Contribution of NR2B Subunits to Synaptic Transmission in Amygdaloid Interneurons

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The Journal of Neuroscience, April 1, 2003, 23(7):2549

Contribution of NR2B Subunits to Synaptic Transmission in Amygdaloid Interneurons
Csaba Szinyei, Oliver Stork, and Hans-Christian Pape
Institute of Physiology, Medical School, Otto-von-Guericke University, 39120 Magdeburg, Germany

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Synaptic responses of interneurons in the rat lateral amygdala (LA) to electrical microstimulation of putative cortical andthalamic afferents were studied in slice preparations in situ.The EPSPs at both thalamic and cortical inputs were composed oftwo major components that were sensitive to 6,7-dinitroxaline-2,3-dioneand DL-2-amino-5-phosphonovaleric acid (APV), indicating mediationthrough AMPA and NMDA receptors. NMDA receptor activation contributedto basal synaptic transmission, as evidenced through a reductionof EPSP amplitudes and integrals by APV. NMDA receptor-mediatedpostsynaptic currents showed magnesium-regulated voltage dependence,and current-voltage relationships displayed a region of negativeslope conductance negative to resting potential. Deactivationof NMDA receptor-mediated currents followed a two exponentialtime course, with both components being significantly reducedby ifenprodil (10 µM), an antagonist of the NR2B subunit of NMDAreceptors. Significant differences were not observed between NMDAcurrents or ifenprodil effects at thalamic and cortical inputs.Furthermore, recordings from a sample of projection neurons inthe LA provided additional evidence for the existence of ifenprodil-sensitivecomponents of thalamically and cortically evoked NMDA receptor-mediatedresponses. Immunohistochemical double-labeling and combined insitu hybridization/immunohistochemistry demonstrated that GABA-immunoreactiveas well as GABA-negative cells express the NR2B subunit. Overall,these results show that GABAergic interneurons in the LA expressfunctional NMDA receptors, which participate in basal synaptictransmission at both thalamic and cortical inputs. The findingthat NR2B subunits are critically involved in NMDA receptor-mediatedsignaling at the two major input pathways to interneurons andprojection cells in the LA is particularly interesting in thelight of previous observations that NR2B antagonists interferewith plastic changes in the LA related to associative fearconditioning.

Key words: lateral amygdala; projection neuron; interneuron; inhibition; NMDA receptors; NR2B subunit

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The amygdaloid complex is known to be important for the regulation of emotional behavior and learning (LeDoux, 2000; Davis,2002) and to be critically involved in neurological disorders,such as temporal lobe epilepsy (Gloor, 1992), post-traumatic stresssyndrome, and depression (Levine et al., 2001). As the main sensoryinput station of the amygdala, the lateral amygdaloid nucleus(LA) receives sensory information from cortical and subcorticalfields. Cortical afferents reach the LA laterally from the externalcapsule, and the subcortical thalamic afferents arrive mediallyfrom the internal capsule (LeDoux et al., 1991; Turner and Herkenham,1991; Romanski and LeDoux, 1993; McDonald, 1998). These two mainsensory inputs converge on populations of principal cells (Liet al., 1996) and interneurons (Lang and Paré, 1998, Szinyeiet al., 2000), which in the LA can be classified based on electrophysiological,neurochemical, and morphological properties (Rainnie et al., 1991;Lang and Paré, 1998; Mahanty and Sah, 1998). In vivo data demonstrateda powerful control through GABAergic inhibition over the activityof projecting principal cells (Lang and Paré, 1997, 1998), whichrenders a special role to the GABAergic interneurons in the controlof excitation in this region. Indeed, GABAergic interneurons arethought to play a crucial role in information processing in theamygdala (Lang and Paré, 1997; Mahanty and Sah, 1999) and toparticipate to the regulation of epileptiform activity (Callahanet al., 1991; Gloor, 1992; Washburn and Moises, 1992a,b) as wellas fear and anxiety (Pesold and Treit, 1995; Sanders, 1995) throughthisregion.

With respect to fast excitation, AMPA and NMDA receptor-mediated responses were shown to coexist at both pathways to LA projectionneurons (Mahanty and Sah, 1999; Weisskopf and LeDoux, 1999). Convergingfast excitatory postsynaptic responses from cortical and thalamicinputs were also found in interneurons of the LA (Szinyei et al.,2000). The cortical glutamatergic inputs onto interneurons inthe lateral and basolateral nucleus of the amygdala were reportedto impinge on AMPA receptors, the Ca²⁺ permeability of which promoted a particular form of long-termsynaptic plasticity, whereas NMDA receptor-mediated signals werereported to be very small or negligible in these types of neurons(Mahanty and Sah, 1998). On the contrary, experiments on LA interneuronsusing pressure application of NMDA showed that the respectivereceptors are functional in interneurons, although the mediatingsynaptic inputs were not identified (Danober et al., 2000).

The present study was undertaken to investigate in detail the possible role of NMDA receptor activation for synaptic signalingin LA interneurons. The following findings were of particularinterest for the design of the study: differences in voltage-dependentproperties of NMDA receptor-mediated synaptic responses associatedwith thalamic and cortical inputs to LA projection neurons (Weisskopfand LeDoux, 1999; but see Mahanty and Sah, 1999) and the criticalcontribution of the NR2B subunits of NMDA receptors to plasticchanges in LA projection neurons associated with fear conditioningin the amygdala (Rodrigues et al., 2001; Bauer et al., 2002).In view of these findings, particular emphasis was put on a comparisonbetween NMDA receptor activation and properties associated withthalamic and cortical input fibers and the contribution of NR2Bsubunits to these responses ininterneurons.

  Materials and Methods

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Whole-cell patch-clamp recordings. Slices containing the amygdala from Long-Evans rats of either sex (postnatal days 21-28)were prepared, and recordings were performed as described previously(Szinyei et al., 2000). Briefly, rats were anesthetized with halothaneand killed by decapitation. After the preparation and equilibrationof 300-µm-thick coronal slices in a sucrose-containing solution[composed of the following (in mM): 20 piperazine-N,N'-bis-2-ethanesulfonate,2.4 KCl, 0.5 CaCl₂, 10 MgSO₄, 10 glucose, and 195 sucrose, withpH adjusted to 7.25 with 1 M NaOH and saturated with O₂], recordingswere obtained under visual guidance (Axioskop FS, Achroplan 40/w;Zeiss, Oberkochen, Germany) using infrared videomicroscopy (C-2400black-and-white camera, Hamamatsu, Hersching, Germany). Experimentswere done at 30°C in a submerged-type chamber. The extracellularsolution contained the following concentration of chemicals (inmM): 125 NaCl, 2.5 KCl, 1.25 NaH₂PO₄, 22 NaHCO₃, 2 MgSO₄, 2 CaCl₂,and 20 glucose, with pH adjusted to 7.3-7.4 through bubbling with95% O₂ and 5% CO₂. Electrophysiological recordings were performedusing the patch-clamp technique in whole-cell mode. Patch pipetteswere pulled from borosilicate glass (2.5-3.5 M $Omega$ , GC150T-10; ClarkElectromedical Instruments, Pangbourne, UK), and experiments wereperformed with a potassium-based internal solution containingthe following (in mM): 95 K-gluconate, 20 K₃-citrate, 10 NaCl,10 HEPES, 0.5 EGTA, 1 MgCl₂, 3 MgATP, and 0.5 NaGTP, with pH adjustedto 7.25 with 1 M KOH. To stimulate afferent fibers, bipolar tungstenstimulation electrodes were placed in the external capsule andin the internal capsule dorsal to the central nucleus of the amygdalasimilarly as described previously (Mahanty and Sah, 1999; Weisskopfand LeDoux, 1999; Heinbockel and Pape, 2000; Szinyei et al., 2000).Stimuli (100 µsec pulse duration, 0.1-5 mA) were used to evokesynaptic responses recorded with an Axopatch 200B amplifier (AxonInstruments, Foster City, CA). Access and input resistance werecontinuously monitored. Access resistance was in the range of8-16 M $Omega$ . Data were omitted if access resistance or input resistancechanged by >20% during the course of the experiment. Liquid junctionpotentials in all voltage-clamp experiments were corrected (Neher,1992). For stimulation, membrane potential control, and data acquisition,pClamp 8.0 software (Axon Instruments) was used. Data were low-pass-filteredat 2 kHz with the Bessel filter of the amplifier and digitizedat 10 kHz by a Digidata 1200 (Axon Instruments). Interneuronswere identified according to their electrophysiological properties(Washburn and Moises, 1992a; Rainnie et al., 1993; Mahanty andSah, 1998; Szinyei et al., 2000). After obtaining the cells involtage-clamp mode, current-clamp mode was chosen to characterizeintrinsic membrane and firing properties of the interneurons.Cells that showed high-frequency firing of fast action potentialsafter the injection of +0.1 to +0.4 nA current with distinct fastafterhyperpolarization after each spike and no apparent spikefrequency adaptation were considered to be interneurons. Classificationwas confirmed through morphological features (lack of dendriticspines) after histologicalprocessing.

Drug application. The following drugs were purchased (if not otherwise stated) from Sigma (St. Louis, MO) and applied duringthe experiments: DL-2-amino-5-phosphonovaleric acid (APV), ifenprodil,and (2S)-3-{[(15)-1-(3,4-dichlorophenyl)ethyl]amino-2-hydroxypropyl)(phenylmethyl)phosphinicacid(CGP55845; obtained from Tocris Cookson, Bristol, UK) were diluteddirectly in the external solution. Picrotoxin was predissolvedat 100 mM in ethanol (95% v/v); 6,7-dinitroxaline-2,3-dione (DNQX)was prepared at 20 mM in 100%DMSO.

Analysis of synaptic responses and drug effects. After baseline stabilization, EPSPs were recorded on alternating stimulationat 0.05 Hz of thalamic and cortical input fibers. Amplitudes wereaveraged from 10 consecutive EPSPs, separately for each pathway,and these were considered controls. The effects of an applieddrug were considered maximal if a stable new baseline was obtained.Amplitudes were averaged from 10 consecutive EPSPs and normalizedwith respect to the control values, separately for each inputpathway. For experiments with repetitive stimulation (10 pulsesat 2 Hz), stimuli were delivered twice at 20 sec intervals. TheAPV-sensitive response component was obtained as the graphic differenceof responses under control conditions and the maximal action ofAPV. Integrals were calculated as the summed amplitudes of EPSPs(sampling rate at 10 kHz) under the different experimental conditions.To obtain current-voltage (I-V) relationships of EPSCs under voltage-clampconditions, interneurons were initially stepped to +50 mV, theresulting outward current was allowed to settle to a steady-statevalue (average holding current at +50 mV was +1.03 ± 0.1 nA; n= 11), and after recording of evoked EPSCs at that potential,less-positive holding potentials were approached in a stepwisemanner. This protocol allowed fair voltage control of EPSCs, asindicated by smooth I-V curves and similar values of reversalpotentials of EPSCs recorded in different cells under differentexperimental conditions. For the construction of I-V relationships,EPSCs were normalized with respect to the absolute value of theEPSC amplitude at $-$ 50 mV in 0.1 mM Mg²⁺ (giving maximal synaptic inwardcurrent).

When standard double-exponential fits were applied to the decay phase of averages of EPSCs, the value of the correlation coefficientwas always >0.96. The following equation was used: y = A₀ + A₁× exp( $-$ t/ $tau$ ₁) + A₂ × exp ( $-$ t/ $tau$ ₂), with A_n and $tau$ _n representingamplitude and time constant,respectively.

Statistical analysis. For statistical analysis, the two-tailed paired t test was applied. Populations were regarded as significantlydifferent if p was <0.05. Data are expressed as means ±SEM.

Histological procedures. Biocytin labeling and light-microscopic morphological analysis were performed as described previously(Szinyei et al., 2000). Briefly, 1% biocytin was added to theintracellular solution. After recording, slices were immersedin 4% paraformaldehyde in PBS. After cryoprotection with a 30%sucrose solution in PBS, slices were resectioned at 100 µm usinga freeze microtome (Leica, Benzheim, Germany). Sections were treatedwith avidin-biotin complex horseradish peroxidase (PK 4000, 1:100;Vector Laboratories, Burlingame, CA) and then treated with (NH₄)₂Ni(SO₄)₂.Finally, sections were dehydrated andcoverslipped.

Immunohistochemistry and in situhybridization. The expression of NR2B subunits on GABA-immunoreactive cells of the LA wasdemonstrated with double-immunohistochemistry and combined insitu hybridization/immunohistochemistry double-labeling. For bothmethods, slices of the LA and adjacent areas after recording werefixed in 4% paraformaldehyde and 0.05% glutaraldehyde overnight.Cryoprotection was done with 30% sucrose, and coronal sectionsof 20 and 40 µm thickness were cut on a freezemicrotome.

Double-immunohistochemistry was performed on 40-µm-thick sections with a free-floating method. After washing in PBS bufferand blocking of unspecific binding with a solution of 10% goatnormal serum, 2% BSA, and 0.3% Triton X-100 in PBS, sections wereincubated overnight with a polyclonal anti-NR2B antibody (Chemicon,Temecula, CA) diluted 1:500 in the blocking solution. After washingin PBS, primary antibodies were detected with biotinylated secondaryantibodies and Cy3-streptavidin complex according to the manufacturer'sprotocol (Sigma). Subsequently, GABA was detected with a monoclonalantibody (Sigma) diluted 1:400 in blocking solution. After overnightincubation and washing in PBS, signals were visualized with Alexagoat anti-mouse fluorescent antibody (obtained from MolecularProbes, Eugene, OR) diluted 1:300 in 0.2% Triton X-100 in PBS.Stained sections were washed, embedded with medium Immu-Mount(Shandon-Lipshaw, Pittsburgh, PA), and coverslipped. Negativecontrols were prepared in parallel experiments with the omissionof anti-NR2B or anti-GABA primaryantibodies.

For in situ hybridization/immunohistochemistry double-labeling, 20-µm-thick sections were cut and thaw-mounted onto silane-coatedslide glasses. After overnight permeabilization with 0.3% TritonX-100 and subsequent quenching of endogenous peroxidase activitywith 0.3% H₂O₂, GABA-immunoreactive cells were detected by immunohistochemistry.Unspecific binding was blocked with 10% normal serum and 2% BSAin PBS, and GABA was detected with a polyclonal antibody fromSigma at a dilution of 1:1000 in blocking solution. Labeling wasdetected using the ABC method (Vectastain) and 3-amino-9-ethylcarbazolechromogen (Sigma), according to the manufacturers' protocols.After development of the GABA staining, sections were immediatelyprocessed for in situ hybridization (Stork et al., 2001). In brief,sections were acetylated, prehybridized for 2 hr at 37°C, andhybridized overnight at 42°C with a digoxigenin-labeled cRNA probegenerated from a 299 bp fragment of the NR2B coding region (3338-3636bp according to sequence NM  008171). Stringency washing was doneat 50°C with 0.1% SSC and 50% formamide as the final concentration,and labeled cells were detected with alkaline-phosphatase-coupledantidigoxigenin antibodies using nitroblue tetrazolium chlorideand 5-bromo-4-chloro-3-indolyl phosphate (Roche Molecular Biochemicals,Mannheim, Germany) as substrate. Staining intensity was optimizedfor double-labeling of LA GABAergic cells. Sections were coveredwith Crystal Mount and embedded in Permount. An Axioplan microscopewith digital image analysis (Metamorph; Visitron, Puchheim, Germany)was used for visualization of these immunohistochemicalpreparations.

  Results

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

NMDA receptor-mediated contribution to synaptic transmission in LA interneurons

Data result from recordings in a total of 83 interneurons in the LA that were identified based on intrinsic membrane properties,firing patterns, and morphological features. Neurons were consideredfor additional analysis if they showed maintained action potentialfiring with little or no spike frequency adaptation during +0.1 $-$ +0.4 nA current injection from the resting membrane potential(Fig. 1Aa). The resting membrane potential, input resistance asmeasured from the steady-state voltage response during a $-$ 50 pAcurrent injection from rest, action potential duration at half-maximalamplitude, and steady-state firing frequency at +0.4 nA currentinjection were $-$ 69.4 ± 1.8 mV, 291 ± 13 M $Omega$ , 0.7 ± 0.02 msec, and80.3 ± 4.2 Hz, respectively (n = 83). In addition, the initialcomponent of hyperpolarizing afterpotentials after an action potentialdisplayed a rapid time course of deactivation, thereby imposinga concave trajectory to the overall form of afterhyperpolarizations(data not shown). Time-dependent inward rectification in the hyperpolarizingdirection was not pronounced. These properties were similar tothose reported previously for interneurons in the LA (Mahantyand Sah, 1998; Szinyei et al., 2000); therefore, we refer to themas such. The intrinsic properties of interneurons were significantlydifferent from those of putative projection cells recorded duringthe course of the present study (n = 17; resting input resistance,186 ± 12 M $Omega$ ; action potential duration at half-maximal amplitude,1.22 ± 0.06 msec; steady-state firing frequency, 19.3 ± 1.4 Hz).Resting membrane potential in projection cells ( $-$ 70 ± 0.9 mV)was not different from that of interneurons. The injection ofbiocytin and subsequent histological processing revealed thatall histologically recovered cells (n = 63) that had been classifiedas interneurons based on electrophysiological criteria possesseddendrites bearing no spines (Fig. 1Ab), thereby corroboratingthat they represent GABAergic interneurons (McDonald, 1982).

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Figure 1. Identification of NMDA receptor-mediated components of EPSPs evoked through stimulation of cortical and thalamic afferent fibers in LA interneurons. A, Electrophysiological (a) and morphological (b) characteristics of a putative interneuron in the LA. Voltage traces (a) represent responses to depolarizing and hyperpolarizing direct current injections (+0.3, $-$ 0.1 nA; current traces not shown). Note the tonic series of action potentials with no apparent frequency adaptation. Staining of the same neuron with biocytin (b) reveals nonspiny dendrites; the region within the white frame is shown at a higher magnification. Scale bar, 100 µm (corresponding to 25 µm in the magnified region). B, EPSPs in an interneuron evoked through single shocks (0.5 mA, 100 µsec) of cortical and thalamic input fibers before (control) and after the application of APV (50 µM). C, Responses to repetitive stimulation (2 Hz) of cortical and thalamic pathways, before and after the application of APV (50 µM). Difference as calculated from graphical subtraction of the APV signal from the control shows the APV-sensitive component. Average represents the average of subtractions from nine interneurons. D, Average of EPSP integrals after APV treatment with respect to controls at the cortical (open columns) and thalamic (closed columns) pathway for 0.05 (a) and 2 Hz (b) afferent stimulation.

The contribution of NMDA receptor-mediated signals was investigated by stimulating the cortical and thalamic fibers with singleshocks at 0.05 Hz and repetitive shocks at 2 Hz and applying APV(50 µM) after a stable baseline of EPSP subthreshold to spikegeneration had been obtained. As is evident from the examples(Fig. 1B,C) and averages calculated from integrals of voltageresponses to single and repetitive stimulation (Fig. 1D), APVdepressed EPSPs at the cortical and thalamic inputs. The amplitudeof cortical and thalamic EPSPs was reduced from 17.9 ± 1.6 and21.6 ± 2.3 mV to 15.5 ± 1.5 and 18.5 ± 2 mV after the applicationof NMDA receptor antagonist, respectively, corresponding to areduction to 85.7 ± 2.1% and 85.6 ± 2.2% of the control value.Calculation of the integrals of EPSPs obtained with single shocksrevealed a significant reduction to 75.2 ± 4.2 and 78.7 ± 4.4%of the control values for cortical and thalamic pathways, respectively(Fig. 1Da) (n = 12). The integrals of EPSPs evoked at 2 Hz werereduced to 69.6 ± 4.2 and 79 ± 4.1%, respectively (Fig. 1Db) (n= 9). The effects of APV at thalamic and cortical pathways weresimilar for stimulation at 0.05 Hz and reached a small but significantdifference (p = 0.016) for stimulation at 2Hz.

Furthermore, the application of DNQX (10 µM) substantially reduced but failed to completely block EPSPs evoked from restingmembrane potential at both thalamic and cortical inputs. Indeed,increasing the stimulation strength under these conditions resultedin a substantial increase in the amplitude of the DNQX-insensitiveresponse components at both input pathways, which were sensitiveto the application of the NMDA receptor antagonist APV (50 µM)(n = 6; data notshown).

These findings indicate that NMDA receptors are functional in LA interneurons, in that they contribute a significant componentto excitatory synaptic responses evoked from resting potentialthrough the activity of the two major sensory input systems. Theproperties of the NMDA receptor-mediated signals were investigatedduring pharmacological isolation using voltage-clamp techniquesin the next experimentalstep.

Voltage dependence of NMDA receptor-mediated EPSCs

Under voltage-clamp conditions, afferent stimulation at different membrane potentials ranging from $-$ 90 to +50 mV revealedEPSCs in interneurons. To pharmacologically isolate NMDA receptor-mediatedactivity, GABA_A and GABA_B receptor-mediated inhibition and AMPAreceptor-mediated excitation were blocked with picrotoxin (100µM), CGP55485 (10 µM), and DNQX (10 µM), respectively, and theconcentration of Mg²⁺ was reduced to 0.1 mM. Under these conditions, maximal EPSC amplitudesof $-$ 765 ± 140 and $-$ 651 ± 130 pA were measured at $-$ 50 mV at thecortical and the thalamic input, respectively (n = 11) (Fig. 2).These EPSCs were sensitive to the application of APV in all testedcells (n = 5; data not shown) and are therefore considered tobe NMDA receptor-mediated synaptic responses. For the constructionof I-V curves, EPSC amplitudes obtained at different holding potentialswere normalized in individual cells with respect to the amplitudeat $-$ 50 mV in 0.1 mM MgCl₂. The normalized and averaged I-V curveobtained from measurements in 11 cells displayed a range of negativeslope conductance between $-$ 90 and $-$ 60 mV and an apparent reversalpotential at 12.8 ± 1.8 and 12.7 ± 1.7 mV for cortical and thalamicEPSCs, respectively (n = 11). There was no significant differencein the I-V relationship of EPSCs associated with the two inputs(Fig. 2). The application of a bathing solution containing 2 mMMg²⁺ led to a voltage-dependent blockade of the EPSCs, with responsesbeing blocked negative to approximately $-$ 50 mV (n = 6) (Fig. 2).The apparent reversal potential was not affected (12.5 ± 1.9 and12.6 ± 1.9 mV for cortical and thalamic afferents, respectively).Furthermore, I-V curves of EPSCs under these conditions did notreveal differences between cortical and thalamic inputs.

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Figure 2. Mg²⁺-sensitive voltage dependence of pharmacologically isolated NMDA receptor-mediated EPSCs in interneurons. All recordings were obtained during the presence of picrotoxin (100 µM), CGP55485 (10 µM), and DNQX (10 µM). In each interneuron, responses were evoked on stimulation of cortical (open symbols) and thalamic (closed symbols) afferents and were compared in bathing solutions containing 0.1 (circles) and 2 (squares) mM Mg²⁺. The holding potential varied in the range $-$ 90 to +50 mV. For the construction of I-V relationships, EPSCs were normalized with respect to the EPSC amplitude at $-$ 50 mV in 0.1 mM Mg²⁺, and responses were averaged from recordings in 11 interneurons. Traces represent original recordings from one interneuron under experimental conditions as indicated. Stimulus artifacts have been removed for clarity.

Contribution of NR2B subunits

To evaluate the possible contribution of NR2B subunits, ifenprodil was used. NR1/NR2B receptor complexes are several-hundred-foldmore sensitive to ifenprodil than are NR1/NR2A receptors, andifenprodil at 10 µM has been reported to near-maximally blockthe NR2B receptor subtype with no substantial effect on the NR2Asubtype (Williams, 1993). In the following experiments, NMDA receptor-mediatedresponses in LA interneurons were pharmacologically isolated asbefore. The application of ifenprodil at 10 µM reduced the NMDAreceptor-mediated EPSPs in all interneurons that were tested (n= 6) (Fig. 3Aa). Inhibition reached a steady-state level ~20 minafter application, corresponding to a reduction of EPSPs to 44.8± 5.4 and 47.9 ± 5.7% of the predrug values at the cortical andthalamic inputs, respectively. Significant differences betweenthe cortical and thalamic input systems with respect to the actionof ifenprodil in interneurons were not observed. In contrast,ifenprodil (10 µM) had no significant effect on DNQX-sensitiveAMPA receptor-mediated EPSCs, which were recorded during the continuouspresence of APV (50 µM) in interneurons held at membrane potentialsclose to the presumed C1 equilibrium potential ( $-$ 75 mV) to minimize the contribution ofGABA_A receptor-mediated synaptic currents (n = 4) (Fig. 3Ab).The AMPA EPSC amplitudes recorded 15 min after the applicationof ifenprodil averaged to 95.7 ± 4.8 and 103.7 ± 5.4% with respectto control values before drug application for the cortical andthalamic pathways, respectively.

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Figure 3. Effects of the NR2B antagonist ifenprodil on NMDA receptor-mediated synaptic responses in interneurons. Aa, Time course of ifenprodil action on NMDA receptor-mediated EPSPs obtained on stimulation of cortical (open symbols) and thalamic (closed symbols) input fibers (n = 6). Responses were obtained at resting potential, during the presence of picrotoxin (100 µM), CGP55485 (10 µM), and DNQX (10 µM). EPSP amplitudes were normalized with respect to baseline values before application, separately for each pathway in each neuron. The bar indicates application of the drug. Traces represent original recordings from one interneuron before and during the maximal action of ifenprodil. Stimulus artifacts were removed for clarity. b, Lack of effect of ifenprodil on AMPA receptor-mediated EPSCs. Examples of cortically and thalamically evoked EPSCs in an LA interneuron obtained during the continuous presence of APV (50 µM), before and 15 min after the application of ifenprodil (10 µM) are shown. The cell was held at $-$ 75 mV. B, Decay kinetics of NMDA receptor-mediated EPSCs. a, Time course of decay of NMDA receptor-mediated EPSCs obtained on stimulation of cortical (left column) and thalamic (right column) afferents in an interneuron before (control) and during maximal action of ifenprodil (at 10 µM) is described by a two exponential function (lines below original traces). b, Fast and slow time constants ( $tau$ ) of EPSC decay, at cortical and thalamic inputs, averaged from recordings in seven interneurons. c, Relative contribution of the fast and slow components to EPSCs before (control) and during the maximal action of ifenprodil (10 µM). Fast and slow components were calculated as A1 and A2 from the equation in Materials and Methods, and the overall amplitudes of EPSCs during ifenprodil (ifenpr.) were normalized with respect to control values. Recordings were obtained during the presence of picrotoxin (100 µM), CGP55485 (10 µM), and DNQX (10 µM).

In various types of cells, synapses with a high NR2B content have been observed to contribute a slow component to the synapticNMDA current, with time constants of decay typically exceeding200 msec (Chen et al., 1999; Lei and McBain, 2002). Therefore,in a subsequent experimental step, the time course of decay ofNMDA currents and the effects of ifenprodil were analyzed in LAinterneurons (n = 7). The time constant of decay of EPSCs wasfitted best by a double-exponential function (Fig. 3Ba) (r > 0.96)at both input pathways, with the two time constants averaging72 ± 6 and 60 ± 5 msec and 423 ± 63 and 285 ± 40 msec at corticaland thalamic inputs, respectively (n = 7) (Fig. 3Bb). The contributionof the fast and the slow components to the total EPSC was 59 ±7.5 and 41 ± 7.5% for the cortical input and 61.8 ± 6.8 and 38.2± 6.8% for the thalamic input (Fig. 3Bc). Differences betweenthe two input pathways were not significant. The application ofifenprodil similarly affected the two components of NMDA receptor-mediatedEPSCs. With ifenprodil, the NMDA receptor-mediated EPSCs werereduced to 30.1 ± 3.7 and 27.2 ± 3.6% of the control value atcortical and thalamic inputs, respectively. The relative contributionof the two components to the overall EPSC remained unchanged (fastcomponent, 60.5 ± 6.4 and 53.7 ± 11.7%; slow component, 39.5 ±6.4 and 46.3 ± 11.7% at the cortical and the thalamic pathway;p = 0.892, cortical; p = 0.475, thalamic) (Fig. 3Bc).

It is noteworthy that significant effects of ifenprodil were also observed on NMDA receptor-mediated EPSPs (n = 3) and EPSCs(n = 5) in a sample of projection neurons recorded during thecourse of the present study, thereby corroborating and extendingrecent findings on the functional importance of NR2B receptorsin this class of LA neurons (Bauer et al., 2002). Interestingly,ifenprodil differentially affected the fast and slow componentsof NMDA currents in projection neurons (n = 5). Under controlconditions, the decay time constants of NMDA currents were fittedbest by a double-exponential function, with the fast and slowcomponents averaging 70 ± 7 and 401 ± 70 msec (cortical input)and 63 ± 9 and 406 ± 41 msec (thalamic input) and contributing50.2 ± 6.3 and 49.8 ± 6.3% (cortical) and 66.8 ± 1.8 and 33.2± 1.8% (thalamic) to the total EPSC. The application of ifenprodilreduced the NMDA EPSCs to 34.5 ± 6.6% (cortical input) and 45± 2.3% (thalamic input) of the control value. The effects of ifenprodilwere significantly larger on the slow compared with the fast component(p = 0.011, cortical; p = 0.035, thalamic), in that (at corticaland thalamic inputs) the fast component contributed 79.1 ± 3.5and 73.2 ± 2%, whereas the slow component contributed 20.9 ± 3.5and 26.8 ± 2% to the residualcurrent.

Expression of NR2B subunits in LA GABA neurons

The expression of NR2B subunits on GABA-immunoreactive neurons of the LA was demonstrated through double-immunohistochemical-labelingand immunohistochemistry/in situ hybridization double-labeling.GABA-immunoreactive neurons were found scattered throughout theslice in cortical and subcortical areas, including the LA (Fig.4Aa). NR2B subunits were widely expressed in these brain areas,and double-immunohistochemical-labeling revealed a colocalizationof NR2B subunits with literally all GABA-immunoreactive cellsin the LA (Fig. 4Ab), in addition to their expression on a largenumber of GABA-negative cells (Fig. 4Ab).

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Figure 4. Expression of NR2B subunit in LA neurons, demonstrated through double-labeling immunohistochemistry (A) and combined in situ hybridization/immunohistochemistry (B). Aa, Green fluorescence in the cell body and proximal dendrites depicts a GABA-immunoreactive interneuron (arrow). Ab, Red fluorescence indicates the localization of NR2B subunits on the same neuron (arrow). Other NR2B-immunoreactive cells are GABA negative and most likely represent projection neurons (arrowheads). B, Red staining indicates GABA-immunoreactive neurons in the LA, some of which are colabeled (red arrows in a and b) for NR2B mRNA (brown reaction product). NR2B mRNA expression is also evident in a number of GABA-negative cells (black arrow in b). Examples of NR2B-negative GABA-immunoreactive cells are indicated by the red arrowheads in b and c. Scale bars, 20 µm.

To validate these immunohistochemical findings further and to confirm that GABA and NR2B subunits were coexpressed in LA neurons,an immunohistochemical labeling of GABA was combined with in situhybridization for NR2B. NR2B mRNA was found to be widely expressedin non-GABAergic cells in the amygdaloid and neocortical structuresof the slice. In addition, a large number of GABA-immunoreactivecell bodies were positive for NR2B mRNA (Fig. 4Ba,b), althoughGABA-immunoreactive NR2B-negative neurons could also be found(Fig. 4Bc). The size and shape of double-labeled cells were reminiscentof the heterogeneous group of class II neurons, which are thoughtto represent the majority of GABAergic interneurons in the LA(McDonald, 1985). Strongly GABA-immunoreactive small perikaryathat may resemble GABAergic class III neurons (McDonald, 1985)could also be found. These were always negative for NR2B, butdetection of NR2B mRNA in such neurogliaform cells may well havebeen prevented by their intense GABA labeling. Occasionally, weaklyGABA-immunoreactive pyramid-shaped neurons were found in the LA;however, the majority of pyramidal cells remained GABA negativeeven after extensive overdevelopment of the staining. In a representativesample of slices (n = 4), 78% of the GABA-immunoreactive neurons(i.e., 193 of a total of 246) were also positive for NR2B, asrevealed through double-immunohistochemical-labeling or immunohistochemistrycombined with in situ hybridization. The actual proportion ofdouble-labeled cells may be even higher, because in some cellsthe immunohistochemical reaction product may have been coveredafter the development of in situhybridization.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The present study was undertaken to elucidate further the functional role of NMDA receptors in synaptic transmission in theLA, with particular emphasis on interneurons and NR2B subunits.The data of the present study indicate the following: (1) NMDAreceptor-mediated responses contribute to basal synaptic transmissionin putative interneurons of the rat LA. (2) NMDA receptor-mediatedcurrents in interneurons display Mg²⁺-dependent voltage dependence. (3) NMDA currents evoked on stimulationof cortical and thalamic inputs to interneurons were not significantlydifferent. (4) Both GABA-immunopositive and GABA-immunonegativeneurons in the rat LA express the NR2B receptor protein. (5) NR2Bsubunits contribute to NMDA receptor-mediated responses associatedwith thalamic and cortical input fibers in both interneurons andprojectionneurons.

NMDA receptor-mediated synaptic responses at cortical and thalamic inputs in interneurons

There is some evidence suggesting that NMDA receptor-mediated excitatory responses exist in interneurons of different brainregions, but these findings are controversial. For instance inthe rat neocortex, interneurons apparently lack NMDA receptor-mediatedresponses (Ling and Benardo, 1995), although evidence for theexistence of NMDA receptors has also been provided (Thomson, 1997).Entorhinal cortical (Jones and Buhl, 1993), thalamic (Pape andMcCormick, 1995; Williams et al., 1996), and hippocampal interneurons(Sah et al., 1990; Morin et al., 1996; Lei and McBain, 2002),however, were shown to possess functional NMDA receptors, althoughsome hippocampal interneuronal populations seem to lack NMDA receptor-mediatedsignals (Sah et al., 1990). In interneurons of the rat lateraland basolateral amygdala, the stimulation of cortical afferentshas been reported to lead to AMPA receptor-mediated responses,with only a minimal or negligible contribution from NMDA receptors(Mahanty and Sah, 1998). However, the results of the present studydemonstrate that activation of NMDA receptors significantly contributesto the glutamatergic response obtained at resting potential inLA interneurons. This contribution of NMDA receptors was observedafter the stimulation of cortical and thalamic input fibers, andmost likely reflects a direct effect of thalamic and corticalfibers acting on postsynaptic NMDA receptors in the interneuronsunder study: (1) Mg²⁺-sensitive voltage dependence of postsynaptic currents typicalof NMDA-mediated currents was apparent when the membrane potentialof the recorded interneurons was changed. This could not be expectedif the mediating NMDA receptors were located at presynaptic sites.(2) Application of APV had no consistent effect on the amplitudeof the postsynaptic response at hyperpolarized levels of the membranepotential. (3) Pharmacologically isolated NMDA currents typicallydisplayed a smoothly rising phase and constant latency, and thekinetics was similar to those observed in other central neurons(Lei and McBain, 2002), thereby suggesting that they representmonosynaptic responses. (4) Substantially higher stimulus intensitieswere needed to evoke EPSPs (and spike firing) in projection cellsthan in interneurons, making it unlikely that EPSPs obtained ata given stimulus strength in interneurons predominantly representfeedback effects via axon collaterals of projection cells. (5)Evidence for the existence of NR2B receptor subunits on GABA-immunoreactiveneurons in the LA was obtained on the mRNA and protein level.In particular, a considerable proportion of GABA-immunoreactiveclass II neurons in the LA appear to expressNR2B.

These results add to our previous findings of functional NMDA receptors in interneurons of the rat LA (Danober et al., 2000)the notion that these receptors contribute to basal synaptic transmissionat both the thalamic and the cortical input system. However, itcannot be deduced from available data whether NMDA and AMPA receptorsubunits are colocalized at the same synapse in interneurons,as has been found for projection neurons of the basolateral amygdala(Farb et al., 1995; Smith and Dudek, 1996).

Experiments performed in Sprague Dawley rats at postnatal days 21-35 indicated that distinct populations of NMDA receptorscontribute to synaptic transmission in LA projection neurons atcortical and thalamic inputs, in that the fractional contributionof NMDA receptors was higher and NMDA responses were more sensitiveto Mg²⁺ at thalamic compared with cortical input synapses (Weisskopfand LeDoux, 1999). A similar study performed in Wistar rats ata slightly younger age (postnatal days 17-25) found no indicationfor differences of NMDA receptor-mediated responses at the twomajor input systems to LA projection neurons (Mahanty and Sah,1999). In LA interneurons recorded in the present study, NMDAreceptors contributed to the evoked synaptic responses at thalamicand cortical inputs. Furthermore, the properties of NMDA currentsappeared similar at the two input systems, with respect to Mg²⁺-sensitive voltage dependence, kinetics, and pharmacological properties(indicating the contribution of NR2B subunits; see below). However,it should be kept in mind that NMDA receptor-mediated events werestudied at the level of evoked synaptic responses, and that thepossibility cannot be excluded that differences between the twoafferent input pathways exist at the level of the unitary and/orquantal events (Gil et al., 1999). In any case, the conclusionis that NMDA receptor-mediated responses do exist in LA interneuronsat thalamic and cortical synaptic inputs, which is in line withour previous hypothesis that these two major afferent systemsto LA interneurons are rather symmetrically organized in functionalterms (Szinyei et al., 2000).

Role of NR2B receptor subunits

Native NMDA receptors are formed by the heteromeric expression of the NR1 subunit with one type or a combination of NR2 subunits(for review, see Dingledine et al., 1999). While the NR1 subunitis required for the ion-channel pore, the NR2 subunits are importantelements in the determination of the unique properties of theNMDA receptors, including unitary conductance, ligand-bindingaffinity, and kinetics of gating, desensitization, and deactivation.In particular, NMDA receptor-mediated currents at synapses bearinga high number of NR2B subunits have been shown to possess relativelyslow decay kinetics compared with synapse-expression NR2A subunits(Monyer et al., 1994; Flint et al., 1997; Chen et al., 1999).In LA interneurons, the decay of the NMDA receptor-mediated currentswas described best by a two exponential function, with the fastand the slow component contributing approximately equally to theoverall current. The slow component with a time constant of >200msec is indicative of synapses with a high NR2B content, as evidencedfrom observations in various cell types (Chen et al., 1999; Leiand McBain, 2002). Indeed, ifenprodil at a concentration thatis considered selective for the NR2B receptor subtype (Williams,1993) significantly reduced the evoked NMDA current in LA interneurons.It is noteworthy that in LA interneurons, fast- and slow-decayingcomponents were similarly reduced by ifenprodil, whereas in thesample of projection neurons, the slow component was predominantlyaffected. This may indicate a difference in the kinetics of NR2B-mediatedcurrents between interneurons and principal cells, similar tothe difference reported for AMPA receptor-mediated EPSCs (Mahantyand Sah, 1998). Interestingly, in developing mouse hippocampalneurons, NMDA components displaying fast versus slow decay kineticswere also found to be equally sensitive to ifenprodil (Kirsonand Yaari, 1996).

The existence of NR2B subunits in both types of LA neurons is corroborated by the results of the combined immunohistochemicaland in situ hybridization experiments. These clearly demonstratedNR2B expression at the cell surface and NR2B mRNA in the perikaryaof GABA-immunoreactive neurons in the LA. GABA immunoreactivityin the LA closely matches the expression pattern of glutamic aciddecarboxylase and appears to be specific for class II and classIII interneurons (McDonald, 1985). Most double-labeled cells,according to their form and size, in fact appeared to be classII neurons (Fig. 4Ba,b). We also found some weakly GABA-labeledpyramidal-shaped cells (Fig. 4Bb), but it was not possible todecide whether these were class I or class II neurons. However,because overdevelopment of the GABA staining did not produce anyadditional labeling in the LA, it appears that the low levelsof metabolic GABA that may be present in its principle neuronshave remained below the detectionlimit.

In various systems, the subunit composition of NMDA receptors is developmentally regulated in that the NR2B subunits tendto be highly expressed at early postnatal stages and are progressivelyreplaced by NR2A subunits during development (Monyer et al., 1994;Flint et al., 1997; Cathala et al., 2000). However, significantnumbers of NMDA receptors with a high level of NR2B compositionalso seem to exist at mature stages, as deduced from recordingsin rat hippocampal interneurons at late postnatal age (later thanpostnatal day 30) (Lei and McBain, 2002). The findings in thepresent study (performed at postnatal days 21-18) are in linewith those observations and suggest that NMDA receptors with ahigh content of NR2B subunits play a role at cortical and thalamicsynapses in interneurons as well as in projection neurons of theLA.

The slow decay kinetics of the NMDA currents with high NR2B content is considered an important element to promote Ca²⁺ entry and induction of synaptic plasticity (Chen et al., 1999).The specific functional importance of NR2B subunits in the amygdalais demonstrated by the recent finding that intra-amygdala infusionof ifenprodil disrupted the acquisition but not the expressionof fear conditioning (Rodrigues et al., 2001). In line with thisis the observation that the application of ifenprodil blockedlong-term potentiation at thalamic input pathways to projectionneurons in vitro (Bauer et al., 2002). Synaptic responses to singleafferent stimuli were found to be reduced by APV but not ifenprodilin that study, which seems to be in contrast to the present findingthat NR2B receptor subtypes contribute to isolated NMDA responsesevoked from a membrane potential close to the resting value. Theunderlying reasons remain unknown, but may relate to the differenttypes of recorded cells or the experimental conditions in thetwo studies [recording of mixed EPSPs (Bauer et al., 2002) vsrecording of isolated NMDA EPSPs/EPSCs (present study)]. In anycase, the results of the present study indicate that synapsesto both projection neurons and interneurons are potential substratesfor NR2B-mediated influences on plastic changes related to fearconditioning. Moreover, the colocalization of NMDA/NR2B and Ca²⁺-permeable AMPA receptors (Mahanty and Sah, 1999) at corticalinputs to LA interneurons could provide multiple routes for Ca²⁺ entry, with an impact on synaptic transmission and plasticity.Overall, our results also support the view that signal processingin amygdaloid synaptic circuits is under the critical controlof GABAergic mechanisms (Lang and Paré, 1997, 1998; Danober andPape, 1998; Szinyei et al., 2000; Stork et al., 2002).

  FOOTNOTES

Received Oct. 10, 2002; revised Dec. 16, 2002; accepted Jan. 7, 2003.

This work was supported by the Deutsche Forschungsgemeinschaft (SFB 426, TP B3) and by the Kultusministerium des Landes Sachsen-Anhalt.We thank R. Ziegler, A. Reupsch, and M. Schmidt for expert technicalassistance.

Correspondence should be addressed to Hans-Christian Pape, Institute for Physiology, Medical School, Otto-von-Guericke University,Leipzigerstrasse 44, 39120 Magdeburg, Germany. E-mail: hans-christian.pape{at}medizin.uni-magdeburg.de.

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Discussion
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