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大鼠原位肝细胞跨膜电位梯度的调节。

Regulation of transmembrane electrical potential gradient in rat hepatocytes in situ.

作者信息

Fitz J G, Scharschmidt B F

出版信息

Am J Physiol. 1987 Jan;252(1 Pt 1):G56-64. doi: 10.1152/ajpgi.1987.252.1.G56.

DOI:10.1152/ajpgi.1987.252.1.G56
PMID:3812689
Abstract

The transmembrane electrical potential gradient (Em) has been measured in hepatocytes from intact anesthetized rats using conventional intracellular microelectrodes under a variety of conditions. Em measurements in control animals were normally distributed around a mean of -35.5 +/- 4.6 mV (SD) with a coefficient of variation (CV) of 13.1% and a range of -26 to -54 mV. In individual livers, however, measurements of Em at a given point in time exhibited little cell-to-cell variation (cv of 4.5%). The Em was noted to fluctuate spontaneously over time and to change consistently in response to a variety of physiological stimuli including fasting (depolarization to -28.5 +/- 3.8 mV) and infusion of glucagon in physiological amounts (hyperpolarization to -45.0 +/- 1.8 mV). Hepatocyte Em abruptly depolarized (2-5 mV) after an intravenous bolus of taurocholate (3 mumol) or alanine (45 mumol), suggesting that both solutes exhibit electrogenic uptake. The Em returned to or below preinfusion values within 5 min. Continued infusion of alanine (10.8 mumol/min), but not taurocholate (810 nmol/min), caused a sustained and unexpected hyperpolarization of Em of 8.2 +/- 3.1 mV that lasted at least 60 min. In separate studies, alanine administration did not alter the biliary excretion of a taurocholate load. Taken together, these observations demonstrate that rat hepatocytes in situ are tightly coupled electrically and that physiological stimuli, including fasting, glucagon, and sodium-coupled solute uptake can change Em considerably over time. The late hyperpolarization of Em caused by alanine appears to offset the rise in intracellular Na+ associated with alanine uptake and preserve the Na+ electrochemical gradient such that Na+-coupled taurocholate transport is maintained.

摘要

使用传统的细胞内微电极,在多种条件下对完整麻醉大鼠的肝细胞跨膜电位梯度(Em)进行了测量。对照动物的Em测量值呈正态分布,平均值为-35.5±4.6 mV(标准差),变异系数(CV)为13.1%,范围为-26至-54 mV。然而,在单个肝脏中,在给定时间点对Em的测量显示细胞间差异很小(CV为4.5%)。Em随时间自发波动,并对包括禁食(去极化至-28.5±3.8 mV)和生理量胰高血糖素输注(超极化至-45.0±1.8 mV)在内的多种生理刺激持续变化。静脉注射牛磺胆酸盐(3 μmol)或丙氨酸(45 μmol)后,肝细胞Em突然去极化(2-5 mV),表明两种溶质均表现出电生成性摄取。Em在5分钟内恢复到输注前值或低于输注前值。持续输注丙氨酸(10.8 μmol/min),但不包括牛磺胆酸盐(810 nmol/min),导致Em持续且意外地超极化8.2±3.1 mV,持续至少60分钟。在单独的研究中,丙氨酸给药未改变牛磺胆酸盐负荷的胆汁排泄。综上所述,这些观察结果表明,原位大鼠肝细胞在电方面紧密耦合,生理刺激,包括禁食、胰高血糖素和钠耦联溶质摄取,可随时间显著改变Em。丙氨酸引起的Em后期超极化似乎抵消了与丙氨酸摄取相关的细胞内Na+升高,并维持了Na+电化学梯度,从而维持了钠耦联牛磺胆酸盐转运。

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