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2,3-丁二酮一肟对大鼠心肌力抑制的机制:细胞内钙离子浓度([Ca2+]i)和横桥动力学的作用

Mechanism of force inhibition by 2,3-butanedione monoxime in rat cardiac muscle: roles of [Ca2+]i and cross-bridge kinetics.

作者信息

Backx P H, Gao W D, Azan-Backx M D, Marban E

机构信息

Department of Medicine, Johns Hopkins University School of Medicine, Baltimore, MD 21205.

出版信息

J Physiol. 1994 May 1;476(3):487-500. doi: 10.1113/jphysiol.1994.sp020149.

DOI:10.1113/jphysiol.1994.sp020149
PMID:8057256
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1160462/
Abstract
  1. We investigated the mechanism of force inhibition by 2,3-butanedione monoxime (BDM) on rat cardiac trabeculae. [Ca2+]i was measured by iontophoretic injection of fura-2 salt. Isometric force was recorded at an end-systolic sarcomere length of 2.1-2.2 microns. 2. With an external [Ca2+] of 1 mM, peak twitch force was monotonically reduced with increasing [BMD]; at 5 and 20 mM [BDM], force was 35 and 1% of the control force. In contrast, the mean peak [Ca2+]i during transients was only reduced at [BDM] > or = 10 mM. 3. The duration of the twitch was dramatically reduced by BDM in a dose-dependent fashion with no significant change in the time course of the underlying Ca2+ transients. The abbreviation of twitch force duration was much greater than expected for the observed reduction in peak force by this agent. 4. The mechanism of the inhibition of force by BDM was explored by examining the relationship between twitch force and Ca2+ transients at various values of external [Ca2+]. In the presence of BDM, the steepness of the relationship between peak force and peak [Ca2+]i was reduced compared to control conditions. As a result, significant elevation in the [Ca2+]i transient was unable to reverse the reduction in force observed in the presence of BDM. 5. The direct inhibitory effects of BDM on the contractile system were examined using ryanodine tetani in intact trabeculae to measure the steady-state force-[Ca2+]i relationship. In contrast to the effects on twitch force at 5 mM BDM, maximal force was only reduced to 71% of control. Furthermore, the [Ca2+]i required for half-maximal activation (Ca50) was increased while the Hill coefficient was reduced slightly by BDM. 6. BDM dramatically slowed the rate of rise of tetanic force. At maximal activation, the time required to reach 90% maximal force was prolonged by a factor of 3-8 in the presence of 5 mM BDM. This suggests that the observed reduction in twitch force and steady-state force may result from slowed kinetics of cross-bridge attachment, consistent with recent biochemical studies. 7. The contribution of altered cross-bridge kinetics to the effects of BDM was investigated using a co-operative cross-bridge model of the contractile system. Changing the rate constants for cross-bridge attachment in the model to mimic the reported biochemical effects of BDM reproduced the observed effects of BDM.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 我们研究了2,3 - 丁二酮一肟(BDM)对大鼠心脏小梁力抑制的机制。通过离子导入法注射fura - 2盐来测量细胞内钙离子浓度([Ca2+]i)。在收缩末期肌节长度为2.1 - 2.2微米时记录等长力。

  2. 细胞外钙离子浓度([Ca2+])为1 mM时,随着BDM浓度增加,峰值收缩力单调降低;在BDM浓度为5 mM和20 mM时,力分别为对照力的35%和1%。相比之下,仅在BDM浓度≥10 mM时,瞬态过程中的平均峰值[Ca2+]i才降低。

  3. BDM以剂量依赖方式显著缩短收缩持续时间,而基础钙离子瞬变的时间进程无显著变化。收缩力持续时间的缩短远大于该试剂引起的峰值力降低所预期的值。

  4. 通过研究在不同细胞外[Ca2+]值下收缩力与钙离子瞬变之间的关系,探讨了BDM抑制力的机制。在存在BDM的情况下,与对照条件相比,峰值力与峰值[Ca2+]i之间关系的斜率降低。因此,钙离子瞬变的显著升高无法逆转在BDM存在时观察到的力的降低。

  5. 使用完整小梁中的雷诺丁强直收缩来测量稳态力 - [Ca2+]i关系,以研究BDM对收缩系统产生的直接抑制作用。与5 mM BDM对收缩力的影响相反,最大力仅降至对照的71%。此外,BDM使达到最大激活一半所需的[Ca2+]i(Ca50)增加,同时希尔系数略有降低。

  6. BDM显著减慢强直收缩力的上升速率。在最大激活时,在5 mM BDM存在下,达到最大力90%所需的时间延长了3 - 8倍。这表明观察到的收缩力和稳态力降低可能是由于横桥附着动力学减慢所致,这与最近的生化研究一致。

  7. 使用收缩系统的协同横桥模型研究了改变的横桥动力学对BDM作用的贡献。在模型中改变横桥附着的速率常数以模拟报道的BDM的生化作用,再现了观察到的BDM的作用。(摘要截断于400字)

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