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高细胞外钙引起的大鼠降钙素分泌细胞系中的膜去极化和细胞内钙离子增加。

Membrane depolarization and intracellular Ca2+ increase caused by high external Ca2+ in a rat calcitonin-secreting cell line.

作者信息

Yamashita N, Hagiwara S

机构信息

Department of Physiology, Jerry Lewis Neuromuscular Research Center, University of California School of Medicine, Los Angeles 90024.

出版信息

J Physiol. 1990 Dec;431:243-67. doi: 10.1113/jphysiol.1990.sp018329.

Abstract
  1. Calcitonin secretion is regulated by the external Ca2+ concentration ([Ca2+]o) via a rise in intracellular Ca2+ concentration ([Ca2+]i). The mechanism which couples an increase in [Ca2+]o to an increase in [Ca2+]i was explored in a rat calcitonin-secreting cell line (rMTC 44-2). [Ca2+]i was monitored using Fura-2 AM, and the membrane potential or current was simultaneously measured. 2. Using the conventional whole-cell clamp, tetrodotoxin-sensitive voltage-gated Na+ channels, T- and L-type Ca2+ channels, and three types of K+ channels, the delayed K+ channel, the A-channel and the inward-rectifying channel were observed. 3. Using the nystatin-perforated whole-cell-clamp technique, the resting potential measured under current clamp in standard extracellular medium was -59.0 +/- 5.0 mV (mean +/- S.D., n = 25), and the input resistance was 3.9 +/- 1.9 G omega (n = 10). In 0.5 mM [Ca2+]o most cells (22/25) showed spontaneous action potentials. 4. An increase in [Ca2+]o depolarized the cell membrane and elevated [Ca2+]i even in the presence of 10 microM-tetrodotoxin. The rise in [Ca2+]i was greatly reduced when action potentials were inhibited by applying hyperpolarizing current. The increase in [Ca2+]i saturated with 3-4 mM [Ca2+]o. In 3 mM [Ca2+]o, [Ca2+]i was 188.9 +/- 40.5% (n = 12) of that in 0.5 mM [Ca2+]o. 5. In high [Ca2+]o the duration of action potentials was prolonged, but the action potential frequency did not always increase. In some cases it even decreased in high [Ca2+]o. 6. Two types of action potential were observed in high [Ca2+]o, one with a shorter duration and the other with a longer duration. [Ca2+]i transiently increased in association with the long-duration action potentials. These long-duration action potentials were also accompanied by a larger after-hyperpolarization. 7. Under voltage clamp, high [Ca2+]o caused a membrane conductance increase to Na+ ions. 8. Even when the membrane potential was clamped at a level below the threshold for Ca2+ channel activation, high [Ca2+]o provoked an increase of [Ca2+]i which was composed of an initial transient increase followed by a sustained increase, indicating an involvement of mechanisms other than Ca2+ influx through voltage-gated channels. The sustained increase was more frequently observed than the initial transient increase. The amplitude of the sustained phase was dependent on [Ca2+]o, and in 5 mM [Ca2+]o it was 120.9 +/- 18.9% (103-194%) (n = 58) of that in 0.5 mM [Ca2+]o.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 降钙素的分泌通过细胞内钙离子浓度([Ca2+]i)的升高受细胞外钙离子浓度([Ca2+]o)的调节。在大鼠降钙素分泌细胞系(rMTC 44-2)中研究了将[Ca2+]o的增加与[Ca2+]i的增加联系起来的机制。使用Fura-2 AM监测[Ca2+]i,并同时测量膜电位或电流。2. 使用传统的全细胞钳制技术,观察到了河豚毒素敏感的电压门控钠离子通道、T型和L型钙离子通道以及三种钾离子通道,即延迟钾通道、A通道和内向整流通道。3. 使用制霉菌素穿孔全细胞钳制技术,在标准细胞外培养基中电流钳制下测得的静息电位为-59.0±5.0 mV(平均值±标准差,n = 25),输入电阻为3.9±1.9 GΩ(n = 10)。在0.5 mM [Ca2+]o时,大多数细胞(22/25)表现出自发动作电位。4. [Ca2+]o的增加使细胞膜去极化并升高[Ca2+]i,即使在存在10 μM河豚毒素的情况下也是如此。当通过施加超极化电流抑制动作电位时,[Ca2+]i的升高大大降低。[Ca2+]i的增加在3 - 4 mM [Ca2+]o时达到饱和。在3 mM [Ca2+]o时,[Ca2+]i是0.5 mM [Ca2+]o时的188.9±40.5%(n = 12)。5. 在高[Ca2+]o时,动作电位的持续时间延长,但动作电位频率并不总是增加。在某些情况下,在高[Ca2+]o时甚至会降低。6. 在高[Ca2+]o时观察到两种类型的动作电位,一种持续时间较短,另一种持续时间较长。[Ca2+]i与持续时间较长的动作电位相关联而短暂增加。这些持续时间较长的动作电位还伴有较大的超极化后电位。7. 在电压钳制下,高[Ca2+]o导致对钠离子的膜电导增加。8. 即使将膜电位钳制在低于钙离子通道激活阈值的水平,高[Ca2+]o也会引发[Ca2+]i的增加,这由初始的短暂增加和随后的持续增加组成,表明除了通过电压门控通道的钙离子内流之外还涉及其他机制。持续增加比初始短暂增加更频繁地被观察到。持续期的幅度取决于[Ca2+]o,在5 mM [Ca2+]o时,它是0.5 mM [Ca2+]o时的120.9±18.9%(103 - 194%)(n = 58)。

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