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在去表皮犬心脏浦肯野细胞中,水母发光蛋白检测到的钙瞬变过程中的快速离子修饰。

Rapid ionic modifications during the aequorin-detected calcium transient in a skinned canine cardiac Purkinje cell.

作者信息

Fabiato A

出版信息

J Gen Physiol. 1985 Feb;85(2):189-246. doi: 10.1085/jgp.85.2.189.

Abstract

A microprocessor-controlled system of microinjections and microaspirations has been developed to change, within approximately 1 ms, the [free Ca2+] at the outer surface of the sarcoplasmic reticulum (SR) wrapped around individual myofibrils (0.3-0.4 micron radius) of a skinned canine cardiac Purkinje cell (2.5-4.5 micron overall radius) at different phases of a Ca2+ transient. Simultaneously monitoring tension and aequorin bioluminescence provided two methods for estimating the peak myoplasmic [free Ca2+] reached during the spontaneous cyclic Ca2+ release from the SR obtained in the continuous presence of a bulk solution [free Ca2+] sufficiently high to overload the SR. These methods gave results in excellent agreement for the spontaneous Ca2+ release under a variety of conditions of pH and [free Mg2+], and of enhancement of Ca2+ release by calmodulin. Disagreement was observed, however, when the Ca2+ transient was modified during its ascending phase. The experiments also permitted quantification of the aequorin binding within the myofibrils and determination of its operational apparent affinity constant for Ca2+ at various [free Mg2+] levels. An increase of [free Ca2+] at the outer surface of the SR during the ascending phase of the Ca2+ transient induced further release of Ca2+. In contrast, an increase of [free Ca2+] during the descending phase of the Ca2+ transient did not cause further Ca2+ release. Varying [free H+], [free Mg2+], or the [Na+]/[K+] ratio had no significant effect on the Ca2+ transient during which the modification was applied, but it altered the subsequent Ca2+ transient. Therefore, Ca2+ appears to be the major, if not the only, ion controlling Ca2+ release from the SR rapidly enough to alter a Ca2+ transient during its course.

摘要

已开发出一种微处理器控制的微注射和微抽吸系统,用于在约1毫秒内改变包裹在去皮犬心脏浦肯野细胞(总半径2.5 - 4.5微米)单个肌原纤维(半径0.3 - 0.4微米)周围肌浆网(SR)外表面的[游离Ca2+],且处于Ca2+瞬变的不同阶段。同时监测张力和水母发光蛋白生物发光提供了两种方法,用于估计在大量溶液[游离Ca2+]持续存在且足够高以使SR过载的情况下,从SR自发循环Ca2+释放过程中达到的肌浆峰值[游离Ca2+]。这些方法在各种pH和[游离Mg2+]条件下以及钙调蛋白增强Ca2+释放的情况下,对自发Ca2+释放给出了非常一致的结果。然而,当Ca2+瞬变在其上升阶段被改变时,观察到了差异。这些实验还允许对肌原纤维内的水母发光蛋白结合进行定量,并确定其在各种[游离Mg2+]水平下对Ca2+的操作表观亲和常数。在Ca2+瞬变上升阶段,SR外表面[游离Ca2+]的增加诱导了Ca2+的进一步释放。相反,在Ca2+瞬变下降阶段[游离Ca2+]的增加并未导致Ca2+的进一步释放。改变[游离H+]、[游离Mg2+]或[Na+]/[K+]比值对施加改变时的Ca2+瞬变没有显著影响,但会改变随后的Ca2+瞬变。因此,Ca2+似乎是主要的(如果不是唯一的)离子,它能足够快地控制从SR释放Ca2+,从而在其过程中改变Ca2+瞬变。

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