光释放的肌醇1,4,5 -三磷酸诱导大鼠门静脉单个平滑肌细胞的反应。

Photoreleased inositol 1,4,5-trisphosphate-induced response in single smooth muscle cells of rat portal vein.

作者信息

Loirand G, Grégoire G, Pacaud P

机构信息

URA CNRS 1489, Bordeaux, France.

出版信息

J Physiol. 1994 Aug 15;479 ( Pt 1)(Pt 1):41-52. doi: 10.1113/jphysiol.1994.sp020276.

DOI:10.1113/jphysiol.1994.sp020276

PMID:7990034

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1155724/

Abstract

The Ca2+ release in response to inositol 1,4,5-trisphosphate (InsP3) was studied in single patch-clamped smooth muscle cells of rat portal vein. InsP3 was photochemically produced from a caged InsP3 precursor included in the pipette solution. Changes in internal Ca2+ concentration ([Ca2+]i) were monitored by measuring Ca(2+)-activated K+ current. 2. Photoreleased InsP3 evoked a transient K+ current which was abolished when 10 mM EGTA or 5 mg ml-1 heparin was included in the pipette. The amplitude and time course of the K+ current responses depended on the light-flash intensity. The amplitude increased, and the latency and the time to peak decreased, with increasing flash intensity, suggesting that the amount of released Ca2+ varied as a function of the amount of InsP3 photoreleased. 3. The K+ current response to photolysis of caged InsP3 was abolished in the presence of 10 mM caffeine; conversely, caffeine was inefficient at inducing at K+ current when applied immediately after a light flash of maximal intensity. 4. The time course of the recovery of the K+ response evoked by a light flash of supramaximal intensity was similar to that obtained for the 10 mM caffeine-induced K+ current. The response recovered to 50% of control with an interval (t1/2) of about 10 s between pulses. The time course of the recovery of submaximal response to photoreleased InsP3 was considerably slower (t1/2 = 1 min), and did not correspond to that obtained for a response of similar amplitude evoked by 2 mM caffeine. 5. Responses to photoreleased InsP3 obtained after the cells were bathed for 3 min in Ca(2+)-free solution were compared with those obtained in 2 mM Ca2+ solution. Responses to light flashes of submaximal intensity were proportionally more inhibited than those evoked by supramaximal stimulations. 6. In portal vein smooth muscle cells, the InsP3-sensitive Ca2+ store seems also to be sensitive to caffeine. Our results suggest that the InsP3-induced Ca2+ release was modulated by regulatory mechanisms.

摘要

在大鼠门静脉的单个膜片钳制平滑肌细胞中研究了对肌醇1,4,5 - 三磷酸（InsP3）的Ca2+释放。InsP3由移液管溶液中包含的笼形InsP3前体光化学产生。通过测量Ca(2+)-激活的K+电流监测细胞内Ca2+浓度（[Ca2+]i）的变化。2. 光释放的InsP3诱发瞬时K+电流，当移液管中加入10 mM乙二醇双乙醚四乙酸（EGTA）或5 mg/ml肝素时该电流消失。K+电流响应的幅度和时间进程取决于闪光强度。随着闪光强度增加，幅度增大，潜伏期和达到峰值的时间缩短，表明释放的Ca2+量随光释放的InsP3量而变化。3. 在10 mM咖啡因存在下，对笼形InsP3光解的K+电流响应消失；相反，在最大强度闪光后立即施加咖啡因时，咖啡因诱导K+电流的效率较低。4. 超最大强度闪光诱发的K+响应的恢复时间进程与10 mM咖啡因诱导的K+电流的相似。响应在脉冲之间间隔约10 s（t1/2）恢复到对照的50%。对光释放的InsP3的次最大响应的恢复时间进程相当慢（t1/2 = 1分钟），且与2 mM咖啡因诱发的类似幅度响应的不同。5. 将细胞在无Ca2+溶液中孵育3分钟后对光释放的InsP3的响应与在2 mM Ca2+溶液中获得的响应进行比较。次最大强度闪光的响应相比超最大刺激诱发的响应受到的抑制比例更大。6. 在门静脉平滑肌细胞中，InsP3敏感的Ca2+储存似乎也对咖啡因敏感。我们的结果表明InsP3诱导的Ca2+释放受调节机制调控。