NMDA Receptor Antagonists Disinhibit Rat Posterior Cingulate and Retrosplenial Cortices: A Potential Mechanism of Neurotoxicity

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The Journal of Neuroscience, April 15, 2002, 22(8):3070-3080

NMDA Receptor Antagonists Disinhibit Rat Posterior Cingulate and Retrosplenial Cortices: A Potential Mechanism of Neurotoxicity
Qiang Li¹^,³, Suzanne Clark¹^,³, Darrell V. Lewis², and Wilkie A. Wilson¹^,³
Departments of ¹ Pharmacology and Cancer Biology and ² Pediatrics (Neurology), Duke University Medical Center, Durham, North Carolina 27710, and ³ Neurology Research, Veterans Administration Medical Center, Durham, North Carolina 27705

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

NMDA receptor antagonists produce region-specific neurodegeneration by an undetermined mechanism, but one proposed mechanisminvolves disinhibition. In certain areas of the brain, NMDA receptorsmediate excitatory drive onto inhibitory interneurons. Thus, NMDAreceptor/channel antagonists may reduce inhibition (i.e., produce"disinhibition"). If a sufficient level of disinhibition is produced,enhanced vulnerability to excitotoxicity may result. Furthermore,if there are region-specific differences in NMDA antagonist-induceddisinhibition, this could underlie region-specific NMDA antagonist-inducedneurotoxicity. In the present study, we tested this hypothesisby exposing rat brain slices to the NMDA receptor antagonist dizocilpinemaleate (MK-801) and measuring MK-801-induced disinhibition inareas of higher and lower vulnerability to neurodegeneration [posteriorcingulate/retrosplenial cortices (PCC/RSC) and parietal cortex,respectively]. Using whole-cell patch-clamp techniques, bicuculline-sensitiveGABA_A receptor-mediated IPSCs were measured in biocytin-labeledpyramidal neurons in the PCC/RSC and parietal cortex. In the PCC/RSC,bath-applied MK-801 (10-40 µM) produced disinhibition, shown asa concentration-dependent decrease in spontaneous IPSC frequencyand amplitude; MK-801 (40 µM) also reduced evoked IPSC amplitudes.In parietal cortex, MK-801 produced significantly less disinhibition.To determine whether disinhibition is caused by presynaptic orpostsynaptic mechanisms, we tested the effects of MK-801 (40 µM)against miniature IPSC (mIPSC) frequency and amplitude in tetrodotoxin(TTX; 0.5 µM)-treated slices and found that MK-801 did not altermIPSC frequency or amplitude. Taken together, these results suggestthat NMDA receptors regulate activity of inhibitory interneuronsand, consequently, GABA release in certain cortical areas. Thisregion-specific reduction in inhibitory input to pyramidal cellscould underlie the region-specific neurotoxicity of NMDAantagonists.

Key words: MK-801; NMDA receptor; IPSCs; disinhibition; pyramidal cells; interneurons; cingulate cortex

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurodegeneration can result from overactivation of NMDA receptors (Rothman and Olney 1986, 1987), causing excitotoxicityproposed to be responsible for certain neurological diseases.Consequently, NMDA antagonists were screened against animal modelsof epilepsy (Avoli and Oliver, 1987), ischemia (Aitken et al.,1988; Ford et al., 1989; Rod and Auer, 1989), and hypoglycemia(Wieloch, 1985).

The results from these studies were perplexing, however. NMDA antagonists were not always effective (Stasheff et al., 1989;Sveinbjornsdottir et al., 1993) nor were they always neuroprotective(MacDonald et al., 1990). In fact, some antagonists actually producedregion-specific neurotoxicity (Olney et al., 1989, 1991). In rats,the most affected areas were posterior cingulate cortex (PCC)and retrosplenial cortex (RSC); other areas were less sensitive(Allen and Iversen, 1990; Olney et al., 1991; Horvath et al.,1997). Pathomorphological changes varied with dose: low dosescaused mitochondrial dilation, higher doses caused neuronal death(Olney et al., 1989, 1991; Fix et al., 1995; Horvath et al., 1997).

How do NMDA antagonists produce neurotoxicity? Olney and colleagues (Olney et al., 1991; Olney and Farber, 1995; Corso etal., 1997) proposed that NMDA antagonists produce neurodegenerationby disrupting inhibition. This disinhibition could be produceddirectly (by disrupting the local excitatory/inhibitory network)or indirectly (by acting through modulatory neurotransmitter systems).Results from in vivo studies have supported Olney's hypothesis;however, no studies have directly tested this hypothesis in vitroin the PCC/RSC.

Using brain slices, we tested these hypotheses. We proposed that NMDA antagonists (1) reduce GABAergic inhibition in the PCC/RSCand (2) are more effective in the PCC/RSC than in less vulnerableregions, such as parietalcortex.

The first proposal is based on reports that NMDA receptors provide excitatory drive onto inhibitory interneurons in severalbrain areas, including the hippocampus (Grunze et al., 1996) andolfactory cortex (Schoppa et al., 1998). Thus, NMDA antagonistsproduce disinhibition in these areas. We extend these findingsto the PCC/RSC. The second proposal is important regarding NMDAantagonist-induced neurodegeneration, because if NMDA antagonistsproduce more disinhibition in PCC/RSC than elsewhere, this mayunderlie their region-specific neurotoxicity. Finally, the useof brain slices may help to determine the level at which NMDAantagonists disrupt inhibition (i.e., in the local excitatory/inhibitorycircuits, versus at the level of extrinsic modulatoryinputs).

To test these proposals, we used the NMDA antagonist dizocilpine maleate (MK-801) to produce disinhibition in slices of PCC/RSCand parietal cortex. Disinhibition was assessed using whole-cellpatch-clamp recordings in pyramidal cells to measure GABA_A-mediatedIPSC frequencies and amplitudes. Here we provide the first directelectrophysiological evidence that NMDA antagonists reduced inhibitorysynaptic drive onto pyramidal cells in the PCC/RSC. Also, themechanism for region-specific vulnerabilities may be explainedby our results, because MK-801 produces more disinhibition incortical areas most vulnerable to NMDA antagonist-inducedneurotoxicity.

Preliminary results have been published previously in abstract form (Li et al., 2000).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cortical slices. Cortical slices were prepared from young, male Sprague Dawley rats (postnatal day 15-25). Rats were isoflurane-anesthetizedand decapitated. The brains were quickly removed from the skullsand placed in cold (4°C) artificial CSF (aCSF) containing (inmM): 120 NaCl, 3.3 KCl, 1.23 NaH₂PO₄, 25 NaHCO₃, 1.2 MgSO₄, 1.8CaCl₂, and 10 D-glucose at pH 7.3, previously saturated with 95%O₂/5%CO₂.Coronal cortical slices (300 µm thickness) containing the PCC/RSCor the parietal cortex (Paxinos and Watson, 1986) were cut witha Vibratome (Model 752; Campden, Berlin, Germany) and incubatedin a holding chamber continuously bubbled with 95% O₂ and 5% CO₂at room temperature (22-24°C).

Whole-cell voltage-clamp recording. Our whole-cell patch-clamp techniques have been described in our previous publication(Mott et al., 1999). For recording, patch pipettes were pulledfrom borosilicate glass capillary tubing (1.5 mm outer diameter,1.05 mm inner diameter; World Precision Instruments, Sarasota,FL) on a Flaming-Brown horizontal microelectrode puller (ModelP-97; Sutter Instrument Co., Novato, CA). Pipettes were filledwith an intracellular solution containing (in mM): 130 Cs-gluconate,7 CsCl, 10 HEPES, 4 Mg-ATP, pH = 7.25. The quaternary lidocainederivative QX-314 (4 mM) (Sigma, St. Louis, MO) was also includedto suppress fast sodium currents. Osmolarity was adjusted to 280mOsm. Pipette resistances generally were in the range of 4-7M $Omega$ .Biocytin (0.3-0.4%) (Sigma) was also added to the intracellularsolution for later visualization of the morphology of the recordedcells.

After >1 hr of incubation in the holding chamber, a slice was transferred to a small submersion chamber maintained at roomtemperature (22-24°C) and secured in place with a bent piece ofplatinum wire resting on the top of the slice. Individual cellswere visualized using an infrared differential interference contrastZeiss Axioskop microscope and a 40× water immersion objective.Tight seals (>1 G $Omega$ ) were obtained on pyramidal-shaped cells, andwhole-cell recordings were made after rupturing the cell membranewith gentle suction. After establishment of the whole-cell recordingconfiguration, stable long-lasting tight-seal recordings wereachieved in most cases. Spontaneous and evoked IPSCs (eIPSCs)were recorded continuously using an Axopatch 1-D amplifier (AxonInstruments, Foster City, CA). Output current signals were DC-coupledto a digital oscilloscope (Nicolet Model 410). Series resistancewas monitored throughout the recordings; a cell was discardedif it changed significantly (>20% of the control). In addition,a PCM/VCR recorder (Model 400; A. R. Vetter Co, Rebersburg, PA)was used to capture all tracings of synaptic events for off-lineanalysis and archiving. The stored signal was further analyzedusing Strathclyde Electrophysiology Software Whole Cell Program(courtesy of Dr. John Dempster, University of Strathclyde, Glasgow,UK) with an interface (BNC-2090; National Instruments, Austin,TX) to a PC-basedcomputer.

Cortical interneurons were selected on the basis of the shape of the soma (small and round under DIC microscopy) and theircharacteristic firing pattern. To determine the firing patternof a cortical interneuron while achieving the tight seal offeredby Cs-gluconate solution under the voltage clamp, the tip of apatch pipette was filled with a solution containing K-gluconate(in mM: 130 K-gluconate, 7 KCl, 10 HEPES, 4 Mg-ATP, and 0.3 Tris-GTP,pH 7.25), then backfilled with a solution containing Cs-gluconate(see above). The dialysis of the recorded cell with the Cs-gluconatesolution could be observed from the distortions of shapes of theaction potentials ~10 min after whole configuration was established.NMDA receptor-mediated EPSCs were then recorded frominterneurons.

Electrical stimulation. A monopolar tungsten electrode (A-M System, Carlsborg, WA) was placed ~50-70 µm lateral to the somaof the recorded pyramidal cells in the same layer. The stimulusthreshold was first determined by increasing the intensity ofthe rectangular wave pulse until detectable responses occurred.Then constant current rectangular stimulus pulses 50% higher thanthreshold intensity with a duration of 0.1 msec and interval of0.0166 Hz were delivered through the electrode by an isolatedstimulator (Grass S88; Grass Instruments, Quincy,MA).

Histological identification of pyramidal cells. During recording, pyramidal cells were filled with biocytin. After the endof the recording, the slice was allowed to stay in the recordingchamber for an additional 10-20 min for further biocytin transportwithin the axon. The slices were then placed overnight in 4% paraformaldehydeand 0.05% glutaraldehyde in 0.1 M PBS. The slices were washedthoroughly in PBS and incubated in 0.1 M Tris-buffered saline(TBS) containing 1% H₂O₂ for 30 min. The slices were then incubatedovernight at 4°C with avidin-biotin-peroxidase complex (ABC kit;Vector Labs, Burlingame, CA) in TBS containing 0.05% Triton X-100.The slices were then rinsed three times in PBS, reacted in a solutioncontaining 3,3'-diaminobenzidine (DAB kit, Vector Labs), thencleared and mounted. The morphology of the biocytin-filled pyramidalcells was examined with a light microscope, and cells were drawnusing a cameralucida.

Statistical analysis of data and drug application. Data were analyzed off-line using Strathclyde Electrophysiological Software.The Kolmogorov-Smirnov (K-S) statistical test was used to comparetwo different cumulative distributions using Origin 5.0 for Windows(MicroCal Software, Norththampton, MA). Paired and unpaired ttests and one-way ANOVA tests were also used, when appropriate.All group data are presented as mean ±SEM.

MK-801 and TTX were purchased from RBI (Natick, MA). D-(-)2-amino-5-phosphonovaleric acid (D-AP5) and bicuculline methiodine(BMI) were purchased from Sigma. All drugs were dissolved directlyin the aCSF and bath-applied in the perfusion medium for ~20 min,unless notedotherwise.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Pyramidal cells were recorded in layers II-VI of the neocortex. We investigated these cortical strata in the PCC/RSC and theparietal cortex. The location of the PCC/RSC and the parietalcortex are illustrated in Figure 1A. Data were acquired from 54pyramidal cells, 6 interneurons in the PCC/RSC, and 49 pyramidalcells from the parietal cortex. According to the location of theirsomata, pyramidal cells are divided into three subgroups: thesuperficial layer (II-III), layer IV, and the deep layer (V-VI).In the PCC/RSC, 25 (46%) pyramidal cells are in the superficiallayer, 13 (24%) in layer IV, and 16 (30%) in the deep layer. Inparietal cortex, 20 (40%) pyramidal cells are in the superficiallayer, 14 (29%) in layer IV, and 15 (31%) in the deep layer. Allsix interneurons are recorded from PCC/RSC layers II and III.Because of the irreversible blockade of NMDA receptors by MK-801,only a single experiment was done from each cortical slice treatedwith MK-801.

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Figure 1. Camera lucida reconstruction of a PCC/RSC pyramidal cell filled with biocytin. A, Coronal section of a cortical slice containing PCC/RSC and parietal cortex. B, Camera lucida reconstruction of a biocytin-filled, layer V pyramidal cell recorded in the PCC/RSC. This pyramidal cell was filled with biocytin during the experiment. An apical dendrite arising from the soma extends toward the pial surface and branches off to form multiple tufts. In addition to a typical apical dendrite tree, a long axon originating from the soma projects to the contralateral side of the hemisphere through the corpus callosum. Another branch of the axon projects ipsilaterally to the lateral cortex. The pia is near the end of the apical dendrite branches. Dashed lines represent the approximate pial surface of the cortex. RSC, Retrosplenial cortices; Par, parietal cortex; CC, corpus callosum; I-VI, cortical lamina; DG, dentate gyrus; 3V, third ventricle; CA, cornus ammonis. Arrows denote axon. Scale bar, 200 µm.

Morphology of dendritic and axonal arbors of pyramidal cells in the PCC/RSC

The morphology of each recorded cell was assessed with biocytin staining to unambiguously distinguish pyramidal cells fromother cell types. We were able to recover histologically ~90%of all recorded cells in the PCC/RSC areas. The dendritic arborof pyramidal cells in the PCC/RSC was characterized by a longapical dendrite that usually extended toward the pial surface,where typically it branched extensively to form multiple smallterminal tufts just under the pial surface. Along the length ofthe apical dendrites are numerous obliquely branched dendriticcollaterals. Basal dendrites extended outward from the lower portionof the soma; these basal dendrites ascended or descended withgradual tapering. The pyramidal cell axonal arbor was denselydistributed around the soma and also extended widely, both horizontallyand vertically. These morphological characteristics are consistentwith cortical pyramidal cells described elsewhere (Kim and Connors,1993; Lubke et al., 1996; Reyes and Sakmann, 1999; Feldmeyer andSakmann, 2000). Figure 1B shows a camera lucida reconstructionof a PCC/RSC pyramidal cell. The soma of this pyramidal cell islocated in layer V, and it sends a long axon projecting to thecontralateral side across the corpus callosum (Sripanidkulchaiand Wyss, 1987).

MK-801 decreases the spontaneous IPSC frequency in pyramidal cells of the PCC/RSC

Spontaneous IPSCs (sIPSCs) were recorded from pyramidal cells in the PCC/RSC using whole-cell voltage-clamp techniques. Theholding potentials were +10 or +30 mV, and the calculated E_CLwas approximately $-$ 40 mV for the internal solution used. Underthese experimental conditions, the sIPSCs were inward currentsat a holding potential of $-$ 70 mV (Fig. 2A) and were robust outwardcurrents at a holding potential of +30 mV (Fig. 2B). At the endof the experiment, the recorded sIPSCs were abolished by bathapplication of a selective GABA_A receptor antagonist, BMI (20µM) (Fig. 2C). NMDA receptor-mediated EPSCs might be present whena cell was depolarized to +40 mV (Hestrin, 1992). Accordingly,we also assessed whether NMDA receptor-mediated EPSCs were alsopresent when a cell was held at +30 mV without blocking excitatorytransmissions. We examined eight PCC/RSC pyramidal cells in thepresence of BMI (20 µM). When the holding potential was held at $-$ 70 mV, fast inward currents mediated by AMPA receptors dominated,and no NMDA receptor-mediated EPSCs were observed (Fig. 2D). NMDAreceptor-mediated EPSCs only become detectable after the holdingpotential was changed to +30 mV (data not shown). However, longslow outward currents were recorded in only four of the nine cellstested, and the frequency of recorded NMDA-EPSCs is very low.These data indicated that the contribution of NMDA receptor-mediatedEPSCs was insignificant and negligible in cells held at +30 mV.Figure 2, E and F, shows evoked IPSCs recorded in a PCC/RSC pyramidalcell in the presence of DNQX (20 µM) and D-AP5 (50 µM). A plotof the amplitude of evoked IPSCs against holding potentials (Fig.2E) indicated an x-intercept of $-$ 39 mV, closely approximatingthe calculated reversal potential of E_CL (Fig. 2F). These resultsindicated that the recorded IPSCs were mediated by the activationof GABA_A receptors.

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Figure 2. GABA_A receptor-mediated IPSCs recorded in PCC/RSC pyramidal cells. Whole-cell recordings were performed using a CsCl-based internal solution at holding potentials of $-$ 70 mV and +30 mV. When the holding potential was $-$ 70 mV (A), inward currents were recorded. When the cell was held at +30 mV, the currents became outward (B). The GABA_A receptor antagonist BMI (20 µM) abolishes the currents (C). In the presence of BMI (20 µM) and at the holding potential of $-$ 70 mV, fast inward currents are recorded from another pyramidal cell and can be blocked by DNQX (20 µM) (D). In the presence of D-AP5 (50 µM) and DNQX (20 µM), amplitudes of evoked IPSCs recorded from another pyramidal cell held at potentials ranged from $-$ 70 to +20 mV (E). An I-V curve was constructed (F) based on the evoked synaptic responses shown in E. The apparent reversal potential was approximately $-$ 39 mV. These findings indicate that the recorded IPSCs were mediated by GABA_A receptors. Calibration: A-C, 500 msec, 0.1 nA; D, 100 msec, 50 pA.

Effects of MK-801 on sIPSCs in PCC/RSC pyramidal cells are demonstrated in Figures 3 and 4. MK-801 suppressed two IPSC properties:amplitude and frequency (the latter reflected as an increase inthe interval between sIPSCs). Figure 3 shows recordings from alayer V pyramidal cell. At a holding potential of +30 mV, therecorded IPSCs were outward currents (Fig. 3A, top panel). Bathapplication of the NMDA antagonist MK-801 (40 µM) caused a significantdecrease in the frequency and amplitude of sIPSCs in this pyramidalcell (Fig. 3A, second panel from top). The IPSCs were abolishedby bath-applied BMI (20 µM) and recovered partially on washout(Fig. 3A, bottom two panels). The cumulative probability distributionsfor these changes are shown in Figure 3B. As shown, bath-appliedMK-801 produced a rightward shift in the distribution of sIPSCintervals (Fig. 3B, left panel), indicating a decrease in sIPSCfrequency (K-S test; p < 0.01). In addition, sIPSC amplitudeswere also reduced significantly (K-S test; p < 0.001), as shownin Figure 3B (right panel). The morphology of this pyramidal cellis shown in Figure 3C.

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Figure 3. MK-801 decreases GABA_A receptor-mediated sIPSCs. A, In a layer V PCC/RSC pyramidal cell held at +30 mV, bath-applied MK-801 (40 µM) decreased the frequency and amplitude of sIPSCs. When BMI (20 µM) was added, sIPSCs were blocked reversibly. Calibration: 500 msec, 0.1 nA. B, In the same cell, the cumulative inter-event interval distribution shows a significant increase in the inter-event interval caused by MK-801 (p < 0.01; K-S test). The cumulative amplitude distribution also shows a significant decrease in amplitude (p < 0.001; K-S test). C, Photomicrograph of the same cell filled with biocytin. I-VI, Cortical lamina. Arrow denotes axon. Scale bar, 100 µm.

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Figure 4. Effect of MK-801 on sIPSCs from a layer III cell. In a layer III PCC/RSC pyramidal cell held at +30 mV, bath-applied MK-801 (40 µM) (B) decreased sIPSCs compared with control (A), an effect similar to that seen in layer V (Fig. 3). Recorded sIPSCs were abolished by BMI (20 µM) (C). Calibration: 500 msec, 0.1 nA. D, Camera lucida reconstruction of the same cell. As shown, this is also a pyramidal cell, with processes slightly different from the cell shown in Figure 3, although the pharmacological responses to MK-801 were similar. I-VI, Cortical lamina. Arrows denote axon. Scale bar, 100 µm.

This effect was not limited to layer V pyramidal cells. A similar effect was also seen in a layer III pyramidal cell of thePCC/RSC, as shown in Figure 4. This pyramidal cell responded tobath-applied MK-801 (40 µM) with a significant decrease in sIPSCfrequency (Figs. 4A, 5B). In addition, amplitudes of sIPSCs werealso attenuated by MK-801. Although large-amplitude sIPSCs apparentlydominated in this layer III pyramidal cell, the morphology ofthis pyramidal cell, as shown in Figure 4D, is similar to thatof the pyramidal cell illustrated in Figure 4C. We found similarMK-801-mediated effects in layers II-VI as well.

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Figure 5. Effect of MK-801 on eIPSCs. A, In a layer IV PCC/RSC pyramidal cell held at +5mV, outward eIPSCs were recorded. These eIPSCs were completely and reversibly blocked by BMI (20 µM), as was seen with sIPSCs (Fig. 2A-C), indicating that eIPSCs were mediated by GABA_A receptors. Calibration: 50 msec, 0.1 nA. B, In a layer V PCC/RSC pyramidal cell held at +5mV, the eIPSC time course after bath-applied MK-801 (40 µM), BMI (20 µM), and washout is shown. Insets illustrate the averaged peak IPSC traces corresponding to each treatment. C, Photomicrograph of the pyramidal cell shown in B filled with biocytin. I-VI, Cortical lamina. Arrow denotes axon. Scale bar, 100 µm.

Inhibitory effects of MK-801 on sIPSCs of pyramidal cells were compared among the three groups. Bath-applied MK-801 (40 µM)reduced sIPSC frequency by 43.3 ± 3.8% (n = 16) compared withthe control in the superficial group (layers II and III), 44.4± 4.6% (n = 11) in layer IV, and 44 ± 3.0% (n = 13) in the deeplayer (layers V and VI). There are no significant differencesin mean IPSC frequency among three groups (p > 0.05; one-way ANOVA),so we pooled data obtained from pyramidal cells recorded in PCC/RSClayers II-VI. Overall, bath application of MK-801 (40 µM) reducedthe frequency of sIPSCs by 43.8 ± 2.2% (n = 40) relative to control(p < 0.05; paired ttest).

We also examined the concentration dependence of MK-801-induced decreases in the frequency of sIPSCs using three concentrationsof MK-801 bath-applied in sequence. We monitored sIPSCs for ~20min after each concentration was applied. Overall, reductionsof mean inter-event intervals were 15.4 ± 1.4, 28.6 ± 2.3, and44.3 ± 3.1% after bath application of MK-801 at the doses of 10,20, and 40 µM, respectively (p < 0.05; one-way ANOVA; n =4).

We also tested the effect of the widely used competitive NMDA receptor antagonist D-AP5. Similar to MK-801, D-AP5 (50 µM)significantly (K-S test; p < 0.05) decreased the frequency ofsIPSCs in two PCC/RSC pyramidal cells tested (data notshown).

MK-801 reduced the amplitude of evoked IPSCs in pyramidal cells in the PCC/RSC

In these experiments, MK-801 was also tested against evoked IPSCs of PCC/RSC pyramidal cells. The pyramidal cells were heldat $-$ 5 or +5mV, and an eIPSC was elicited by a single pulse deliveredlateral to the recording electrode (see Materials and Methods).These eIPSCs were abolished by bath application of GABA_A receptorantagonist BMI (20 µM), indicating that eIPSCs are mediated byGABA_A receptors (Fig. 5A).

The time course of the MK-801-induced effect on eIPSC of a layer V PCC/RSC is shown in Figure 5B. As shown, the evoked IPSCswere gradually, but significantly, reduced by bath-applied MK-801.At a holding potential of +5mV, recordings were made in controlsolution for 10 min, then MK-801 (40 µM) was bath-applied. Fiveminutes after addition of MK-801, the eIPSCs began to decline.By 30 min after treatment, eIPSCs were reduced from 1.0 to 0.5nA (i.e., 50% of control). Again, the eIPSCs were blocked by bath-appliedBMI (20 µM) and recovered during BMI washout. Overall, MK-801(40 µM) significantly reduced evoked responses to 51.3 ± 2.3%of control (n = 13; p < 0.05; paired ttest).

Comparison of effects of MK-801 on sIPSCs and eIPSCs in the PCC/RSC and the parietal cortex

Several in vivo animal studies have demonstrated that pathomorphological changes induced by NMDA antagonists occur in a numberof different areas of the brain, but with different sensitivitiesamong the affected areas (Olney et al., 1991; Fix et al., 1993;Horvath et al., 1997). For example, MK-801 causes more severedamage to neurons in the PCC/RSC, whereas some other corticalareas were lessaffected.

We hypothesize that one mechanism by which MK-801 produces region-specific neurodegeneration is that MK-801 more effectivelyproduces disinhibition in a vulnerable area (e.g., PCC/RSC) thana less vulnerable area (e.g., parietal cortex). To address this,we recorded sIPSCs and eIPSCs from 49 pyramidal cells in the parietalcortex.

Figure 6 shows the effect of MK-801 on sIPSCs recorded in a layer V parietal pyramidal cell. The sIPSCs were only slightlyreduced by MK-801 (40 µM) (Fig. 6A). Although MK-801 significantlyincreased the inter-event intervals (K-S test; p < 0.05) (Fig.6B, left panel), MK-801 did not have a significant effect on thecumulative amplitude distribution (K-S test; p > 0.05) (Fig. 6B,right panel).

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Figure 6. MK-801 is less effective on sIPSCs of pyramidal cells in the parietal cortex. A, At the holding potential of +30 mV, bath-applied MK-801 (40 µM) decreased sIPSCs in a layer V pyramidal cell in the parietal cortex. When BMI (20 µM) was added, sIPSCs were abolished, then recovered after washout. Calibration: 500 msec, 0.1 nA. B, In the same cell, the cumulative inter-event interval distribution shows a slight but significant increase in the inter-event interval (p < 0.05; K-S test). In contrast, MK-801 did not significantly decrease the sIPSC amplitude in the parietal cortex, as shown by the cumulative amplitude distribution (p > 0.05; K-S test). C, Photomicrograph of the same cell filled with biocytin. I-VI, Cortical lamina. Arrow denotes axon. Scale bar, 100 µm. (In the main dendrite, the small apparent gaps are artifacts: they arose after coverslipping. During the experiment, the dendrite was intact, as in all other experiments.)

Depressive effects of MK-801 on pyramidal cell sIPSCs were also compared among the three groups. Bath-applied MK-801 (40 µM)reduced frequency of sIPSCs by 21.9 ± 4.8% (n = 14) compared withcontrol in the superficial group (layers II and III), 23.9 ± 5.4%(n = 12) in layer IV, and 23.4 ± 3.5% (n = 13) in the deep layers(layers V and VI). No significant differences in mean IPSC frequencyamong three groups were observed (p > 0.05; one-way ANOVA). Accordingly,we also pooled data obtained from pyramidal cells recorded inlayers II-VI of parietal cortex. Bath application of MK-801 (40µM) reduced the frequency of sIPSCs by 22.9 ± 2.6% (n = 39) relativeto control (p < 0.05; paired t test). In contrast, in the PCC/RSC,mean sIPSC frequency was reduced by 43.8 ± 2.2% (n = 40). In addition,we found that in ~19% pyramidal cells recorded in parietal cortex,mean sIPSC frequency was reduced by MK-801 (40 µM) <10% (rangingfrom 2 to 10%), compared with 5% of those in the PCC/RSC.

Overall inhibitory effect of MK-801 on sIPSC frequency of each group recorded from two brain regions is summarized in Figure7. There is a significantly greater depression of sIPSC frequencyby MK-801 in the PCC/RSC versus the parietal cortex (unpairedt test; p < 0.05) (Fig. 7A). The amplitudes of IPSCs are alsosuppressed by MK-801 in the PCC/RSC. Taken together, these resultsindicate that, at a dose of 40 µM, MK-801 caused greater disinhibitionof pyramidal cells in the RSC than in the parietal cortex.

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Figure 7. Comparison of MK-801 on sIPSCs and eIPSCs of pyramidal cells in the PCC/RSC and the parietal cortex. A, Graph shows data indicating the reduction in sIPSC frequency in PCC/RSC pyramidal cells [superficial layers (n = 16), layer IV (n = 11), and the deep layers (n = 13)] and in the parietal cortex [superficial layer (n = 14), layer IV (n = 12), and the deep layers (n = 13)]. MK-801 (40 µM) significantly decreased the average sIPSC frequency of pyramidal cells in the PCC/RSC compared with those in the parietal cortex (*p < 0.05; unpaired t test). B, Graph shows that MK-801 (40 µM) significantly inhibited the average peak amplitude of eIPSCs in pyramidal cells (n = 10) in the PCC/RSC compared with the parietal cortex (n = 9) (*p < 0.05; unpaired t test).

Similar differences were also observed on eIPSCs of pyramidal cells in the parietal cortex as shown in Figure 7B. The meanamplitude of eIPSCs of pyramidal cells recorded from the PCC/RSCwas decreased by 52 ± 1.8% (n = 10) of control. However, the averageeIPSCs amplitude of pyramidal cells recorded from the parietalcortex was decreased by only 27 ± 2.1% (n = 9) of control afterbath application of 40 µM MK-801. There is a significant differencebetween two groups (p < 0.05; unpaired ttest).

MK-801 inhibits NMDA receptor-mediated EPSCs in PCC/RSC interneurons

It has been demonstrated that excitability of interneurons in the entorhinal cortex (Jones and Buhl, 1993) and auditory cortex(Bandrowski et al., 2001), the olfactory bulb (Schoppa et al.,1998) of rats can be modulated via excitatory synaptic input mediatedby NMDA receptors. To assess whether MK-801 has a direct effecton NMDA receptor-mediated EPSCs in GABAergic interneurons, weisolated NMDA receptor-mediated EPSCs from six PCC/RSC layer II-IIIinterneurons. Figure 8B shows a typical firing pattern of a PCC/RSClayer III interneuron (Kawaguchi, 1995; Zhou and Hablitz, 1998)compared with that of a PCC/RSC layer IV pyramidal cell (Fig.8A). When the interneuron was held at $-$ 70 mV, DNQX-sensitive orAMPA/kainate receptor-mediated fast EPSCs were dominant (Fig.8C). When the holding potential was changed to +50 mV, there werefew, very long slow outward currents (Fig. 8D). These could beblocked by D-APV (n = 2; data not shown), suggesting they areNMDA receptor mediated.

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Figure 8. MK-801 blocks NMDA receptor-mediated EPSCs in PCC/RSC interneurons. A, Current-clamp recording of a PCC/RSC layer IV pyramidal cell in response to depolarizing current injection. The firing pattern of this pyramidal cell shows slow action potentials and frequency adaptation, characteristics typical for pyramidal cells. B, Current-clamp recording of a PCC/RSC layer III interneuron in response to depolarizing current injection. This interneuron fires rapidly and lacks frequency adaptation, characteristics typical for interneurons. Calibration: A, B, 200 msec, 20 mV, 80 pA. C, At the holding potential of $-$ 70 mV and in the presence of BMI (20 µM), DNQX-sensitive fast inward EPSCs are dominant in the interneuron. Calibration: 500 msec, 50 pA. D, When this interneuron was voltage-clamped at +50 mV and in the presence of BMI (20 µM), the long slow EPSCs were dominant. Calibration: 1000 msec, 100 pA. E, The slow EPSCs were blocked after administration of MK-801 (40 µM). Calibration: 1000 msec, 50 pA.

Twenty minutes after bath-applied MK-801 (40 µM), these NMDA receptor-mediated EPSCs were abolished (Fig. 8E). MK-801 completelyblocked NMDA receptor-mediated EPSCs in all six PCC/RSC interneuronstested. These results suggested that PCC/RSC interneurons receiveNMDA receptor-mediated input; the absence of excitatory afferentdrive onto the PCC/RSC interneurons could result in a decreaseof inhibitory transmission from interneurons onto pyramidalcells.

MK-801 did not inhibit mIPSCs of pyramidal cells in the PCC/RSC

The results described above demonstrated that a block of NMDA receptors by the NMDA antagonist MK-801 reduced GABA_A receptor-mediatedIPSCs in PCC/RSC pyramidal cells. To determine whether the decreaseof sIPSCs and eIPSCs in pyramidal cells was caused by a reductionof action potential-dependent or action potential-independentmechanisms, we used TTX, a Na⁺ channel blocker, to block synaptic events that are dependenton action potentials. Under such conditions, synaptic responsesobtained in the presence of TTX are caused by quantal releaseand referred to as miniature IPSCS(mIPSCs).

We investigated the effect of MK-801 on mIPSCs in pyramidal cells in the PCC/RSC and found that MK-801 did not affect mIPSCfrequency or amplitude. Figure 9A shows recordings of sIPSCs froma PCC/RSC pyramidal cell in layer III before and after applicationof TTX (0.5 µM). TTX caused a decrease in the mean sIPSC amplitude,indicating that a significant portion of the sIPSCs was causedby action potential-dependent GABA release from inhibitory interneurons.In the presence of TTX and at a holding potential of +30 mV, theaverage mIPSC frequency in the pyramidal cells was 4.5 ± 0.26/secand the mean amplitude was 35 ± 6.2 pA (n = 5). After pretreatmentof the slice with TTX for >30 min, bath application of MK-801(40 µM) had no effect on the frequency (4.2 ± 0.23/sec) or amplitude(33 ± 5.8 pA) of mIPSCs (Fig. 9A). In contrast to the effectsof MK-801 on spontaneous IPSCs, there were no significant changesin the cumulative probability distribution of either mIPSC frequency(Fig. 9B, left panel) or amplitude (Fig. 9B, right panel) afterbath application of MK-801 (K-S; p > 0.05). These results indicatedthat MK-801 exerts its inhibitory effect on IPSCs of pyramidalcells through an action potential-dependent mechanism.

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Figure 9. MK-801 does not suppress mIPSCs. A, In a PCC/RSC layer III pyramidal cell held at +30 mV, bath-applied TTX (0.5 µM) abolished all action potential-dependent IPSCs, leaving only mIPSCs. Bath-applied MK-801 (40 µM) had no effect on mIPSCs, whereas BMI (20 µM) reversibly blocked mIPSCs. Calibration: 500 msec, 0.05 nA. B, Cumulative mIPSC inter-event and amplitude distributions were not significantly changed (K-S test; p > 0.05), indicating that MK-801 produces disinhibition through an action potential-dependent mechanism. C, Camera lucida reconstruction of the same cell filled with biocytin. I-VI, Cortical lamina. Arrows denote axon. Scale bar, 100 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Using whole-cell patch-clamp techniques combined with morphological identification of neurons in rat brain slices, we haveinvestigated the effect of the noncompetitive NMDA receptor antagonistMK-801 on sIPSCs and eIPSCs in pyramidal cells of PCC/RSC andparietal cortex. Our results demonstrate that in PCC/RSC pyramidalcells, GABA_A receptor-mediated synaptic transmission is reducedby NMDA receptor antagonists. These observations suggest thatNMDA receptor-mediated excitation of interneurons facilitatesGABAergic inhibition of PCC/RSC pyramidalcells.

The modulation of GABAergic inhibition by MK-801 in two regions with different vulnerabilities to NMDA antagonist-induced neurotoxicity

MK-801 has neuroprotective effects in certain CNS disorders (Foster et al., 1988; Dirnagl et al., 1990). However, MK-801 alsohas negative effects in vivo, including altered behavior (Sams-Dodd,1997) and temperature regulation (Colbourne et al., 1999). Severalin vivo studies reported that chronic injection of low-dose MK-801[or other NMDA receptor antagonists, e.g., phencyclidine (PCP)]causes neuronal vacuolization in the PCC/RSC (Olney et al., 1989;Fix et al., 1993; Corso et al., 1997). This vacuolization canbe reversible at low doses; however, irreversible neuronal damageoccurs after high doses or repeated low doses (Fix et al., 1993).

Given these results, a fundamental question arose: how could an agent that had been expected to be neuroprotective turn outto be neurotoxic? On the basis of their whole animal studies,Olney and others proposed that these drugs might impair neuronalinhibition, leading to hyperactivity and neuronal death (Olneyet al., 1991; Corso et al., 1997; Horvath et al., 1997). However,neurotoxic mechanisms underlying this phenomenon may be complexand could include those mediated by direct disruption of GABAergicfunction (Olney et al., 1991) or through a more indirect mechanismvia modulatory neurotransmitters acting in vulnerable regions[such as cholinergic (Olney et al., 1991;), serotoninergic (Loscherand Honack, 1991), adrenergic (Loscher and Honack, 1991; Farberet al., 1995a), and dopaminergic (Sharp et al., 1994; Farber etal., 1996). Either way, a significant loss of inhibition couldresult in hyperexcitability, and this could lead to excitotoxicity.Consistent with these proposals are studies in which MK-801 increasedglucose utilization in regions vulnerable to neurotoxicity, includingthe cingulate and entorhinal cortices (Kurumaji and McCulloch,1990; Nehls et al., 1990; Patel and McCulloch, 1995). These resultssuggest that the vulnerable areas were highly activated by MK-801.The use of brain slices allowed us to assess disinhibition withless interference from modulating inputs and to determine theextent of disinhibition produced within localized networks. Inour study, we have found that NMDA antagonists greatly reduceIPSCs in the PCC/RSC, an area of high susceptibility to NMDA antagonist-inducedneurotoxicity.

With respect to the regional vulnerability to NMDA antagonist-induced neurotoxicity in vivo, the PCC/RSC is more susceptiblethan other cortical areas detected with a range of methods, includinghematoxylin and eosin, silver stains, and electron microscopy(Olney et al., 1989; Fix et al., 1993; Corso et al., 1997; Horvathet al., 1997). We have found regional differences in the disinhibitoryeffects of MK-801 in vitro that parallel in vivo histopathologicalstudies. Specifically, PCC/RSC pyramidal sIPSCs were significantlydecreased by MK-801, whereas parietal pyramidal sIPSCs were lessaffected. Similar to this weak effect of MK-801 on parietal sIPSCs,Salin and Prince (1996) demonstrated that D-APV, a competitiveNMDA receptor antagonist, only minimally inhibited sIPSC frequencyin rat somatosensory cortex, another area less vulnerable to MK-801-inducedneurotoxicity (Olney et al., 1989, 1991). We therefore postulatethat these regional differences in disinhibition may explain,at least in part, the regional difference in the vulnerabilityto NMDA antagonists-inducedneurotoxicity.

Our data indicate that MK-801-induced reduction in excitatory synaptic input onto GABAergic interneurons could be responsiblefor reducing pyramidal cell sIPSC frequency, although this isindirect evidence. However, we also isolated NMDA receptor-mediatedEPSCs in interneurons and found that MK-801 blocked these EPSCs,providing more direct evidence for NMDA antagonist-induced disinhibition.Entorhinal interneurons receive NMDA receptor-mediated input (Jonesand Buhl, 1993); however, some hippocampal interneurons may nothave NMDA receptors (McBain and Dingledine, 1993). Similar tothe hippocampal interneurons (McBain and Dingledine, 1993; Mottet al., 1997), cortical interneurons have heterogeneous anatomicmorphologies and physiological functions (Kawaguchi 1995; Kawaguchiand Kubota, 1996). These differences may contribute to regionalvulnerabilities in MK-801-inducedneurotoxicity.

Systemic administration of MK-801 results in altered field potentials, specifically limited to layer III of rat medial entorhinalcortex (Gloveli et al., 1997). A marked increase in immediateearly gene c-fos expression in layer III was also noted in ratspretreated with MK-801 (Vaisanen et al., 1999). These resultssuggested that cells in layer III are more sensitive to NMDA receptorantagonists. However, our experiments demonstrated that reductionin inhibitory transmission or disinhibition induced by MK-801is not layer specific, although there are interlaminar differencesin sIPSC frequency in rat somatosensory cortex (Salin and Prince,1996).

MK-801 modulates pyramidal cell IPSCs via an action potential-dependent mechanism

Reduction of inhibitory transmission by NMDA antagonists has been observed in hippocampus (Hablitz and Langmoen, 1986; Grunzeet al., 1996) and basolateral amygdala (Rainnie et al., 1991).In rat olfactory bulb, NMDA receptor activation is required fordendrodendritic inhibition (Schoppa et al., 1998). Direct infusionof D-APV bilaterally into the accessory olfactory bulb producedepileptiform seizures in adult female mice (Brennan and Keverne,1989), an effect consistent with disinhibition. These investigatorssuggested that reduced inhibitory transmission could result froma loss of excitatory drive onto interneurons in the localcircuit.

Our findings are compatible with this mechanism. MK-801 dramatically reduced the frequency of sIPSCs and the amplitude ofeIPSCs but did not affect the frequency or amplitude of TTX-insensitivemIPSCs. This argues that MK-801 did not affect the postsynapticefficacy of released GABA and did not affect quantal size or probabilityof spontaneous release. [Disinhibition produced by presynapticmechanisms has been observed elsewhere, such as in studies ofthe effects of opioids and cannabinoids (Cohen et al., 1992; Hoffmanand Lupica 2000)]. MK-801 seemed to affect action potential-dependentGABA release, compatible with an effect in inhibitory interneuronson either action potential-induced calcium influx into the presynapticterminal or an effect on action potential initiation or propagation.Consequently, future experiments will focus on the effects ofMK-801 on synaptic currents and resting spontaneous activity ininterneurons.

Relation to proposed models

These results support the hypothesis that NMDA antagonists produce disinhibition within a PCC/RSC excitatory/inhibitory network.This disinhibition may be attributable partially to a local effect,because these findings were obtained in brain slices in whichmany of the modulatory input fibers have beensevered.

These results, however, do not rule out the importance of inputs from other brain areas shown to play a role in NMDA antagonist-inducedneurotoxicity [e.g., inputs from the anterior thalamus (Tomitakaet al., 2000) or cholinergic nuclei (Corso et al., 1997)]. Thismay be important, because it is not clear whether disinhibitionalone is sufficient to produce neurodegeneration in the PCC/RSC.For example, if disinhibition is sufficient, then local injectionof NMDA antagonists into the PCC or RSC might be expected to producelocalized neurodegeneration. However, the results vary regardingthe in vivo effects of direct injections of NMDA antagonists:D-APV injected directly into the cingulate caused neuronal vacuolization(Olney et al., 1989), whereas MK-801 injected into the RSC didnot induce HSP70 heat shock protein, but instead, HSP70 was inducedafter bilateral (but not unilateral) MK-801 injections into theanterior thalamus (Tomitaka et al., 2000). Based on the latterfindings, a model was constructed in which excitatory connectionsfrom the anterior thalamus to the RSC mediate MK-801-induced neurotoxicity,and it is within the thalamus that local modulation of GABAergicinhibition occurs (Tomitaka et al., 2000). That model is entirelyconsistent with their findings. However, our results suggest thatthere also is modulation of GABAergic function at the local corticallevel. It is possible that locally mediated disinhibition (asseen in our slices) may not be sufficient to produce neurodegeneration.However, local disinhibition could become critical when modulatedby other neurotransmitters or external excitatory inputs, thenleading to full-blown neurodegeneration. Given that region-specificdisinhibition seen in vitro does parallel region-specific neurodegenerationseen in vivo, it is plausible that disinhibition may be a candidatemechanism underlyingneurotoxicity.

Clinical significance

These findings may have wide-ranging clinical significance because drugs with NMDA antagonist activity are being used clinically,and many more are under development. These include drugs for pain,epilepsy, and Parkinson's disease (Subramaniam et al., 1995; Boyceet al., 1999; Parsons et al., 1999). Also, certain abused drugs,such as PCP and ketamine, are NMDA antagonists (Olney et al.,1987). Potent NMDA antagonists such as PCP produce bizarre anddisturbing behavioral effects in humans, but it has not been determinedwhether this reflects neurotoxicity. If so, it will be importantto better understand the neurotoxic mechanisms and to reduce therisk of damage. One strategy involves using NMDAR-glycine siteantagonists, which lack neurotoxicity (Berger et al., 1994; Auer,1997). However, noncompetitive channel antagonists may still proveuseful, so it will be important to better understand their neurotoxicmechanisms and the characteristics that increase vulnerabilityto neurotoxicity [e.g., age or gender (Auer, 1996; Wozniak etal., 1996)].

Also, NMDA antagonists are proposed to model psychiatric conditions such as schizophrenia (Ellison, 1995; Farber et al., 1995b).If there are shared mechanisms between drug-induced neurotoxicityand the etiologies of schizophrenia, these findings may have broadimplications forpsychiatry.

  FOOTNOTES

Received July 5, 2001; revised Feb. 5, 2002; accepted Feb. 5, 2002.

This work was supported by the Department of Defense (Neurotoxin Exposure Treatment Research Program, DAMA17-99-1-9541; Q.L,S.C., D.V.L., W.A.W.), The Department of Veteran Affairs (W.A.W.,S.C), and the National Institutes of Health (DA-06735; D.V.L).

Correspondence should be addressed to Dr. Qiang Li, Neurology Research, Veterans Administration Medical Center, Room 24, Building16, 508 Fulton Street, Durham, NC 27705. E-mail: Liq{at}duke.edu.

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