Relation Between Bicarbonate Concentration and Voltage Dependence of Sodium Currents in Freshly Isolated CA1 Neurons of the Rat

doi:10.1152/jn.01083.2002

Relation Between Bicarbonate Concentration and Voltage Dependence of Sodium Currents in Freshly Isolated CA1 Neurons of the Rat

C. Bruehl and O. W. Witte

Department of Neurology; Friedrich-Schiller-University; 07745 Jena, Germany

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Bruehl, C. and O. W. Witte. Relation Between Bicarbonate Concentration and Voltage Dependence of Sodium Currents in Freshly Isolated CA1 Neurons of the Rat. J. Neurophysiol. 89: 2489-2498, 2003. It recently has been shown that whole cell calcium and sodium currents are modulated by CO₂/HCO-bufferedsaline. While the bicarbonate ion, but not CO₂, has been provento modulate calcium currents, this information is lacking forsodium currents. Furthermore, it is not known whether the strengthof modulation dependents on the bicarbonate concentration or whetherit is an all-or-nothing phenomenon. To answer these questions,we used the whole cell voltage-clamp technique on freshly isolatedhippocampal CA1 neurons from the rat. A voltage step from $-$ 130to $-$ 20 mV elicited a sodium current with an amplitude of $-$ 5.1± 0.5 nA (mean ± SE, n = 17) when cells were superfused with HEPES-bufferedsaline. The amplitude of this current increased during a subsequentsuperfusion with solutions containing increasing amounts of bicarbonateand CO₂ (%CO₂/mM HCO: 2.5/5.6; 5.0/18;10/37), with a maximal increment in 10% CO₂/37 mM HCOof $-$ 6.9 ± 0.8 nA. The increase in amplitude was associated witha linear negative shift (slope: $-$ 0.7 mV/mM HCO)of the potential of half-maximal activation ( $Delta$ V_h,a: $-$ 19.4 ± 1.8mV in 10% CO₂) but not with an alteration in the maximal conductance(g_max: HEPES: 203.1 ± 21.0 nS and 10% CO₂/37 mM HCO:207.3 ± 21.3 nS). In addition, the potential of half-maximal inactivation(V_h,i) shifted to more negative potentials (slope: $-$ 0.6 mV/mMHCO) with increasing amounts of bicarbonateand CO₂ (HEPES: $-$ 53.6 ± 11.8 mV; 10% CO₂/37 mM HCO: $-$ 69.8 ± 2.1 mV), making the amplitude of the current highly sensitivefor small potential changes at resting membrane potential. Thesame negative shift in voltage dependence arose when cells wereexposed to solutions with different amounts of bicarbonate (5.6;18; 26 mM) but constant CO₂ (5%) with slope rates of $-$ 0.5 mV/mMHCO for V_h,a and $-$ 0.5 mV/mM HCOfor V_h,i. Again, there was no correlation between bicarbonateconcentration and the size of g_max. When currents were evokedin solutions containing a constant concentration (18 mM) of bicarbonatebut different amounts of CO₂ (2.5; 5.0 10%), no significant changeshave been observed. The present data demonstrate that bicarbonateions, and not CO₂, modulate voltage-gated sodium currents in aconcentration-dependent manner. Because the amplitude of the sodiumcurrent becomes highly sensitive to membrane potential changesconcomitant with increased bicarbonate amounts, this may be criticalfor the excitability of the neuronal network in situations (likemetabolic acidosis, respiratoric alkalosis and hypercapnia) inwhich the concentration of this ion canalter.

	INTRODUCTION

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Solutions containing CO₂/HCO, which act as the pH buffering system, have recently been shown tomodulate whole cell calcium as well as sodium currents (Bruehlet al. 2000; Gu et al. 2000). Furthermore, the excitability ofneurons in the slice preparation is different when the tissueis superfused with CO₂/HCO-bufferedsaline instead of a solution buffered with the artificial pH bufferHEPES (Church 1992, 1999; Church and McLennan 1989; Cowan andMartin 1995, 1996; Gu et al. 2000). Moreover, we have demonstratedthat the voltage-dependent properties of calcium currents andtheir maximal conductance are concentration dependent modulatedwhen the amount of bicarbonate ions was raised from 0 up to 37mM (Bruehl et al. 2000). Gu et al. (2000) showed a strong negativeshift in the voltage dependence of voltage-gated sodium currentsafter the exchange of a HEPES-buffered saline for a solution bufferedwith 26 mM HCO and 5% CO₂. Moreover,they demonstrated a largely reduced excitability of the CA1 neuronsduring the CO₂/HCO situation whencells were held in current-clamp mode. Switching from a nominallyCO₂/HCO-free HEPES to a CO₂/HCO-containingmedium cannot distinguish between bicarbonate or CO₂ as the modulatingfactor to evoke these effects. Furthermore, it is not clear whetherthese alterations are an all-or-nothing phenomenon or whetherthey depend on the concentration/gas-pressure of the modulator(i.e., HCO or CO₂).

Because CO₂/HCO is the mayor pH buffer system in the CNS and alterations in the concentrationof both CO₂ and HCO can occur duringnormal, as well as patho-physiological conditions, it is importantto investigate whether and to what extent CO₂/HCO-bufferedsaline can modulate ion conductances like the whole cell sodiumcurrent. Therefore we undertook the present study to unravel whichof both components induces the modulation of the sodium currentproperties and whether there is a concentration dependence ascan be seen on whole cell calciumcurrents.

For this purpose, we used the conventional whole cell voltage-clamp technique on freshly isolated hippocampal CA1 neuronsof young Wistarrats.

	METHODS

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Cell preparation

CA1 pyramidal neurons were enzymatically isolated from male Wistar rats (50-75 g) as described in detail previously (Vreugdenhiland Wadman 1992). Slices (500 µm) were cut from both hippocampi,and the CA1 area was dissected. These tissue pieces were incubatedfor 38 min at 32°C in oxygen-saturated dissociation solution (inmM/l: 120 NaCl, 5 KCl, 1 CaCl₂, 1 MgCl₂, 20 PIPES, 25 D-glucose;pH: 7.0; osmolarity: 295 mosmol) containing 1 mg/ml trypsin (BovineType XI). Following enzymatic treatment, tissue was washed twiceand kept in the dissociation solution without trypsin at 19°C.Directly before measurements tissue pieces were dispersed in HEPES-bufferedbath solution by trituration through Pasteur pipettes with decreasingtip diameter, and cells were allowed to settle in the perfusionchamber.

To assure total solution exchange, we used a bath chamber with a volume of ~120 µl, which was perfused with a constant flowrate of 1 ml/min. Bath solutions contained (in mM/l): 37 NaCl,5 KCl, 2.5 CaCl₂, 1 MgCl₂, 5 4-aminopyridine (4-AP), 30 TEA-Cl,72 choline-Cl, and 25 D-glucose and 100 µM CdCl₂; pH was set at7.3 (unless otherwise stated), with an osmolarity of 318 mosmol/l.For seal formation, the majority of cells were patched in thepreceding mentioned solution, plus 10 mM HEPES as the pH-buffersystem. Bath solutions containing CO₂/HCOinstead of HEPES were thoroughly gassed with different amountsof CO₂ (2.5; 5.0;10%) before the corresponding amount of HCOwas added. NaCl was replaced equimolarily by NaHCO,and osmolarity was adjusted with glucose to 318 mosmol/l whennecessary. Special care was taken to assure that the solutionswere always equilibrated with CO₂ throughout the course of theexperiment because otherwise CaCO₃ and CdCO₃ would have precipitated.Liquid-junction potentials may occur at the tip of the patch electrodesdue to the different ion compositions of the solutions and mayin some cases mislead the measurements. Therefore we measuredthe electrode potentials in HEPES- and bicarbonate-buffered solutions.The observed junction potentials never exceeded ±0.5 mV and weretherefore regarded asnegligible.

All chemicals were obtained from Sigma (Deisenhofen, Germany) or Merck (Darmstadt,Germany).

Current recording

Currents were measured under whole cell voltage-clamp conditions at room temperature using patch pipettes of 2-4 M $Omega$ resistance.Electrode solution contained (in mM/l): 5 NaCl, 115 CsF, 2 MgCl₂,0.5 CaCl₂, 115 TEA-Cl, 10 EGTA, 5 phosphocreatine, 2 MgATP, 0.1NaGTP, and 0.1 leupeptin (pH set at 7.3) and 50 units/ml phosphocreatinekinase. Osmolarity was adjusted to 300 mosmol/l, when necessary,by adding glucose. The solution was heavily buffered by 50 mMHEPES to minimize intracellular pH changes following the introductionof CO₂/HCO-buffered solution. Currentswere measured with an Axopatch 200B amplifier (Axon Instruments)and stored on an Atari ST computer (10-kHz sample frequency).Capacitive transients were corrected and series resistances (<10M $Omega$ ) were compensated for >90% on-line. Data were evaluated off-lineusing a custom-made computer program. All current traces werecorrected for aspecific linear leak (reversal potential: 0 mV)determined at holding potential. Rundown phenomena were neverobserved during the recording period and any neuron that escapefrom voltage clamp was rejected from the analysis. Such an escapewas characterized by a slow activation of the currents, a delayedachievement of the peak amplitude and/or by the occurrence ofmore than one current peaks during the voltagestep.

Experimental protocols

Sodium currents were activated, following a prepotential of $-$ 130 mV (500 ms), using 10-ms voltage steps to voltage levelsbetween $-$ 70 and +15 mV (increment: 5 mV). Holding potential waskept at $-$ 80 mV. The steady-state inactivation of the sodium currentwas determined using a standard depolarization to $-$ 20 mV afterthe cell was polarized for 500 ms to various levels between $-$ 110and $-$ 45 mV (increment: 5mV).

First, neurons were normally bathed in HEPES-buffered saline, and the voltage protocols that determine activation and inactivationproperties were performed. Second, the HEPES-buffered saline wasreplaced by CO₂/HCO-buffered saline.During solution changes a test pulse stepping from $-$ 130 mV (500ms) to $-$ 20 mV was applied (10 ms), to monitor current amplitudechanges and to ensure the stability of the final condition. A3-min period was allowed to guarantee total solution exchangebefore the same protocols were applied as with HEPES-containingsolution. During this period, the current amplitude increasedwithin seconds after solution exchange and reached its final valuewithin the followingminute.

Current analysis

Peak amplitudes of the currents (I) evoked with the activation protocol were plotted as a function of membrane potential (V).The resulting I-V relations were fitted with a combination ofa third-order Boltzmann activation function and the Goldman-Hodgkin-Katz(GHK) current-voltage relation (Hille 1992; Kortekaas and Wadman1997)

(1)

with $alpha$ = F/RT and g_max = $alpha$ FP₀ [Na⁺]_out, where g_max is the maximal membrane conductance (which is proportional to the maximalpermeability and the extracellular sodium concentration), V_h isthe potential of half-maximal activation, and V_c is proportionalto the slope of the curve at V_h. F represents the Faraday constant,R the gas constant, P₀ is the maximal permeability, and T theabsolutetemperature.

The voltage dependence of steady-state inactivation of the sodium current was estimated from the relation of peak currentamplitude versus the prepotential. This relation was well describedby a Boltzmann function, which also normalized the current

<IT>N</IT>(<IT>V</IT>)<IT>=</IT><FR><NU><IT>I</IT>(<IT>V</IT>)</NU><DE><IT>I</IT><IT>max</IT></DE></FR> where <IT>I</IT>(<IT>V</IT>)<IT>=</IT><FR><NU><IT>I</IT><IT>max</IT></NU><DE><IT>1+</IT>exp <FENCE><FR><NU><IT>V</IT><IT>h</IT><IT>−</IT><IT>V</IT></NU><DE><IT>V</IT><IT>c</IT></DE></FR></FENCE></DE></FR> (2)

where N(V) is the level of steady-state inactivation determined from the current amplitude I(V) normalized to I_max, V isthe prepulse potential, V_h is the potential of half-maximal inactivation,and V_c is a factor proportional to the slope of the curve at V_h.

Kinetics of the whole cell sodium currents were determined using a fit procedure which implies a third-order exponential termfor activation and two exponentials describing the inactivationkinetics. The following function was applied

(3)

where I1 and I2 are the amplitudes of the two current components and $tau$ _a; $tau$ _i,1 and $tau$ _i,2 represent the time constants for activationand inactivation after the start of the voltage step at timet0.

Statistics

Values are presented as the mean ± SE. Statistical comparisons were made with Student's t-test, if not stated otherwise. P< 0.05 was used to indicate significantdifferences.

	RESULTS

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Concentration dependent effect of CO₂/HCO₃-buffered solution on whole cell sodium currents

ACTIVATION IN HEPES-BUFFERED SALINE. In a HEPES-buffered saline, whole cell sodium currents could be evoked in all neurons (n = 16) tested (Fig. 1). They showeda fast activation and an almost complete inactivation when elicitedfrom a potential of $-$ 130 mV (Fig. 2A, left). A voltage protocolthat steps to different voltage levels (between $-$ 70 and +15 mV)revealed the typical current voltage relation (Fig. 2B, bottom)with an mean peak amplitude of $-$ 5.4 ± 0.5 nA at around $-$ 15 mV.When those I-V curves were fitted with Eq. 1, they delivered threevariables, i.e., the maximal sodium conductance (g_max), the potentialof half-maximal activation (V_h,a), and the slope factor at thepoint of V_h,a (V_c). For the cells tested in this way, g_max wasevaluated to be 203.1 ± 21.0 nS (Fig. 3, left) and 50% of thechannels were activated at a voltage of V_h,a:-27.4 ± 1.4 mV witha slope of V_c: 4.3 ± 0.3 mV (Fig. 2B, top). With regards to thedifferent ion compositions and evaluation methods (third- vs.first-order Boltzmann activation functions), these values resembleddata previously been published from freshly isolated CA1 neurons(Gu et al. 2000; Ketelaars et al. 2001).

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Fig. 1. Sodium currents evoked from a CA1 neuron. Activation protocol was preceded by a period of 500 ms at a voltage of -130 mV to remove inactivation totally. Currents were elicited at voltages ranging from -70 to 15 mV (see inset). Within the test period of 10 ms, sodium currents did not fully inactivate.

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Fig. 2. A: whole cell sodium current evoked by a voltage step from $-$ 130 to $-$ 20 mV (see inset) of a CA1 neuron. Cell was subsequently bathed in 4 solutions containing either HEPES as the pH buffer, or CO₂/HCO with different concentrations. The amplitude of this current increased in parallel with increasing amounts of bicarbonate. B: I-V relationship (bottom) and activation properties (top) of the voltage-gated sodium current in relation to the concentration of bicarbonate and CO₂. Currents are activated from a prepotential of $-$ 130 mV. The peak amplitude increased and shifted to more negative potentials, when the amount of CO₂/HCO was elevated. This phenomenon underlies a negative shift of the Boltzmann curves of activation, which results in an increased driving force for the sodium ions.

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Fig. 3. Bar-graph showing the maximal conductances (g_max), as were evaluated with Eq. 1 for 3 different bicarbonate and CO₂ combinations (see subtitles) and the HEPES-buffered solution. The observed increase in sodium current amplitude was not accompanied by an increase in maximal conductance when neurons (n = 16) were successively bathed in solutions with increasing amounts of CO₂/HCO.

INACTIVATION IN HEPES-BUFFERED SALINE. To investigate the steady-state inactivation properties, we evoked currents with a voltage step to $-$ 20 mV (10 ms) followinga 500-ms period at different prepotentials ( $-$ 110 to $-$ 45 mV; increment:5 mV). When the measured peak amplitudes were plotted againstthe prepotential voltage, it gives a Boltzmann-like inactivationcurve that was best described by Eq. 2. The values received bya fit with this equation; i.e., the half-maximal potential ofsteady-state inactivation (V_h,i) and the slope of the Boltzmanncurve at this potential (V_c) amounted to $-$ 53.6 ± 1.8 and $-$ 6.1± 0.2 mV,respectively.

KINETICS IN HEPES-BUFFERED SALINE. When evoked by potential changes from $-$ 130 mV to more positive values, currents activated rapidly and inactivated almost completelywithin the time window of 20 ms. The kinetic of activation andinactivation could be best described using a combination of athird-order exponential term for the activation of the currentand two exponential terms for the inactivating part (Eq. 3). Applicationof this algorithm usually leads to fit results within the noiselevel (Fig. 4, top). The evaluation of the time constants wasrestricted to test voltages of $-$ 35 up to $-$ 5 mV and delivered timeconstants for activation, which decreased with more positive voltages,starting with 0.39 ± 0.11 ms at $-$ 35 mV and ending with 0.08 ±0.01 ms (n = 16) at $-$ 5 mV. The time constants for inactivationwere also voltage dependent and were estimated to be in the rangeof 7.98 ± 1.46 ms (at $-$ 35 mV) and 3.11 ± 0.24 ms (at $-$ 5mV) forthe slow component and 1.33 ± 0.43 and 0.51 ± 0.03 ms (n = 16),for the fast inactivating component (Fig. 4, $open circle$ ).

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Fig. 4. Activation and inactivation kinetics of the whole cell sodium current. The original current (

; top) was best fitted (scattered line) with a 3rd-order exponential for activation (time constant $tau$ _a) and a double exponential for inactivation (time constants $tau$ _i,1 and $tau$ _i,2). Increasing the amounts of CO₂ and HCO led to a decline of the time constant of activation in the voltage range of $-$ 35 to $-$ 20 mV (left, bottom), while the time constants of inactivation decreased over the entire voltage range with increasing CO₂/HCO (middle and right).

ACTIVATION IN CO₂/HCO-BUFFERED SALINE. After performing the described protocols the bath perfusion was switched from HEPES buffer to solutions containing differentamounts of CO₂ and HCO. Cells weresubjected to solutions containing 2.5% CO₂/5.6 mM HCO,5% CO₂/18 mM HCO, and 10% CO₂/37 mMHCO, with the same pH of 7.3 for allsolutions. Half the cells were tested with solutions in ascendingorder of the amounts of CO₂ and HCO,while the other half were tested with solutions in descendingorder to avoid any hysteresis effect induced by the order of solutionchanges. Because the effects were fully reversible, no differencewas found between the two sequences of solution exchanges. Datawere pooled and are presented as mean values. No sign of a solutiondependent alteration in g_max was observed (Fig. 3) during theseexperiment. None of the g_max values obtained in the three CO₂/HCO-bufferedsolutions was significantly different from the value seen in HEPES-bufferedsolution, which could be shown by one-way ANOVA analysis (Table1). Changing to a solution with low CO₂/HCObuffering (i.e.: 2.5% CO₂ and 5.6 mM HCO)following the HEPES condition induced only small alterations ofthe currents (Fig. 2A, top). The mean peak amplitude (at $-$ 15 mV)was merely unaffected (Fig. 2B, $black-triangle$ ) with a value of $-$ 5.4 ± 0.6nA, while the potential of half-maximal activation V_h,a was negativelyshifted by $-$ 5.8 ± 2.1 mV (Fig. 5B1) to a voltage of $-$ 33.2 ± 2.7,and the slope (V_c) was almost unchanged 3.8 ± 0.4 mV. Increasingthe amounts of CO₂ and HCO in thebath solution led to a more pronounced negative shift of V_h,aand to a significant increase of the current amplitude. The additionof the 5% CO₂/18 mM HCO-buffered salineresulted in a shift of V_h,a by $-$ 13.1 ± 1.8 mV to $-$ 40.5 ± 2.2 mV,which was significantly different from the V_h,a measured in HEPESsolution (one-way ANOVA: P < 0.05, Fig. 5B1), and in a raise ofthe peak amplitude to $-$ 6.7 ± 0.8 nA (at $-$ 25 mV). Again the slopeV_c was only slightly affected (3.4 ± 0.4 mV). The shift of voltagedependence and increase in amplitude was most pronounced in the10% CO₂/37 mM HCO-containing solution,with $Delta$ V_h,a: $-$ 19.4 ± 1.8 mV (V_h,a: $-$ 46.9 ± 1.8 mV; P < 0.05) anda peak amplitude value of $-$ 7.9 ± 1.0 nA (at $-$ 35 mV; P < 0.05).No alteration of the slope V_c (3.5 ± 0.6 mV) was observed (Figs.2B and 5B1). The shift of V_h,a, induced by increasing amountsof CO₂ and HCO, was almost linearwithin the concentration-range measured with a slope-rate of $-$ 0.7mV/mM HCO. Nevertheless it cannotbe excluded that with even higher amounts of CO₂ and HCO,this function will break away from linearity. A subtraction ofthe I-V curves obtained in HEPES-buffered solution from thosein CO₂/HCO-containing solutions revealedan increase in current amplitude that was most prominent in thevoltage range of $-$ 50 to $-$ 30 mV (Fig. 5A1).

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Table 1. Whole cell calcium current properties in HEPES- and CO₂/HCO-buffered solutions

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Fig. 5. A: mean differential current constructed by subtracting I-V curves obtained in HEPES-buffered solution from I-V curves derived with CO₂/HCO in the bathing solution. A prominent increase in current amplitude and a shift to more negative potentials was seen when both CO₂ and HCO were raised (A1). The huge amplitude in differential current reflects also the negative shift of the potential of half-maximal activation during these experiments. The same alterations take place when only the concentration of bicarbonate was increased and CO₂ was held constant at 5% (A2). When CO₂ was increased but not HCO (18 mM), no differences between the 3 CO₂/HCO-buffered solution could be observed (A3). The maximal increase in current amplitude was observed in the voltage range of -50 to -30 mV in all experiments. B, 1-3: bar-charts showing shifts of the voltage dependence of activation (

) and inactivation (

) following superfusion with solutions containing different amounts of CO₂/HCO. Both, the potential of half-maximal activation (V_h,a) and inactivation (V_h,i) were negatively shifted with respect to the amount of CO₂/HCO (B1). Qualitatively the same shifts of V_h,i and V_h,a were observed when only the concentration of bicarbonate was increased while CO₂ was kept stable (B2). There was no correlation in the shifts of the V_h,i and V_h,a when the concentration of CO₂ (2.5, 5.0; 10%) was increased and the concentration of bicarbonate was held constant at 18 mM (B3). Insets: numbers of cells measured for the corresponding pairs of data in A and B.

Despite the pronounced increase in current amplitude, no sign of a solution-dependent alteration in g_max was observed becausethe values for the three CO₂/HCO-bufferedsolutions were (in ascending order): 197.3 ± 20.9, 205.5 ± 22.8,and 207.3 ± 21.3 nS (Fig. 3).

INACTIVATION IN CO₂/HCO-BUFFERED SALINE. Concomitantly with the shift of voltage dependence of activation, also the voltage parameters of the steady-state inactivationwere negatively shifted when the concentrations of CO₂/HCOwere elevated (Fig. 5B1). The potential of half-maximal inactivationwas shifted almost linearly (within the concentration-range measured;slope-rate: $-$ 0.6 mV/mM HCO) by $-$ 2.8± 1.2, $-$ 8.8 ± 1.1, and $-$ 16.2 ± 1.0 mV when CO₂/HCOwas added in ascending order (absolute values: $-$ 56.4 ± 1.9 mV, $-$ 62.4 ± 2.0 mV, P < 0.05; $-$ 69.8 ± 2.1 mV; P < 0.05). As with activation,no alteration of the slope (V_c) at the point V_h,i was observed(Table 1). The calculation of the pairwise difference betweenthe potentials of half-maximal activation and inactivation showedno significant difference among the solutions (-25.4 ± 2.2, $-$ 25.0± 2.8, $-$ 24.0 ± 2.1, and $-$ 24.0 ± 2.1 mV; n = 14). This demonstratedthat the effect took place to the same degree on the activationas well as on the inactivation properties of thecurrents.

KINETICS IN CO₂/HCO-BUFFERED SALINE. The prominent shift in voltage dependence of the current characteristics with increasing amounts of CO₂ and HCOwere accompanied by alterations of the inactivation and activationkinetics (Fig. 4, bottom). Both time constants for inactivationdecreased when CO₂ and HCO were increased,yielding values, in the 10% CO₂/37 mM HCO-containingsolution, of 4.13 ± 0.36 and 1.64 ± 0.25 ms ( $-$ 35 and $-$ 5 mV; n= 17) for the slow component and 0.64 ± 0.06 and 0.31 ± 0.03 msfor the fast current component. The time constant for activationshowed qualitatively the same reduction when cells were exposedto increasing amounts of bicarbonate and CO₂ with minimal valuesof 0.13 ± 0.01 ms ( $-$ 35 mV) and 0.12 ± 0.01 ms ( $-$ 5 mV) in the solutioncontaining 10% CO₂/37 mM HCO.

Bicarbonate but not CO₂ shifts the voltage dependence of sodium currents

In the first set of experiments, both compounds of the CO₂/HCO buffer were altered to keep theextracellular pH constant. It was therefore not possible to statewhether CO₂ or bicarbonate modulates the whole cell sodium current.In a second series of experiments, the concentration of CO₂ washeld constant at 5%, and the concentration of bicarbonate wasaltered (5.6; 18; 26 mM). Under these circumstances, extracellularpH varies considerably between the CO₂/HCO-bufferedsolutions (pH: 6.96; 7.30; 7.44; respectively). Therefore experimentswere carried out in which only one switch, from HEPES-bufferedsaline to the concerned CO₂/HCO-bufferedsaline was performed. The pH value of the HEPES- buffered salinewas adjusted to match the CO₂/HCO-bufferedsaline to avoid any effect by a difference in pH_o. The concentrationof the high bicarbonate containing solution (i.e., 37 mM HCO)was reduced to 26 mM HCO to preventprecipitation of CaCO₃ and CdCO₃. In total, 58 neurons wereinvestigated.

When I-V curves of the whole cell sodium current were constructed from the data obtained in HEPES-buffered solutions, a depressionof the current amplitude over the entire voltage range was observedwith more acidic pH_o values (Fig. 6B). This reduction was mainlydue to a slight, but not significant, decrease of g_max, concomitantlywith the decreased pH_o. As previously observed (Tombaugh and Somjen1996), only small and not significant shifts in the potentialsof half-maximal activation and inactivation could be elicited.The following switch to the corresponding CO₂/HCO-bufferedsolutions led to a clear evidence for a bicarbonate-concentration-dependenteffect on the voltage properties of activation and inactivation(Fig. 5B2). The potential of half-maximal activation and inactivationwas negatively shifted, in a significant way, with increasingbicarbonate amounts, when compared with values achieved in thecorresponding HEPES-buffered saline (Table 1). Within the concentrationrange measured the half-maximal potentials shifted by 0.5 mV/mMdissolved HCO. Again, it could beshown by calculating the pairwise difference between V_h,a andV_h,i that both the activation and inactivation properties wereeffected in the same manner. When the differences of currentsobtained in HEPES- and CO₂/HCO-bufferedsolutions were plotted, it became obvious, that the increase incurrent amplitude was most prominent in the voltage range between-50 to -30 mV (Fig. 5A2). This effect was similar to the experimentalseries described before. The slope parameters (V_c) for inactivationand activation remained unchanged and showed no concentration-dependenteffect. The same applied to the maximal sodium conductance, whichdid not significantly increase during these experiments.

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Fig. 6. The role of intra- and extracellular pH on the modulation of sodium currents. A: the current-voltage relationship of the current was slightly shifted to more negative potentials and amplitude was moderately depressed when neurons were exposed to 23 mM acetate, which induces an intracellular acidification. The differential current showed a different course than was seen after a change to CO₂/HCO-buffered solutions because it was negative in the range $-$ 50 to $-$ 20 mV and became than positive with more positive voltages. B: extracellular pH differences lead to an increase in amplitude with more alkaline pH values, but not to a shift of the I-V curve.

Lack of modulation by CO₂

As a complementary series of experiments, also CO₂/HCO-buffered solutions were tested, which containedequal quantities of bicarbonate (18 mM) but different amountsof CO₂ (2.5, 5.0, and 10%). This was done to justify whether bicarbonatealone can modulate the whole cell sodium currents or whether CO₂has an additional effect. Again the pH values of the HEPES-bufferedsolutions were adjusted to fit with the values of the correspondingCO₂/HCO-buffered saline (pH: 7.5,7.30, 7.0). Briefly, the use of solutions with different CO₂ concentrations,but constant amounts of bicarbonate, did not change any of thecurrent parameters in a concentration- and CO₂-dependent manner.The potential of half-maximal activation V_h,a was negatively shiftedby about the same amount in all three solutions (Fig. 5B3) with $-$ 11.4 ± 2.5 mV (6), $-$ 12.8 ± 1.6 mV (18), and $-$ 8.5 ± 1.3 mV (n= 6). A similar result was obtained for the half-maximal potentialof inactivation ( $Delta$ V_h,i: 9.9 ± 1.3, 9.0 ± 1.1, and 8.2 ± 0.4 mV).Also the slope factors (V_c) of both activation and inactivationand, furthermore, the maximal sodium conductance did not differbetween the solutions tested. Finally, the difference (Fig. 5A3)between I-V curves obtained in HEPES- and CO₂/HCO-bufferedsolutions was similar for all three CO₂ amounts, indicating thatvariations of CO₂ do not modulate the voltage dependence of thewhole cell sodiumcurrents.

Effects of internal pH on whole cell sodium currents

The role of pH in the modulation of sodium currents has previously been demonstrated (Tombaugh and Somjen 1996). To estimatethe fraction of effect, which could be attributed to an alterationof intracellular pH, we conducted a small experimental seriesin which neurons were exposed to bath solutions containing 23mM Na-acetate. Because the acetic acid crosses the membrane likethe carbonic acid, this solution mimics the acid load of the neurons,which can be assumed during exposure to CO₂/HCO-containingsolutions. The intracellular pH during these experiments was controlledby only 10 mM HEPES, instead of 50 mM, to show the maximum effectof the intracellular pHchanges.

With this weak intracellular pH buffering, several changes of the sodium current properties were observed during the measurements.The maximal conductance was decreased by 23 ± 12% (112.4 ± 6.5vs. 87.2 ± 14.9 nS; P = 0.11; n = 5), which is opposite to theeffects seen with CO₂/HCO-bufferedsolution, where a small, but not significant, increase was found.Negative shifts of the potentials of half-maximal activation ( $-$ 9.6± 1.6 mV; n = 5; P < 0.05) and inactivation ( $-$ 4.3 ± 1.0 mV; P< 0.05) were observed when acetate was introduced. Neverthelessthis shift was grossly only half the size of the maximal shiftobserved with CO₂/HCO-containing solutions.Because the shift in the voltage sensitivity and the decreaseof g_max have opposite effects on the peak size of the I-V curve,only a small, but not significant, decrease of the peak amplitudewas observed (Fig. 6A). Furthermore the difference current fromthe I-V curves derived under the acetate and nonacetate conditionshowed a clearly different course than was seen with CO₂/HCO-bufferedsolution. Because in the voltage range $-$ 40 to $-$ 30 mV, the currentwas negative, like in the other experiments, while in the rangemore positive than $-$ 25 mV, it gained positivevalues.

	DISCUSSION

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Bicarbonate modulates sodium current activation and inactivation

The present study indicates the potential role of bicarbonate ions as a modulator of voltage dependent properties of wholecell sodium currents in CA1 neurons of the rat. Bicarbonate, ina concentration-dependent manner, shifts the potential of half-maximalactivation and inactivation to more negative voltages, leavingthe slopes of the activation and inactivation curves unaffected.Variation of the CO₂ contents of the solutions (from 2.5 to 10%)did not have any additional effect, showing that bicarbonate alonemodulates the voltage dependence of the sodium currents. The negative,bicarbonate-dependent shift of V_h,i made the mean peak currentamplitude highly sensitive to small voltage changes close to themembrane potential, which is different to the situation in HEPES-bufferedsaline. Bicarbonate did not change the maximal conductance ofthe investigated sodium currents. The latter effect is in contrastto the result found on whole cell calcium currents from the sametype of neurons. In this case, a prominent reduction of the maximalconductance induced by bicarbonate ions was observed (Bruehl etal. 2000). This difference is responsible for the fact that undercertain circumstances, the amplitude of the sodium currents increaseswith the increase of bicarbonate concentration rather than decreasesas demonstrated for calcium currents. The increase of the sodiumcurrent amplitude can further be explained by the negative shiftof the activation threshold (resp. the V_h,a), which results inan increase of the number of sodium channels being opened at morenegative membrane voltages at which the sodium ions are subjectto a stronger drivingforce.

The lack of effect on the sodium conductance and the prominent reduction of the calcium conductance points toward the possibilitythat bicarbonate ions act in a different way on both channeltypes.

Sodium current amplitude and amount of bicarbonate

Recently, Gu et al. (2000) demonstrated that CO₂/HCO-buffered saline can shift both the potentialof half-maximal activation and inactivation to more negative potentialsin mice neurons. This is in line with the present study. In addition,they stated that this saline did not change the total amplitudeof the whole cell sodium current. In contrast, the present studydemonstrates a strong voltage sensitivity of the sodium currentamplitude, depending on the amount of dissolved bicarbonate. Increasingconcentrations of bicarbonate shifted the Boltzmann curve of inactivationin negative direction (up to $-$ 70 mV) to voltages close to restingmembrane potential (i.e., approximately $-$ 65 mV). With the steepslope of the curve close to resting potential, it is expectedthat even small voltage changes strongly alter the number of inactivatedsodium channels. Therefore the sodium current amplitude and theresulting action potential will be larger with potentials morenegative than about -70 mV and much smaller with potentials positiveto this value. This feature of the sodium current in CO₂/HCO-bufferedsaline is different from the situation in solutions with low concentrationsof bicarbonate or even in HEPES-buffered saline. Under these circumstances,the potential of half-maximal inactivation is far away (approximately $-$ 54 mV) from the resting potential value, which leaves the sodiumcurrent amplitude almost independent from voltage changes aroundrestingpotential.

Previous studies have shown that the excitability of the neuronal network is reduced when brain slices or cell cultures aresuperfused with CO₂/HCO-buffered salineinstead of a HEPES-buffered solution (Cowan and Martin 1995, 1996;Gu et al. 2000). This observation fits with the presented data $---$ inthe case that bicarbonate is low enough $---$ and the previous findingthat whole cell calcium currents are reduced (Bruehl et al. 2000),when CO₂/HCO is used as the pH buffersystem. The present study also points out that the excitabilitymight be increased under certain conditions when the bicarbonateconcentration is sufficiently high (Church 1992, 1999; Churchand McLennan 1989) and neurons are temporarily hyperpolarizedbeyond resting potential. Under these conditions, the shift inactivation increases the sodium current amplitude, while the steady-stateinactivation has little effect. Regarding the negative shift ofthe potential of half-maximal activation (V_h,a), one can predictthat the action potential threshold also should shift to morenegative potentials with increasing concentrations of dissolvedbicarbonate. Indeed, such a shift of activation threshold wasfound by Church and McLennan (1989) on intracellular recordedCA1 neurons in slice preparations. They found the activation thresholdlowered $<=$ 9 mV, when the bath solution was switched from 26 to72 mM bicarbonate, and a positive shift ( $<=$ 16 mV) following a switchto bicarbonate-free (HEPES-buffered) media (Church 1992). Furthermore,both studies demonstrated that neurons that were quiet in low-or bicarbonate-free media became spontaneously firing when higherbicarbonate concentrations were used. This again can be explainedby a threshold for action potential firing that is closer to therestingpotential.

The present study also demonstrates that the inactivation kinetics of the sodium current is strongly affected by bicarbonate.The time constants of both components decreased over the entirevoltage range measured, while the time constant of activationdecreased only in the range between $-$ 35 up to $-$ 25 mV, but remainedunchanged at more positive values. Consequently, the inactivationbecomes more efficient in terminating the current at potentialsmore positive to -25 mV, for example during the generation ofaction potentials. The lack of a so-called overshoot of the actionpotential, which occasionally occurs in vivo (Witte et al. 1996)but also in vitro (Gu et al. 2000); see there Fig. 2A), may bea consequence of this faster inactivation in CO₂/bicarbonate-bufferedsolution because the current shuts down before the zero voltagelevel has beenreached.

The concentration values at which bicarbonate acts on the whole cell sodium current are clearly in the physiological rangeobserved in brain in vivo, which has been shown to be 24-26 mMduring normal activity (Betz et al. 1989). During pathophysiologicalprocesses, like metabolic acidosis, respiratoric alkalosis orhypercapnia this normal level can be changed by 10-15 mM in bothdirections. Under these circumstances, it is most likely thatthe excitability of the network changes, not only by pH alterations(Church 1999; Tombaugh and Sapolsky 1990, 1996, 1997) but alsoby differences in bicarbonate concentration in the braintissue.

Changes of the intracellular pH

When bicarbonate/CO₂-free bath solutions are exchanged by solutions containing these compounds, the trans-membraneous passageof CO₂ into cells leads, at least transiently, to a decline ofthe intracellular pH, due to liberation of protons in accordanceto the Henderson-Hasselbalch equation. It is conceivable thatsuch changes contributed to the alterations of sodium currentsin our experiments. Nevertheless, our data obtained by superfusingneurons with bath solutions containing 23 mM Na-acetate, a solutionthat mimics the acid introducing properties of HCO/CO₂-bufferedmedia, showed only subtle alterations of the currents. The intracellularpH was only weakly buffered by 10 mM HEPES during these experiments.First, the maximal conductance decreased and the mean peak amplitudewas merely unchanged. Second, the potentials of half-maximal activationor inactivation showed smaller potential shifts in negative directionas was seen in HCO/CO₂-buffered solution.Furthermore, Tombaugh and Somjen (1997) have shown that an increaseof the intracellular buffering power by enhancing the HEPES concentrationblunted pH-related effects on whole cell calcium currents by $>=$ 50%.These observations indicate that the alteration of sodium currentsby bicarbonate-buffered solutions are mainly related to the modulatingaction of the bicarbonate ions, and are only minimally contaminatedby pH-related effects. Further evidence for this conclusion arisesfrom the experiment in which bicarbonate was kept constant (at18 mM) and CO₂ was altered from 2.5 to 10%. This should alterintracellular pH values and cause cumulative changes of the sodiumcurrent properties. However, such changes of the sodium currentswere notobserved.

As for the modulating action of bicarbonate ions on whole cell calcium currents, we still do not know how these ions can interactwith the sodium channel pores. The mechanisms underlying the modulationof sodium currents by protons were discussed earlier in detail(Hille 1992) and might help to understand the way of modulationby bicarbonate ions. First of all, modulation of the channelsneeds charged ions, which can interfere with the charged domainsof the channel proteins. This theoretically rules out any actionof the uncharged molecule CO₂. In practice, our data stronglysupport this hypothesis. Three theories have been proposed ofhow protons may alter the characteristics of the sodium channels.Two titration theories that assume that protons may titrate negativesurface charges or negative acid groups within the channel havebeen favored. The covering of the sodium ion attracting sitesshould end up in a decrease of the single channel conductance,which explains the reduced sodium permeability at low extracellularpH. A reduced sodium conductance has not been observed in thepresent study, when bicarbonate ions act as the modulator. Thisfinding supports the third explanation, the gating theory, becausean influence of the modulator on the gating properties of thechannels does not result in an alteration of the conductance,but in a shift of voltage dependence of the activation and inactivation.In fact alterations of the gating properties of sodium channelsby CO₂/HCO solutions have been demonstratedby Gu et al. 2000. Taken together, the lack of effect on the conductanceand the shift in activation and inactivation, shown in the presentstudy, plus the findings of Gu makes the gating theory, the mostconceivable mechanism of how bicarbonate ions act on sodium currentchannels. To substantiate this assumption, further studies onthe single channel level and/or binding studies arenecessary.

	ACKNOWLEDGMENTS

The authors thank M. Sreji $c'$ and D. Steinhoff for perfect technicalassistance.

The investigations were supported by Sonder Forschungsbereich 194B2.

	FOOTNOTES

Address for reprint requests: C. Bruehl, Dept. of Neurology; Friedrich-Schiller-University; Erlanger Allee 101, 07745 Jena,Germany (E-mail: bruehl{at}med.uni-jena.de).

REFERENCES

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ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Betz AL, Goldstein GW, and Katzmann R. Blood-brain-cerebrospinal fluid barriers. In: Basic Neurochemistry, edited by Siegel GJ, Agranoff BW, Albers RW, and Molinoff PB. New York: Raven, 1989, p. 591-606.
Bruehl C, Wadman WJ, and Witte OW. Concentration dependence of bicarbonate-induced calcium current modulation. J Neurophysiol 84: 2277-2283, 2000[Abstract/Free Full Text].
Church J. A change from HCO₃( $-$ )-CO₂- to HEPES-buffered medium modifies membrane properties of rat CA1 pyramidal neurons in vitro. J Physiol 455: 51-71, 1992[Abstract/Free Full Text].
Church J. Effects of pH changes on calcium-mediated potentials in rat hippocampal neurons in vitro. Neuroscience 89: 731-742, 1999[ISI][Medline].
Church J, and McLennan H. Electrophysiological properties of rat CA1 pyramidal neurons in vitro modified by changes in extracellular bicarbonate. J Physiol 415: 85-108, 1989[Abstract/Free Full Text].
Cowan AI, and Martin RL. Simultaneous measurement of pH and membrane potential in rat dorsal vagal motoneurons during normoxia and hypoxia: a comparison in bicarbonate and HEPES buffers. J Neurophysiol 74: 2713-2721, 1995[Abstract/Free Full Text].
Cowan AI, and Martin RL. Ionic basis of the membrane potential responses of rat dorsal vagal motoneurones to HEPES buffer. Brain Res 717: 69-75, 1996[ISI][Medline].
Gu XQ, Yao H, and Haddad GG. Effect of extracellular HCO(3)( $-$ ) on Na(+) channel characteristics in hippocampal CA1 neurons. J Neurophysiol 84: 2477-2483, 2000[Abstract/Free Full Text].
Hille B. Ionic Channels of Excitable Membranes., Sunderland, MA: Sinauer, 1992.
Ketelaars SO, Gorter JA, van Vliet EA, Lopes da Silva FH, and Wadman WJ. Sodium currents in isolated rat CA1 pyramidal and dentate granule neurones in the post-status epilepticus model of epilepsy. Neuroscience 105: 109-120, 2001[ISI][Medline].
Kortekaas P, and Wadman WJ. Development of HVA and LVA calcium currents in pyramidal CA1 neurons in the hippocampus of the rat. Brain Res Dev Brain Res 101: 139-147, 1997[Medline].
Tombaugh GC, and Sapolsky RM. Mild acidosis protects hippocampal neurons from injury induced by oxygen and glucose deprivation. Brain Res 506: 343-345, 1990[ISI][Medline].
Tombaugh GC, and Somjen GG. Effects of extracellular pH on voltage-gated Na⁺, K⁺, and Ca²⁺ currents in isolated rat CA1 neurons. J Physiol 493: 719-732, 1996[ISI][Medline].
Tombaugh GC, and Somjen GG. Differential sensitivity to intracellular pH among high- and low-threshold Ca²⁺ currents in isolated rat CA1 neurons. J Neurophysiol 77: 639-653, 1997[Abstract/Free Full Text].
reugdenhil M, and Wadman WJ. Enhancement of calcium currents in rat hippocampal CA1 neurons induced by kindling epileptogenesis. Neuroscience 49: 373-381, 1992[ISI][Medline].
Witte OW, Bruehl C, and Hossmann KA. Metabolic and electrophysiological effects of focal epileptic discharges on surrounding and remote brain tissue in the rat cortex. Epilepsy Res Suppl 12: 157-162, 1996[Medline].

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Relation Between Bicarbonate Concentration and Voltage Dependence of Sodium Currents in Freshly Isolated CA1 Neurons of the Rat

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