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本文引用的文献

1
Interactions between the regulation of the intracellular pH and sodium activity of sheep cardiac Purkinje fibres.绵羊心脏浦肯野纤维细胞内pH调节与钠活性之间的相互作用。
J Physiol. 1980 Jul;304:471-88. doi: 10.1113/jphysiol.1980.sp013337.
2
Intracellular pH.细胞内pH值
Physiol Rev. 1981 Apr;61(2):296-434. doi: 10.1152/physrev.1981.61.2.296.
3
Stoichiometry and ion dependencies of the intracellular-pH-regulating mechanism in squid giant axons.鱿鱼巨大轴突中细胞内pH调节机制的化学计量学和离子依赖性。
J Gen Physiol. 1983 Mar;81(3):373-99. doi: 10.1085/jgp.81.3.373.
4
Intracellular pH regulation in the renal proximal tubule of the salamander. Basolateral HCO3- transport.蝾螈肾近端小管中的细胞内pH调节。基底外侧HCO3-转运。
J Gen Physiol. 1983 Jan;81(1):53-94. doi: 10.1085/jgp.81.1.53.
5
Ca2+ ions can affect intracellular pH in mammalian cardiac muscle.钙离子可影响哺乳动物心肌细胞内的pH值。
Nature. 1983 Feb 10;301(5900):522-4. doi: 10.1038/301522a0.
6
Analysis of Cl- -HCO3(-) exchange during recovery from intracellular acidosis in cardiac Purkinje strands.心脏浦肯野纤维束细胞内酸中毒恢复过程中Cl⁻-HCO₃⁻交换的分析
Am J Physiol. 1984 May;246(5 Pt 1):C391-400. doi: 10.1152/ajpcell.1984.246.5.C391.
7
Voltage-dependent inactivation of inward-rectifying single-channel currents in the guinea-pig heart cell membrane.豚鼠心肌细胞膜内向整流单通道电流的电压依赖性失活
J Physiol. 1984 Feb;347:659-83. doi: 10.1113/jphysiol.1984.sp015089.
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Chloride activity and its control in skeletal and cardiac muscle.骨骼肌和心肌中氯离子活性及其调控
Philos Trans R Soc Lond B Biol Sci. 1982 Dec 1;299(1097):537-48. doi: 10.1098/rstb.1982.0150.
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Effects of monovalent cations on sodium permeability of human red cells.单价阳离子对人体红细胞钠通透性的影响。
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10
Membrane proteins related to anion permeability of human red blood cells. I. Localization of disulfonic stilbene binding sites in proteins involved in permeation.与人类红细胞阴离子通透性相关的膜蛋白。I. 二磺酸芪结合位点在参与通透的蛋白质中的定位。
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绵羊心脏浦肯野纤维中的Na(+)-HCO3-同向转运体

Na(+)-HCO3- symport in the sheep cardiac Purkinje fibre.

作者信息

Dart C, Vaughan-Jones R D

机构信息

University Laboratory of Physiology, Oxford.

出版信息

J Physiol. 1992;451:365-85. doi: 10.1113/jphysiol.1992.sp019169.

DOI:10.1113/jphysiol.1992.sp019169
PMID:1403816
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1176166/
Abstract
  1. Intracellular pH (pHi) was recorded in isolated sheep cardiac Purkinje fibres using liquid sensor ion-selective microelectrodes in conjunction with conventional (3 M-KCl) microelectrodes (to record membrane potential). 2. In HEPES-buffered solution (pH0 7.4), pHi recovery from an intracellular acid load (20 mM-NH4Cl removal) was blocked by 1 mM-amiloride, consistent with the inhibition of Na(+)-H+ exchange. Replacement of the HEPES buffer with CO2-HCO3- caused a transient acidosis followed by an amiloride-resistant recovery of pHi to more alkaline levels (n = 43). This implies the presence of a HCO3(-)-dependent pHi regulatory mechanism. 3. Comparison of the membrane potential with the equilibrium potential for HCO3- ions (EHCO3) estimated during amiloride-resistant pHi recovery, showed that for polarized fibres (membrane potential Em approximately -80 mV), there was a net outward electrochemical driving force for HCO3- ions. Hence the amiloride-resistant pHi recovery cannot be explained in terms of passive HCO3- influx through membrane channels. 4. Removal of external Na+ (Na0+ replaced by N-methyl-D-glucamine) inhibited HCO3(-)-dependent pHi recovery, whereas removal of external Cl- (leading to depletion of internal Cl-; Cl0- replaced by glucuronate) or short-term removal of extracellular K+ had no inhibitory effect. We suggest that a Na(+)-HCO3- co-influx causes the recovery. Replacement of external Na+ with Li+ greatly reduced HCO3(-)-dependent pHi recovery indicating that Li0+ cannot readily substitute for Na0+ on the co-transport. 5. The stilbene drug DIDS (4,4-diisothiocyano-stilbene-disulphonic acid, 500 microM) slowed HCO3(-)-dependent pHi recovery. 6. Depolarization of the membrane potential in high K0+ (44.5 mM) solution or with 5 mM-BaCl2 had no effect upon the rate of HCO3(-)-sensitive pHi recovery. This observation, when coupled with the fact that activation of HCO3(-)-dependent pHi recovery was associated with no consistent change of membrane potential, suggests that the Na(+)-HCO3- co-influx is electroneutral and voltage insensitive. 7. HCO3(-)-dependent pHi recovery was unaffected by the Na(+)-K(+)-2Cl- co-transport inhibitor, bumetanide (150 microM). 8. The contribution of Na(+)-H+ exchange and Na(+)-HCO3- co-transport to net acid efflux was assessed. At a pHi of 6.6, we estimate that the co-transport should account for 20% of total acid equivalent efflux.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 使用液体传感器离子选择性微电极结合传统的(3M - KCl)微电极(用于记录膜电位),在分离的绵羊心脏浦肯野纤维中记录细胞内pH值(pHi)。2. 在HEPES缓冲溶液(pH 7.4)中,1 mM氨氯吡咪可阻断细胞内酸负荷(去除20 mM - NH4Cl)后pHi的恢复,这与抑制Na(+) - H+交换一致。用CO2 - HCO3-取代HEPES缓冲液会导致短暂的酸中毒,随后pHi出现氨氯吡咪抗性恢复至更碱性水平(n = 43)。这意味着存在一种依赖HCO3(-)的pHi调节机制。3. 在氨氯吡咪抗性pHi恢复过程中,将膜电位与估计的HCO3-离子平衡电位(EHCO3)进行比较,结果表明,对于极化纤维(膜电位Em约为 - 80 mV),存在HCO3-离子的净外向电化学驱动力。因此,氨氯吡咪抗性pHi恢复不能用HCO3-通过膜通道的被动内流来解释。4. 去除细胞外Na+(用N - 甲基 - D - 葡糖胺取代Na0+)会抑制依赖HCO3(-)的pHi恢复,而去除细胞外Cl-(导致细胞内Cl-耗竭;用葡糖醛酸盐取代Cl0-)或短期去除细胞外K+则无抑制作用。我们认为是Na(+) - HCO3-共内流导致了恢复。用Li+取代细胞外Na+大大降低了依赖HCO3(-)的pHi恢复,表明Li0+不能轻易替代共转运中的Na0+。5. 芪类药物DIDS(4,4 - 二异硫氰基芪 - 二磺酸,500 microM)减缓了依赖HCO3(-)的pHi恢复。6. 在高K0+(44.5 mM)溶液中或用5 mM - BaCl2使膜电位去极化,对依赖HCO3(-)的pHi恢复速率没有影响。这一观察结果,再加上依赖HCO3(-)的pHi恢复激活与膜电位无一致变化这一事实,表明Na(+) - HCO3-共内流是电中性且对电压不敏感的。7. 依赖HCO3(-)的pHi恢复不受Na(+) - K(+) - 2Cl-共转运抑制剂布美他尼(150 microM)的影响。8. 评估了Na(+) - H+交换和Na(+) - HCO3-共转运对净酸外排的贡献。在pHi为6.6时,我们估计共转运应占总酸当量外排的20%。(摘要截短至400字)