Electrophysiological response of rat atrial myocytes to acidosis

doi:10.1152/ajpheart.01000.2001

Electrophysiological response of rat atrial myocytes to acidosis

Kimiaki Komukai, Fabien Brette, and Clive H. Orchard

School of Biomedical Sciences, University of Leeds, Leeds LS2 9NQ, United Kingdom

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

The effect of acidosis on the electrical activity of isolated rat atrial myocytes was investigated using the patch-clamp technique.Reducing the pH of the bathing solution from 7.4 to 6.5 shortenedthe action potential. Acidosis had no significant effect on transientoutward or inward rectifier currents but increased steady-stateoutward current. This increase was still present, although reduced,when intracellular Ca²⁺ was buffered by 1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraaceticacid (BAPTA); BAPTA also inhibited acidosis-induced shorteningof the action potential. Ni²⁺ (5 mM) had no significant effect on the acidosis-induced shorteningof the action potential. Acidosis also increased inward currentat $-$ 80 mV and depolarized the resting membrane potential. Acidosisactivated an inwardly rectifying Cl current that was blocked by 4,4'-diisothiocyanostilbene-2,2'-disulfonicacid (DIDS), which also inhibited the acidosis-induced depolarizationof the resting membrane potential. It is concluded that an acidosis-inducedincrease in steady-state outward K⁺ current underlies the shortening of the action potential andthat an acidosis-induced increase in inwardly rectifying Cl current underlies the depolarization of the resting membranepotential duringacidosis.

action potential; potassium current; chloride current; perforated patch

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

CARDIAC MUSCLE becomes acidic in a number of pathological conditions (27). Acidosis decreases the strength of contractionof the heart [for review see Orchard and Kentish (27)] and caninduce arrhythmias [for review see Orchard and Cingolani (26)],both of which impair cardiac function. There are many mechanismswhereby acidosis can induce arrhythmias, among which is changingaction potential duration: longer action potentials can producetriggered activity, shorter action potentials decrease the refractoryperiod and can lead to premature contraction, and regional effectson the action potential can produce QT dispersion and reentrytachyarrhythmia. Previous studies have shown marked effects ofacidosis on the action potential in ventricular cells (3, 19,21) that could produce arrhythmias by these mechanisms. However,despite the prevalence of atrial arrhythmias, the effect of acidosison the atrial action potential isunknown.

We have recently shown that acidosis prolongs the action potential in rat ventricular cells by inhibition of the steady-stateK⁺ current (I_SS). However, the response in atrial cells may be different.These cells have three distinct Ca²⁺-independent, depolarization-induced outward K⁺ currents: a rapidly activating, rapidly inactivating current(fast transient outward current, I_TO,f), a rapidly activatingslowly inactivating current (slow transient outward current, I_TO,s),and a rapidly activating noninactivating current (I_SS) (5,6). Although the kinetics of atrial I_SS are similar to thoseof ventricular I_SS, which is inhibited by acidosis, rat atrialI_SS is carried by Kv1.5 (1, 2, 4, 25), whereas ratventricular I_SS appears to be carried by Kv1.2 or Kv2.1 (29).Thus the response of the action potential to acidosis may be differentin rat atrial and ventricularcells.

Acidosis also depolarizes the resting membrane potential in ventricular cells, but the mechanism is unknown (26). Althougha change in resting membrane potential will contribute to theelectrophysiological response to acidosis, the response of theresting membrane potential to acidosis in atrial cells isunknown.

In the present study we investigated the effect of acidosis on the action potential and resting membrane potential and theunderlying currents in rat atrialcells.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Cell Isolation

Male Wistar rats weighing 220~250 g were stunned and then killed by cervical dislocation. The heart was quickly removed andwashed with isolation solution (see Solutions and Chemicals) containing0.5 mM CaCl₂. The aorta was cannulated and retrogradely perfusedwith isolation solution containing 0.5 mM CaCl₂ at 10-12 ml/minand at a temperature of 36.5 ± 0.5°C. After good contraction ofthe heart was confirmed, it was perfused with isolation solutioncontaining 0.1 mM EGTA (Sigma Chemical, St. Louis, MO) for 4 minand then with isolation solution containing 0.8 mg/ml collagenase(Type I, Worthington Biochemical) and 0.08 mg/ml protease (TypeXIV, Sigma) for 10 min. At the end of the perfusion, both atrialappendages were dissected from the heart and cut into small pieces,which were incubated with isolation solution containing 1% bovineserum albumin in addition to the above enzymes, for 10 min at37°C. The tissue was filtered and the filtrate centrifuged at40 g for 60 s. The supernatant was removed, and the cells wereresuspended in isolation solution containing 0.5 mM CaCl₂ andstored at room temperature. This process was repeated four tofive times with the remainingtissue.

Experimental Setup

An aliquot of cells was transferred to the experimental chamber, which was mounted on the stage of an inverted microscope(Diaphot, Nikon; Tokyo, Japan). In some experiments, the cellswere illuminated with long wavelength (>600 nm) light, and theimage was detected using a CCD camera (WAT-92A, Watec, Japan)and monitor (model PM-950, Ikegami Tsushinki; Utsunomiya,Japan).

The patch-clamp amplifier (8800 Total Clamp System; Dagan, MN) was controlled by a personal computer through an analog-digitalinterface (model 1401, Cambridge Electronic Design; Cambridge,UK) by using CED Patch and Voltage Clamp Software (Cambridge ElectronicDesign), which was also used for data acquisition. Voltage andcurrent were also monitored with the use of an oscilloscope (OS4100,Gould; Hainault,UK).

Measurement of Action Potential and K+ Currents

The perforated patch-clamp technique was used to monitor the action potential and K⁺ currents (14, 15, 19, 20). Electrodes (2-4 M $Omega$ ) were madefrom glass capillaries (GC150F-15, Clark Electromedical Instruments;Reading, UK) by using a vertical puller (PP-83, Narishige; Tokyo,Japan). The tip of the electrode was filled with pipette solution(see Solutions and Chemicals) and backfilled with pipette solutioncontaining 200-400 µg/ml amphotericin B. When the electrode tipwas in the bath, junction potential was electronically offsetto zero. After a seal was made (>1 G $Omega$ ), capacitance was compensatedand holding potential was set to $-$ 40 mV. Five-millivolt depolarizingsteps (20 ms in duration) were applied to monitor pore formation.The pipette solution contained 1 mM CaCl₂ to ensure that accidentalrupture of the membrane resulted in cell death. Electrical accesswas usually obtained within 15-30 min. After the capacity transientsbecame constant, series resistance was compensated and measurementswere made. Changing between control and acid solutions while theelectrode tip was in the bath solution was used to ensure theabsence of artifactual changes of potential. Action potentialswere measured in current clamp mode. Three- to five-millisecondcurrent pulses, sufficient to trigger an action potential, wereinjected every 2 s from the amplifier. The duration of the actionpotential was measured at 25, 50, and 90% repolarization (APD₂₅,APD₅₀, and APD₉₀, respectively). Depolarization-induced K⁺ currents were recorded in the presence of 0.1 mM CdCl₂ (as werethe recordings shown in Fig. 3 when K⁺ was replaced with Cs⁺) to block Ca²⁺ current (I_Ca). 4-Aminopyridine (4-AP) was not used for theseexperiments because of its nonspecific inhibitory effects on K⁺ currents (5). To measure I_TO,f, holding potential was setto $-$ 80 mV. After a 40-ms prepulse to $-$ 40 mV [to inactivate Na⁺ current (I_Na)], 500-ms test pulses to voltages between $-$ 40 and+40 mV were applied; pulses were applied every 2 s. I_TO,f wasmeasured as the difference between the peak outward current andthe current remaining at the end of pulse. I_SS was monitored froma holding potential of $-$ 20 mV to avoid contamination by transientoutward current (I_TO), which is inactivated at this potential(Ref. 6, see also Fig. 3A). A series of 500-ms test pulsesto voltages between $-$ 40 and +40 mV was applied; pulses were appliedevery 2 s. I_SS was measured at the end of the pulses. Inward rectifiercurrent (I_K1) was monitored from a holding potential of $-$ 40 mV.A series of 500-ms pulses to voltages between $-$ 120 and $-$ 30 mVwas applied; pulses were applied every 2 s. I_K1 was measured atthe end of the pulses. All experiments were performed at roomtemperature.

Measurement of Cl $-$ Current

Conventional whole cell patch clamp was used to measure Cl currents (I_Cl) because Cl diffusion between the pipette and the cell interior is restrictedin the perforated patch configuration. A 3 M KCl-agar bridge-AgClpellet was used as the bath electrode. Holding potential was setto $-$ 40 mV. Two-second test pulses to voltages between $-$ 120 and+40 mV (in 20-mV increments) followed by 400-ms pulses to +40mV were applied; pulses were applied every 10 s (10). Currentwas measured at 2 s. All experiments were performed at roomtemperature.

Solutions and Chemicals

During isolation and cell storage, the isolation solution used contained (in mM) the following: 130 NaCl, 5.4 KCl, 1.4 MgCl₂· 6H₂O, 0.4 NaH₂PO₄, 10 creatine (Sigma), 20 taurine (Sigma),5 HEPES (Sigma), and 10 glucose. pH was adjusted to 7.30 withNaOH. When the action potential and K⁺ currents were measured using the perforated patch-clamp technique,the composition of the extracellular solution was (in mM) thefollowing: 108 NaCl, 5 KCl, 1 Na₂HPO₄ · 12H₂O, 1 MgSO₄ · 7H₂O,20 Na acetate, 10 glucose, 1 CaCl₂, 10 HEPES, and 5 U/l insulin.pH was first adjusted to 7.40 with NaOH, and then HCl was usedto decrease the pH of an aliquot of this solution to 6.50. Thecomposition of the pipette solution was (in mM) the following:130 KCl, 10 NaCl, 1.4 MgCl₂ · 6H₂O, 1 CaCl₂, and 5 HEPES. pH wasadjusted to 7.10 with KOH. When I_Cl was measured by using conventionalwhole cell clamp, the composition of the extracellular solutionwas (in mM) the following: 120 TEACl (Sigma), 10 CsCl (Sigma),1 MgCl₂ · 6H₂O, 10 HEPES, 2 BaCl₂ (Sigma), and 10 glucose, 1 CaCl₂,2 4-AP (Sigma), and 0.01 nifedipine (Sigma). pH was first adjustedto 6.5 with TEAOH (Sigma), and then an aliquot of the solutionwas adjusted to pH of 7.4 by further addition of TEAOH. The compositionof the pipette solution was (in mM) the following: 110 CsCl, 20TEACl, 5 MgATP (Sigma), 5 EGTA, and 5 HEPES. pH was adjusted to7.1 withCsOH.

All chemicals were purchased from BDH Laboratory Supplies (Poole, UK) unless otherwise mentioned. Amphotericin B was purchasedfrom Sigma, and a 50 mg/ml stock solution was made with DMSO (Sigma)immediately before the experiments and diluted into the pipettesolution before use. 1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraaceticacid (BAPTA)-AM was purchased from Molecular Probes (Eugene, OR),and a 1 mM stock solution was made with DMSO. A 10 mM stock solutionof nifedipine and a 100 mM stock solution of 4,4'-diisothiocyanostilbene-2,2'-disulfonicacid (DIDS; Sigma) were made with DMSO and kept in light-resistantcontainers. A 10 mM stock solution of strophanthidin (Sigma) wasmade with ethanol. All stock solutions were diluted into the perfusateimmediately before use. Addition of DIDS (final concentrationup to 0.1 mM) did not alter pH ofperfusate.

Statistical Analysis

Data are expressed as means ± SE for n cells. Paired or unpaired t-tests (two-tailed) were performed as appropriate. Whenan unpaired t-test was used, the variances were tested by F test.Statistical significance was taken as P < 0.05.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Effect of Acidosis on Action Potential in Atrial Myocytes

Isolated atrial myocytes were current clamped at 0.5 Hz. Figure 1 shows representative action potentials recorded at controlpH and during acidosis. Acidosis significantly shortened APD₉₀from 79 ± 7 to 48 ± 6 ms (P < 0.05, n = 5) but did not alter APD₂₅(4 ± 0 ms at control pH, 4 ± 0 ms in acidosis) or APD₅₀ (12 ±1 ms at control pH, 11 ± 1 ms in acidosis). Acidosis also causeddepolarization of the resting membrane potential from $-$ 79 ± 1mV at control pH to $-$ 76 ± 2 mV during acidosis (P < 0.05, n =5). This change in resting potential is similar to that reportedpreviously in ventricular cells. However, the abbreviation ofthe action potential by acidosis is in contrast to the prolongationreported in ventricular cells (see INTRODUCTION).

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Fig. 1. Effect of acidosis on the atrial action potential. Action potentials recorded from a representative atrial cell at control pH and during acidosis. Dashed line indicates 0 mV.

Subsequent experiments were designed to investigate the current(s) responsible for these changes. Currents were normalizedto cell capacitance and presented as current density. Mean cellcapacitance, calculated from capacitance transients during a 10-mVhyperpolarizing pulse from $-$ 80 mV, was 53 ± 3 pF (n =38).

Effect of Acidosis on I_TO in Atrial Myocytes

The I_TO in rat atrial myocytes has two components: I_TO,f and I_TO,s (6), which have time constants of inactivation of ~180ms and ~3 s, respectively (6). Thus at the end of the 500-msvoltage-clamp pulses used to monitor I_TO (see METHODS), I_TO,fwill have decayed by ~94%, whereas I_TO,s will have decreased byonly ~15%. In addition, at the stimulation frequency used in thepresent study I_TO,s will be mostly inactivated due to its slowrecovery from inactivation (6). Thus the current measured asthe difference between peak current and current at the end ofthe pulse (see METHODS) will reflect predominantly I_TO,f.

Figure 2, A and B, shows original traces of total outward current in a representative cell, elicited using the protocol describedin the METHODS and shown in the inset in Fig. 2A, at control pH(A) and during acidosis (B). Figure 2C shows the current at +60mV in control and acidosis. When the currents are superimposedby offsetting one of the currents, it is apparent that the amplitudeand time course of I_TO,f were identical in control and acidosis(Fig. 2C, inset); because the currents can be superimposed inthis way, this suggests that the acidosis-induced increase inoutward current (compare Fig. 2, B with A) is a rapidly activating,noninactivating current (see Effect of Acidosis on I_SS in AtrialMyocytes), but that I_TO,f is unchanged during acidosis. Figure2D shows mean current density-voltage relationships of I_TO,f showingthat acidosis did not alter I_TO,f: current at +60 mV was 8.0 ±1.0 pA/pF in control and 6.7 ± 1.5 pA/pF in acidosis [not significant(NS), n = 6].

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Fig. 2. Effect of acidosis on depolarization-induced outward current from a holding potential of $-$ 80 mV. A and B: original traces of depolarization-induced outward current in a representative atrial cell in control (A) and acidosis (B). Inset: schematic of protocol: cell was held at $-$ 80 mV and depolarized to a series of test voltages between $-$ 40 and +60 mV for 500 ms at 0.5 Hz. Arrow indicates zero current level. Capacitance of the cell was 40 pF. C: original traces of the current at +60 mV in control ( $open circle$ ) and acidosis (

). When the currents are superimposed, it is clear that the amplitude and time course were identical (inset). D: mean ± SE current density-voltage relationship of fast transient outward current (I_TO,f) in atrial cells at control pH and during acidosis. Transient outward current was measured as the difference between the peak outward current and the current remaining at the end of pulses (see text for details).

At the end of the voltage-clamp pulse used to elicit I_TO,f (Fig. 2), membrane current is due to a small residual I_TO,f (seeabove), I_TO,s and I_SS (see Effect of Acidosis on I_SS in AtrialMyocytes). Thus although I_TO,s will be small under the conditionsof the present experiments (see Effect of Acidosis on I_TO in AtrialMyocytes), it is possible to estimate this current by subtractingI_SS at the end of a 500-ms test pulse from a holding potentialof $-$ 20 mV (see Effect of Acidosis on I_SS in Atrial Myocytes) fromthe current at the end of the 500-ms test pulse to the same potential,but from a holding potential of $-$ 80 mV, used to elicit I_TO (seealso Ref. 6). Although small, I_TO,s estimated in this way wasnot altered by acidosis: the current at +60 mV was 2.0 ± 0.7 pA/pFin control and 2.5 ± 0.6 pA/pF in acidosis (NS, n =6).

Thus acidosis does not appear to alter I_TO,f or I_TO,s making it unlikely that changes in I_TO underlie the observed changesin the actionpotential.

Effect of Acidosis on I_SS in Atrial Myocytes

I_SS was evoked from a holding potential of $-$ 20 mV to avoid contamination by I_TO,f and I_TO,s, which are inactivated at thispotential, and was measured at the end of 500-ms test pulses (Fig.3A, inset, and see METHODS). Figure 3A shows original traces ofI_SS in a representative cell at control pH. The cell is the sameas presented in Fig. 2, A-C; note that I_TO is absent at this holdingpotential (cf. Fig. 2). Figure 3B shows original traces from thesame cell during acidosis showing that acidosis increased thiscurrent. Figure 3C shows the effect of acidosis on the currentdensity-voltage relationship showing that acidosis significantlyincreased I_SS at all potentials: at +60 mV the current increasedfrom 10.5 ± 1.8 to 14.7 ± 2.2 pA/pF (P < 0.01, n = 6).

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Fig. 3. Effect of acidosis on depolarization-induced outward current from a holding potential of $-$ 20 mV. A and B: original traces of depolarization-induced outward current in the same cell as in Fig. 2, A-C, in control (A) and during acidosis (B). Inset: schematic protocol: the cell was held at $-$ 20 mV and hyperpolarized or depolarized to a series of test voltages between $-$ 40 and +60 mV for 500 ms at 0.5 Hz. Arrow indicates zero current level. C: mean ± SE current density-voltage relationship of steady-state current (I_SS) in atrial cells at control pH and during acidosis. *P < 0.05 vs. control. **P < 0.01 vs. control. D: mean ± SE current density-voltage relationship of I_SS in atrial cells at control pH and during acidosis when K⁺ in the pipette solution and perfusate was replaced with Cs⁺. I_SS was measured at the end of pulse as described in the text.

To determine whether this current was carried by K⁺, the effect of replacing the K⁺ in the pipette and bathing solutions with Cs⁺ was investigated. Figure 3D shows that Cs⁺ almost completely abolished this current at control pH, and thatin the presence of Cs⁺, acidosis did not increase outward current. Thus it appears thatI_SS is carried by K⁺ and increased byacidosis.

Effect of Acidosis on I_SS in Presence of Intracellular Ca²+ Buffering

In rat ventricular myocytes, acidosis increases intracellular [Ca²⁺] and hence Ca²⁺-sensitive outward current (15). It seemed possible, therefore,that the increase in I_SS observed during acidosis in the presentstudy was due to the Ca²⁺-sensitive outward current. The above experiment was thereforerepeated in the presence of BAPTA to buffer intracellular Ca²⁺. After the perforated patch configuration was established, 200-msdepolarizing pulses from $-$ 40 to 0 mV were applied every 2 s, andI_Ca and cell contraction were monitored. The cell was then exposedto 5 µM BAPTA-AM for 10 min; contraction was completely abolishedwithin 5 min, although I_Ca remained. The perfusate was changedto BAPTA-free Tyrode solution, and measurements were made as describedabove from a holding potential of $-$ 20mV.

Figure 4A shows the mean current-voltage relationship obtained at control pH and during acidosis in the presence of BAPTA.At control pH, BAPTA did not significantly alter I_SS at any testpotential (compare Fig. 3C and Fig. 4A, open symbols). In thepresence of BAPTA, acidosis still increased I_SS: at +60 mV thecurrent increased from 8.0 ± 1.1 to 9.3 ± 1.7 pA/pF (n = 7, P< 0.01) and returned to 7.6 ± 1.1 pA/pF after acidosis (NS vs.precontrol). However, Fig. 4B shows the difference current (acidosis $-$ control; i.e., the increase in current produced by acidosis)in the absence and presence of BAPTA, showing that the increaseinduced by acidosis was significantly smaller in the presenceof BAPTA.

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Fig. 4. Effect of acidosis on depolarization-induced outward current in the presence of intracellular Ca²⁺ buffering. A: mean ± SE current density-voltage relationship of I_SS in atrial cells in the presence of BAPTA at control pH and during acidosis. After treatment with 5 µM BAPTA/AM, the same protocol was used as in Fig. 3 (see text for details). *P < 0.05 vs. control. **P < 0.01 vs. control. B: means ± SE difference currents (acidosis-control) obtained in the absence and presence of BAPTA. *P < 0.05 vs. in the presence of BAPTA. C: action potentials recorded from a representative atrial cell after treatment with BAPTA at control pH and during acidosis. Dashed horizontal line indicates 0 mV.

Because BAPTA reduced the acidosis-induced increase of I_SS, its effect on the response of the action potential to acidosiswas investigated to test whether the increase in I_SS might underliethe acidosis-induced abbreviation of the action potential. Figure4C shows that BAPTA altered the configuration of the action potentialat control pH (compare Fig 4C, control with Fig. 1, control),presumably by buffering the Ca²⁺ transient and hence inhibiting inward Na⁺/Ca²⁺ exchange current (I_Na/Ca) during the action potential (inhibitionof the exchange using Ni²⁺ had a similar effect on action potential configuration, see Fig.5). In the presence of BAPTA, acidosis caused a smaller decreaseof action potential duration (Fig. 4C; APD₉₀ decreased from 53± 10 to 41 ± 9 ms, n = 6, P < 0.01, i.e., by 11 ± 3 ms, comparedwith a decrease of 31 ± 10 ms in the absence of BAPTA).

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Fig. 5. Effect of acidosis on action potentials in the presence of Ni²⁺. Action potentials recorded from a representative atrial cell in the presence of 5 mM Ni²⁺ at control pH and during acidosis. Dashed horizontal line indicates 0 mV.

These data are compatible with the idea that an acidosis-induced increase in BAPTA-sensitive and BAPTA-insensitive I_SS underliethe abbreviation of the action potential observed during acidosis(see DISCUSSION).

Effect of Acidosis on Action Potential in Presence of Ni²+

It seems possible that changes in I_Na/Ca during acidosis might also contribute to the abbreviation of the action potential(in which case inhibition of I_Na/Ca by BAPTA would be expectedto inhibit action potential shortening during acidosis). Thisseems feasible because Na⁺/Ca²⁺ exchange is inhibited by acidosis (14, 20, 28, 34) andmodulated by intracellular Ca²⁺. To test this idea, we investigated the effect of acidosis onthe action potential in the presence of 5 mM NiCl₂ to block I_Na/Ca(8). In the presence of Ni²⁺, acidosis still shortened the action potential (APD₉₀ decreasedfrom 72 ± 17 to 53 ± 17 ms, n = 3, P < 0.05) (Fig. 5). This decreasewas not significantly different from that observed in the absenceof Ni²⁺, making it unlikely that changes in I_Na/Ca contribute significantlyto the abbreviation of the action potential observed during acidosis(although the decrease observed in the presence of Ni²⁺ was slightly smaller than that observed in control, suggestingthat I_Na/Ca may play a smallrole).

Effect of Acidosis on I_K1 in Atrial Myocytes

I_K1 is responsible for late repolarization and maintenance of the resting membrane potential. Thus I_K1 was measured at controlpH and during acidosis to investigate whether it could contributeto the observed changes in the action potential or resting potential.However, acidosis had no significant effect on I_K1 (not shown):at $-$ 120 mV the current measured at the end of the 500-ms testpulses used was $-$ 10.5 ± 1.1 pA/pF at control pH, $-$ 10.4 ± 1.2 pA/pFin acidosis (NS, n = 5). It thus appears unlikely that I_K1 playsa role in the observed changes in the action potential and restingpotential.

Mechanism of the Resting Membrane Potential Depolarization During Acidosis

To investigate the mechanism responsible for the depolarization of the resting membrane potential during acidosis, the inwardshift of holding current at $-$ 80 mV at control pH and during acidosiswas monitored. Figure 6C shows that acidosis significantly increasedthe inward current at $-$ 80 mV, and that this shift was not significantlydifferent in the presence of BAPTA, when K⁺ in the pipette and bathing solutions was replaced with Cs⁺ or when pipette and bathing K⁺ was replaced with Cs⁺, and 5 mM Ni²⁺, 0.1 mM Ba²⁺, and 20 µM strophanthidin were present in the bathing solution(extracellular MgSO₄ was replaced with MgCl₂, and Na₂HPO₄ wasomitted to avoid precipitation with Ba²⁺). Thus it appears unlikely that changes in Ca²⁺-sensitive currents (including I_Na/Ca), I_Ca, K⁺ currents, or Na pump current (I_Na/K), underlie the acidosis-induceddepolarization of resting membrane potential.

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Fig. 6. Effect of acidosis on resting membrane potential. A: action potentials recorded from representative atrial cell in the presence of 50 µM 4,4'-diisothiocyanostilbene-2,2'-disulfonic acid (DIDS) at control pH and during acidosis. B: mean ± SE acidosis-induced depolarization of resting membrane potential (from top to bottom): in control; +5 mM Ni²⁺; + intracellular BAPTA; +50 µM DIDS. *P < 0.05 vs. control. C: mean ± SE acidosis-induced inward shift of holding current at $-$ 80 mV (from top to bottom) in control; + intracellular BAPTA; with replacement of K⁺ in the pipette solution and perfusate with Cs⁺; with K⁺ in the pipette solution and perfusate replaced with Cs⁺, and 5 mM Ni²⁺, 0.1 mM Ba²⁺, 20 µM strophanthidin present in the perfusate. Numbers of cells are shown in parentheses. All changes in resting membrane potential and holding current were significantly different from baseline (P < 0.05) except that in the presence of DIDS (NS, not significant).

Figure 6B shows that acidosis significantly depolarized the resting membrane potential in control, in the presence of Ni²⁺ and BAPTA, as expected from the results above, but that 50 µMDIDS inhibited the acidosis-induced depolarization of the restingmembrane potential (Fig. 6, A and B), suggesting that the depolarizationis due to acidosis-induced activation of a DIDS-sensitive I_Cl.To test this idea further, the effect of acidosis on I_Cl wasinvestigated.

Figure 7, A and B, shows original traces of I_Cl recorded from a representative cell at control pH (Fig. 7A) and during acidosis(Fig. 7B) in the absence of Na⁺ and K⁺ and the presence of Cs⁺, TEA⁺, Ba²⁺, nifedipine, 4-AP, and internal EGTA as described in METHODS.Under these conditions (pipette [Cl] = 130 mM), an inwardly rectifying current was recorded witha reversal potential of $-$ 10 mV (Fig. 7C, open circles); reducingpipette [Cl] to 20 mM (replaced with aspartate) markedly decreased the measured current and shifted the reversalpotential to $-$ 46 mV (Fig. 7C, open triangles). The similarityof the measured reversal potentials to the calculated Cl reversal potentials ( $-$ 2 mV and $-$ 49 mV, respectively) suggeststhat the measured current is carried predominantly by Cl; the difference between the calculated and measured reversalpotentials may represent imperfect equilibration between pipetteand intracellular solutions. Acidosis increased inward current(Fig. 7C, filled symbols): when pipette [Cl] was 130 mM, current at $-$ 120 mV increased from $-$ 4.0 ± 2.1 to $-$ 6.5 ± 2.5 pA/pF (n = 5, P < 0.05). Figure 7D shows that the currentinduced by acidosis (i.e., current in acidosis minus that at controlpH) shows strong inward rectification and is decreased when pipette[Cl] is decreased: the current induced by acidosis at $-$ 120 mV wasreduced from $-$ 2.5 ± 0.6 pA/pF (n = 5) to $-$ 0.4 ± 0.2 pA/pF (n =3; P < 0.05) when pipette [Cl] was reduced from 130 to 20 mM. The acidosis-induced increasein current was completely inhibited by DIDS (Fig. 7E), althoughDIDS had no significant effect on membrane current at controlpH under these conditions or on resting membrane potential undercontrol conditions (not shown). These data suggest, therefore,that the acidosis-induced depolarization of the resting membranepotential is due to activation of a DIDS-sensitive, inwardly rectifyingI_Cl (I_Cl,ir).

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Fig. 7. Effect of acidosis on Cl current. A and B: original traces of Cl current monitored using ruptured patch in a representative atrial cell at control pH (A) and during acidosis (B); pipette [Cl] 130 mM. Cell was held at $-$ 40 mV and hyperpolarized to a series of test voltages between $-$ 120 and +40 mV in 20-mV increments for 2 s followed by 400-ms pulses to +40 mV at 0.1 Hz. Arrow indicates zero current level. C: means ± SE current density-voltage relationships of Cl current at control pH (open symbols) and during acidosis (filled symbols) when pipette [Cl] was 130 mM (circles) or 20 mM (triangles). *P < 0.05 vs. control pH. D: means ± SE difference current (acidosis $-$ control) when pipette [Cl] was 130 mM (

) or 20 mM ( $black-triangle$ ). *P < 0.05 vs. 130 mM pipette [Cl]. E: means ± SE difference current in the absence (

) and presence (

) of 0.1 mM DIDS; pipette [Cl] 130 mM. *P < 0.05 vs. in the absence of DIDS.

Relationship Between Resting Membrane Potential and Action Potential Duration

To test whether the observed change in action potential duration might be secondary to the acidosis-induced change in restingmembrane potential per se, current injection was used to depolarizethe resting membrane potential by 5 mV. However, this maneuvertended to prolong action potential duration (not shown), makingthisunlikely.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

In the present study, acidosis was produced by decreasing the extracellular pH (pH_o) from 7.4 to 6.5. Measurement of intracellularpH (pH_i) using the fluorescent dye 2',7'-bis(2-carboxyethyl)-5(6)-carboxyfluoresceinhas shown that pH_i decreases by ~0.5 pH units in response to thischange in pH_o (20). These changes are, therefore, within therange observed pathophysiologically (27). pH_i reaches a newsteady state within 3 min; measurements in the present study weretherefore carried out after 5 min exposure to the acid solution(15). In ventricular cells, the presence of a perforated patchelectrode containing 5 mM HEPES does not affect the change ofpH_i that occurs on exposure to the acid solution (not shown);it therefore seems unlikely that it would do so in atrial cells.The perforated patch-clamp technique was used because acidosisalters the intracellular environment, increasing intracellular[Ca²⁺] (12), intracellular [Na⁺] (12), calcium-calmodulin-dependent kinase (CaMKII) activityvia the increase in intracellular [Ca²⁺] (13) and inhibiting protein phosphatase activity (23). Wetherefore used the perforated patch-clamp technique where possibleto minimize disruption to these normal responses, to investigatethe physiological response toacidosis.

Effect of Acidosis on Atrial Action Potential

Role of I_Ca and I_Na/Ca. We have previously shown that acidosis has little effect on I_Ca in rat ventricular cells when the perforated patch-clamp techniqueis used (14, 19, 20). Because the channel that carries thiscurrent in atrial cells appears to be the same as in ventricularcells, it seems likely that acidosis has little effect on I_Cain atrial cells. Although inhibition of I_Ca by Ni²⁺ may contribute to the change in action potential configurationobserved in the presence of Ni²⁺, the observation that acidosis-induced shortening of the actionpotential still occurred in these conditions suggests that changesin I_Ca are not necessary to account for this abbreviation of theactionpotential.

Inhibition of Na⁺/Ca²⁺ exchange shortens action potential duration (30). Acidosis-induced inhibition of Na⁺/Ca²⁺ exchange (14, 20, 28, 34) could, therefore, explain theobserved abbreviation of the action potential during acidosis.However, the present study shows that acidosis shortened the actionpotential even after the exchange had been inhibited by 5 mM Ni²⁺ (Fig. 5), making it unlikely that inhibition of Na⁺/Ca²⁺ exchange plays a major role in the acidosis-induced shorteningof the action potential, although it is possible that it playsa small role (see RESULTS).

Role of I_TO,f and I_TO,s. In the present study, acidosis did not alter I_TO,f (Fig. 2) consistent with the observation that acidosis did not alter earlyrepolarization (Fig. 1). Although atrial I_TO,f is distinct fromventricular I_TO with respect to its time course of activationand inactivation, the same channels (Kv4.2/4.3) are thought tounderlie both currents. The present result is therefore consistentwith the observation that acidosis does not alter I_TO in rat ventricularcells when holding potential is negative to $-$ 60 mV (15). Thesedata make it unlikely that the effect of acidosis on the actionpotential is mediated by a change in I_TO,f.

It is also unlikely that I_TO,s is involved in the acidosis-induced shortening of the action potential because I_TO,s is mostlyinactivated in the conditions used in the present study and appearsto be unaffected by acidosis (see RESULTS), consistent with previousreports that Kv1.2, which appears to carry I_TO,s, is unaffectedby acidosis (32).

Role of I_SS. Kv1.5 is the most likely candidate for rat atrial I_SS (25), because the time- and voltage-dependent properties of heterologouslyexpressed Kv1.5 channels are similar to those of rat atrial I_SS,and anti-Kv1.5 antibody shows high levels of binding in rat atrialcells (2) and exposure of rat atrial cells to antisense oligodeoxynucleotidesfor Kv1.5 significantly inhibits I_SS (4).

The present data show that I_SS is inhibited by replacing K⁺ with Cs⁺, consistent with a K⁺ current. I_SS also appeared to have a Ca²⁺-insensitive component and a Ca²⁺-sensitive component that was only observed during acidosis (BAPTAdecreased I_SS during acidosis but had no effect on I_SS at controlpH; Figs. 3 and 4). We are unaware of any previous work showingthat I_SS is Ca²⁺ dependent or has two components. However, it is not clear whetherthese are two different components of I_SS or whether the apparentlyCa²⁺-insensitive component is due to incomplete buffering of Ca²⁺ by BAPTA. In support of the latter suggestion, both componentsshowed the same kinetics (rapidly activating, noninactivating;not shown), and acidosis increased both components of I_SS (Fig.4B).

Previous work has shown that acidosis decreases I_SS in rat ventricular cells (see INTRODUCTION), although this may be becausein rat ventricle I_SS is carried by Kv1.2 or Kv2.1 (29). However,acidosis (pH 7.3-6.3) also inhibits Kv1.5 current expressed inXenopus oocytes (32), although this difference may be due todifferences in the channel's environment and regulation in thetwo cell types (e.g., 9). The mechanism of action of acidosison I_SS is unclear but is likely to be an effect on channel conductancerather than inactivation; the observation that the increase inI_SS produced by acidosis is voltage independent (Fig. 3C) alsosuggests that it is unlikely that the effect of protons is withinthe channelpore.

The observation that BAPTA inhibited the acidosis-induced decrease in action potential duration (Fig. 4C) is compatible withthe idea that an acidosis-induced increase in the BAPTA-sensitivecomponent of I_SS is responsible for much of the action potentialshortening observed duringacidosis.

Role of I_K1. In the present study, acidosis did not alter I_K1, making it unlikely that changes in I_K1 are responsible for the changes inthe action potential observed duringacidosis.

I_K1 in the rat ventricle appears to be carried by Kir2.1 (24). Although the identity of rat atrial I_K1 has not been established,Kir2.1 is pH insensitive (37), consistent with the presentdata.

Mechanism of acidosis-induced shortening of the atrial action potential. In the present study, acidosis shortened the action potential of rat atrial cells. This is in contrast to previous work, whichshowed that acidosis prolongs the action potential of rat ventricularcells under identical experimental conditions. The abbreviationobserved in the present study is unlikely to be due to the effectsof acidosis on I_Na/Ca, I_Ca, I_TO,f, I_TO,s I_K1, or I_Cl,ir, or secondaryto the depolarization of the resting membrane potential (see above),but could be due predominantly to the effect of acidosis on I_SS,which is increased in atrial cells, but inhibited in ventricularcells and which could, therefore, account for the different responsein the two cell types. Unfortunately, there is no specific inhibitorof I_SS with which to test this hypothesis, although the observationthat BAPTA inhibited the increase in I_SS and the abbreviationof the action potential supports theidea.

One problem with this hypothesis is that the effect of acidosis on I_SS is greater at more positive potentials (Fig. 3), whereasthe effect on the action potential is greater at more negativepotentials (Fig. 1). Because many of the repolarizing currentsare voltage and time dependent, the comparison of the action potentialand the currents monitored under voltage clamp is not straightforward.However, a similar relationship between the configuration of theaction potential and a change in I_SS to that observed in the presentstudy has been reported in response to phenylephrine (11), whichproduced a prolongation of late depolarization that was ascribedto a decrease in I_SS. It seems possible that the effect of theacidosis-induced increase in I_SS on the action potential is maskedduring the early phase (APD₂₅, APD₅₀) of the action potentialby the presence of other large currents (e.g., I_Na, I_TO,f) andthus that an increase in I_SS, possibly with a small contributionby altered I_Na/Ca (see RESULTS), could underlie the abbreviationof the atrial action potential duringacidosis.

Effect of Acidosis on Resting Potential

Acidosis-induced depolarization of the resting membrane potential has been observed by many investigators [for review seeOrchard and Cingolani (26)], although the mechanism has remainedobscure. The present study shows that the acidosis-induced increasein inward current, and hence resting membrane potential, is unlikelyto be due to changes in Ca²⁺-sensitive currents (including I_Na/Ca), I_Ca, K⁺ currents, or I_Na/K (Fig. 6, B and C).

However, acidosis markedly increased I_Cl,ir, monitored using whole cell clamp (Fig. 7). This current and the acidosis-inducedincrease in current were reduced when pipette [Cl] was decreased (Fig. 7, C and D): when pipette [Cl] was 20 mM, within the physiological range (10-20 mM; Ref. 16),the acidosis-induced increase in current at $-$ 80 mV was 0.19 ±0.12 pA/pF, similar to the increase in inward current observedduring acidosis using perforated patch-clamp recording under morephysiological conditions (~0.5 pA/pF; Fig. 6). The slightly highercurrent observed during perforated patch recording might be dueto the high [Cl] in the pipette and a small permeability of the perforated patchto Cl causing a small increase in intracellular [Cl]. The observation that the increase in inward current inducedby acidosis was inhibited by decreasing pipette [Cl] and by DIDS (Fig. 7, D and E), which also abolished the depolarizationof the resting membrane potential (Fig. 6), suggests that thedepolarization of the resting membrane potential is due to acidosis-inducedactivation of a DIDS-sensitive I_Cl,ir. Assuming a membrane resistanceof 118 M $Omega$ (range in rat ventricular myocytes 20-200 M $Omega$ , Ref. 36),the small (28 pA) inward shift of current at $-$ 80 mV could accountfor the 3.3-mV depolarization observed duringacidosis.

I_Cl,ir does not appear to be due to protein kinase A-dependent I_Cl, Ca²⁺-activated Cl current, or swelling-induced I_Cl, because these do not show inwardrectification (18, 31, 16). However, this current showssimilarities to that carried by volume-regulated Cl (ClC-2) channels,which have recently been found in atrial and ventricular cells(7, 10); the I_Cl carried by these channels shows inward rectification(10, 17), is of comparable magnitude to that recorded in thepresent study (10), and is increased by acidosis in Xenopusoocytes (17). The presence of Cd²⁺, which blocks ClC-2, during measurement of depolarization-inducedK⁺ currents (see METHODS) could then explain why this current wasnot observed during these K⁺ current measurements, although the amplitude of I_Cl,ir at physiologicalintracellular [Cl] is sufficiently small (Figs. 6 and 7) that it would be difficultto detect during measurement of relatively large K⁺ currents, even in the absence of Cd²⁺. One problem with this hypothesis is that these channels havebeen reported to be insensitive to stilbene derivatives such asDIDS, which agrees with the observation in the present study thatDIDS did not alter I_Cl,ir at control pH. It is possible, therefore,that acidosis alters the response to DIDS, either by affectingDIDS itself, or DIDS may block the stimulatory action of H⁺ on ClC-2. Alternatively acidosis may increase I_Cl,ir, not byacting on the channel, but by causing a DIDS-sensitive increaseof intracellular [Cl], although the possible mechanism is unclear: the Cl/OH exchange (or H⁺-Cl coinflux) mechanism described by Sun et al. (33) is DIDS insensitive,whereas the DIDS-sensitive Na⁺-HCO cotransporter and Cl/HCO₃ exchanger (22) would be inhibited in the HEPES-buffered (HCOfree) solutions used in the present study (33). In either case,it appears likely that ClC-2 channels carry the acidosis-inducedI_Cl,ir that underlies the depolarization of the resting membranepotential duringacidosis.

	ACKNOWLEDGEMENTS

This work was supported by British Heart Foundation and WellcomeTrust.

	FOOTNOTES

Address for reprint requests and other correspondence: C. H. Orchard, School of Biomedical Sciences, Univ. of Leeds, LeedsLS2 9NQ, UK (E-mail: c.h.orchard{at}leeds.ac.uk).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

April 11, 2002;10.1152/ajpheart.01000.2001

Received 14 November 2001; accepted in final form 8 April 2002.

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