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一种化学磷酸酶对分离的豚鼠心室肌细胞单个钙通道及全细胞钙电流失活的影响。

The effect of a chemical phosphatase on single calcium channels and the inactivation of whole-cell calcium current from isolated guinea-pig ventricular myocytes.

作者信息

Allen T J, Chapman R A

机构信息

British Heart Foundation Research Group, School of Veterinary Science, Bristol, UK.

出版信息

Pflugers Arch. 1995 May;430(1):68-80. doi: 10.1007/BF00373841.

DOI:10.1007/BF00373841
PMID:7545282
Abstract

A chemical phosphatase, butanedione monoxime (BDM, at 12-20 mM), reduced open probability (P0) of single cardiac L-type Ca2+ channels in cell-attached patches from guinea-pig ventricular myocytes, without effect on the amplitude of single-channel current, the mean open time or the mean shorter closed time, but it increased mean longer closed time and caused a fall in channel availability. A decrease in the mean time between first channel opening and last closing within a trace was principally due to an inhibition of the longer periods of activity. As a result, the time course of the mean currents, which resolved into an exponentially declining and a sustained component, was changed by an increase in the rate of the exponential phase and a profound reduction of the sustained current. Essentially similar results were obtained when studying whole-cell Ba2+ currents. The inactivation of the whole-cell Ca2+ currents was composed of two exponentially declining components with the slower showing a significantly greater sensitivity to BDM, an effect that was much more pronounced in myocytes exposed to isoprenaline with adenosine 5'-O-(3-thiotriphosphate) (ATP[gamma S]) in the pipette solution. The actions of BDM, which are the opposite of those produced by isoprenaline, suggest that the level of phosphorylation affects processes involved in the slow regulation of channel activity under basal conditions and that several sites (and probably several kinases) are involved. Channels with an inherently slow inactivation would seem to be converted into channels with a rapid inactivation by a dephosphorylation process.

摘要

一种化学磷酸酶,丁二酮单肟(BDM,浓度为12 - 20 mM),降低了豚鼠心室肌细胞贴附式膜片上单通道心脏L型Ca2+通道的开放概率(P0),而不影响单通道电流幅度、平均开放时间或平均较短关闭时间,但增加了平均较长关闭时间并导致通道可用性下降。一次记录中首次通道开放与最后关闭之间平均时间的减少主要是由于较长活动期受到抑制。结果,分解为指数衰减和持续成分的平均电流的时间进程发生了变化,表现为指数相速率增加和持续电流大幅减少。在研究全细胞Ba2+电流时也得到了基本相似的结果。全细胞Ca2+电流的失活由两个指数衰减成分组成,较慢的成分对BDM表现出明显更高的敏感性,在移液管溶液中含有异丙肾上腺素和腺苷5'-O-(3-硫代三磷酸)(ATP[γS])的心肌细胞中,这种效应更为明显。BDM的作用与异丙肾上腺素产生的作用相反,这表明磷酸化水平影响基础条件下通道活动缓慢调节所涉及的过程,并且涉及多个位点(可能还有多种激酶)。具有内在缓慢失活特性的通道似乎通过去磷酸化过程转变为具有快速失活特性的通道。

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Pflugers Arch. 1993 Jan;422(4):325-31. doi: 10.1007/BF00374287.
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