NMDA Receptor-Mediated Na+ Signals in Spines and Dendrites

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The Journal of Neuroscience, June 15, 2001, 21(12):4207-4214

NMDA Receptor-Mediated Na⁺ Signals in Spines and Dendrites
Christine R. Rose and Arthur Konnerth
Institut für Physiologie, Ludwig-Maximilians-Universität München, D-80802 München, Germany

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Spines and dendrites of central neurons represent an important site of synaptic signaling and integration. Here we identifya new, synaptically mediated spine signal with unique properties.Using two-photon Na⁺ imaging, we show that suprathreshold synaptic stimulation leadsto transient increases in Na⁺ concentration in postsynaptic spines and their adjacent dendrites.This local signal is restricted to a dendritic domain near thesite of synaptic input. In presumed active spines within thisdomain, the Na⁺ level increases by 30-40 mM even during short bursts of synapticstimulation. During a long-term potentiation induction protocol(100 Hz, 1 sec), the Na⁺ level in the active spines reaches peak amplitudes of ~100 mM.We find that the Na⁺ transients are mainly mediated by Na⁺ entry through NMDA receptor channels and are detected duringthe coincident occurrence of synaptic potentials and backpropagatingaction potentials. The large amplitudes of the Na⁺ transients and their location on dendritic spines suggest thatthis signal is an important determinant of electrical and biochemicalspinecharacteristics.

Key words: dendrite; spine; two-photon imaging; sodium; NMDA; coincidence detection; hippocampus

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Dendritic spines represent the major postsynaptic input site for excitatory transmission in the brain (Harris and Kater, 1994).Despite this central feature, their role in information processingis still not completely understood (Koch and Zador, 1993; Harris,1999; Segal et al., 2000). So far, two classes of spine signalshave been observed during synaptic transmission. One class ofsynaptically induced spine signals is changes in the membranepotential. These can be recorded only at distant sites, becausespines themselves are inaccessible to direct electrical measurements.In recent years, the development of high-resolution imaging techniqueshas enabled the detection of a second spine signal (Denk et al.,1996) that is composed of transient elevations in the intracellularCa²⁺ concentration (Eilers and Konnerth, 1997; Yuste et al., 2000).

When the postsynaptic membrane is sufficiently depolarized, influx of Ca²⁺ into spines can be mediated through NMDA receptors and induceactivity-dependent changes in synaptic properties such as long-termpotentiation (LTP) or long-term depression (LTD) (Malenka, 1994).Close to the resting potential, another type of glutamate receptor,the so-called AMPA receptor, which in general is much less permeableto Ca²⁺, isactivated.

The major current carrier for both glutamate-gated channels, however, is Na⁺. Therefore, excitatory synaptic transmission is also expectedto significantly alter the postsynaptic Na⁺ concentration. Indeed, dendritic Na⁺ accumulation induced by synaptic stimulation was observed incerebellar Purkinje and hippocampal CA1 neurons (Lasser-Ross andRoss, 1992; Miyakawa et al., 1992; Callaway and Ross, 1997). Inthese studies, however, no spatial resolution of spines was obtained,and an analysis of the spatial distribution of the signals couldnot be performed. Moreover, no estimate concerning the actualamplitude of the Na⁺ changes wasmade.

A more detailed knowledge of postsynaptic Na⁺ transients is desirable because changes in the electrochemical Na⁺ gradient will alter the reversal potential of excitatory synapticcurrents and Na⁺-dependent transporters such as Na⁺/Ca²⁺-exchange (Blaustein and Lederer, 1999) and therefore could significantlyinfluence synaptic function. Moreover, several studies indicatedthat Na⁺ might play a role in activity-dependent synaptic plasticity.An earlier report showed that Na⁺ influx through AMPA receptor channels is required for the inductionof LTD in cerebellar Purkinje neurons (Linden et al., 1993). Inhippocampal neurons, intracellular Na⁺ increases have been proposed to increase the open probabilityof NMDA receptors via activation of the protein tyrosine kinaseSrc and thus might control the gain of excitatory transmission(Yu and Salter, 1998).

In the present study we used two-photon Na⁺ imaging in combination with whole-cell patch-clamp recordings (Rose et al., 1999)to measure action potential (AP)-induced and synaptically inducedNa⁺ signals in spines and dendrites in a hippocampal slice preparation.This technique is particularly well suited for measurement ofNa⁺ transients in small cellular compartments because excitationis limited to the focal plane, allowing imaging in the intact,scattering tissue (Denk et al., 1990). Our results demonstratethe presence of local postsynaptic Na⁺ transients in spines and dendrites. We provide evidence thatNa⁺ transients are mediated mainly by Na⁺ entry through NMDA receptor-gatedchannels.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Tissue preparation and patch-clamp recordings. CD-1 mice (Charles River; 3-5 weeks old) were anesthetized and decapitated.Transverse hippocampal slices (300 µm) were prepared as describedpreviously, and standard techniques were used for somatic whole-cellpatch-clamp recordings (Edwards et al., 1989). CA1 pyramidal cellswere generally held at membrane potentials of $-$ 60 to $-$ 65 mV; granulecells of the dentate gyrus were held at $-$ 75 to $-$ 80 mV. Becauseof better space-clamp characteristics, voltage-clamp experimentswere exclusively performed on granule cells. The intracellularsolution for patch-clamp experiments contained (in mM): 120 K⁺-gluconate, 10 HEPES, 32 KCl, 4 NaCl, 0.16 EGTA, 4 Mg-ATP, 0.4NaGTP, 2 tetraammonium salt of sodium-binding benzofuran isophthalate(SBFI) (Molecular Probes, Eugene, OR) and was titrated with KOHto a pH of 7.3. During experiments, slices were perfused withphysiological saline containing (in mM): 125 NaCl, 4 KCl, 1.25NaH₂PO₄, 26 NaHCO₃, 2 CaCl₂, 1 MgCl₂, 20 glucose, continuouslybubbled with 95% O₂/5% CO₂ resulting in a pH of 7.4. GABAergictransmission was blocked by using 10 µM bicuculline methiodide.Experiments were performed at room temperature (22-24°C). To mimicburst activity of CA3 neurons, Schaffer collaterals were electricallystimulated by five 2 msec square pulses delivered at 50 Hz viaa thin glass pipette filled with saline. To activate granule cells,the stimulation electrode was placed in the molecular layer ofthe dentate gyrus. The stimulation pipettes were placed at a distanceof 10-15 µm from the dendrites. Stimulation strength was set justbelow action potential firing threshold for subthreshold stimulationand just above firing threshold for suprathresholdstimulation.

Na⁺ imaging. Imaging was performed using a custom-built two-photon laser-scanning microscope based on a mode-locked Ti:sapphirelaser system operated at 790 nm center wavelength, 80 MHz pulserepeat, <100 fsec pulse width (Tsunami and Millenia, Spectra Physics,Mountain View, CA), and a laser-scanning system (MRC 1024, Bio-Rad,Herts, UK) mounted on an upright microscope (BX50WI, Olympus,Tokyo, Japan) equipped with 20 × 0.5 NA and 60 × 0.9 NA waterimmersion objectives (Olympus). Neurons were filled with SBFIvia the patch pipette for at least 45 min before the recordingswere started. Images were acquired at 4-8 Hz. Background-correctedimages were analyzed off-line with a custom-written routine inLabView (National Instruments, Austin, TX). In situ calibrationof SBFI fluorescence with Na⁺ ionophores enabled the determination of the actual magnitudeof the Na⁺ changes (Rose and Ransom, 1997; Rose et al., 1999). Unless specifiedotherwise, data are expressed as means ± SEM, and data tracesshown are averages of one to three consecutive trials. Data werestatistically analyzed by a Student's t test (significance level,p < 0.005).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

By combining whole-cell patch-clamp recordings with two-photon laser-scanning microscopy (Denk et al., 1990), we analyzedsynaptically and action potential-induced Na⁺ changes in apical dendrites and spines of neurons in hippocampalslice preparations of 3- to 5-week-old mice. Common patterns ofactivity in the hippocampus are bursts of two to seven actionpotentials (Otto et al., 1991; Lisman, 1997). To induce such burstactivity in CA1 pyramidal neurons, Schaffer collaterals were electricallystimulated by trains of five pulses delivered at 50 Hz. Granulecells of the dentate gyrus were similarly activated by placingthe stimulation electrode in the molecular layer of the dentategyrus.

Spatial profile of Na⁺ transients

Suprathreshold synaptic activation leads to widespread elevations of Ca²⁺ throughout the dendritic tree because of backpropagation of actionpotentials and the resulting opening of voltage-gated Ca²⁺ channels (Jaffe et al., 1992; Markram et al., 1995; Sprustonet al., 1995b; Yuste and Denk, 1995). Because apical dendritesof CA1 pyramidal neurons also express voltage-gated Na⁺ channels (Stuart et al., 1997), we first determined the spatialprofile of synaptically induced dendritic Na⁺ accumulations. Figure 1 shows intracellular Na⁺ transients induced by suprathreshold synaptic stimulation (fivestimuli resulting in four to five postsynaptic APs) (Fig. 1b)along different regions of a secondary apical dendrite of a CA1pyramidal neuron.

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Figure 1. Local dendritic Na⁺ transients induced by synaptic stimulation. a, Reconstruction of a stack of 27 optical sections taken at 1.5 µm intervals through part of a CA1 pyramidal neuron filled with 2 mM SBFI (objective: 60 × 0.9 NA). The brackets numbered 1-6 indicate the dendritic regions from which fluorescence measurements in c were obtained. The position of the stimulation electrode is indicated schematically. Scale bar, 20 µm. Distance of region 1 from the cell body is 120 µm. b, Membrane potential change at the soma (V_m) induced by five afferent stimuli at 50 Hz as indicated in the bottom trace. c, Na⁺ transients in the dendritic regions 1-6 caused by suprathreshold afferent stimulation as in b. Na⁺ transients were maximal in region 4, which was closest to the stimulation pipette. Na⁺ changes in the different regions were measured successively, because the focal plane did not include the complete dendrite. d, Bar graph summarizing the normalized amplitude of activity-induced dendritic Na⁺ transients (mean ± SEM). The bars represent 4-16 observations taken from 16 cells. The bar at $-$ 40 µm summarizes data from two experiments. The amplitude of Na⁺ transients decayed monoexponentially with increasing distance from the region of maximal response with a length constant ( $lambda$ ) of ~30 µm. The arrowhead in c indicates the time of synaptic stimulation.

When the stimulation electrode was placed in close proximity to the dendrite (10-15 µm) (Fig. 1a), synaptically induced Na⁺ transients were maximal in the dendritic region, which was near(10-50 µm) the pipette (Fig. 1c). Synaptic activation of the postsynapticdendrite is expected from Ca²⁺ imaging measurements that were performed under similar conditions(Kovalchuk et al., 2000). Furthermore, to assure that these changeswere not caused by direct activation of voltage-sensitive channelsby the stimulation current, we applied the postsynaptic blockers6-cyano-7-nitroqionoxaline-2,3-dione (CNQX; 10 µM) and DL-2-amino-5-phosphovalericacid (APV; 100 µM). During perfusion with these drugs, both membranepotential changes and Na⁺ transients were abolished, indicating that they were indeed causedby synaptic activity (n = 4; data notshown).

The amplitudes of Na⁺ transients reached ~10 mM in the experiment depicted in Figure 1 [for calibration procedures, see Roseet al. (1999)]. This region of maximal response extended acrossa dendritic length of 20-30 µm. With increasing distance fromthe region of maximal response, the site of synaptic input, theamplitude of the Na⁺ transients decayed in a monoexponential fashion with a lengthconstant ( $lambda$ _Na⁺) of ~30 µm (n = 16 cells) (Fig.1d). In other dendritic branches, small Na⁺ signals just above the detection threshold (~1-2 mM) were observed.This is in line with an earlier study in which we showed thatshort bursts of backpropagating action potentials cause only minorchanges in Na⁺ concentration throughout the dendritic tree (Rose et al., 1999).

These results demonstrate that suprathreshold stimulation leads to local Na⁺ transients that occur in dendritic domains near the site of synapticactivation. In all subsequent experiments, the analysis of Na⁺ transients was confined to dendritic regions and their adjacentspines ~15-20 µm proximal and distal to the position of the stimulationpipette.

Na⁺ transients require suprathreshold stimulation

Whereas suprathreshold activation has been reported to induce widespread dendritic Ca²⁺ transients (Markram et al., 1995; Yuste and Denk, 1995; Jaffeand Brown, 1997), subthreshold stimulation can elicit local dendriticCa²⁺ signals that are confined to the site of activation (Markramand Sakmann, 1994; Eilers et al., 1995; Yuste and Denk, 1995;Kovalchuk et al., 2000). Synaptically induced dendritic Na⁺ signals, however, could be detected only with suprathresholdsynaptic stimulation (Fig. 2). When the stimulation strength wasset just below the threshold for action potential firing, no measurablechange in the Na⁺ level was observed. Increasing the stimulation strength justabove firing threshold, in contrast, resulted in prominent Na⁺ transients in the apical dendrites of CA1 pyramidal cells (n= 25) (Fig. 2a,b). The amplitudes of these Na⁺ transients were dependent on the number of suprathreshold stimuli.Five stimuli (four to five action potentials) resulted in dendriticNa⁺ transients that amounted to 13.4 ± 1.1 mM (n = 33 cells) (Fig.3e) and three stimuli (two to three action potentials) evokedNa⁺ transients of 8.6 ± 1.7 mM (n = 6 cells; data not shown), whereasa single stimulus resulting in one action potential evoked a Na⁺ rise close to the detection threshold (4.3 ± 1.0; n = 7 cells;data not shown).

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Figure 2. Na⁺ transients require suprathreshold stimulation. a, Left, Reconstruction of a stack of 24 optical sections taken at 5 µm intervals through an SBFI-filled CA1 pyramidal cell. The white box indicates the area enlarged in the right panel. Right, Spiny dendrite from the same cell taken at higher resolution (15 stacks at 0.4 µm). The position of the stimulation electrode is indicated schematically. The arrows indicate the dendritic region from which measurements in b were obtained. b, Suprathreshold synaptic stimulation (top traces) induced a prominent Na⁺ transient in the dendrite, whereas subthreshold stimulation (bottom traces) did not result in a measurable Na⁺ increase. c, Left, Stack of 20 optical sections (3.5 µm intervals) through a granule cell of the dentate gyrus filled with SBFI. The white box indicates the area enlarged on the right. Right, Spiny dendrite from the same cell (15 stacks at 0.7 µm); the stimulation electrode is indicated schematically. The arrows indicate the dendritic region from which measurements in d were obtained. d, Suprathreshold stimulation evoked a Na⁺ transient in the dendrite (top traces). Subthreshold stimulation, in contrast, did not result in a Na⁺ transient (bottom traces). Scale bars: a, 50 µm, inset, 5 µm; c, 20 µm, inset, 5 µm. Arrowheads in b and d indicate the time of synaptic stimulation. Calibration for d is shown in b.

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Figure 3. Synaptically induced Na⁺ transients in spines. a, Image of the spiny dendrite of a CA1 pyramidal cell chosen for the experiment depicted in b and c. Closed arrowheads indicate active spines; open arrowheads indicate passive spines from which measurements in c were taken. Scale bar: 5 µm; distance from the cell body: 140 µm. b, Suprathreshold stimulation (5 afferent stimuli at 50 Hz) induced five APs as measured at the soma. c, Left, Average activity-induced Na⁺ transient in spines (average of 19 spines) and in the dendrite (top traces). Middle traces, Na⁺ transients in three single passive spines. Bottom traces, Na⁺ transients in three single active spines. Data points of single spine traces were binned by a factor of 2 to improve the signal-to-noise ratio. Right, The recovery of dendritic Na⁺ transients and passive spines could be fitted by a monoexponential decay with similar time constants ( $tau$ ). Recovery in active spines followed a biexponential time course ( $tau$ _f, fast decay constant; $tau$ _s, slow decay time constant). The spine traces on the right represent averages of the single spine traces depicted on the left. d, Histogram of peak Na⁺ transients of all spines. Individual data were pooled in steps of 2.5 mM Na⁺. The data were fitted by two Gaussian functions revealing a bimodal distribution. e, Top, Mean amplitudes ± SEM of activity-induced Na⁺ increases in dendrites and spines. The amplitude in active spines was significantly higher than those in passive spines and dendrites. Bottom, Mean decay time constants ( $tau$ ) ± SEM of activity-induced Na⁺ increases. The fast time constant ( $tau$ _f) of active spines was significantly different from the slow time constant ( $tau$ _s). Arrowheads in c indicate the time of synaptic stimulation.

Activity-induced Na⁺ transients were not restricted to CA1 pyramidal cells but could also be evoked in granule cells of thedentate gyrus. As observed for CA1 pyramidal cells, measurabledendritic Na⁺ transients were elicited only with suprathreshold synaptic stimulation( $Delta$ Na⁺ = 11.6 ± 1.5 mM; n = 8) (Fig. 2c,d).

Na⁺ transients in spines

We next attempted to identify "active" spines (Denk et al., 1995; Yuste and Denk, 1995), that is, the spines directly activatedduring synaptic stimulation. As reported above for dendritic Na⁺ transients, synaptically induced Na⁺ signals in spines were observed only with suprathreshold stimulation(the signal-to-noise ratio allowed reliable detection of Na⁺ transients in single spines of ~5 mM). Unambiguous identificationof active spines was difficult because suprathreshold stimulationproduced Na⁺ transients in all spines of the active domain. The plotting ofa distribution histogram of peak Na⁺ transients of all spines, however, revealed a bimodal distributionof response amplitudes, clearly indicating the presence of twoclasses of spines (Fig. 3d).

In the first class of spines (75% of 152 spines; n = 18 cells), the Na⁺ level rose by 14.6 ± 1.8 mM (stimulation parameters set to fivepulses at 50 Hz) (Fig. 3b), a level that was only slightly higherthan that of the dendrites (~13 mM; see above and Fig. 3c-e).Moreover, the decay of the Na⁺ transients in these spines and in dendritic regions was monoexponentialwith time constants of 8.8 ± 1.6 sec (spines) and 9.0 ± 2.1 sec(dendrites; n = 16 cells) (Fig. 3c,e). In contrast, in the secondclass of spines (25% of 152; n = 18 cells), activity-induced Na⁺ transients were two to three times higher than those of the adjacentdendrite, reaching up to 35-40 mM (mean 35.7 ± 4 mM) (Fig. 3).Recovery followed a biexponential decay with a fast time constant( $tau$ _f) of 1.6 ± 0.5 sec and a slow time constant ( $tau$ _s) that was verysimilar to the dendritic decay constant (8.5 ± 1.9 sec) (Fig.3e). We assume, therefore, that these spines were the sites ofsynaptic input and thus the sites of synaptic Na⁺ influx (active spines). In the other class of spines, in whichthe amplitude and the time course of Na⁺ transients corresponded to that of the dendrites, the Na⁺ signals were probably caused by diffusion of free and SBFI-boundNa⁺ ions from their site of entry ("passive"spines).

Because of the relatively low image sampling frequency (4-8 Hz) and the required additional binning to improve the signal-to-noiseratio of the fluorescence signals from single spines, our measurementsvery likely underestimated the peak amplitude of the Na⁺ increase in active spines. Earlier calculations estimated thata single presynaptic action potential results in a rapid Na⁺ increase by ~30 mM in postsynaptic spines during excitatory transmission(Sejnowski and Qian, 1992). For the same reasons, $tau$ _f, which mostlikely represents both active Na⁺ extrusion and diffusion of Na⁺ from spines to dendrites (Majewska et al., 2000), is probablyoverestimated. Furthermore, although SBFI concentration was low(2 mM) in comparison with the observed Na⁺ changes (~35 mM in spines), the dye will act as a buffer forNa⁺ and might alter Na⁺ dynamics in spines and dendrites, as has been reported for Ca²⁺ signals measured with fluorometric Ca²⁺ indicators (Helmchen et al., 1996). Finally, decay times of Na⁺ transients are dependent on temperature. In an earlier study,we showed that increasing the bath temperature from 23 to 33°Cdecreased the dendritic decay constant of action potential-inducedNa⁺ transients by a factor of 1.7, indicating that Na⁺/K⁺-ATPase activity plays a dominant role in restoring the electrochemicalNa⁺ gradient (Rose et al., 1999).

NMDA receptor dependence

To further analyze the mechanism of activity-induced Na⁺ transients, we studied the contribution of ionotropic glutamate receptors.In these and all subsequent experiments (except for those illustratedin Fig. 7a,b), fluorescence signals from all spines of a givendendrite were averaged. This resulted in average spine Na⁺ transients that were slightly larger than those of the parentdendrites (compare Figs. 3c, 4-6, 7c).

Blocking of glutamate receptors of the NMDA type with APV resulted in a reversible reduction of the stimulus-induced Na⁺ transients by ~80% in spines and dendrites, although the stimulationstill elicited action potentials (Figs. 4a, 5c) (n = 6). Duringperfusion with CNQX (10 µM), a blocker of non-NMDA receptors,the stimulation failed to elicit action potentials, and the activity-inducedNa⁺ transient was reduced by ~93% (Figs. 4b, 5c) (n = 4). Increasingthe stimulus intensity caused a pronounced depolarization andrestored the Na⁺ transient (Fig. 4b) (n = 2). This was most likely caused by anefficient removal of the Mg²⁺ block of NMDA receptor channels at the site of synaptic input.

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Figure 4. NMDA dependence of synaptically induced Na⁺ transients. a, Blocking glutamate receptors of the NMDA type with APV strongly reduced the stimulus-induced Na⁺ transient in the spines and the dendrite. b, CNQX, a blocker of non-NMDA receptors, blocked activity-induced Na⁺ transients. Increasing the stimulus intensity restored the Na⁺ transients. a, CA1 pyramidal neuron; b, dentate gyrus granule cell. Arrowheads in a and b indicate the time of synaptic stimulation. Calibration for b is shown in a; distance from the cell body in a = 120 µm; in b = 80 µm.

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Figure 5. Membrane potential dependence of Na⁺ transients. a, Na⁺ transients induced by suprathreshold stimulation were suppressed when cells were held in the voltage-clamp mode. Removing extracellular Mg²⁺ relieved this voltage dependence. b, In the absence of extracellular Mg²⁺, the amplitudes of the Na⁺ transients were similar when the cells were held in the current-clamp and voltage-clamp mode. c, Normalized mean amplitudes of dendritic activity-induced Na⁺ transients ± SEM in control conditions (1), during perfusion with APV (2), CNQX (3), during voltage clamp (4), and during voltage clamp in 0 Mg²⁺ (5). d, Normalized mean amplitudes of activity-induced Na⁺ transients ± SEM during current clamp and voltage clamp. a, b, Dentate gyrus granule cells; distance from the cell body in a = 60 µm; in b = 90 µm. Arrowheads in a and b indicate the time of synaptic stimulation.

Na⁺ transients induced by suprathreshold stimulation were suppressed by >77% during voltage clamp. Removing extracellular Mg²⁺ relieved this voltage dependence and resulted in the expectedaugmentation of the amplitude of the Na⁺ increase to ~172% of control levels (Fig. 5a,c) (n = 7). In theabsence of extracellular Mg²⁺, the amplitudes of the Na⁺ transients were undistinguishable between stimulations performedwhen cells were held in the current-clamp mode (allowing the generationof action potentials) compared with those in the voltage-clampmode (Fig. 5b,d) (n = 9). This demonstrates that the influx ofNa⁺ through voltage-gated Na⁺ channels during backpropagating action potentials does not significantlycontribute to the observed Na⁺ transients, even during concomitant synaptic activation of NMDAreceptors.

These results indicate that the observed postsynaptic Na⁺ transients are largely mediated by Na⁺ entry through NMDA receptor channels, whereas Na⁺ entry through AMPA receptor channels or voltage-gated Na⁺ channels plays only a minor role. Indeed, because of the considerablylonger time course of synaptic NMDA receptor currents (Sprustonet al., 1995a), Na⁺ influx through these NMDA channels will be larger by far thanthat through AMPA-gatedchannels.

To further quantify the Na⁺ influx through NMDA receptors, we performed experiments in which cells were held in the voltage-clampmode in the absence of extracellular Mg²⁺ and in the presence of CNQX, and the stimulation intensity wasincreased stepwise (Fig. 6a) (n = 6). We then plotted the measuredcharge against the corresponding Na⁺ increase and found a linear correlation with a slope of 5.3 pC/mMNa⁺ (Fig. 6b,c). This result corresponds closely to the predictionbecause the influx of 1 mM Na⁺ into a given dendrite with a length of 20 µm and a diameter of2 µm will result theoretically in a loss of 6 pC negative charge.

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Figure 6. Correlation between charge and Na⁺ increase. a, Membrane currents (I_NMDA) and corresponding Na⁺ transients at four different increasing stimulation intensities. Experiments were performed in the voltage-clamp mode in the absence of extracellular Mg²⁺ and in the presence of CNQX. b, Plot of the mean values ± SEM of six experiments. Individual data points were pooled in steps of 5 mM Na⁺. The mean values follow a linear regression line (r = 0.994) with a slope of 5.3 pC/mM Na⁺. c, Histogram of mean values ± SEM for measured charge per millimolar Na⁺ for experiments in which no CNQX was present (1; compare Fig. 5a) and for experiments in which CNQX was added to the saline (2). Experiments were performed in dentate gyrus granule cells; distance from the cell body in a = 100 µm.

In the voltage-clamp experiments performed in the presence of CNQX (see above), the correlation between charge and [Na⁺] increase was not significantly different from the experimentsperformed with no CNQX added (Figs. 5a, third row, 6c). This controlexperiment clearly confirms that the influx of Na⁺ through AMPA-gated channels does not contribute significantlyto the measured, synaptically induced Na⁺transients.

Na⁺ transients during an LTP induction protocol

Repetitive activation of excitatory synapses in the hippocampus causes a long-lasting increase in synaptic strength calledLTP that is considered to be a cellular model for learning andmemory (Bliss and Collingridge, 1993; Malenka, 1994). Usually,LTP is induced by a tetanic synaptic stimulation using stimulationfrequencies of 100 Hz for 1 sec. The critical trigger for LTPis a rise in intracellular Ca²⁺ after NMDA receptor channel opening (Malenka, 1994).

To analyze Na⁺ changes during a typical LTP induction protocol, we performed a synaptic stimulation at 100 Hz for 1 sec whilemeasuring Na⁺ transients in dendrites and spines of CA1 pyramidal neurons.In these experiments, the calcium chelator BAPTA (10 mM) was addedto the pipette solution to prevent postsynaptic Ca²⁺ accumulation and LTP induction. As illustrated in Figure 7, aand b, the Na⁺ concentration increased by 44.6 ± 4.2 mM (n = 7) in dendritesduring the tetanus. Again (compare Fig. 3), two classes of spinescould be distinguished. Although Na⁺ transients in passive spines were similar to those measured inthe dendrite, Na⁺ increased to values of >100 mM in active spines. These resultsdemonstrate that tetanic stimulation causes enormous postsynapticNa⁺ transients, which may play a role in the induction process ofLTP. Furthermore, during a short period (1-2 sec), the drivingforce for Na⁺ will break down and synaptic transmission will collapse. It isimportant to note that Na⁺ entry through cation channels activated by metabotropic glutamatereceptors may partially contribute to the Na⁺ transients during this prolonged stimulation (Congar et al.,1997).

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Figure 7. Na⁺ transients during tetanic stimulation and during coincident presynaptic and postsynaptic activity in CA1 pyramidal cells. a, Image of the spiny dendrite chosen for the experiment depicted in b. Closed arrowheads indicate active spines; open arrowheads indicate passive spines from which measurements in b were taken. Scale bar, 5 µm. b, Top, Membrane potential change induced by synaptic stimulation at 100 Hz/1 sec. Bottom, Average Na⁺ transients in 16 spines and in the dendrite induced by the tetanic stimulation; Na⁺ transients in two single passive spines; and Na⁺ transients in two single active spines. Data points of single spine traces were binned by a factor of 2 to improve the signal-to-noise ratio. c, Effect of coincident presynaptic and postsynaptic activity on the amplitude of synaptically induced Na⁺ transients. Suprathreshold synaptic activation caused Na⁺ transients in both dendrite and adjacent spines, whereas subthreshold stimulation did not result in measurable Na⁺ increases. Backpropagating APs evoked only minor Na⁺ changes. Combining backpropagating APs with subthreshold synaptic stimulation, however, resulted in a supralinear summation of Na⁺ transients of both spines and dendrites. d, Histogram comparing the normalized mean amplitudes ± SEM of activity-induced Na⁺ transients during suprathreshold stimulation (1), subthreshold stimulation (2), backpropagating APs (3), and pairing of backpropagating APs with subthreshold stimulation (4). The arrowheads in b and c indicate the time of synaptic stimulation; distance from the cell body in a = 150 µm; in c = 250 µm.

Na⁺ transients during coincident presynaptic and postsynaptic activity

Na⁺ spikes actively invade dendrites of hippocampal pyramidal cells (Jaffe et al., 1992; Spruston et al., 1995b), and the coincidenceof presynaptic and postsynaptic activity can lead to supralinearincreases in postsynaptic Ca²⁺ (Magee and Johnston, 1997; Markram et al., 1997; Koester andSakmann, 1998; Schiller et al., 1998). To analyze whether sucha supralinearity also exists for postsynaptic Na⁺ signals in dendrites and spines, we investigated the effect ofcoincident presynaptic and postsynaptic activity on the amplitudeof synaptically induced Na⁺ transients. Figure 7c shows such an experiment. As illustratedabove (compare Fig. 2), suprathreshold synaptic activation causeda prominent Na⁺ transient, whereas subthreshold stimulation did not result inmeasurable Na⁺ increases. Backpropagating APs, evoked by 2 msec square pulsecurrent injection at the soma at 50 Hz, caused no or only minorNa⁺ changes (on average 17% of control) (Fig. 7d) (cf. Rose et al.,1999). Combining backpropagating APs with subthreshold synapticstimulation, however, resulted in a supralinear summation of Na⁺ influx into both spines and dendrites. The pairing of presynapticand postsynaptic activity induced Na⁺ transients that reached ~75% of those with suprathreshold stimulation(Fig. 7d) (n = 7/8 cells). These results demonstrate that theoccurrence of postsynaptic APs in coincidence with presynapticactivity was the critical parameter for the induction of NMDA-receptor-mediatedpostsynaptic Na⁺transients.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Local Na⁺ transients in apical dendrites and spines

Our results demonstrate a new and unique type of synaptically induced signal in dendrites and spines that consists of postsynapticNa⁺ transients. Although a direct comparison is problematic becausespatial and temporal characteristics of measured ion changes dependon the binding characteristics of the indicator used (Helmchenet al., 1996), the Na⁺ signals appear to differ in several ways from postsynaptic Ca²⁺ signals reported earlier. First, suprathreshold stimulation protocolsevoke widespread elevations in Ca²⁺ because of influx of Ca²⁺ through voltage-gated Ca²⁺ channels activated by backpropagating action potentials (Jaffeet al., 1992; Markram et al., 1995; Spruston et al., 1995b; Yusteand Denk, 1995). Na⁺ transients elicited by suprathreshold stimulation seem to bemore restricted to defined dendritic regions directly at and adjacentto the stimulation site. As reported earlier (Rose et al., 1999),influx of Na⁺ via voltage-gated Na⁺ channels during short trains of backpropagating action potentialscauses only minor Na⁺ increases throughout the dendritictree.

Second, postsynaptic Na⁺ signals in spines as well as in dendrites were observed only with suprathreshold stimulation, whereasalready single, subthreshold stimuli induce Ca²⁺ signals in spines (Denk et al., 1995; Eilers et al., 1995, Yusteand Denk, 1995, Koester and Sakmann, 1998; Schiller et al., 1998).The absence of subthreshold Na⁺ signals in spines might be related to the fact that these signalswere too small to be detected with our technique. In any case,this result indicates that Na⁺ accumulations in active spines during subthreshold stimulationare probably negligible (<5 mM) in comparison with those evokedby suprathreshold stimulation (30-40 mM).

Third, our results strongly suggest that the dominating pathways for Na⁺ entry during suprathreshold synaptic activation are NMDA receptorchannels. Postsynaptic Ca²⁺ signals, in contrast, can be mediated by several mechanisms:influx through NMDA receptor channels, influx through voltage-gatedCa²⁺ channels, and release from intracellular stores (Markram andSakmann, 1994; Denk et al., 1995; Nakamura et al., 1999; Yusteet al., 1999; Kovalchuk et al., 2000; Schiller et al., 2000).

Our ability to detect large Na⁺ gradients between active spines and the adjacent dendrite with our relatively low image-samplingfrequency (4-8 Hz) was surprising. The existence of such gradientsthat were maintained over hundreds of milliseconds suggests theexistence of a diffusion barrier or a buffer system, or both,for Na⁺ in the spines. The apparent diffusion coefficient for free Na⁺ is ~13 × 10⁶ cm²/sec (Push and Neher, 1988) and about twice that value for SBFI-boundNa⁺ [assuming that the diffusion coefficient is similar to that offura-2 (Push and Neher, 1988)]. Unrestricted equilibration ofNa⁺ and SBFI-bound Na⁺ between distances of ~1 µm will be accomplished, therefore, withinmilliseconds. Because diffusion from spines to the adjacent dendriteis slowed by a factor of 10-100 by the spine neck (Svoboda etal., 1996), Na⁺ gradients between spine and adjacent dendrites should be largelyequilibrated within ~100msec.

Significant gradients between spines and the adjacent dendritic shaft have also been reported for Ca²⁺ signals (Jaffe and Brown, 1997; Yuste et al., 1999; Kovalchuket al., 2000; Majewska et al., 2000), suggesting that spines maybe chemically isolated from dendrites. In addition to the diffusionbarrier caused by spine necks, calcium pumps or other Ca²⁺ uptake systems and Ca²⁺ buffers might be responsible for the observed biochemical isolationof spines (Koch and Zador, 1993; Maeda et al., 1999). Similarlyone could speculate about a high presence of Na⁺ pumps (Na⁺-K⁺-ATPase) in spine necks that might account for the compartmentalizationin Na⁺. Alternatively, the spine head may contain molecules that bindand buffer Na⁺.

Functional implications of postsynaptic Na⁺ transients

The NMDA receptor channels are widely accepted as coincident detectors of presynaptic and postsynaptic activity (Malenka,1994). They were shown to mediate a supralinear increase in postsynapticCa²⁺ signals during pairing of an action potential with synaptic stimulation(Yuste and Denk, 1995; Magee and Johnston, 1997; Markram et al.,1997; Koester and Sakmann, 1998; Schiller et al., 1998). Our resultsindicate that NMDA receptor activity might be involved in yetanother signal for coincidence detection, which consists of Na⁺ transients. Postsynaptic Na⁺ transients seem to be ideally suited for coincidence detectionbecause they are restricted to the site of activation and exhibitall-or-none characteristics in that they require the occurrenceof postsynaptic APs in coincidence with presynapticactivity.

Although the direct physiological role of Na⁺ accumulations in spines is unclear, it is firmly established that the inwardlydirected Na⁺ gradient regulates many cellular processes, among them intracellularCa²⁺ homeostasis via Na⁺/Ca²⁺ exchange (Blaustein and Lederer, 1999). In presynaptic terminalsof cultured hippocampal cells, an elevation of Na⁺ was accompanied by an increase in Ca²⁺, causing enhanced transmitter release (Bouron and Reuter, 1996).A reduction in the Na⁺ gradient slowed Ca²⁺ extrusion in cerebellar neurons (Kiedrowski et al., 1994; Fierroet al., 1998). In granule cell presynaptic terminals, Ca²⁺ extrusion via the Na⁺/Ca²⁺ exchange leads to Na⁺ accumulation (Regehr, 1997). These studies indicate that Na⁺ accumulations in spines might shape the time course of postsynapticCa²⁺ transients and vice versa. Therefore, activation of Na⁺/Ca²⁺ exchange also might contribute partly to the synaptically inducedNa⁺ transients observed in our study. The Na⁺ changes measured during tetanic stimulation in the presence of10 mM BAPTA, however, indicate that considerable Na⁺ increases also occur without a contribution of Na⁺/Ca²⁺ exchange. Furthermore, a rise in postsynaptic Na⁺ will slow the Na⁺-dependent uptake of glutamate or may even lead to its reversaland therefore could influence excitatory transmission (Attwellet al., 1993).

Another emerging possibility is that increases in Na⁺ concentration might induce synaptic plasticity by selectively increasingthe open probability of NMDA receptors, a process that is controlledby a channel-associated Src kinase (Yu and Salter, 1998). Thismechanism might be especially powerful during more intensive stimulationprotocols and could be important in the Src-dependent inductionof LTP in CA1 hippocampal neurons (Lu et al., 1998). Thus, synapticallyinduced NMDA-dependent Na⁺ accumulations in spines might provide an efficient mechanismof autoregulation of NMDA conductance and input-specific strengtheningof active synapses. It is important to note that in isolated patchrecordings, [Na⁺] elevations by 30-40 mM were sufficient to upregulate the NMDAreceptor function (Yu and Salter, 1998). Under our conditionsof stimulation with an LTP-inducing protocol, we saw Na⁺ peak levels of >100 mM in activespines.

Finally, an important possibility that must be considered is that increases in intracellular Na⁺ will reduce the driving force for glutamatergic currents. Atrest, the reversal potential of AMPA and NMDA receptor-mediatedcurrents is close to 0 mV. Short synaptic bursts will brieflyreduce their reversal potential to approximately $-$ 35 mV [calculationbased on assumed peak intracellular concentrations of 35 mM Na⁺ (see Results) and 130 mM K⁺, and extracellular concentrations of 145 mM Na⁺ and 8 mM K⁺ ; see Materials and Methods and Dietzel and Heinemann (1985)].At this potential, NMDA receptor currents are already significantlyreduced because of voltage-dependent block by Mg²⁺ (Spruston et al., 1995a). With more intense synaptic activityand larger ion changes, the reversal potential for glutamatergiccurrents will be even more negative, which would eventually resultin dendritic saturation (Sejnowski and Qian, 1992; Bush and Sejnowski,1994). Glutamatergic currents will be largely diminished, therebyprotecting the postsynaptic input sites from excessive accumulationsof Na⁺ and Ca²⁺, which have been implicated in inducing cellular excitotoxicity(Lee et al., 1999). This intriguing prediction, however, willprobably be difficult to test experimentally at present, becausepeak ionic changes persist for only very short periods (Fig. 7).Nevertheless, it seems reasonable to speculate that dendriticsaturation caused by increases in postsynaptic Na⁺ levels during excitatory synaptic transmission could play animportant role in the input-specific protection of overexcitationof synapses. The development of specific Na⁺ chelators that are effective in the range of tens of millimolarwill help to test thishypothesis.

  FOOTNOTES

Received March 2, 2001; revised April 3, 2001; accepted April 5, 2001.

This study was supported by the Deutsche Forschungsgemeinschaft and the Bundesministerium für Bildung undForschung.
Correspondence should be addressed to Christine R. Rose, Institut für Physiologie, Ludwig-Maximilians-Universität München,Biedersteiner Strasse 29, D-80802 München, Germany. E-mail: rose{at}lrz.uni-muenchen.de.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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