Reduced Inhibition in an Animal Model of Cortical Dysplasia

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The Journal of Neuroscience, December 1, 2000, 20(23):8925-8931

Reduced Inhibition in an Animal Model of Cortical Dysplasia
Wei Jian Zhu¹ and Steven N. Roper¹^,²
¹ Department of Neurological Surgery, University of Florida, and ² Malcolm Randall Veterans Administration Medical Center, Gainesville, Florida 32610-0265

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cortical dysplasia has a strong association with epilepsy in humans, but the underlying mechanisms for this are poorly understood.In utero irradiation of rats produces diffuse cortical dysplasiaand neuronal heterotopia in the neocortex and hippocampus. Usingin vitro neocortical slices, whole-cell patch-clamp recordingswere obtained from pyramidal neurons in dysplastic cortex andcontrol neocortex. Spontaneous IPSCs were reduced in amplitude(35%) and frequency (70%) in pyramidal cells from dysplastic cortex.Miniature IPSCs were reduced in frequency (66%) in dysplasticcortex. Two additional measures of cortical inhibition, monosynapticevoked IPSCs and paired pulse depression of evoked EPSCs, werealso impaired in dysplastic cortex. Spontaneous EPSCs were increasedin amplitude (42%) and frequency (77%) in dysplastic cortex, butminiature EPSCs were not different between the two groups. Thesedata demonstrate significant physiological impairment in inhibitorysynaptic transmission in experimental cortical dysplasia. Thissupports previous immunohistochemical findings in this model andobservations in humans of a reduction in the density of inhibitoryinterneurons in dysplasticcortex.

Key words: cortical dysplasia; GABA; neocortex; development; local circuits; epilepsy

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Disorders of cortical development are common findings in people with intractable epilepsy and impaired cognitive development(Taylor et al., 1971; Palmini et al., 1991; Raymond et al., 1995).Cortical dysplasia is one type of such disorders and is characterizedby loss of normal lamination in the neocortex, abnormal spatialorientation of the neurons, cytoskeletal abnormalities, and abnormalitiesof cell commitment (Mischel et al., 1995). Despite a strong associationbetween cortical dysplasia and epilepsy, the exact relationshipbetween structural abnormalities and seizure activity is not clear.A causal relationship between some types of focal cortical dysplasiaand epilepsy is suggested by the fact that surgical resectionof these lesions can abolish the person's seizures (Hirabayashiet al., 1993; Palmini et al., 1995). In other cases, corticaldysplasia can be present in people who never haveseizures.

A number of animal models have been used to examine genetic control of cortical development and response to early corticalinjury and to relate structural features of cortical dysplasiawith functional abnormalities. In utero irradiation of rats isone such model. Exposure of pregnant rats and their fetuses toexternal irradiation on gestational day 17 produces offspringwith microcephaly, diffuse cortical dysplasia, subcortical andperiventricular heterotopic gray matter, heterotopic neurons inthe hippocampus, and agenesis or hypoplasia of the corpus callosum(Riggs et al., 1956; Cowan and Geller, 1960; Roper et al., 1995).Previous studies have shown that the affected rats have an increasedpropensity for electrographic seizures in the presence of certainsedating agents (Roper et al., 1995). In vitro slices of dysplasticneocortex demonstrate enhanced epileptiform activity in the presenceof the GABA_A receptor antagonist bicuculline methiode when comparedwith control neocortex (Roper et al., 1997b). Immunohistochemicalstudies have demonstrated a selective reduction in inhibitoryinterneurons (cells immunoreactive for parvalbumin and calbindin-D28k)in dysplastic cortex (Roper et al., 1999). The current study wasperformed to study possible alterations in excitatory and inhibitoryconnections in cortical dysplasia using whole-cell patch-clamprecordings of spontaneous and evoked postsynaptic currents. Wepresent evidence for a significant reduction in inhibitory connectionsin experimental cortical dysplasia when compared with controlneocortex.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals and irradiation. All procedures used in the study adhered to guidelines approved by the Institutional Animal Careand Use Committee at the University of Florida. Female SpragueDawley rats with known insemination times were obtained (HarlanSprague Dawley, Indianapolis, IN). The day of insemination wasdesignated embryonic day 0 (E0). Pregnant rats were housed separately,and pups were weaned at postnatal day 28. All animals were maintainedon 12 hr light/dark cycles and were provided food and water adlibitum. Offspring from six irradiated (n = 20 animals) and sevencontrol (n = 21 animals) mothers were used for the experiments.Irradiation was performed on E17. Pregnant rats were placed ina Plexiglas box to limit movement and exposed to 225 cGy of external $gamma$ irradiation from a linear acceleratorsource.

Brain slice preparation. In vitro brain slices were obtained from 28- to 35-d-old rats using procedures similar to those describedpreviously (Roper et al., 1997b). After decapitation, the brainwas rapidly removed and submerged in ice-cold artificial CSF (ACSF)containing (in mM): NaCl 124, KCl 2.5, KH₂PO₄ 1.25, MgCl₂ 2.5,CaCl₂ 0.5, NaHCO₃ 26, and glucose 10, pH 7.4 (300 mOsm/kg). Threehundred- to 400-µm-thick, coronal, hemispheric brain slices wereobtained at the rostrocaudal level of the anterior commissureusing a Vibratome (Campden Instruments). The slices were incubatedin oxygenated (5% CO₂ and 95% O₂) ACSF at 32-34°C for 30 min andthen maintained at room temperature (22-25°C) until they weretransferred to a submersion-type recordingchamber.

Electrophysiological recording. Neocortical pyramidal neurons were identified using infrared differential interference contrast(IR-DIC) videomicroscopy with a fixed-stage microscope (Axioskop-FS,equipped with a 40×, 0.80 W water-immersion lens; Zeiss, Oberkochen,Germany), according to their characteristic somata and apicaldendrites. All of the recordings were made at room temperature(22-25°C) from slices kept under constant (2-3 ml/min) perfusionof ACSF as given above, with the exception that MgCl₂ and CaCl₂concentrations were 1 and 2 mM, respectively. Drugs were appliedto slices by gravity perfusion. Evoked synaptic responses wereobtained in neocortical pyramidal cells using a twisted platinum-iridiumwire (diameter, 76 µm) with current pulses (0-500 µA; duration,0.1 msec) applied to the white matter adjacent to the recordedcell. Analysis of all evoked responses was based on averages of10 trials per event with 30 sec intervals betweenstimuli.

Spontaneous and miniature postsynaptic currents. Tight-seal (>1 G $Omega$ ) whole-cell recordings were obtained from the cell bodyof neocortical pyramidal cells. Patch electrodes had a resistanceof 3-5 M $Omega$ when filled with (in mM): potassium gluconate 120, NaCl8, HEPES 10, MgATP 4, Na₃GTP 0.4, EGTA 0.2, and biocytin 0.1%,pH 7.2 (280 mOsm/kg) for EPSCs and CsCl 125, HEPES 10, MgATP 5,Na₃GTP 0.4, MgCl₂ 4, EGTA 5, and biocytin 0.1%, pH 7.2 (280 mOsm/kg)for IPSCs. Neurons were voltage-clamped at $-$ 65 mV (for EPSCs)or $-$ 60 mV (for IPSCs) using an Axopatch 1D amplifier (Axon Instruments,Foster City, CA). Access resistance (10-25 M $Omega$ ) was monitored regularlyduring recordings, and cells were rejected if it changed >15%during the experiment. Data were filtered at 2 kHz, digitizedat 10 kHz, and stored in a computer using pClamp 8 software (AxonInstruments) for off-line data analysis. In some experiments,inhibitory currents were blocked using the GABA_A receptor antagonistspicrotoxin (100 µM) and bicuculline methiodide (BMI; 10 µM). GABA_A-gatedIPSCs were recorded in the presence of DL-2-amino-5-phosphonopentanoicacid (AP-5; 50 µM) and 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX;10 µM) in the bath solution to block fast glutamatergic transmission.Miniature EPSCs (mEPSCs) and mIPSCs were recorded in the presenceof tetrodotoxin (TTX; 1 µM).

Histology. Slices with biocytin-filled cells were fixed by immersion in 4% paraformaldehyde in 0.15 M phosphate buffer overnightat 4°C and then rinsed three times in PBS (0.01 M). The sliceswere incubated in PBS containing 10% methanol and 3% H₂O₂ for1 hr to remove endogenous peroxidase activity and rinsed threetimes in PBS. Slices with biocytin-filled cells were then incubatedin avidin-biotin-horseradish peroxidase complex (ABC Elite kit;Vector Laboratories, Burlingame, CA) in PBS (1:100), pH 7.3, containing2% Triton X-100 for 48-72 hr at 4°C. The slices were rinsed andreacted with 3,3'-diaminobenzidine tetrahydrochloride (0.06%)and H₂O₂ (0.003%) in PBS, pH 7.4. The slices were mounted on subbedslides, air-dried overnight, dehydrated through a graded seriesof ethanols (70-100%), andcoverslipped.

Data analysis and statistics. Event analysis was performed on continuous segments of spontaneous synaptic current records(sIPSCs, mIPSCs, sEPSCs, and mEPSCs) lasting 3-5 min in a semiautomatedmanner. Histograms were made of two parameters extracted fromthe continuous records (amplitude and interevent time interval),and these data were converted to probability density functionsfor comparison. Synaptic events per period were detected usinga threshold crossing of the derivative with parameters set foreach cell and kept constant for the whole session (Mini AnalysisProgram; Synaptosoft Inc., Leonia, NJ). The events detected werethen visually inspected to remove electrical artifacts beforefinal analysis. Their peak amplitude and 10-90% rise time weremeasured, and the decay phase of individual events could be fittedby one exponential. Individual EPSCs that did not overlap withother events were selected at random and averaged together toform composite EPSCs for analysis. All results are given as mean± SD. The large sample approximation of the Kolmogorov-Smirnofftest was used to compare the distributions of sIPSC, mIPSC, sEPSC,and mEPSC parameters between individual representative neurons.Paired or unpaired Student's two-tailed t test was used to comparegroup results. Statistical significance was defined as p < 0.05.

Drugs. CNQX and AP-5 were obtained from Tocris Cookson (Ballwin, MO); TTX, BMI, and picrotoxin were from Sigma (St. Louis,MO).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Histological effects

Histological abnormalities found in the irradiated rats have been described in detail previously (Riggs et al., 1956; Cowanand Geller, 1960; Roper et al., 1995). All slices used in thisstudy demonstrated cortical dysplasia and subcortical neuronalheterotopia. Dyplastic cortex (DC) was characterized by thinningof the cortex with loss of lamination and loss of the normal orientationof some pyramidal cells with respect to the pial surface (Fig.1B). DC and heterotopic gray matter were easily visualized witha low-power objective (10×) at the time of physiological recordingsusing IR-DIC videomicroscopy. Cresyl violet staining of some fixedslices was performed after recording to confirm these changes.

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Figure 1. Morphological and physiological properties of a pyramidal neuron in dysplastic cortex. A, Composite videomicrograph of a representative biocytin-filled pyramidal cell with the soma lying in the center of the dysplastic cortex, dendrites extending to the pial surface (top), and the axon extending into the white matter. Scale bar, 100 µm. B, Photomicrograph of a cresyl violet-stained section of dysplastic cortex (40 µm thick) demonstrating thinning of the cortex, loss of laminar organization, and loss of orientation of pyramidal cells (pial surface is at top) Scale bar, 100 µm. C, Current-clamp recording (top trace) of a pyramidal neuron from dysplastic cortex demonstrating the response to depolarizing current (bottom trace). Elicited action potentials show frequency adaptation that is indicative of a regular spiking neuron.

Basic membrane properties in pyramidal neurons

Whole-cell recordings were performed in the somatosensory cortex overlying the lateral ventricle. In control cortex we recordedfrom neurons in superficial layers (II/III) and in layer V. InDC we recorded from neurons throughout the cortical mantle. Pyramidalneurons were identified using morphological properties of theirtriangular somata and prominent apical dendrites under IR-DICvideomicroscopy using a 40× objective. As shown in Figure 1A,recorded cells filled with biocytin had apical and basal dendriteswith many spines and main axons extending to the underlying whitematter. Morphological features of pyramidal cells in DC were similarto those of control pyramidal cells, although the orientationof the neuron with respect to the pial surface was sometimes abnormal.No systematic analysis of dendritic or axonal distribution orbranching patterns was performed; therefore, the possibility ofmore subtle structural differences between pyramidal cells incontrol and dysplastic cortex cannot be excluded. With step-wisedepolarization in whole-cell current-clamp recordings, all pyramidalneurons tested (control, n = 24; DC, n = 22) responded initiallywith a high frequency of action potentials (APs), adapting toa lower, sustained frequency (Fig. 1C) as described for regularspiking cells (McCormick et al., 1985; Chagnac-Amitai and Connors,1989). The resting potentials in all neurons recorded were morenegative than $-$ 60 mV. Membrane and AP properties of neurons fromlayers II/III and V in control neocortex were not different, andthese values were not different from those observed in the pyramidalneurons of DC (Table 1).


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Table 1. Membrane properties and postsynaptic currents in the pyramidal neurons of cortex

Impaired GABAergic synaptic transmission in dysplastic cortex

Whole-cell voltage-clamp recordings were made from pyramidal neurons in dysplastic and control neocortex. Spontaneously occurringinward currents were observed at a holding potential of $-$ 60 mVin the presence of CNQX (10 µM) and AP-5 (50 µM). These currentswere completely blocked by the GABA_A receptor antagonists picrotoxin(100 µM) and BMI (10 µM), indicating that the synaptic currentswere GABAergic. The measured amplitude and frequency of thesecurrents showed no consistent developmental change in the cellsfrom animals aged from postnatal day 28 (P28) to P35 (data notshown), and the kinetics, amplitude, and frequency of sIPSCs betweenlayer II/III and V pyramidal neurons in control neocortex werenot significantly different (Table 1). In this study, we groupedneurons from layers II/III and V together in the statistical analysisof IPSCs andEPSCs.

As shown in Figure 2A, the frequency of sIPSCs in pyramidal neurons from DC was reduced in comparison with control neurons.However, the 10-90% rise time (control, 1.75 ± 0.12 msec; n =20; DC, 1.88 ± 0.11 msec; n = 19; p = 0.42) and the decay timeconstant (control, 10.96 ± 0.61 msec; n = 20; DC, 11.47 ± 0.82msec; n = 19; p = 0.64) of sIPSCs were not different between controland dysplastic cortex. Mean amplitude and frequency of sIPSCsin pyramidal neurons from control (n = 20) and dysplastic cortex(n = 19) are shown in Figure 2, B and C. Both amplitude and frequencywere significantly reduced by 35 and 70%, respectively, in pyramidalneurons from DC.

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Figure 2. Decreased amplitude and frequency of sIPSCs from pyramidal neurons in dysplastic cortex. A, Representative traces of voltage-clamp recordings from pyramidal neurons in control neocortex and dysplastic cortex in the presence of AP-5 (50 µM) and CNQX (10 µM). B, C, Group comparison of amplitude and frequency of sIPSCs and mIPSCs from pyramidal neurons in control neocortex and DC. Graphs show data for amplitude (B) and frequency (C) of sIPSCs (left) and mIPSCs (right). B, Mean values of sIPSC amplitude were decreased in DC (p < 0.001), but the mIPSC amplitude was not different (p = 0.83). C, Mean frequencies of both sIPSCs and mIPSCs were significantly reduced in DC (p < 0.001 for both measures).

Miniature IPSCs resulting from the spontaneous, action potential-independent release of GABA from individual vesicles in theaxon terminals were recorded in the presence of TTX (1 µM) (Fig.3A). To determine whether inhibitory synaptic activity was impairedin DC, the amplitude, frequency, and kinetics of mIPSCs from pyramidalcells in DC were compared with those from pyramidal cells in controlneocortex. The decay time constant of mIPSCs was not changed betweenthe two groups (control, 10.1 ± 0.72 msec; n = 17; DC, 9.35 ±0.78 msec; n = 18; p = 0.48). Also, there was no significant differencein the 10-90% rise time of mIPSCs (control, 1.75 ± 0.12 msec,n = 17; DC, 1.71 ± 0.13 msec; n = 18; p = 0.67). Amplitude distributionhistograms were similar between representative pyramidal neuronsfrom control and dysplastic cortex (Fig. 3B). The mean amplitudeof mIPSCs (Fig. 2B) was also not different between control (n= 17) and dysplastic cortex (n = 18). However, cumulative probabilitycurves demonstrated an increase of the interevent interval inDC when representative neurons were compared (Fig. 3D). In thegroup comparison, the mean frequency of mIPSCs was significantlyreduced by 66% in DC (n = 17) compared with control (n = 18) neocortex(Fig. 2C).

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Figure 3. Decreased frequency of mIPSCs in pyramidal neurons from dysplastic cortex. A, Representative voltage-clamp recordings of mIPSCs from pyramidal neurons from control and dysplastic cortex in the presence of AP-5 (50 µM), CNQX (10 µM), and TTX (1 µM). B, Distribution histograms of mIPSC amplitude from these cells show similar patterns. Normalized cumulative probability curves show no difference between control and dysplastic cortex for mIPSC amplitude (C; p = 0.16), but the interevent interval (D) is shifted to the right (consistent with decreased frequency) in the neuron from dysplastic cortex (p < 0.0001).

Decreased monosynaptic evoked IPSCs in pyramidal neurons from dysplastic cortex

At a holding potential of $-$ 60 mV, single-pulse stimulation was applied by a bipolar platinum-iridium electrode positioned150-200 µm away from the recorded soma to directly activate localinterneurons. Monosynaptic evoked IPSCs (eIPSCs) of pyramidalneurons were recorded in the presence of CNQX (10 µM) and AP-5(50 µM), and stimulus amplitudes were increased in intensity (0-500µA) until they reached a maximal response. To verify that monosynapticeIPSCs were GABA_A-mediated, in some experiments a GABA_A receptorantagonist (BMI, 10 µM, or picrotoxin, 100 µM) was applied tothe bath solution, showing a complete and reversible abolishmentof evoked postsynaptic currents (data not shown). Evoked IPSCsdisplayed a fast-onset inward current with a small delay afterthe stimulation (Fig. 4A). Failures were more frequent at lowerintensities. In pyramidal neurons from DC, mean rise time anddecay time constants were 5.2 ± 1.12 and 25.68 ± 2.34 msec (n= 20), respectively, which were not significantly different fromthose in control neurons. However, the mean maximal amplitudeof monosynaptic eIPSCs was significantly decreased by 48% in pyramidalneurons from DC (n = 16) compared with controls (n = 20; failuresnot included) (Fig. 4B).

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Figure 4. Monosynaptic evoked IPSCs recorded from pyramidal neurons from control and dysplastic cortex in the presence of AP-5 (50 µM) and CNQX (10 µM). A, Representative recordings of monosynaptic eIPSCs show a smaller response in the neuron from dysplastic cortex (bottom trace) compared with the control neuron (top trace). B, Group comparison of data from control and dysplastic cortex shows a significant reduction in monosynaptic eIPSC amplitude in pyramidal neurons from dysplastic cortex (p < 0.002).

Absence of paired pulse depression in pyramidal neurons from dysplastic cortex

To examine excitatory synaptic transmission in DC, neocortical pyramidal neurons were voltage-clamped at $-$ 65 mV, close tothe Cl equilibrium potential, with potassium gluconate intracellularsolution. Evoked EPSCs (eEPSCs) were induced by placing a bipolarplatinum-iridium electrode in the white matter beneath the neocortex,showing increased inward currents with an increase in the stimulationintensity (0-500 µA). The average 10-90% rise time and decay timeconstants were 1.85 ± 0.09 and 7.9 ± 0.38 msec (n = 16), respectively,in control neocortex. Bath perfusion of CNQX (10 µM) and AP-5(50 µM) completely and reversibly blocked the eEPSCs. We observedthat the fast-onset inward peak current of eEPSCs was usuallyfollowed by a group of high-frequency, inward currents in pyramidalcells from DC (Fig. 5A), but this activity was rare in controls(control, 3 of 16 cells; DC, 15 of 18 cells). The delayed inwarddischarges could be abolished by bath application of CNQX andAP-5, indicating that they are glutamate-mediated events. EvokedEPSCs in pyramidal neurons from DC (n = 14) showed a 52% increasein amplitude compared with controls (n = 22; Fig. 5B), and thetotal charge transfer during eEPSCs was significantly increasedin pyramidal neurons from DC compared with controls (Fig. 5C).The 10-90% rise time was not significantly changed in DC.

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Figure 5. Evoked EPSCs recorded at the reversal potential of GABAgeric currents in pyramidal neurons from control and dysplastic cortex. A, Representative recordings of eEPSCs in pyramidal neurons from control and dysplastic cortex. Evoked EPSCs from dysplastic cortex typically demonstrated a complex response comprising multiple inward currents. B, Group comparison of data from control and dysplastic cortex shows an increase in eEPSC peak amplitude in dysplastic cortex (p < 0.001). C, The averaged area of eEPSCs in dysplastic cortex was also significantly increased (p < 0.001).

To examine the competency of feedback inhibition in the neural circuits of DC, paired pulse stimulation (interpulse interval,20 msec) was applied while eEPSCs were recorded in pyramidal cellsat a holding potential of $-$ 65 mV. As shown in Figure 6A, the secondeEPSC amplitude was smaller than the first response in controlneocortex. However, the second synaptic response was increasedcompared with the first one in DC, suggesting an impairment offeedback inhibition in DC neuronal circuits. This difference wasmaintained when group data from control neocortex (n = 14) andDC (n = 16) were compared (Fig. 6B).

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Figure 6. Paired pulse modulation of evoked EPSCs recorded from pyramidal neurons in control and dysplastic cortex with an interpulse interval of 20 msec. A, Representative recordings of paired eEPSCs in pyramidal cells from control and dysplastic cortex show that the amplitude of the second response was reduced in the control neuron but increased in the neuron from dysplastic cortex. B, Group data from control and dysplastic cortex demonstrate an absence of paired pulse depression in dysplastic cortex (p < 0.001).

Enhanced excitatory synaptic transmission in pyramidal neurons from dysplastic cortex

Spontaneous EPSCs were recorded from neocortical pyramidal neurons voltage-clamped at $-$ 65 mV (Fig. 7A). Bath application ofCNQX and AP-5 completely and reversibly abolished the spontaneouslyoccurring inward currents observed at this holding potential.As observed in IPSCs, the amplitude and frequency of EPSCs didnot change with age (P28-P35) and were not different between layerII/III and V pyramidal neurons (Table 1). The 10-90% rise times(control, 1.85 ± 0.09 msec; n = 25; DC, 2.02 ± 0.16 msec; n =28; p > 0.05) and decay times (control, 7.92 ± 0.38 msec; n =25; DC, 7.38 ± 0.7 msec; n = 28; p > 0.05) of sEPSCs were notdifferent between pyramidal cells from control neocortex and DC.In representative neurons, the distribution of sEPSCs showed largeramplitudes in DC than in control neurons (Figs. 7B), and cumulativeprobability curves were shifted to larger amplitudes (Fig. 7C).In the group analysis, the mean sEPSC amplitude was increasedby 42% in pyramidal neurons from DC (n = 28) compared with controls(n = 25) (Fig. 8A). In representative neurons, cumulative probabilitycurves showed a decrease in interevent intervals for sEPSCs inpyramidal cells from DC (Fig. 7D). Group comparisons showed thatmean sEPSC frequency was significantly higher in DC (n = 28) comparedwith controls (n = 25) (Fig. 8B).

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Figure 7. Increased amplitude and frequency in sEPSCs in pyramidal neurons from control and dysplastic cortex. A, Representative voltage-clamp recordings demonstrate a significant increase in amplitude and frequency of sEPSCs in the pyramidal neuron from dysplastic cortex compared with the control neuron. B, Amplitude distribution histograms of sEPSCs from pyramidal neurons from control and dysplastic cortex show that sEPSCs were skewed toward larger amplitudes, especially in dysplastic cortex. C, Normalized cumulative probability curves of sEPSC amplitude show that values from the dysplastic cortex neuron were significantly shifted to the right (p < 0.0001), indicating an increase in sEPSC amplitude in this cell. D, Normalized cumulative probability curves of interevent intervals are significantly shifted to the left in the pyramidal neuron from dysplastic cortex compared with the control neuron (p < 0.0001), indicating an increase in sEPSC frequency in the dysplastic cortex neuron.

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Figure 8. Group comparisons of amplitude and frequency of sEPSCs and mEPSCs from pyramidal neurons from control and dysplastic cortex. Graphs show data for amplitude (A) and frequency (B) of sEPSCs (left) and mEPSCs (right). Mean values of sEPSC amplitude were increased in dysplastic cortex (p < 0.001), but there was no difference in mean mEPSC amplitude between the two groups (p = 0.21). Mean sEPSC frequency was increased in dysplastic cortex (p < 0.001), but there was no difference in mean frequency of mEPSCs between the two groups (p = 0.67).

Miniature EPSCs were recorded in the presence of TTX (1 µM) from pyramidal cells voltage-clamped at $-$ 65 mV to examine presynapticor postsynaptic mechanisms of increased excitability in the neuronalcircuits of dysplastic cortex. In contrast to sEPSCs, there wasno difference in mean amplitude or frequency of mEPSCs betweenpyramidal neurons from control (n = 15) and dysplastic (n = 12)cortex (Fig. 8). There was also no difference in rise time, decaytime, or distribution of mEPSC amplitude or interevent interval.Therefore, blocking action potential-dependent activity abolishedthe increased spontaneous excitatory activity in pyramidal neuronsfromDC.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study has demonstrated significant impairment of inhibition in the in utero irradiation model of cortical dysplasia.The reduction in frequency of miniature IPSCs recorded from pyramidalcells with no difference in amplitude suggests that the principalabnormality is presynaptic rather than postsynaptic. This couldresult from an impaired release mechanism from the presynapticterminals or simply from a reduction in the number of GABAergicterminals on the pyramidal cells. This second explanation is supportedby previous studies from this laboratory that showed a reductionin density of parvalbumin- and calbindin D28k-immunoreactive neuronsin dysplastic cortex from irradiated rats (Roper et al., 1999),because a reduced number of inhibitory neurons would likely resultin a reduced number of inhibitory connections by these neuronsonto adjacent pyramidal cells. In addition, the similar frequencyof both spontaneous and miniature IPSCs may indicate a relativelylow level of spontaneous activity in inhibitory interneurons indysplasticcortex.

Decreases in paired pulse inhibition and monosynaptic evoked IPSCs also provide evidence for impaired inhibition in dysplasticcortex but do not give any additional information regarding thespecific mechanisms of this impairment. In this study, pairedpulse depression of excitatory postsynaptic responses was selectedas a common measure of cortical inhibition (Burdette and Gilbert,1995; Ramoa and Sur, 1996) to either support or contradict thespontaneous IPSC results. Whole-cell recordings from paired corticalneurons have confirmed that, with an interstimulus interval of20 msec, pyramidal cell pairs generally show paired pulse depression,whereas pyramidal interneuron pairs show paired pulse facilitation(Thomson, 1997). However, short-term synaptic plasticity is affectedby many variables, such as presynaptic release probability (Oleskevichet al., 2000), postsynaptic receptors and cell properties (Rozovand Burnashev, 1999), and presynaptic GABA_B receptors (Deisz,1999), and other explanations for our reported changes in pairedpulse depression arepossible.

In this study we used neurons from both supragranular and infragranular layers of control neocortex for comparison with neuronsfrom DC. DC in this model has no clear laminar pattern, so thereare no anatomic cues on which to base a comparison between thesame cortical layers in both the control and experimental groups.Neurons in DC are most likely to represent neurons that shouldhave assumed an infragranular location, because the irradiationoccurs at a time when the early cortical plate has already formed,and neurons destined for the deeper layers arrive first in corticaldevelopment. The irradiation treatment kills immature, migratingneurons (Bayer and Altman, 1991) as well as radial glia (Roperet al., 1997a) with relative sparing of the cortical plate neuronsand the neuroepithelium. After irradiation, some neurons are trappedin the periventricular and subcortical regions and go on to formneuronal heterotopias, but some may still migrate out to the corticalplate. Therefore the resultant dysplastic cortex (as opposed tothe underlying heterotopic gray matter) probably represents anamalgam of neocortical neurons with a heavier representation fromneurons originally destined for the deeper cortical layers. Becauseof these factors, it is difficult to assign a specific categoryof neurons from control neocortex to serve as the appropriatecontrol group. For this reason we have studied pyramidal cells(which can clearly be identified morphologically in both controland dysplastic neocortex) from both supragranular and infragranularlayers in control neocortex as the comparison group. This raisesthe possibility that our study could produce a spurious resultif, for instance, one group of control neurons had a significantlyhigher frequency of miniature IPSC's when the appropriate comparisonwas actually with the control subset with a lower frequency. Toaddress this problem we compared the supragranular control neuronswith the infragranular control neurons and found no differencesbetween the two groups with respect to basic membrane propertiesor amplitude or frequency of sIPSCs or sEPSCs. On the basis ofthese findings it seems appropriate to use the pooled data fromsupragranular and infragranular neurons in control neocortex forcomparison with neurons from DC in thisstudy.

The findings of partial loss of inhibition in this model are consistent with observations in human cortical dysplasia. Twogroups have reported a qualitative reduction in inhibitory interneuronsin specimens of human focal cortical dysplasia surgically resectedfor the treatment of intractable epilepsy (Ferrer et al., 1992,1994; Spreafico et al., 1998). In addition, physiological abnormalitieshave been reported in human cortical dysplasia. Surface recordings(electrocorticography) from focal cortical dysplasia can showcontinuous ictal activity that is rarely seen in other types epilepsy(Palmini et al., 1995). In addition, in vitro brain slices ofhuman dysplastic cortex demonstrate prolonged epileptiform dischargesthat are not seen from "control" human temporal neocortex thatis removed during anterior temporal lobectomy for medial temporallobe epilepsy (Mattia et al., 1995). Although these physiologicalabnormalities document an increased propensity for epileptiformactivity, they do not specifically indicate impaired inhibition,and other mechanisms could explain thesefindings.

There are several other animal models of cortical dysplasia that have been studied. In utero administration of the alkylatingagent methylazoxymethanol acetate produces histological changessimilar to those in the in utero irradiation model. Physiologicalabnormalities in this model have included an increase in the numberof intrinsically bursting neurons in the hippocampus (Barabanand Schwartzkroin, 1995) and neocortex (Sancini et al., 1998).In the current study, we did not find intrinsically bursting neuronsin either control or dysplastic neocortex. Intrinsically burstingpyramidal neurons were originally described in layer V of normalneocortex using sharp intracellular microelectrodes (McCormicket al., 1985; Chagnac-Amitai and Connors 1989). Because of thelarge tip diameter of microelectrodes used in whole-cell patch-clamprecordings, the electrode-filling solution communicates freelywith the cytoplasm of the recorded cell. Because intrinsic firingproperties are significantly affected by intracellular calciumlevels (Friedman and Gutnick, 1989), it is possible that alterationsin intracellular calcium attributable to washout or bufferingfrom the microelectrode-filling solution make detection of intrinsicallybursting cells unlikely. In addition to this, there are differencesin age of the animals and the temperature of the recording chambersbetween these studies that might affect intrinsic firing patterns.Of note, Kawaguchi (1993) used whole-cell patch-clamp recordingtechniques similar to those used in the current study in controlneocortex and also found no intrinsically bursting neurons inrat frontal cortex. Additional studies using sharp intracellularmicroelectrodes may provide better detection and quantificationof intrinsically bursting cells inDC.

One model of focal cortical dysplasia involves creating a cortical freeze lesion on P0 or P1 that persists as a microsulcus.These animals develop an area of hyperexcitable cortex just adjacentto the actual lesion, the paramicrogyral cortex. Although thereis a loss of parvalbumin-immunoreactive neurons in supragranularlayers of the microsulcus and adjacent cortex in early postnataldevelopment, this deficit recovers by P21. There is a permanentdecrease in parvalbumin-immunoreactive neurons in the infragranularcortex in the microgyrus and paramicrogyral cortex in this model(Rosen et al., 1998). Spontaneous and evoked IPSCs are increasedin amplitude but not frequency in the paramicrogyral cortex (Princeet al., 1997), and current theories on epileptogenesis in thismodel involve synaptic reorganization with exuberant thalamocorticalconnections in the paramicrogyral cortex attributable to lossof normal targets in the microsulcus (Jacobs et al., 1999). DeFazioand Hablitz (1999, 2000) have provided evidence for a delay orarrest of normal maturation of GABA receptors (DeFazio and Hablitz,1999) and NMDA receptors (DeFazio and Hablitz, 2000) in neuronsof the paramicrogyral cortex in thismodel.

In addition to reduced inhibitory currents, we have also demonstrated an increase in the frequency of sEPSCs in pyramidalcells from DC. This difference was abolished when action potentialswere blocked with TTX. This suggests that the increased sEPSCsdid not represent a primary increase in the number of excitatorypresynaptic terminals on the pyramidal cells or a primary alterationin glutamatergic receptors. It could be a consequence of reducedinhibition in the local circuit, because a reduction of inhibitorytone would allow excitatory cells to fire more often. It couldalso result from an increase in the number of intrinsically burstingneurons in dysplasticcortex.

This study is the first to quantitatively demonstrate a physiological impairment in inhibition in an animal model of hyperexcitabledysplastic cortex. Paired with previous data that showed a persistent,selective reduction of inhibitory interneurons in the same areas(Roper et al., 1999), these results demonstrate a selective vulnerabilityof the inhibitory system to in utero irradiation. We do not knowwhether this is a direct effect of the radiation on immature neuronsthat would have become inhibitory neurons or whether it is a secondaryeffect of the treatment. It is even possible that the inhibitoryneurons are still present but misplaced. Preliminary studies haveshown inhibitory interneurons in subcortical and periventricularheterotopic gray matter in these animals, but no quantitativestudies have been performed (Roper and Houser, 1992). Whole-cellrecordings from heterotopic pyramidal neurons in this model haveshown the presence of inhibitory activity, but this has not beenquantified (Smith et al., 1999).

The majority of inhibitory interneurons of the neocortex originate outside the cortical mantle in the lateral and median ganglioniceminence (Anderson et al., 1997, 1999; Tamamiki et al., 1997).This necessitates a longer migratory pathway to the cortical plateand may make these immature inhibitory neurons more susceptibleto in utero injury, because migrating neurons are among the mostvulnerable to in utero irradiation (Altman et al., 1968; Bayerand Altman, 1991). Alternatively, the putative inhibitory neuronseither may arrive at the cortical plate and not develop theirappropriate phenotype or may die off during development becauseof some secondary abnormality in the dysplastic cortex such asincreased excitatory activity or alterations in subcortical afferents.The current data do not provide evidence to address these questions,and further studies are needed. At this point, these studies havedemonstrated a selective vulnerability of inhibitory interneuronsto in utero injury that may have far-reaching implications forother disorders of corticaldevelopment.

  FOOTNOTES

Received July 11, 2000; revised Sept. 7, 2000; accepted Sept. 20, 2000.

This work was supported by National Institute of Neurological Disorders and Stroke Grant NS35651 to S.N.R. Special thanksto Dr. F. E. Dudek for critiques and suggestions and Dr. FrankBova for assistance withirradiation.
Correspondence should be addressed to Dr. Steven N. Roper, Department of Neurological Surgery, University of Florida, P.O.Box 100265, Gainesville, FL 32610-0265. E-mail: roper{at}neurosurgery.ufl.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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