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小鼠红白血病细胞的质膜电位:测量方法及细胞密度依赖性证据

Plasma membrane potential of murine erythroleukemia cells: approach to measurement and evidence for cell-density dependence.

作者信息

Arcangeli A, Olivotto M

出版信息

J Cell Physiol. 1986 Apr;127(1):17-27. doi: 10.1002/jcp.1041270104.

DOI:10.1002/jcp.1041270104
PMID:3457015
Abstract

The plasmamembrane potential (delta psi p) of murine erythroleukemia (MEL) cells has been determined by measuring the distribution of the lipophilic cation tetraphenylphosphonium (TPP+) across the plasmamembrane. TPP+ accumulation within the cells (experimental accumulation ratio, AR exp) was measured by adding 2 microM TPP+ directly to the culture flasks, avoiding any other perturbation of the experimental system. The mitochondrial contribution to AR exp, evaluated by adding carbonyl cyanide p-trifluoromethoxyphenylhydrazone (FCCP) or 2,4-dinitrophenol (DNP), was apparently negligible in standard cultures, AR exp being substantially the same in either the absence or presence of these uncouplers. However, the addition of oligomycin produced a strong AR exp enhancement, which was abolished by FCCP, suggesting that MEL cell mitochondria are in state 3. The aspecific TPP+ binding was estimated by a new mathematical approach worked out to fit AR exp values measured in the presence of valinomycin at various extracellular K+ concentrations and plotted against the ratio of intracellular to extracellular K+ concentration ([K+]i/[K+]e). This binding was found to be close to zero in MEL cells. By applying the Nernst equation directly to AR exp values, delta psi p of these cells was then measured; this potential varying from -65 mV to -16 mV (inside negative) is inversely related to the cell density on the culture surface on which the cells sediment (cells/cm2; CD). The dependence of delta psi p on CD is practically eliminated by valinomycin and appears to be related to a cell interaction with the culture surface of the flasks, suggesting that in the immediate environment of MEL cells one or more factors are produced that modulate the K+ plasma membrane permeability (PK).

摘要

通过测量亲脂性阳离子四苯基鏻(TPP +)在质膜上的分布,测定了小鼠红白血病(MEL)细胞的质膜电位(δψp)。通过将2μM TPP +直接添加到培养瓶中,避免实验系统受到任何其他干扰,测量细胞内TPP +的积累(实验积累率,AR exp)。通过添加羰基氰化物对三氟甲氧基苯腙(FCCP)或2,4-二硝基苯酚(DNP)评估线粒体对AR exp的贡献,在标准培养中显然可以忽略不计,无论是否存在这些解偶联剂,AR exp基本相同。然而,添加寡霉素会导致AR exp强烈增强,而FCCP可消除这种增强,这表明MEL细胞线粒体处于状态3。通过一种新的数学方法估算非特异性TPP +结合,该方法用于拟合在不同细胞外K +浓度下缬氨霉素存在时测得的AR exp值,并与细胞内与细胞外K +浓度之比([K +] i / [K +] e)作图。发现这种结合在MEL细胞中接近于零。通过将能斯特方程直接应用于AR exp值,然后测量这些细胞的δψp;这种从-65 mV到-16 mV(内负)变化的电位与细胞沉降所在培养表面上的细胞密度(细胞/cm2;CD)成反比。缬氨霉素实际上消除了δψp对CD的依赖性,并且似乎与细胞与培养瓶培养表面的相互作用有关,这表明在MEL细胞的直接环境中产生了一种或多种调节K +质膜通透性(PK)的因子。

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