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大鼠近端曲管基底外侧膜H⁺/OH⁻/HCO₃⁻转运机制。一种钠偶联的电生性过程。

Mechanism of basolateral membrane H+/OH-/HCO-3 transport in the rat proximal convoluted tubule. A sodium-coupled electrogenic process.

作者信息

Alpern R J

出版信息

J Gen Physiol. 1985 Nov;86(5):613-36. doi: 10.1085/jgp.86.5.613.

Abstract

In order to examine the mechanism of basolateral membrane H+/OH-/HCO-3 transport, a method was developed for the measurement of cell pH in the vivo doubly microperfused rat proximal convoluted tubule. A pH-sensitive fluorescein derivative, (2',7')-bis(carboxyethyl)-(5,6)-carboxyfluorescein, was loaded into cells and relative changes in fluorescence at two excitation wavelengths were followed. Calibration was accomplished using nigericin with high extracellular potassium concentrations. When luminal and peritubular fluids were pH 7.32, cell pH was 7.14 +/- 0.01. Decreasing peritubular pH from 7.32 to 6.63 caused cell pH to decrease from 7.16 +/- 0.02 to 6.90 +/- 0.03. This effect occurred at an initial rate of 2.4 +/- 0.3 pH units/min, and was inhibited by 0.5 mM SITS. Lowering the peritubular sodium concentration from 147 to 25 meq/liter caused cell pH to decrease from 7.20 +/- 0.03 to 6.99 +/- 0.01. The effect of peritubular sodium concentration on cell pH was inhibited by 0.5 mM SITS, but was unaffected by 1 mM amiloride. In addition, when peritubular pH was decreased in the total absence of luminal and peritubular sodium, the rate of cell acidification was 0.2 +/- 0.1 pH units/min, a greater than 90% decrease from that in the presence of sodium. Cell depolarization achieved by increasing the peritubular potassium concentration caused cell pH to increase, an effect that was blocked by peritubular barium or luminal and peritubular sodium removal. Lowering the peritubular chloride concentration from 128 to 0 meq/liter did not affect cell pH. These results suggest the existence of an electrogenic, sodium-coupled H+/OH-/HCO-3 transport mechanism on the basolateral membrane of the rat proximal convoluted tubule.

摘要

为了研究基底外侧膜H⁺/OH⁻/HCO₃⁻转运机制,开发了一种在体内对大鼠近端曲管进行双微灌注时测量细胞pH值的方法。一种对pH敏感的荧光素衍生物(2',7')-双(羧乙基)-(5,6)-羧基荧光素被加载到细胞中,并跟踪两个激发波长下荧光的相对变化。使用尼日利亚菌素和高细胞外钾浓度进行校准。当管腔液和肾小管周围液的pH值为7.32时,细胞pH值为7.14±0.01。将肾小管周围pH值从7.32降至6.63导致细胞pH值从7.16±0.02降至6.90±0.03。这种效应的初始速率为2.4±0.3 pH单位/分钟,并被0.5 mM SITS抑制。将肾小管周围钠浓度从147降至25 meq/升导致细胞pH值从7.20±0.03降至6.99±0.01。肾小管周围钠浓度对细胞pH值的影响被0.5 mM SITS抑制,但不受1 mM氨氯吡咪影响。此外,当在完全没有管腔液和肾小管周围液钠的情况下降低肾小管周围pH值时,细胞酸化速率为0.2±0.1 pH单位/分钟,比有钠存在时降低了90%以上。通过增加肾小管周围钾浓度实现的细胞去极化导致细胞pH值升高,这种效应被肾小管周围钡或去除管腔液和肾小管周围液中的钠所阻断。将肾小管周围氯浓度从128降至0 meq/升不影响细胞pH值。这些结果表明,在大鼠近端曲管的基底外侧膜上存在一种电生的、钠耦联的H⁺/OH⁻/HCO₃⁻转运机制。

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