首页> 美国卫生研究院文献>Biophysical Journal >Simultaneous measurements of intracellular pH in the leech giant glial cell using 27-bis-(2-carboxyethyl)-56-carboxyfluorescein and ion-sensitive microelectrodes.
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Simultaneous measurements of intracellular pH in the leech giant glial cell using 27-bis-(2-carboxyethyl)-56-carboxyfluorescein and ion-sensitive microelectrodes.

机译:使用27-双-(2-羧乙基)-56-羧基荧光素和离子敏感微电极同时测量水ech巨大神经胶质细胞的细胞内pH。

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摘要

We have employed two independent techniques to measure the intracellular pH (pHi) in giant glial cells of the leech Hirudo medicinalis, using the fluorescent dye 2',7'-bis-(2-carboxyethyl)-5,6-carboxyfluorescein (BCECF) and double-barreled neutral-carrier, pH-sensitive microelectrodes, which also record the membrane potential. We have compared two procedures for calibrating the ratio of the BCECF signal, excited at 440 nm and 495 nm: 1) the cell membrane was H(+)-permeabilized with nigericin in high-K+ saline at different external pH (pHo) values, and 2) the pHi of intact cells was perturbed in CO2/HCO3(-) -buffered saline of different pH, and the BCECF ratio was calibrated according to a simultaneous microelectrode pH reading. As indicated by the microelectrode measurements, the pHi did not fully equilibrate to the pHo values in nigericin-containing, high-K+ saline, but deviated by -0.12 +/- 0.02 (mean +/- SEM, n = 37) pH units. In intact cells, the microelectrode readings yielded up to 0.15 pH unit lower values than the calibrated BCECF signal. In addition, larger dye injections into the cells (> 100 microM) caused an irreversible membrane potential loss indicative of some damage to the cells. The amplitude and kinetics of slow pHi changes were equally followed by both sensors, and the dye ratio recorded slightly higher amplitudes during faster pHi shifts as induced by the addition and removal of NH4+.
机译:我们已使用两种独立的技术,使用荧光染料2',7'-双-(2-羧乙基)-5,6-羧基荧光素(BCECF),来测量水ech水giant巨胶质细胞的细胞内pH(pHi)。以及双管中性载体,pH敏感的微电极,它们也记录膜电位。我们比较了两种校准440 nm和495 nm激发的BCECF信号比例的方法:1)在不同外部pH(pHo)值下,在高K +盐溶液中用尼日利亚菌素对细胞膜进行H(+)渗透, 2)将完整细胞的pHi在不同pH的CO2 / HCO3(-)缓冲盐水中扰动,并根据微电极的同时pH读数校准BCECF比率。如微电极测量所示,pHi不能完全平衡至含尼日菌的高K +盐水中的pHo值,但会偏离-0.12 +/- 0.02(平均值+/- SEM,n = 37)pH单位。在完整的细胞中,微电极读数比校准的BCECF信号低0.15个pH单位。此外,向细胞中注入较大的染料(> 100 microM)会导致不可逆的膜电位损失,这表明细胞受到了一定程度的损害。两个传感器均等地跟踪缓慢pHi变化的幅度和动力学,并且在由于添加和去除NH4 +引起的较快pHi移动期间,染料比率记录了稍高的幅度。

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