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完整淋巴细胞中的钙稳态:用一种新的细胞内捕获荧光指示剂监测细胞质游离钙。

Calcium homeostasis in intact lymphocytes: cytoplasmic free calcium monitored with a new, intracellularly trapped fluorescent indicator.

作者信息

Tsien R Y, Pozzan T, Rink T J

出版信息

J Cell Biol. 1982 Aug;94(2):325-34. doi: 10.1083/jcb.94.2.325.

DOI:10.1083/jcb.94.2.325
PMID:6980885
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2112871/
Abstract

A new, fluorescent, highly selective Ca2+ indicator , "quin2", has been trapped inside intact mouse and pig lymphocytes, to measure and manipulate cytoplasmic free Ca2+ concentrations, [Ca2+]i. Quin2 is a tetracarboxylic acid which binds Ca2+ with 1:1 stoichiometry and an effective dissociation constant of 115 nM in a cationic background mimicking cytoplasm. Its fluorescence signal (excitation 339 nm, emission 492 nm) increases about fivefold going from Ca-free to CA-saturated forms. Cells are loaded with quin2 by incubation with its acetoxymethyl ester, which readily permeates the membrane and is hydrolyzed in the cytoplasm, thus trapping the impermeant quin2 there. The intracellular quin2 appears to be free in cytoplasm, not bound to membranes and not sequestered inside organelles. The fluorescence signal from resting cells indicates a [Ca2+]i of near 120 nM. The millimolar loadings of quin2 needed for accurately calibrated signals do not seem to perturb steady-state [Ca2+]i, but do somewhat slow or blunt [Ca2+]i transients. Loadings of up to 2mM are without serious toxic effects, though above this level some lowering of cellular ATP is observed. [Ca2+]i was well stabilized in the face of large changes in external Ca2+. Alterations of Na+ gradients, membrane potential, or intracellular pH had little effect. Mitochondrial poisons produced a small increase in [Ca2+]i, probably due mostly to the effects of severe ATP depletion on the plasma membrane. Thus intracellulary trapped chelators like quin2 offer a method to measure or buffer [Ca2+]i in hitherto intractable cell types.

摘要

一种新型的、荧光性的、高选择性钙离子指示剂“喹啉-2”(quin2)已被载入完整的小鼠和猪淋巴细胞内,用于测量和调控细胞质游离钙离子浓度[Ca²⁺]i。喹啉-2是一种四羧酸,它与钙离子以1:1化学计量比结合,在模拟细胞质的阳离子背景下,有效解离常数为115 nM。其荧光信号(激发波长339 nm,发射波长492 nm)从无钙形式转变为钙饱和形式时增加约五倍。通过与乙酰氧基甲酯一起孵育,细胞被载入喹啉-2,乙酰氧基甲酯能轻易透过细胞膜并在细胞质中水解,从而将不能透过膜的喹啉-2截留在那里。细胞内的喹啉-2似乎在细胞质中是游离的,不与膜结合,也不被隔离在细胞器内。静息细胞的荧光信号表明[Ca²⁺]i接近120 nM。为获得精确校准信号所需的毫摩尔浓度的喹啉-2载入量似乎不会干扰稳态[Ca²⁺]i,但会在一定程度上减缓或减弱[Ca²⁺]i瞬变。高达2 mM的载入量没有严重的毒性作用,不过高于此水平会观察到细胞ATP有所降低。面对外部钙离子的大幅变化,[Ca²⁺]i能很好地保持稳定。钠离子梯度、膜电位或细胞内pH的改变影响很小。线粒体毒物使[Ca²⁺]i略有增加,这可能主要是由于严重的ATP耗竭对质膜的影响。因此,像喹啉-2这样细胞内截留的螯合剂为测量或缓冲迄今为止难以处理的细胞类型中的[Ca²⁺]i提供了一种方法。

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Calcium homeostasis in intact lymphocytes: cytoplasmic free calcium monitored with a new, intracellularly trapped fluorescent indicator.完整淋巴细胞中的钙稳态:用一种新的细胞内捕获荧光指示剂监测细胞质游离钙。
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