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单个小鼠胰腺β细胞中动作电位和电压钳钙电流引发的胞吐作用。

Exocytosis elicited by action potentials and voltage-clamp calcium currents in individual mouse pancreatic B-cells.

作者信息

Ammälä C, Eliasson L, Bokvist K, Larsson O, Ashcroft F M, Rorsman P

机构信息

Department of Medical Biophysics, Gothenburg University, Sweden.

出版信息

J Physiol. 1993 Dec;472:665-88. doi: 10.1113/jphysiol.1993.sp019966.

DOI:10.1113/jphysiol.1993.sp019966
PMID:8145165
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1160506/
Abstract
  1. Measurements of membrane capacitance, as an indicator of exocytosis, and intracellular Ca2+ concentration ([Ca2+]i) were used to determine the Ca2+ dependence of secretion in single pancreatic B-cells. 2. Exocytosis was dependent on a rise in [Ca2+]i and could be evoked by activation of voltage-dependent Ca2+ currents. The threshold for depolarization-induced release was 0.5 microM [Ca2+]i. Once the [Ca2+]i threshold was exceeded, exocytosis was rapidly (< 50 ms) initiated. When individual pulses were applied, exocytosis stopped immediately upon repolarization and the Ca2+ channels closed, although [Ca2+]i remained elevated for several seconds. 3. During repetitive stimulation (1 Hz), when [Ca2+]i attained micromolar levels, exocytosis also took place during the interpulse intervals albeit at a slower rate than during the depolarizations. 4. Exocytosis could be initiated by simulated action potentials. Whereas a single action potential only produced a small capacitance increase, and in some cells even failed to stimulate release, larger and more consistent responses were obtained with > or = four action potentials. 5. Comparison of the rates of exocytosis measured in response to depolarization, mobilization of Ca2+ from intracellular stores or infusion of Ca2+ through the patch pipette suggests that [Ca2+]i at the secretory sites attains a concentration of several micromolar. This is much higher than the average [Ca2+]i detected by microfluorimetry suggesting the existence of steep spatial gradients of [Ca2+]i within the B-cell. 6. Inclusion of inhibitors of Ca2+/calmodulin-dependent protein kinase II in the intracellular solution reduced the depolarization-induced exocytotic responses suggesting this enzyme may be involved in the coupling between elevation of [Ca2+]i to stimulation of the secretory machinery. 7. The size of the unitary exocytotic event was 2 fF, corresponding to a secretory granule diameter of 250 nm. 8. Over short periods, exocytosis may be extremely fast (1 pF/s or 500 granules/s), which is much higher than the rate of endocytosis (18 fF/s or 9 granules/s). Since the latter is in better agreement with the maximum rate of insulin secretion from islets (approximately 2 granules/s), we suggest that membrane retrieval may set an upper limit on the rate of exocytosis during extended periods of secretion.
摘要
  1. 作为胞吐作用指标的膜电容测量以及细胞内Ca2+浓度([Ca2+]i)测量,被用于确定单个胰腺β细胞中分泌的Ca2+依赖性。2. 胞吐作用依赖于[Ca2+]i的升高,并且可由电压依赖性Ca2+电流的激活所诱发。去极化诱导释放的阈值为0.5微摩尔[Ca2+]i。一旦超过[Ca2+]i阈值,胞吐作用迅速(<50毫秒)启动。当施加单个脉冲时,胞吐作用在复极化时立即停止且Ca2+通道关闭,尽管[Ca2+]i仍升高数秒。3. 在重复刺激(1赫兹)期间,当[Ca2+]i达到微摩尔水平时,胞吐作用在脉冲间隔期间也会发生,尽管其速率比去极化期间慢。4. 胞吐作用可由模拟动作电位引发。单个动作电位仅产生较小的电容增加,并且在一些细胞中甚至未能刺激释放,而≥四个动作电位则可获得更大且更一致的反应。5. 对去极化、细胞内储存库中Ca2+的动员或通过膜片吸管注入Ca2+所测得的胞吐作用速率进行比较表明,分泌位点处的[Ca2+]i达到数微摩尔的浓度。这远高于通过微量荧光测定法检测到的平均[Ca2+]i,提示β细胞内存在[Ca2+]i的陡峭空间梯度。6. 在细胞内溶液中加入Ca2+/钙调蛋白依赖性蛋白激酶II抑制剂可降低去极化诱导的胞吐反应,提示该酶可能参与[Ca2+]i升高与分泌机制刺激之间的偶联。7. 单个胞吐事件的大小为2飞法,对应于直径为250纳米的分泌颗粒。8. 在短时间内,胞吐作用可能极快(1皮法/秒或500个颗粒/秒),这远高于内吞作用的速率(18飞法/秒或9个颗粒/秒)。由于后者与胰岛胰岛素分泌的最大速率(约2个颗粒/秒)更相符,我们认为在长时间分泌期间,膜回收可能为胞吐作用速率设定了上限。

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