Mechanisms of stretch-induced changes in [Ca2+]i in rat atrial myocytes -: Role of increased troponin C affinity and stretch-activated ion channels

被引:90
|
作者
Tavi, P
Han, CL
Weckström, M
机构
[1] Univ Oulu, Dept Physiol, FIN-90220 Oulu, Finland
[2] Univ Oulu, Dept Phys Sci, Div Biophys, FIN-90220 Oulu, Finland
[3] Univ Oulu, Bioctr Oulu, FIN-90220 Oulu, Finland
关键词
stretch; myocyte; Frank-Starling; Ca2+; action potential;
D O I
10.1161/01.RES.83.11.1165
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
To study the effects of stretch on the function of rat left atrium, we recorded contraction force, calcium transients, and intracellular action potentials (APs) during stretch manipulations. The stretch of the atrium was controlled by intra-atrial pressure. The Frank-Starling behavior of the atrium was manifested as a biphasic increase of the contraction force after increasing the stretch level. The development of the contraction force after step increase of the stretch (intra-atrial pressure from 1 to 3 mm Hg) was accompanied by the increase in the amplitude of the calcium transients (P<0.05, n=4) and decrease in the time constant of the Ca2+ transient decay. The APs of the individual myocytes were also affected by stretch; the duration of the AP was decreased at positive voltages (AP duration at 15% repolarization level, P<0.001; n = 13) and increased at negative voltages (AP duration at 90% repolarization level, P<0.01; n=13). To study the mechanisms causing these changes we developed a mathematical model describing [Ca2+](i) and electrical behavior of single rat atrial myocytes. Stretch was simulated in the model by increasing the troponin (TnC) sensitivity and/or applying a stretch-activated (SA) calcium influx. We mimicked the Ca2+ influx by introducing a nonselective cationic conductance, the SA channels, into the membrane. Neither of the 2 plausible mechanosensors (TnC or SA channels) alone could produce similar changes in the Ca2+ transients or APs as seen in the experiments. The model simulated the effects of stretch seen in experiments best when both the TnC affinity and the SA conductance activation were applied simultaneously. The SA channel activation led to gradual augmentation of Ca2+ transients, which modulated the APs through increased Na+/Ca2+-exchanger inward current. The role of TnC affinity change was to modulate the Ca2+ transients, stabilize the diastolic [Ca2+](i) and presumably to produce the immediate increase of the contraction force after stretch seen in experiments. Furthermore, we found that the same mechanism that caused the normal physiological responses to stretch could also generate arrhythmogenic afterpotentials at high stretch levels in the model.
引用
收藏
页码:1165 / 1177
页数:13
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