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从分离的肌浆网中快速释放钙是通过附着的横管系统触发的。

Rapid calcium release from the isolated sarcoplasmic reticulum is triggered via the attached transverse tubular system.

作者信息

Ikemoto N, Antoniu B, Kim D H

出版信息

J Biol Chem. 1984 Nov 10;259(21):13151-8.

PMID:6490650
Abstract

Rapid replacement of 0.15 M K gluconate with 0.15 M choline Cl led to multiphasic Ca2+ release from a heavy fraction of rabbit skeletal muscle microsomes. Following the initial lag period (0-50 ms), about 15 nmol of Ca2+/mg of protein was rapidly released with first-order rate constants k = 60-140 s-1. Subsequently, a larger amount of Ca2+ (up to 56 nmol/mg) was released at a slower rate (k = 0.8-1.5 s-1). The Ca2+ released in both rapid and slow phases was reaccumulated within 60 s. In agreement with a previous report (Caswell, A. H., Lau, Y. H., Garcia, M., and Brunschwig, J-P. (1979) J. Biol. Chem. 254, 202-208), French press treatment of the tubule/sarcoplasmic reticulum (SR) complex results in dissociation of transverse tubular membrane (T-tubules) from SR. Subsequent incubation with 0.4 M potassium cacodylate results in the reassociation of the complex, as shown by sucrose density-gradient sedimentation. Upon T-tubule dissociation, both rapid and slow Ca2+ release was inhibited. Upon reassociation, the rapid Ca2+ release was completely restored and the slow phase partially restored. The results indicate that the T-tubule associated with SR plays a crucial role in triggering rapid Ca2+ release induced by ionic replacement. Other types of Ca2+ release, e.g. those induced by Ca2+ alone or with drugs such as caffeine and quercetin, are unaffected by T-tubule dissociation, and hence produced by direct stimulation of the SR membrane.

摘要

用0.15 M氯化胆碱快速替换0.15 M葡萄糖酸钾会导致兔骨骼肌微粒体的重组分出现多相Ca2+释放。在初始延迟期(0 - 50毫秒)之后,约15 nmol的Ca2+/mg蛋白质以一级速率常数k = 60 - 140 s-1快速释放。随后,大量的Ca2+(高达56 nmol/mg)以较慢的速率(k = 0.8 - 1.5 s-1)释放。在快速和慢速阶段释放的Ca2+在60秒内重新积累。与之前的一份报告(Caswell, A. H., Lau, Y. H., Garcia, M., and Brunschwig, J-P. (1979) J. Biol. Chem. 254, 202 - 208)一致,用法国压榨机处理小管/肌浆网(SR)复合体导致横管膜(T小管)与SR解离。随后用0.4 M二甲胂酸钾孵育会导致复合体重新结合,蔗糖密度梯度沉降显示了这一点。在T小管解离时,快速和慢速Ca2+释放均受到抑制。重新结合后,快速Ca2+释放完全恢复,慢速阶段部分恢复。结果表明,与SR相关的T小管在触发离子替换诱导的快速Ca2+释放中起关键作用。其他类型的Ca2+释放,例如仅由Ca2+或与咖啡因和槲皮素等药物一起诱导的释放,不受T小管解离的影响,因此是由SR膜的直接刺激产生的。

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