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豚鼠平滑肌去极化和药物机械偶联过程中的游离钙和力瞬变

Free-calcium and force transients during depolarization and pharmacomechanical coupling in guinea-pig smooth muscle.

作者信息

Himpens B, Somlyo A P

机构信息

Pennsylvania Muscle Institute, University of Pennsylvania, School of Medicine, Philadelphia 19104-6083.

出版信息

J Physiol. 1988 Jan;395:507-30. doi: 10.1113/jphysiol.1988.sp016932.

Abstract
  1. Fura2 was loaded by permeation and hydrolysis of the acetoxymethyl ester into smooth muscle cells of intact thin sheets of the longitudinal layer of the small intestine of the guinea-pig, to record Ca2+ transients during contraction. 2. Cytoplasmic Ca2+ ([Ca2+]i) was monitored by computing the ratio of the fluorescence signal excited at 340 and 380 nm wavelengths. The dye loading and the exposure to UV light required for the experiments had no significant effect on the contractile parameters observed. 3. Spontaneous, rhythmic increases in [Ca2+]i were often observed, preceding the onset of force. Removal of extracellular Ca2+ caused a very transient increase in [Ca2+]i accompanied by a phasic force transient; this was followed by a decline in [Ca2+]i and tension below control levels. Elevated Ca2+ from 1.2 to 15 mM also caused a fall in [Ca2+]i and a relaxation of basal tension. 4. Elevation of [K+]o increased [Ca2+]i. Graded concentrations of K+ caused graded changes in both fluorescence ratio and tension. 5. Carbachol evoked a transient increase in [Ca2+]i and contraction. Thereafter, in spite of the continued presence of the drug, both signals declined, presumably as the result of cholinergic desensitization. The initial phasic force response to carbachol was usually followed by an 'after-contraction', that was only occasionally accompanied by a similar (small) secondary rise in the fluorescence signal. 6. In depolarized smooth muscle, both in the presence and in the absence of extracellular Ca2+, carbachol induced a transient increase in [Ca2+]i, indicating that Ca2+ release from intracellular stores is a major mechanism of pharmacomechanical coupling. 7. In some preparations an applied stretch caused, after a few seconds, a rise in [Ca2+]i and force development.
摘要
  1. 通过乙酰氧甲基酯的渗透和水解将Fura2加载到豚鼠小肠纵肌层完整薄片的平滑肌细胞中,以记录收缩过程中的Ca2+瞬变。2. 通过计算在340和380 nm波长激发的荧光信号的比率来监测细胞质Ca2+([Ca2+]i)。实验所需的染料加载和紫外线照射对观察到的收缩参数没有显著影响。3. 经常观察到在力量开始之前,[Ca2+]i会自发、有节奏地增加。去除细胞外Ca2+会导致[Ca2+]i非常短暂的增加,并伴有阶段性力量瞬变;随后[Ca2+]i和张力下降至对照水平以下。将Ca2+从1.2 mM升高到15 mM也会导致[Ca2+]i下降和基础张力松弛。4. 升高[K+]o会增加[Ca2+]i。不同浓度的K+会导致荧光比率和张力的分级变化。5. 卡巴胆碱引起[Ca2+]i短暂增加和收缩。此后,尽管药物持续存在,但两个信号都下降了,推测是胆碱能脱敏的结果。对卡巴胆碱的初始阶段性力量反应通常会接着出现“后收缩”,这种后收缩仅偶尔伴有荧光信号类似的(小的)二次升高。6. 在去极化的平滑肌中,无论有无细胞外Ca2+,卡巴胆碱都会诱导[Ca2+]i短暂增加,表明从细胞内储存释放Ca2+是药物机械偶联的主要机制。7. 在一些制剂中,施加的拉伸在几秒钟后会导致[Ca2+]i升高和力量发展。

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Am J Physiol. 1960 Sep;199:553-9. doi: 10.1152/ajplegacy.1960.199.3.553.
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