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二羰花青染料荧光与处于不同唐南平衡状态下的人红细胞膜电位之间的关系。

The relation between dicarbocyanine dye fluorescence and the membrane potential of human red blood cells set at varying Donnan equilibria.

作者信息

Freedman J C, Hoffman J F

出版信息

J Gen Physiol. 1979 Aug;74(2):187-212. doi: 10.1085/jgp.74.2.187.

Abstract

The fluorescence, F, of two dicarbocyanine dyes, diS-C3(5) and diI-C3(5), depends both on the membrane potential, E, and on the intracellular pH, pHc, or human red blood cells. Compositions of isotonic media have been devised in which the equilibrium Donnan potential, E, varies at constant pHc and in which pHc varies at constant E. Dye fluorescence measurements in these suspensions yield calibrations of +1.7 % delta F/mV for diS-C3(5) and +0.6 % delta F/mV for diI-C3 (5). While pHo does not affect F of either dye, changes in pHc of 0.1 unit at constant E cause changes of F equivalent to those induced by 2--3mV. Based on these results, a method is given for estimating changes in E from dye fluorescence in experiments in which E and pHc co-vary. The relation of F to E also depends in a complex way on the type and concentration of cells and dye, and the wavelengths employed. The equilibrium calibration of dye fluorescence, when applied to diffusion potentials induced by 1 microM valinomycin, yields a value for the permeability ratio, PK.VAL/PCl, of 20 +/- 5, in agreement with previous estimates by other methods. The calibration of F is identical both for diffusion potentials and for equilibrium potentials, implying that diC-C3(5) responds to changes in voltage independently of ionic fluxes across the red cell membrane. Changes in the absorption spectra of dye in the presence of red cells in response to changes in E show that formation of nonfluorescent dimers contributes to fluorescence quenching of diS-C3(5). In contrast, only a hydrophobic interaction of dye monomers need be considered for diI-C3(5), indicating the occurrence of a simpler mechanism of fluorescence quenching.

摘要

两种双碳菁染料diS-C3(5)和diI-C3(5)的荧光强度F,既取决于膜电位E,也取决于细胞内pH值(pHc),对于人类红细胞而言也是如此。已设计出等渗介质的组成,其中平衡唐南电位E在恒定pHc下变化,且pHc在恒定E下变化。在这些悬浮液中进行的染料荧光测量得出,diS-C3(5)的校准值为+1.7%ΔF/mV,diI-C3(5)的校准值为+0.6%ΔF/mV。虽然细胞外pH值(pHo)不影响任何一种染料的荧光强度F,但在恒定E下,pHc变化0.1个单位会导致F的变化,其变化量等同于由2 - 3mV引起的变化量。基于这些结果,给出了一种在E和pHc共同变化的实验中,根据染料荧光估计E变化的方法。F与E的关系还以复杂的方式取决于细胞和染料的类型及浓度,以及所采用的波长。当将染料荧光的平衡校准应用于由1微摩尔缬氨霉素诱导的扩散电位时,得出的通透率PK.VAL/PCl值为20±5,这与之前用其他方法的估计结果一致。对于扩散电位和平衡电位,F的校准是相同的,这意味着diC-C3(5)对电压变化的响应与跨红细胞膜的离子通量无关。在红细胞存在的情况下,染料吸收光谱随E的变化表明,非荧光二聚体的形成有助于diS-C3(5)的荧光猝灭。相比之下,对于diI-C3(5),只需考虑染料单体的疏水相互作用,这表明存在一种更简单的荧光猝灭机制。

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