[犬实验性心肌梗死晚期浦肯野纤维异常活动的机制]。

E P Aniukhovskiĭ, G G Beloshapko, L V Rozenshtraukh
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引用次数: 0

摘要

将犬左冠状动脉降支闭塞24小时后缺血区异常活跃的心内膜下浦肯野纤维(PF)根据其对灌注液离子组成变化的反应分为2组。第一组AAPF频率随[Ca2+]o的升高而降低,随[Ca2+]o的降低而升高,并与[Na+]o成正比。第二组AAPF频率在增加[Ca2+]i的作用下升高([Ca+]o升高,[Na+]o降低),在减少[Ca2+]i的作用下下降([Ca2+]o降低,[Na+]o升高)。在短期(10 s)高频刺激后,第一组纤维的AAPF频率保持不变或短暂性减慢。在II组纤维中,高频刺激后的AA频率保持不变或短暂性不显著升高。I群纤维的异常活性可以被河豚毒素阻断,而维拉帕米实际上无效。第二组的异常活动被两种药物阻断。因此,我们得出结论,在PF缺血区LDCA闭塞后一天,可能存在异常自动性和触发机制引起的异常活动。引起异常自动性的起搏器电流可能是由缺血修饰的钠离子通道摄取Na+引起的。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
[Mechanisms of the anomalous activity of the Purkinje fibers in the late stage of experimental myocardial infarct in dogs].

The anomalously active (AA) subendocardial Purkinje's fibers (PF) in the ischemic zone 24 hours after occlusion of the left descending coronary artery (LDCA) in dogs are proposed to be divided into 2 groups according to their reaction to the changes in the ionic composition of perfusion solution. The AAPF frequency in the first group decreased by increase in [Ca2+]o, increased by fall in [Ca2+]o and was proportional to [Na+]o. In the second group AAPF frequency rose under actions increasing [Ca2+]i (increase in [Ca+]o, decrease in [Na+]o), and fell under actions reducing [Ca2+]i (decrease in [Ca2+]o, increase in [Na+]o). After short-term (10 s) high frequency stimulation the AAPF frequency in the group I fibers either remained unchanged or insignificant transitory slowing down was registered. In the group II fibers the AA frequency after high frequency stimulation either remained unchanged or insignificant transitory elevation was observed. The anomalous activity in the group I fibers could be blocked by tetrodotoxin, while verapamil was practically ineffective. In the second group anomalous activity was blocked by both drugs. We conclude thus that one day after the occlusion of LDCA in the ischemic zone PF with anomalous activity caused by anomalous automaticity as well as by trigger mechanism may be present. The pacemaker current inducing anomalous automaticity is possibly caused by Na+ intake through ischemically modified natrium channels.

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