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大鼠心室肌和血管平滑肌肌浆网再充盈过程中细胞内[Ca2+]的变化。

Changes of intracellular [Ca2+] during refilling of sarcoplasmic reticulum in rat ventricular and vascular smooth muscle.

作者信息

Baró I, O'Neill S C, Eisner D A

机构信息

Department of Veterinary Preclinical Sciences, University of Liverpool.

出版信息

J Physiol. 1993 Jun;465:21-41. doi: 10.1113/jphysiol.1993.sp019664.

Abstract
  1. Intracellular calcium concentration ([Ca2+]i) was measured in single myocytes isolated from either the cardiac ventricle or the mesenteric artery of the rat. 2. In both cardiac and smooth muscle, the application of caffeine produced an increase of [Ca2+]i which spontaneously decayed back to resting levels. In vascular smooth muscle cells, removal of caffeine produced a transient fall of [Ca2+]i to below the resting level. [Ca2+]i then returned to control levels. A transient undershoot of [Ca2+]i on removal of caffeine was also sometimes seen in cardiac cells. When the undershoot was absent in cardiac cells it could be induced by elevating [Ca2+]o. 3. In vascular smooth muscle cells noradrenaline increased [Ca2+]i and an undershoot of [Ca2+]i could be produced by its removal. In cardiac cells a small undershoot could sometimes be seen following the systolic Ca2+ transient produced by electrical stimulation. 4. In both cardiac and vascular cells the time constant of decay of the caffeine response (tau caff) was less than that of the recovery from the undershoot (tau us). On average the ratio tau us:tau caff was about 5 in smooth muscle. In cardiac cells the recovery of the undershoot was also considerably slower than that of the caffeine response. 5. If caffeine was removed before the rise of [Ca2+]i had fully decayed spontaneously then the magnitude of the undershoot was reduced. 6. It is suggested that the undershoot of [Ca2+]i on removal of caffeine results from refilling of the SR decreasing [Ca2+]i. The data from vascular cells can be fitted by this model if the dissociation constant, Kd, of the surface membrane Ca2+ pump for [Ca2+]i is about 1 microM. 7. Using the model, it is concluded from the ratio of the time constants shown above that the caffeine releasable content of the sarcoplasmic reticulum constitutes about 80% of total cellular calcium in both cardiac and smooth muscle.
摘要
  1. 在从大鼠心室或肠系膜动脉分离出的单个肌细胞中测量细胞内钙浓度([Ca2+]i)。2. 在心肌和平滑肌中,应用咖啡因都会使[Ca2+]i升高,随后其会自发衰减至静息水平。在血管平滑肌细胞中,去除咖啡因会使[Ca2+]i短暂降至静息水平以下,然后[Ca2+]i又恢复到对照水平。在心肌细胞中,去除咖啡因时有时也会出现[Ca2+]i的短暂下冲。当心肌细胞中不存在下冲时,可通过提高[Ca2+]o诱导产生。3. 在血管平滑肌细胞中,去甲肾上腺素会增加[Ca2+]i,去除去甲肾上腺素会产生[Ca2+]i的下冲。在心肌细胞中,电刺激产生的收缩期Ca2+瞬变之后有时会出现小的下冲。4. 在心肌细胞和血管细胞中,咖啡因反应衰减的时间常数(tau caff)小于下冲恢复的时间常数(tau us)。在平滑肌中,tau us与tau caff的平均比值约为5。在心肌细胞中,下冲的恢复也比咖啡因反应的恢复慢得多。5. 如果在[Ca2+]i自发升高完全衰减之前去除咖啡因,则下冲的幅度会减小。6. 有人提出,去除咖啡因时[Ca2+]i的下冲是由于肌浆网再充盈导致[Ca2+]i降低所致。如果表面膜Ca2+泵对[Ca2+]i的解离常数Kd约为1 microM,则该模型可以拟合血管细胞的数据。7. 使用该模型,根据上述时间常数的比值得出结论,在心肌和平滑肌中,肌浆网中可被咖啡因释放的钙含量约占细胞总钙含量的80%。

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