Glutamate Release through Volume-Activated Channels during Spreading Depression

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The Journal of Neuroscience, August 1, 1999, 19(15):6439-6445

Glutamate Release through Volume-Activated Channels during Spreading Depression
Trent A. Basarsky, Denise Feighan, and Brian A. MacVicar
Department of Physiology and Biophysics, Neuroscience Research Group, University of Calgary, Calgary, Alberta T2N 4N1, Canada

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Volume-sensitive organic anion channels (VSOACs) in astrocytes are activated by cell swelling and are permeable to organicanions, such as glutamate and taurine. We have examined the releaseof glutamate through VSOACs during the propagation of spreadingdepression (SD). SD was induced by bath application of ouabainin hippocampal brain slices and was monitored by imaging intrinsicoptical signals, a technique that provides a measure of cellularswelling. The onset of SD was associated with increased lighttransmittance, confirming previous studies that cellular swellingoccurs during SD. NMDA receptor antagonists, either noncompetitive(MK-801, 10-50 µM) or competitive (CGS-17355, 100 µM), reducedthe rate of propagation of SD, indicating that glutamate releasecontributes to SD onset. SD still occurred in zero Ca²⁺-EGTA (0-Ca²⁺-EGTA) solution, a manipulation that depresses synaptic transmission.HPLC measurements indicated that, even in this solution, therewas significant glutamate release. Two lines of experiments indicatedthat glutamate was released through VSOACs during SD. First, 5-nitro-2-(3-phenylpropylamino)benzoic acid (NPPB), a blocker of VSOACs, depressed the rate ofpropagation of SD in a manner similar to NMDA antagonists. Second,NPPB inhibited the release of glutamate during SD in 0-Ca²⁺-EGTA external solution. These results indicate that cellularswelling during SD causes the activation of VSOACs and the releaseof glutamate by permeation through this channel. Cellular swellingis a result of neuronal activity and is observed during excitotoxicity.Therefore, glutamate release from VSOAC activation could occurunder conditions of cell swelling and contribute to excitotoxicdamage.

Key words: volume-sensitive organic anion channels; astrocytes; volume-sensitive chloride channels; NMDA receptors; intrinsic optical imaging; ischemia; CLC-3; swelling

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Volume-sensitive organic anion channels (VSOACs) [also called volume-sensitive chloride channels (I_cl,vol)] are a potentialsource of glutamate efflux in the CNS because they are permeableto glutamate (Strange et al., 1996). Volume changes in astrocytesactivate VSOACs in a process involving mitogen-activated proteinand tyrosine kinases (Crepel et al., 1998) and the cytoskeleton(Lascola et al., 1998). VSOACs have also been described recentlyin cerebellar neurons (Patel et al., 1998). Efflux of Cl and anions, such as glutamate, aspartate, and taurine, throughVSOACs helps to restore volume through a process called regulatoryvolume decrease (RVD) that also involves K⁺ channels (Pasantes-Morales and Schousboe, 1989; Pasantes-Moraleset al., 1990, 1994a,b). We designed these experiments to testthe hypothesis that glutamate efflux through volume-activatedchannels occurs during spreading depression(SD).

SD is a wave of glial and neuronal depolarization and cellular swelling that slowly propagates through gray matter of theCNS (Van Harreveld and Khattab, 1967; Leao, 1944; Somjen et al.,1992; Jing et al., 1994; Nicholson and Sykova, 1998). Intrinsicoptical signals, which measure the changes in light transmittancein tissue, provide an indirect measure of cell volume changesbecause increased light transmittance through brain slices isassociated with cellular swelling (MacVicar and Hochman, 1991;Andrew and MacVicar, 1994; Holthoff and Witte, 1996). We previouslyrecorded intrinsic optical signals during SD and found that thepropagation of SD could be mapped by a wave of swelling (Basarskyet al., 1998). Activation of glutamate-permeable VSOACs by swellingof astrocytes and possibly neurons could contribute to glutamaterelease duringSD.

In our previous study, we mapped SD by imaging intrinsic optical signals and simultaneously monitored intracellular calciumdynamics by measuring fura-2 fluorescence (Basarsky et al., 1998).In normal artificial CSF (aCSF) containing calcium, an intracellularcalcium wave was associated with SD. However, SD still propagatedin 0 external Ca with 2 mM EGTA with no detectable changes inintracellular calcium. Because glutamate release is thought tocontribute to the propagation of SD (Mody et al., 1987; Lauritzenet al., 1988; Marrannes et al., 1988; Lauritzen and Hansen, 1992),we hypothesized that at least some of the glutamate efflux duringSD could be attributable to VSOAC activation not involving calcium-dependentrelease from neurons and/or astrocytes. If glutamate release throughVSOAC was contributing to SD, then we predict the following. First,NMDA receptor antagonists should depress the propagation of SDin isolated brain slices (Marrannes et al., 1988; Lauritzen andHansen, 1992). Second, 5-nitro-2-(3-phenylpropylamino) benzoicacid (NPPB), an antagonist for VSOACs (Crepel et al., 1998), shoulddepress the propagation of SD. Third, glutamate should still bereleased from brain slices during SD, even after depressing synaptictransmission in solutions containing 0 external calcium and 2mM EGTA. Finally, NPPB should depress the Ca-insensitive releaseof glutamate from brain slices during SD. We have used intrinsicoptical imaging of ouabain-induced SD and HPLC measurement ofglutamate efflux to demonstrate that glutamate release from VSOACscontributes to the propagation ofSD.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experiments were performed as described previously (Basarsky et al., 1998). A brief description of these methods is givenbelow.

Slices. Hippocampal slices (400 µm) were prepared from 16- to 23-d-old Sprague Dawley rats. Slices were maintained in aCSFaerated with 95% O₂-5% CO₂ for a minimum of 1 hr after preparationbefore experiments were performed. For all experiments, the sliceswere transferred to a superfusion chamber mounted to the imagingsetup described below. Slices were maintained at 33-34°C and heldin place with platinum wires during the experiment. Control experimentswere always performed each day on slices obtained from the sameanimal from which the experimental slices were prepared. Controlexperiments were alternated with experiments in which transmitterantagonists were applied to ensure that the slices were healthyand that there was no rundown in the quality of thetissue.

Imaging. The intrinsic optical imaging system was composed of a COHU 4982 charge-coupled device camera connected to an AxonImage Lightning 2000 frame grabber (Axon Instruments, Foster City,CA) that was driven by Axon Imaging Workbench (version 2.1; AxonInstruments). The illumination source was a standard Zeiss (Oberkochen,Germany) tungsten bulb whose output was directed through a 750DF20discriminating filter. Typically, four frames were averaged foreach image. This approach allowed the visualization of SD at asampling frequency of 1 Hz, which was sufficiently fast giventhe relatively slow propagation rate of SD. The intrinsic opticalsignals were recorded and presented as subtracted images, withthe first image acquired during acquisition serving as the referenceimage, which was then subtracted from all subsequent images duringacquisition. The intrinsic optical signals were acquired at afrequency of 1 Hz but were saved to disk at a variable frequencyof between 0.008 and 1.0 Hz to reduce data storage requirements.We described the rate of change of intrinsic optical signals duringspreading depression as the change in the intensity in a specifiedzone region of the subtracted image per second ( $Delta$ T/T%). Quantificationof intrinsic optical signals during SD was performed as describedby Basarsky et al. (1998), their Figure3.

Solutions. Regular aCSF contained (in mM): NaCl, 124; KCl, 5; MgCl₂, 1.3; CaCl₂, 2; glucose, 10; and NaHCO₃, 26.2. For thezero calcium aCSF (0-Ca²⁺ aCSF), calcium was replaced with magnesium, and 2 mM EGTA wasadded, yielding a 0-Ca²⁺ aCSF that contained (in mM): NaCl, 114; KCl, 5; MgCl₂, 3.3; glucose,10; NaHCO₃, 26.2; and EGTA, 2. The pH was adjusted to 7.37 forboth of these solutions. NPPB was purchased from BIOMOL">Biomol (PlymouthMeeting,PA).

HPLC. The methods described by Saleh et al. (1997) were used to measure amino acid content in the superfusate, with the followingmodifications. One milliliter samples were collected at 1 minintervals. These samples were lyophilized and reconstituted into50 µl aliquots for HPLC analysis. This ensured that the concentrationof glutamate was well within detection limits and also allowedfor the perfusion of the slice at flow rates that minimized slicedeterioration. Although taurine is often measured during cellularswelling experiments, it was not possible to always discern thetaurine peak from the arginine peak in our HPLC experiments. Consequently,taurine was notanalyzed.

Statistics. Unless otherwise stated, all statistics were performed with the Mann-Whitney U test. GB-STAT version 3.53 (DynamicMicrosystems) was used for all statisticalcalculations.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glutamate is involved in the initial phase of spreading depression

In hippocampal brain slices in normal aCSF, ouabain induced spreading depression, which propagated throughout the hippocampus,and was measured as a transient increase in tissue transmittance(Fig. 1A). Previous reports (Marrannes et al., 1988; Gill et al.,1992; McLachlan, 1992; Nellgard and Wieloch, 1992; Martin et al.,1994; Willette et al., 1994; Obrenovitch and Zilkha, 1996; Tatlisumaket al., 1998) have demonstrated that spreading depression in vivois delayed or inhibited by glutamate receptor antagonists. Inhippocampal brain slices, application of the noncompetitive NMDAreceptor antagonist MK-801 (50 µM) inhibited the onset of spreadingdepression (Fig. 1B). In the presence of MK-801, there was a slowand uniformly distributed increase in tissue transmittance throughoutthe CA1 region. This widespread increase was followed by a propagatingdecrease in light transmittance (Fig. 1B). In contrast, in controlconditions, there was a rapidly propagating increase in lighttransmittance that was followed by a decrease in transmittance(Fig. 1A).

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Figure 1. Time course of ouabain-induced spreading depression in hippocampal slices. A, Spreading depression in control conditions. SD rapidly initiated in CA1 and propagated throughout the entire CA1 region as a wave of increased light transmittance followed by a rapid decrease. B, Spreading depression in the presence of 50 µM MK-801, after preincubation for 20 min in MK-801. The waveform of SD was different in that the initial increase in light transmittance was slow, but this was still followed by a rapidly propagating wave of decreased transmittance. C, Bright-field image of the slice used in A. The purple dot denotes a typical region used for measurements, and the CA1 region has been shown in A and B. Ouabain (100 µM) was added at 1 minute 30 seconds. All times are given in minutes:seconds. Scale bar, 100 µm.

The time course of the light transmittance changes during SD at a single region in the stratum radiatum of CA1 is shown fromsingle experiments in Figure 2 and is summarized in Figure 3.In addition to the noncompetitive antagonist MK-801, we also examinedthe effects of the competitive NMDA receptor antagonist CGS-19755(100 µM). Both MK-801 and CGS-197555 inhibit the onset of spreadingdepression. Furthermore, the effect of MK-801 was approximatelyfourfold greater at 50 µM than at 10 µM. Quantification of thekinetics of spreading depression revealed that MK-801 and CGS-19755greatly inhibited the onset slope of spreading depression (Fig.3B) and that MK-801 at the highest concentration attenuated thepeak change in transmittance (Fig. 3A). In paired control slices,the onset slope was typically 10 $Delta$ T/sec. After bath applicationof antagonist, the onset slope decreased to 0.4 ± 0.02 $Delta$ T/sec(n = 21) in 10 µM MK-801, 0.4 ± 0.04 $Delta$ T/sec (n = 21) in 100 µMCGS-19755, and 0.1 ± 0.01 $Delta$ T/sec (n = 18) in 50 µM MK-801. Incontrast, CNQX, an antagonist to the AMPA receptor, did not alterSD. We preapplied CNQX at 30 µM, which we have observed completelyblocks AMPA-mediated synaptic potentials (data not shown) andfound it had no significant effect on the peak amplitude of SD(65 ± 8 $Delta$ T; n = 5; vs CNQX, 63 ± 5 $Delta$ T; n = 5) or the maximum rateof rise (control, 2.2 ± 0.7; n = 5; vs CNQX, 2.1 ± 0.4; n = 5).Together, these data indicate that glutamate plays an importantrole the initial phase of spreading depression; inhibition ofNMDA-type glutamate receptors suppresses the onset of spreadingdepression.

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Figure 2. Time course of spreading depression in the presence of NMDA receptor antagonists. Each trace represents the change in transmittance in a single region of interest (as denoted in Fig. 1) recorded in separate brain slices. The top trace is a profile of spreading depression in a control slice. The bottom three traces are profiles of spreading depression in separate brain slices incubated in the indicated NMDA receptor antagonist. Both the competitive antagonist (CGS-19755) and the noncompetitive antagonist (MK-801) reduced the onset of SD, and the effects of MK-801 were dose-dependent. Solid bar represents the time of application of ouabain (100 µM).

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Figure 3. Quantification of the effects of NMDA receptor antagonists on spreading depression. A, The amplitude of the peak response was only reduced significantly by 50 µM MK-801 (p < 0.01) but was not significantly affected by CGS-19755 (100 µM) or MK-801 (10 µM) (p > 0.05). B, The onset slope was reduced by both the competitive (CGS-19755) and noncompetitive (MK-801) NMDA receptor antagonists. Note that the scale in B is split to enable the display of both control and antagonist measurements.

Inhibition of VSOACs inhibits the initial phase of spreading depression

We examined the effects of the VSOAC antagonist NPPB (100 µM) under normal conditions and under conditions in which synapticrelease of neurotransmitter is inhibited. In normal Ca externalsolution, the addition of NPPB slowed the decline of the SD waveform.The decline at 30 sec is reduced from 47 ± 6% (n = 14) in controlsolution with calcium to 2 ± 0.5% (n = 14) in control with NPPB.This is consistent with the role for Cl channels in regulatoryvolume decrease after the swelling during SD. In external 0-Ca²⁺, spreading depression occurs in a normal manner, albeit withslower kinetics (Jing et al., 1993; Herreras et al., 1994) (Figure4B) as we have shown previously (Basarsky et al., 1998). Underthese conditions, inhibition of VSOACs by NPPB further reducedthe onset slope of spreading depression (Fig. 4A,B). Incubationof slices with 100 µM NPPB caused a significant reduction in theonset slope from 1.43 ± 0.4 $Delta$ T/sec in paired controls in 0-Ca²⁺ to 0.53 ± 0.05 $Delta$ T/sec in NPPB (p < 0.01; n = 7). The declineof the SD signal in 0-Ca²⁺ was also slowed from 35 ± 2% (n = 21) to 19 ± 2% (n = 18) inNPPB. We also examined the effects of threo-hydroxy- $beta$ -aspartate(THBA), which has been shown to block glutamate release causedby reverse transport in astrocytes after extracellular application(Rutledge and Kimelberg, 1996). A 40 min preapplication of 1 mMTHBA had no effect on the maximum signal in SD (control, 77 ±5%; vs THBA, 80 ± 8%; n = 10) nor on the maximum rate of riseof the SD signal (control, 4.1 ± 0.6%/sec; vs THBA, 4.5 ± 0.6%/sec).

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Figure 4. NPPB, a VSOAC antagonist, inhibited the onset of spreading depression. A, Representative traces of the light transmittance changes in the presence and absence of external calcium and in the presence of the VSOAC antagonist NPPB (100 µM). B, Summary data for the effects of 0-Ca²⁺ and NPPB on the onset slope of spreading depression. In the absence of calcium, NPPB significantly inhibited the onset slope. Solid bar denotes the time of application of ouabain (100 µM).

Inhibition of VSOACs inhibits the release of glutamate during spreading depression

We next determined whether VSOACs are involved in the release of glutamate during spreading depression when synaptic transmissionwas greatly depressed in 0-Ca²⁺-EGTA solution. To do this, we used HPLC to measure glutamatelevels in the superfusate and examined the effect of the VSOACantagonist NPPB on glutamate release during spreading depression.Not surprisingly, HPLC measurements showed that, during SD incontrol solution with calcium, there was substantial increasein glutamate efflux to 2668 ± 1444% (n = 3) of control levels.When SD was observed in the brain slice in 0-Ca²⁺-EGTA solution, HPLC measurement showed that there was still asubstantial increase in the release of glutamate, GABA, and glutamine,although it was approximately eightfold less (Fig. 5). Incubationof slices with 100 µM NPPB resulted in a significant inhibitionof the release of glutamate (Fig. 5A,B). However the release ofboth GABA and glutamine was not depressed by NPPB, consistentwith previous observations that these amino acids do not significantlypermeate VSOACs. Together, these data are consistent with themodel that activation of VSOACs during spreading depression resultsin the calcium-independent release of glutamate, which contributesto the rapid onset of spreading depression. Inhibition of thesechannels inhibits the release of glutamate and delays the onsetof spreading depression.

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Figure 5. Inhibition of VSOACs inhibited the calcium-independent release of glutamate. All data were collected from brain slices incubated in 0-Ca²⁺-EGTA solution for at least 20 min before the start of the experiment. A, Representative HPLC measurements of glutamate release in the superfusate before and during SD in two separate brain slices. The initial onset of SD was measured using intrinsic optical signals and is taken as t = 0. SD propagated throughout the brain slice during the collection of superfusate and induced the release of glutamate, even in the 0-Ca²⁺-EGTA solution. Preincubation with NPPB (100 µM) reduced the release of glutamate during spreading depression. B, Effect of NPPB on glutamate, GABA, and glutamine release during spreading depression. Each point represents the increase in the indicated amino acid 7 min after the initiation of spreading depression from at least n = 5 separate brain slices. All numbers are expressed normalized to the initial levels before spreading depression. NPPB significantly depressed the release of only glutamate during SD (*p < 0.01) and had no effect on the release of either GABA or glutamine.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

These results provide the first evidence that glutamate release through VSOACs in the hippocampus contributes to the propagationof spreading depression. We confirmed the importance of glutamaterelease in spreading depression by describing the inhibition ofspreading depression by NMDA receptor antagonists. Using HPLC,we measured a significant release of glutamate during spreadingdepression, even in 0-Ca²⁺ aCSF in which conventional synaptic release is blocked. NPPB,an antagonist to VSOAC channels, depressed this calcium-insensitiverelease of glutamate and inhibited the rate of propagation ofspreadingdepression.

This study continues our previous work using intrinsic optical imaging to map spreading depression in the hippocampal slice(Basarsky et al., 1998). Intrinsic optical signals arise fromthe dynamics of light transmittance. For example, cellular swellingdecreases light scattering, resulting in an increase in lighttransmittance through the slice, whereas cellular shrinkage doesthe reverse (MacVicar and Hochman, 1991; Andrew and MacVicar,1994; Holthoff and Witte, 1996). The pattern of increased lighttransmittance during the onset of spreading depression indicatesthat there is substantial cellular swelling during spreading depression.In our previous study (Basarsky et al., 1998), we simultaneouslyimaged intrinsic optical signals and intracellular calcium changesusing fura-2 fluorescence measurements and found that a calciumwave was normally associated with spreading depression. However,we made the surprising discovery that, in 0-Ca²⁺ aCSF, spreading depression still occurred, and there were noassociated changes in intracellular calcium. These results, combinedwith the volume changes suggested by the intrinsic optical signals,indicated that spreading depression is a calcium-independent phenomenoninvolving cellularswelling.

In astrocytes and other cell types, swelling activates VSOACs that are permeant to chloride ions and organic anions, includingglutamate (Jackson and Strange, 1993; Sanchez-Olea et al., 1993;Pasantes-Morales et al., 1994a,b; Roy, 1994, 1995; Gonzalez etal., 1995; Lascola and Kraig, 1996; Strange et al., 1996; Crepelet al., 1998). The efflux of organic anions and Cl through VSOACs can contribute to the active process called RVDto restore the initial cellular volume (Pasantes-Morales et al.,1994a,b). The efflux of K⁺ through other channels also contributes to RVD. VSOACs have notbeen widely investigated in neurons but have recently been describedin cerebellar granule cells (Patel et al., 1998). CLC-3, a clonedCl-selective ion channel, is a good candidate for the VSOAC (Duanet al., 1997) and is highly expressed in the CNS and the hippocampus(Kawasaki et al., 1994). Therefore, VSOACs are present in thehippocampus and are likely found in both astrocytes andneurons.

We used NPPB to block the VSOAC for two reasons. First, NPPB has been reported to inhibit the VSOAC and the efflux of aminoacids activated by cell swelling in astrocytes and other celltypes (Rutledge et al., 1998). Second, NPPB inhibits the VSOACin a nonvoltage-dependent manner (Crepel et al., 1998), whichsuggests that NPPB will effectively inhibit the VSOAC in astrocytesat both the resting potential and the depolarized levels reachedduringSD.

The profile of the amino acid efflux during SD and the selective inhibition of glutamate release by NPPB are consistent withrelease of glutamate through VSOACs. The HPLC data showed thatglutamate and GABA are both released from hippocampal brain slicesduring SD in 0-Ca²⁺ aCSF. Glutamine was released to a lesser extent. Under theseconditions, synaptic transmission is negligible in brain slices(Schweitzer et al., 1992), and we have shown previously that thereare no detectable changes in intracellular calcium during SD (Basarskyet al., 1998). Therefore, we conclude that both glutamate andGABA can be released in high levels by non-Ca²⁺-dependent mechanisms. The relative contribution of glutamaterelease during SD through these mechanisms appears to be lessthan that caused by calcium-dependent exocytosis judging by theHPLC measurements of glutamate release. Only the glutamate effluxwas depressed by NPPB, which is consistent with studies that haveshown that glutamine does not permeate the VSOAC (Pasantes-Moraleset al., 1994a,b; Rutledge et al., 1998). We have not investigatedthe mechanisms by which GABA efflux occurs, but it is presumablybecause of anothertransporter.

The potential roles for reversed glutamate transport are difficult to unequivocally rule out because most inhibitors are competitiveand would not be expected to act on reverse transport (Kanai etal., 1993). However, the glial transporter is inhibited by externalapplication of THBA (Rutledge and Kimelberg, 1996). We have foundno effect of THBA onSD.

Previous studies have shown that NMDA receptor antagonists depress the activation of spreading depression in vivo (Marranneset al., 1988; Gill et al., 1992; McLachlan, 1992; Nellgard andWieloch, 1992; Martin et al., 1994; Willette et al., 1994; Obrenovitchand Zilkha, 1996; Tatlisumak et al., 1998). Our results pointto a pivotal role for NMDA receptor activation in the initialonset of SD. NMDA receptor antagonists decreased the rate of onsetof SD. This was observed with both the competitive antagonistCGS-197555 and the noncompetitive antagonist MK-801. The similarityof action of both types of NMDA antagonists is reassuring becauseMK-801 can affect other ion channels at higher concentrations(>100 µM) (ffrench-Mullen and Rogawski, 1989).

The results in this study suggest a new addition to the cellular mechanisms contributing to SD. The original hypothesis statedthat increased external K⁺ caused depolarization of both postsynaptic processes and presynapticterminals (Leao, 1944; Kraig and Nicholson, 1978; Van Harreveld,1978; Nicholson and Kraig, 1981; Somjen et al., 1992). Presynapticdepolarization of terminals evoked calcium-dependent synaptictransmission and the release of glutamate, which in turn furtherdepolarized postsynaptic elements and caused further increasesin external K⁺. This was thought to result in positive feedback between K⁺ accumulation and glutamate release leading to regenerative depolarizations.SD was thought to be a propagating wave of high K⁺-induced glutamate release and depolarization. However, studiesin brain slices in which synaptic transmission could be blockeddemonstrated that SD still occurred in calcium-free solution (Herreraset al., 1994). Our results further illustrate the dichotomy betweenthe calcium studies and the glutamate hypothesis and provide apartial although incomplete explanation. We found that spreadingdepression propagated normally in external solutions in whichsynaptic transmission would be blocked or at least greatly depressed.However, the propagation of SD under these conditions was stillinfluenced by the activation of NMDA receptors because the propagationrate of SD was reduced in the presence of either competitive ornoncompetitive NMDA receptor antagonists. Therefore, this studyindicates that swelling, which has long been known to be associatedwith SD (Van Harreveld and Khattab, 1967; Jing et al., 1994),is an important factor in its generation. Previously, glutamatewas thought to be the factor that caused swelling during SD. However,we suggest that swelling is a contributing factor in causing therelease ofglutamate.

We suggest the following addition to the mechanisms underlying spreading depression. Swelling, perhaps as a result of intenseneuronal activity (Nicholson and Sykova, 1998), opens VSOACs thatare permeable to glutamate. The efflux of glutamate activatesNMDA receptors on neurons, which increases extracellular K⁺ leading to further astrocyte swelling. The swelling attributableto K⁺ accumulation causes additional activation of VSOACs and furtherrelease of glutamate through this channel. The net result is positivefeedback with a central role for swelling-induced glutamaterelease.

Conclusion

Spreading depression may represent an extreme example of a normal process that occurs regularly on a less dramatic scale.In normal conditions, cellular swelling is known to occur in conjunctionwith neuronal activity (Nicholson and Sykova, 1998). Our resultssuggest that activity-induced cellular swelling may activate VSOACsand thereby cause glutamate release from these channels. A similarmechanism may contribute to ischemic-induced excitotoxicity becauseof the associated cellular swelling. Interestingly, NPPB has beenreported to decrease the efflux of glutamate from ischemic brainregions (Phillis et al., 1997). Therefore, the release of glutamatethrough volume-activated channels could have widespread implicationsin theCNS.

  FOOTNOTES

Received Dec. 7, 1998; revised April 28, 1999; accepted May 10, 1999.

This work was supported by the Medical Research Council of Canada (MRC). T.A.B. is a postdoctoral fellow of the Alberta HeritageFoundation for Medical Research (AHFMR). B.A.M. is an MRC SeniorScientist and an AHFMR Scientist. We thank Lorenzo Bauce for performingthe HPLC measurements and Drs. J. Armstrong and V. Parpura foruseful comments on earlier versions of thismanuscript.
Correspondence should be addressed to Dr. B. A. MacVicar, Department of Physiology and Biophysics, Neuroscience Research Group,University of Calgary, 3330 Hospital Drive N.W., Calgary, AlbertaT2N 4N1,Canada.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Andrew RD, MacVicar BA (1994) Imaging cell volume changes and neuronal excitation in the hippocampal slice. Neuroscience 62:371-383[ISI][Medline].
Basarsky TA, Duffy SN, Andrew RD, MacVicar BA (1998) Imaging spreading depression and associated intracellular calcium waves in brain slices. J Neurosci 18:7189-7199[Abstract/Free Full Text].
Crepel V, Panenka W, Kelly ME, MacVicar BA (1998) Mitogen-activated protein and tyrosine kinases in the activation of astrocyte volume-activated chloride current. J Neurosci 18:1196-1206[Abstract/Free Full Text].
Duan D, Winter C, Cowley S, Hume JR, Horowitz B (1997) Molecular identification of a volume-regulated chloride channel. Nature 390:417-421[Medline].
ffrench-Mullen JM, Rogawski MA (1989) Interaction of phencyclidine with voltage-dependent potassium channels in cultured rat hippocampal neurons: comparison with block of the NMDA receptor-ionophore complex. J Neurosci 9:4051-4061[Abstract].
Gill R, Andine P, Hillered L, Persson L, Hagberg H (1992) The effect of MK-801 on cortical spreading depression in the penumbral zone following focal ischaemia in the rat. J Cereb Blood Flow Metab 12:371-379[ISI][Medline].
Gonzalez E, Sanchez-Olea R, Pasantes-Morales H (1995) Inhibition by Cl channel blockers of the volume-activated, diffusional mechanism of inositol transport in primary astrocytes in culture. Neurochem Res 20:895-900[Medline].
Herreras O, Largo C, Ibarz JM, Somjen GG, Martin del Rio R (1994) Role of neuronal synchronizing mechanisms in the propagation of spreading depression in the in vivo hippocampus. J Neurosci 14:7087-7098[Abstract].
Holthoff K, Witte OW (1996) Intrinsic optical signals in rat neocortical slices measured with near-infrared dark-field microscopy reveal changes in extracellular space. J Neurosci 16:2740-2749[Abstract/Free Full Text].
Jackson PS, Strange K (1993) Volume-sensitive anion channels mediate swelling-activated inositol and taurine efflux. Am J Physiol 265:C1489-C1500[Abstract/Free Full Text].
Jing J, Aitken PG, Somjen GG (1993) Role of calcium channels in spreading depression in rat hippocampal slices. Brain Res 604:251-259[ISI][Medline].
Jing J, Aitken PG, Somjen GG (1994) Interstitial volume changes during spreading depression (SD) and SD-like hypoxic depolarization in hippocampal tissue slices. J Neurophysiol 71:2548-2551[Abstract/Free Full Text].
Kaai Y, Smith CP, Hediger MA (1993) The elusive transporters with a high affinity for glutamate. Trends Neurosci 16:365-370[ISI][Medline].
Kawasaki M, Uchida S, Monkawa T, Miyawaki A, Mikoshiba K, Marumo F, Sasaki S (1994) Cloning and expression of a protein kinase C-regulated chloride channel abundantly expressed in rat brain neuronal cells. Neuron 12:597-604[ISI][Medline].
Kraig RP, Nicholson C (1978) Extracellular ionic variations during spreading depression. Neuroscience 3:1045-1059[ISI][Medline].
Lascola CD, Kraig RP (1996) Whole-cell chloride currents in rat astrocytes accompany changes in cell morphology. J Neurosci 16:2532-2545[Abstract/Free Full Text].
Lascola CD, Nelson DJ, Kraig RP (1998) Cytoskeletal actin gates a Cl channel in neocortical astrocytes. J Neurosci 18:1679-1692[Abstract/Free Full Text].
Lauritzen M, Hansen AJ (1992) The effect of glutamate receptor blockade on anoxic depolarization and cortical spreading depression. J Cereb Blood Flow Metab 12:223-229[ISI][Medline].
Lauritzen M, Rice ME, Okada Y, Nicholson C (1988) Quisqualate, kainate and NMDA can initiate spreading depression in the turtle cerebellum. Brain Res 475:317-327[ISI][Medline].
Leao AAP (1944) Spreading depression of activity in the cerebral cortex. J Neurophysiol 7:359-390[Free Full Text].
MacVicar BA, Hochman D (1991) Imaging of synaptically evoked intrinsic optical signals in hippocampal slices. J Neurosci 11:1458-1469[Abstract].
Marrannes R, Willems R, De Prins E, Wauquier A (1988) Evidence for a role of the N-methyl-D-aspartate (NMDA) receptor in cortical spreading depression in the rat. Brain Res 457:226-240[ISI][Medline].
Martin H, Warner DS, Todd MM (1994) Effects of glycine receptor antagonism on spreading depression in the rat. Neurosci Lett 180:285-289[ISI][Medline].
McLachlan RS (1992) Suppression of spreading depression of Leao in neocortex by an N-methyl-D-aspartate receptor antagonist. Can J Neurol Sci 19:487-491[ISI][Medline].
Mody I, Lambert JD, Heinemann U (1987) Low extracellular magnesium induces epileptiform activity and spreading depression in rat hippocampal slices. J Neurophysiol 57:869-888[Abstract/Free Full Text].
Nellgard B, Wieloch T (1992) NMDA-receptor blockers but not NBQX, an AMPA-receptor antagonist, inhibit spreading depression in the rat brain. Acta Physiol Scand 146:497-503[ISI][Medline].
Nicholson C, Kraig RP (1981) The behaviour of extracellular ions during spreading depression. In: The application of ion-selective electrodes (Zeuthen T, ed), pp 217-238. Amsterdam: Elsevier.
Nicholson C, Sykova E (1998) Extracellular space analysis revealed by diffusion analysis. Trends Neurosci 21:207-215[ISI][Medline].
Obrenovitch TP, Zilkha E (1996) Inhibition of cortical spreading depression by L-701,324, a novel antagonist at the glycine site of the N-methyl-D-aspartate receptor complex. Br J Pharmacol 117:931-937[ISI][Medline].
Pasantes-Morales H, Schousboe A (1989) Release of taurine from astrocytes during potassium-evoked swelling. Glia 2:45-50[ISI][Medline].
Pasantes-Morales H, Moran J, Schousboe A (1990) Volume-sensitive release of taurine from cultured astrocytes: properties and mechanism. Glia 3:427-432[ISI][Medline].
Pasantes-Morales H, Murray RA, Lilja L, Moran J (1994a) Regulatory volume decrease in cultured astrocytes. I. Potassium- and chloride-activated permeability. Am J Physiol 266:C165-C171[Abstract/Free Full Text].
Pasantes-Morales H, Murray RA, Sanchez-Olea R, Moran J (1994b) Regulatory volume decrease in cultured astrocytes. II. Permeability pathway to amino acids and polyols. Am J Physiol 266:C172-C178[Abstract/Free Full Text].
Patel AJ, Lauritzen I, Lazdunski M, Honore E (1998) Disruption of mitochondrial respiration inhibits volume-regulated anion channels and provokes neuronal cell swelling. J Neurosci 18:3117-3123[Abstract/Free Full Text].
Phillis JW, Song D, O'Regan MH (1997) Inhibition by anion channel blockers of ischemia-evoked release of excitotoxic and other amino acids from rat cerebral cortex. Brain Res 758:9-16[ISI][Medline].
Roy G (1994) Channels for amino acids and metabolites activated by cell volume regulation. Jpn J Physiol [Suppl 44] 2:S37-S42.
Roy G (1995) Amino acid current through anion channels in cultured human glial cells. J Membr Biol 147:35-44[ISI][Medline].
Rutledge EM, Kimelberg HK (1996) Release of [3H]-D-aspartate from primary astrocyte cultures in response to raised external potassium. J Neurosci 16:7803-7811[Abstract/Free Full Text].
Rutledge EM, Aschner M, Kimelberg HK (1998) Pharmacological characterization of swelling-induced D-[3H]aspartate release from primary astrocyte cultures. Am J Physiol 274:C1511-C1520[Abstract/Free Full Text].
Saleh TM, Bauce LG, Pittman QJ (1997) Glutamate release in parabrachial nucleus and baroreflex alterations after vagal afferent activation. Am J Physiol 272:R1631-R1640[Abstract/Free Full Text].
Sanchez-Olea R, Pena C, Moran J, Pasantes-Morales H (1993) Inhibition of volume regulation and efflux of osmoregulatory amino acids by blockers of Cl transport in cultured astrocytes. Neurosci Lett 156:141-144[ISI][Medline].
Schweitzer JS, Patrylo PR, Dudek FE, Snow RW, Taylor CP (1992) Prolonged field bursts in the dentate gyrus: dependence on low calcium, high potassium, and nonsynaptic mechanisms. J Neurophysiol 68:2016-2025[Abstract/Free Full Text].
Somjen GG, Aitken PG, Czeh GL, Herreras O, Jing J, Young JN (1992) Mechanism of spreading depression: a review of recent findings and a hypothesis. Can J Physiol Pharmacol 70:S248-S254.
Strange K, Emma F, Jackson PS (1996) Cellular and molecular physiology of volume-sensitive anion channels. Am J Physiol 270:C711-C730[Abstract/Free Full Text].
Tatlisumak T, Takano K, Meiler MR, Fisher M (1998) A glycine site antagonist, ZD9379, reduces number of spreading depressions and infarct size in rats with permanent middle cerebral artery occlusion. Stroke 29:190-195[Abstract/Free Full Text].
Van Harreveld A (1978) Two mechanisms for spreading depression in the chicken retina. J Neurobiol 9:419-431[ISI][Medline].
Van Harreveld A, Khattab FI (1967) Changes in cortical extracellular space during spreading depression investigated with the electron microscope. J Neurophysiol 30:911-929[Free Full Text].
Willette RN, Lysko PG, Sauermelch CF (1994) A comparison of (+)SK&F 10047 and MK-801 on cortical spreading depression. Brain Res 648:347-351[ISI][Medline].

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