pigment (glial) cells, and in the extracellular space, in the superfused, cut, retina. The effect of photostimulation was studied: 20 msec light flashes, intense enough to evoke receptor potentials of maximum amplitude were presented, 1/sec, in a train lasting about 2 min. 3. In photoreceptors with membrane potentials greater than or equal to 50 mV aK in the dark was 79 mM, S.D. = 27 mM, n = 11. During photostimulation aK fell by 21.5 +/- 9.5 mM with a half-time of 30 +/- 22 sec. (A tentative conversion from activities to free concentrations can be made by taking the activity coefficient as 0.70 its value in the Ringer solution). 4. In pigment cells with membrane potentials greater than or equal to 50 mV, aK in the dark was 52 mM, S.D. = 13 mM, n = 11. During photostimulation aK increased by 14 +/- 5 mM. 5. In the extracellular space aK increased during photostimulation with a mean half-time of less than 1.3 sec to a maximum (mean value 14 mM, S.D. = 8.4 mM, n = 22), and then fell to a plateau. 6. It is estimated from the anatomy that the photoreceptors occupy approximately 38% of the total volume of the retina, the pigment cells 57%, and extracellular space 5%. Hence, it seems possible that during photostimulation nearly all the net loss of potassium from the photoreceptors is temporarily stored in the pigment cells. 7. Recordings were made in the extracellular space of the intact animal by passing the electrode through a hole in the cornea. The mean aK in the dark was 7.7 mM, S.E. = 0.4 mM, n = 22. In the superfused retina, aK in the dark was 6.3 mM, S.E. = 0.7 mM, n = 22, even though aK in the Ringer solution was 2.2 mM. Increasing the aK of the Ringer solution to 7.0 mM had no apparent effect on aK in the extracellular space at depths greater than 20 micron. 8. In the intact animal the amplitude and time course of the change in extracellular aK evoked by the standard pattern of photostimulation were within the range observed in the superfused preparation.
摘要
  1. 研制了一种双管钾敏感微电极,其精细程度足以记录雄蜂视网膜中的细胞内电位和钾活性(aK)。2. 在光感受器细胞、色素(神经胶质)细胞以及灌流的离体视网膜的细胞外空间中测量了aK。研究了光刺激的效应:以每秒1次的频率呈现持续约2分钟的20毫秒光脉冲,其强度足以诱发最大幅度的感受器电位。3. 在膜电位大于或等于50 mV的光感受器中,暗处的aK为79 mM,标准差 = 27 mM,n = 11。光刺激期间,aK下降了21.5 +/- 9.5 mM,半衰期为30 +/- 22秒。(通过将活度系数视为其在林格溶液中的值0.70,可以进行从活性到游离浓度的初步换算)。4. 在膜电位大于或等于50 mV的色素细胞中,暗处的aK为52 mM,标准差 = 13 mM,n = 11。光刺激期间,aK增加了14 +/- 5 mM。5. 在细胞外空间中,光刺激期间aK增加,平均半衰期小于1.3秒,达到最大值(平均值14 mM,标准差 = 8.4 mM,n = 22),然后降至平稳状态。6. 根据解剖结构估计,光感受器约占视网膜总体积的38%,色素细胞占57%,细胞外空间占5%。因此,在光刺激期间,光感受器中几乎所有钾的净损失似乎都暂时储存在色素细胞中。7. 通过将电极穿过完整动物角膜上的一个孔,在其细胞外空间进行记录。暗处的平均aK为7.7 mM,标准误 = 0.4 mM,n = 22。在灌流的视网膜中,暗处的aK为6.3 mM, 标准误 = 0.7 mM,n = 22,尽管林格溶液中的aK为2.2 mM。将林格溶液的aK增加到7.0 mM对深度大于20微米处的细胞外空间中的aK没有明显影响。8. 在完整动物中,由标准光刺激模式诱发的细胞外aK变化的幅度和时间进程在灌流制剂中观察到的范围内。

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