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使用钙离子电极和水母发光蛋白同时测量肌肉中的钙离子。可扩散的细胞质成分降低了水母发光蛋白与钙离子无关的发光。

Simultaneous measurement of Ca2+ in muscle with Ca electrodes and aequorin. Diffusible cytoplasmic constituent reduces Ca(2+)-independent luminescence of aequorin.

作者信息

Blatter L A, Blinks J R

机构信息

Department of Pharmacology, Mayo Foundation, Rochester, Minnesota 55905.

出版信息

J Gen Physiol. 1991 Dec;98(6):1141-60. doi: 10.1085/jgp.98.6.1141.

DOI:10.1085/jgp.98.6.1141
PMID:1783896
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2229069/
Abstract

Estimates of cytoplasmic Ca2+ concentration ([Ca2+]i) were made essentially simultaneously in the same intact frog skeletal muscle fibers with aequorin and with Ca-selective microelectrodes. In healthy fibers under truly resting conditions [Ca2+]i was too low to be measured reliably with either technique. The calibration curves for both indicators were essentially flat in this range of [Ca2+], and the aequorin light signal was uniformly below the level to be expected in the total absence of Ca2+. When [Ca2+]i had been raised to a stable level below the threshold for contracture by increasing [K+]o to 12.5 mM, [Ca2+]i was 38 nM according to aequorin and 59 nM according to the Ca-selective microelectrodes. These values are not significantly different. Our estimates of [Ca2+]i are lower than most others obtained with microelectrodes, probably because the presence of aequorin in the cells allowed us to detect damaging microelectrode impalements that otherwise we would have had no reason to reject. The observation that the light emission from aequorin-injected fibers in normal Ringer solution was below the level expected from the Ca(2+)-independent luminescence of aequorin in vitro was investigated further, with the conclusion that the myoplasm contains a diffusible macromolecule (between 10 and 30 kD) that interacts with aequorin to reduce light emission in the absence of Ca2+.

摘要

利用水母发光蛋白和钙选择性微电极,在同一完整的青蛙骨骼肌纤维中基本同时进行了细胞质钙离子浓度([Ca2+]i)的测定。在真正的静息条件下,健康纤维中的[Ca2+]i过低,无法用这两种技术可靠地测量。在这个[Ca2+]范围内,两种指示剂的校准曲线基本是平的,并且水母发光蛋白的光信号始终低于完全没有Ca2+时预期的水平。当通过将[K+]o提高到12.5 mM使[Ca2+]i升高到低于挛缩阈值的稳定水平时,根据水母发光蛋白测定的[Ca2+]i为38 nM,根据钙选择性微电极测定为59 nM。这些值没有显著差异。我们对[Ca2+]i的估计值低于大多数用微电极获得的其他值,可能是因为细胞中存在水母发光蛋白使我们能够检测到有损伤的微电极刺入,否则我们没有理由拒绝。进一步研究了在正常林格氏液中注射了水母发光蛋白的纤维发出的光低于体外水母发光蛋白的非钙依赖性发光预期水平这一现象,得出的结论是肌浆中含有一种可扩散的大分子(10至30 kD之间),它与水母发光蛋白相互作用,在没有Ca2+的情况下减少发光。

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