Synaptic Plasticity in the Amygdala in a Model of Arthritic Pain: Differential Roles of Metabotropic Glutamate Receptors 1 and 5

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The Journal of Neuroscience, January 1, 2003, 23(1):52-63

Synaptic Plasticity in the Amygdala in a Model of Arthritic Pain: Differential Roles of Metabotropic Glutamate Receptors 1 and 5
Volker Neugebauer¹, Weidong Li¹, Gary C. Bird¹, Gautam Bhave², and Robert W. Gereau IV²
¹ Department of Anatomy and Neurosciences and Marine Biomedical Institute, The University of Texas Medical Branch, Galveston, Texas 77555-1069, and ² Division of Neuroscience, Baylor College of Medicine, Houston, Texas 77030

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Pain has a strong emotional-affective dimension, and the amygdala plays a key role in emotionality. Mechanisms of pain-relatedchanges in the amygdala were studied at the cellular and molecularlevels in a model of arthritis pain. The influence of the arthriticcondition induced in vivo on synaptic transmission and group Imetabotropic glutamate receptor (mGluR1 and mGluR5) function wasexamined in vitro using whole-cell voltage-clamp recordings ofneurons in the central nucleus of the amygdala (CeA). G-protein-coupledmGluRs are implicated in various forms of neuroplasticity as wellas in neurological and psychiatric disorders. Synaptic transmissionwas evoked by electrical stimulation of afferents from the basolateralamygdala (BLA) and the pontine parabrachial (PB) area in brainslices from control (untreated or saline-injected) rats and fromarthritic rats. This study shows enhanced synaptic transmissionof nociceptive-specific inputs (PB $right-arrow$ CeA synapse) and polymodalsensory inputs (BLA $right-arrow$ CeA synapse) in the arthritis model. CeA neuronsfrom arthritic rats also developed increased excitability comparedwith control CeA neurons. Synaptic plasticity in the CeA was accompaniedby increased presynaptic mGluR1 function and upregulation of mGluR1and mGluR5. A selective mGluR1 antagonist reduced transmissionin CeA neurons from arthritic animals but not in control neurons,and increased levels of mGluR1 and mGluR5 protein were measuredin the CeA of arthritic rats compared with controls. Our resultsshow that plastic changes in the amygdala in an arthritis modelthat produces prolonged pain involve a critical switch of presynapticmGluR1 expression andfunction.

Key words: amygdala; arthritis pain; electrophysiology; metabotropic glutamate receptors; nociception; patch-clamp; plasticity; synaptic transmission

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The amygdala plays a key role in the emotional-affective aspects of behavior, the emotional evaluation of sensory stimuli,emotional learning and memory, and related disorders (Davis, 1998;Cahill, 1999; Davidson et al., 1999; Gallagher and Schoenbaum,1999; Maren, 1999; Aggleton, 2000; LeDoux, 2000; Rasia-Filho etal., 2000). The amygdala is also implicated in the emotional-affectivecomponent of pain (Bernard and Bandler, 1998; Manning et al.,2001; Schneider et al., 2001; Neugebauer and Li, 2002).

The amygdala exhibits a high degree of plasticity in models of tetanic, pharmacologically induced, and behavioral long-termmodification of synaptic transmission (McKernan and Shinnick-Gallagher,1997; Neugebauer et al., 1997a, 2000; Maren, 1999; Wang and Gean,1999; LeDoux, 2000; Martin et al., 2000; Bauer et al., 2001; Blairet al., 2001; Lin et al., 2001). Such neuroplasticity is believedto be involved in associative learning and in certain neurologicaland psychiatricdisorders.

The amygdala receives purely nociceptive information through the spino-parabrachio-amygdaloid pain pathway, which connectsthe pontine parabrachial area and spinal cord with the centralnucleus of the amygdala (CeA) (Bernard et al., 1993; Jasmin etal., 1997; Buritova et al., 1998) (see Fig. 1). Polymodal sensory,including nociceptive, information reaches the amygdala from thalamicand cortical areas through connections with the lateral and basolateralamygdaloid nuclei, which then project to the CeA, the output nucleusfor major amygdala functions (Pitkanen et al., 1997; Doron andLeDoux, 1999; Linke et al., 1999; Shi and Davis, 1999; LeDoux,2000; Smith et al., 2000) (see Fig. 1).

Accumulating evidence implicates the amygdala in pain processing and modulation. Electrical stimulation of the amygdala elicitsvocalizations that are accompanied by emotional reactions in monkeys(Jurgens et al., 1967; Jurgens, 1982). Lesions or temporary inactivationof the amygdala decrease higher integrated emotional pain responseswithout affecting normal behavior or baseline nociceptive responses(Charpentier, 1967; Calvino et al., 1982; Helmstetter, 1992; Maieret al., 1993; Fox and Sorenson, 1994; Watkins et al., 1998; Borszcz,1999; Tershner and Helmstetter, 2000). Single-unit recordingsin anesthetized rats defined the capsular division of the CeAas the "nociceptive amygdala," because the vast majority of theseneurons respond exclusively or preferentially to painful stimuli(Bernard et al., 1992; Neugebauer and Li, 2002).

The role of the amygdala in prolonged, and chronic pain is mostly unknown. This study is the first to address cellular andmolecular mechanisms of synaptic plasticity in the amygdala ina well established model of arthritic pain arising from a localizedinflammation of one knee joint (Neugebauer et al., 1993, 1994,1995, 1996). We focus on group I metabotropic glutamate receptors(mGluRs), which are involved in neuroplasticity associated withnormal brain functions as well as in neurological and psychiatricdisorders (Fundytus, 2001; Neugebauer, 2001a, 2002). Group I mGluRscomprise mGluR1 and mGluR5 subtypes. These couple through G_q/11-proteinsto the activation of phospholipase C and protein kinase C, andthey also regulate various other signal transduction pathways.Accumulating evidence suggests an important role of mGluRs inpain processing (Fundytus, 2001; Karim et al., 2001; Neugebauer,2001a,b; Neugebauer, 2002; Neugebauer and Carlton, 2002; Varneyand Gereau, 2002).

  Materials and Methods

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Electrophysiological and biochemical data were obtained from control rats (untreated normal rats and saline-injected "sham"rats) and rats with monoarthritis (6-8 hr after induction). MaleSprague Dawley rats (110-250 gm) were individually housed in standardplastic boxes (40 × 20 cm) in a temperature-controlled room andmaintained on a 12 hr day/night cycle. Standard laboratory chowand tap water were available ad libitum. On the day of the experiment,rats were transferred from the animal facility and allowed toacclimate to the laboratory for at least 1hr.

Arthritis pain model
In one group of rats ("arthritis"), arthritis was induced in one knee joint as described in detail previously (Neugebaueret al., 1989, 1993, 1994, 1995, 1996; Neugebauer and Schaible,1990). A kaolin suspension (4%, 80-100 µl) was slowly injectedinto the joint cavity through the patellar ligament with a syringeand needle (1 ml, 25G5/8). After repetitive flexions and extensionsof the knee for 15 min, a carrageenan solution (2%, 80-100 µl)was injected into the knee joint cavity, and the leg was flexedand extended for another 5 min. This treatment paradigm reliablyleads to localized inflammation and swelling of the injected kneewithin 1-3 hr. The inflammation persists for up to 2 weeks. Itdoes not spread systemically (Neugebauer et al., 1989, 1993, 1994,1995, 1996; Neugebauer and Schaible, 1990; Min et al., 2001).
Another group of rats ("shams") received injections of a sterile physiological saline solution into one knee joint similarto the kaolin and carrageenan injections of the arthritis group.The knee joint was rhythmically flexed and extended as in thearthritis group (see above). The intra-articular saline injectioncaused a temporary swelling of the knee joint, which did not persistbeyond 2 hr afterinjection.
The third group of rats ("normal") did not receive any injections but was kept under the same conditions as the arthritisand sham rats before brain slices were obtained for electrophysiologicaland molecularstudies.

Behavioral tests
Evoked and spontaneous pain-related behavior was tested in rats from which brain slices were obtained for electrophysiologyand Western blot analysis. Behavioral data were measured in controlrats, which consisted of untreated normal rats and shams, andarthriticrats.
Evoked behavior. Hindlimb withdrawal and vocalization thresholds were measured and determined as follows: mechanical stimuliof gradually increasing intensity (steps of 50 gm/30 mm²) were applied to the hindpaw by means of a forceps with a forcetransducer, whose calibrated output was amplified and displayedin g on an liquid crystal display screen. Threshold was definedas the minimum stimulus intensity that evoked withdrawal of thehindlimb or vocalization. The threshold stimulus intensity wasthen tested again three times to verify the presence of the withdrawalreflex or vocalization in at least 50% oftrials.
Spontaneous behavior. Exploratory behavior was measured using an activity box, which monitors exploratory activity in termsof the frequency at which the animal interrupts one of six beamsof UV light over 45 min. A computer tracked the activity and provideda report of exploratory activity over time in terms of parameterssuch as entries, distance traveled, and time spentresting.

Electrophysiology
Whole-cell voltage-clamp recordings were made from CeA neurons in brain slices from control and arthritic rats (6-8 hr afterinduction of arthritis). Monosynaptic EPSCs were evoked at theparabrachial (PB) $right-arrow$ CeA synapse (nociceptive-specific input) andthe basolateral amygdala (BLA) $right-arrow$ CeA synapse (polymodal sensory,including nociceptive, inputs) (Fig. 1). Drugs dissolved in artificialCSF (ACSF) were applied by superfusion. ACSF contained (in mM):117 NaCl, 4.7 KCl, 1.2 NaH₂PO₄, 2.5 CaCl₂, 1.2 MgCl₂, 25 NaHCO₃,and 11glucose.
Amygdala slice preparation. Brain slices containing the CeA were obtained as previously described (Neugebauer et al. 1997a,2000) (see Fig. 1). Rats were decapitated, and the brains quicklydissected out and blocked in cold (4°C) ACSF (see above). ACSFwas oxygenated and equilibrated to pH 7.4 with a mixture of 95%O₂and 5% CO₂. Coronal brain slices (350-500 µm) were preparedusing a Vibroslice (Camden Instruments, London, UK). After incubationin ACSF at room temperature (21°C) for at least 1 hr, a singlebrain slice was transferred to the recording chamber and submergedin ACSF (31 ± 1°C), which superfused the slice at ~2 ml/min.
Whole-cell patch-clamp recording. Whole-cell recordings using the "blind" patch technique (Blanton et al., 1989) or differentialinterference contrast (DIC)-enhanced infrared (IR) videomicroscopy(Dodt and Zieglgansberger, 1990, 1998) (see Fig. 1) were obtainedfrom CeA neurons using patch electrodes made from 1.5 mm borosilicateglass capillaries (1.5 mm outer diameter, 1.12 mm inner diameter;Drummond, Broomall, PA) pulled on a Flaming-Brown micropipettepuller (P-80/PC; Sutter Instrument Co., Novato, CA). Recordingelectrodes were positioned in the central medial and lateral capsulardivisions of the CeA under visual control. The boundaries of theCeA were discerned under light microscopy (see Fig. 1); each slicewas matched with the corresponding level of Paxinos and Watson(1998). The internal solution of the recording electrodes (3-5M $Omega$ tip resistance) contained (in mM): 122 K-gluconate, 5 NaCl,0.3 CaCl₂, 2 MgCl₂, 1 EGTA, 10 HEPES, 5 Na₂-ATP, and 0.4 Na₃-GTP,pH was adjusted to 7.2-7.3 with KOH and osmolarity to 280 mOsm/kgwithsucrose.
After tight (>2G $Omega$ ) seals were formed and the whole-cell configuration was obtained, neurons were included in the sample ifthe resting membrane potential was more negative than $-$ 50 mV,and action potentials overshooting 0 mV were evoked by directcathodal stimulation. Voltage and current signals were low-pass-filteredat 1 kHz with a dual four-pole Bessel filter (Warner InstrumentCorp., Hamden, CT), digitized at 5 kHz (Digidata 1200 interface;Axon Instruments, Foster City, CA), and stored on a computer (GatewayPerformance Pentium III). Data were also continuously recordedon a pen chart recorder (3400; Gould Instruments, Valley View,OH). Evoked potential and evoked current data were acquired andanalyzed using pCLAMP8 software (Axon Instruments). Discontinuoussingle-electrode voltage-clamp recordings were acquired usingan Axoclamp-2B amplifier (Axon Instruments) with a switching frequencyof 5-6 kHz (30% duty cycle), gain of 3-8 nA/mV, and time constantof 20 msec. Phase shift and the antialias filter were optimized.The head stage voltage was monitored continuously on a digitaloscilloscope (Gould 400) to ensure precise performance of theamplifier. Neurons were voltage-clamped at $-$ 60mV.
Synaptic stimulation. The CeA represents the major output nucleus of the amygdala and processes information from other amygdalanuclei and from widespread brain areas. We studied two lines ofinput to the CeA: the BLA $right-arrow$ CeA synapse and the pontine PB $right-arrow$ CeA synapse(see introductory remarks and Fig. 1). Using two concentric bipolarstimulating electrodes (Kopf Instruments) of 22 k $Omega$ resistance,EPSCs were evoked in CeA neurons by electrical stimulation (usingan S88 stimulator; Grass Instruments) of the two afferent synapsesto the CeA (see Fig. 1): the PB $right-arrow$ CeA synapse, which provides nociceptiveinputs from the spinal cord and brainstem (PB; Bernard et al.,1993; Harrigan et al., 1994; Alheid et al., 1995), and the BLA-CeAsynapse, which provides highly integrated polymodal sensory, includingnociceptive, information from thalamic and cortical areas (seeintroductory remarks). For stimulation of the PB, the electrodewas positioned under microscopic control on the fibers dorsomedialto the CeA and ventral to but outside the caudate-putamen (Bernardet al., 1993). Electrical stimuli (150 µsec square-wave pulses)were delivered at frequencies <0.25 Hz. Thresholds for EPSCs andspiking were defined as the respective intensity that evoked aresponse in at least 5 of 10 trials with mean amplitude determinedfrom the 10 trial stimulations. Input-output relationships wereobtained by increasing the stimulus intensity in 50 µA steps.For evaluation of a drug effect on synaptically evoked responses,the stimulus intensity was adjusted to 75-80% of the intensityrequired for orthodromic spikegeneration.
Paired-pulse facilitation. Paired-pulse facilitation (PPF) is being used to distinguish presynaptic versus postsynaptic mechanismsin the CNS (McKernan and Shinnick-Gallagher, 1997, and referencestherein). Two orthodromic synaptic stimuli of equal intensitywere applied at varying intervals, and the resulting EPSCs wererecorded. PPF refers to the phenomenon that the amplitude of thesecond EPSC is usually larger than the initial EPSC if the interstimulusinterval is sufficiently small. In whole-cell voltage clamp, peakamplitudes were measured as the difference between the currentlevel before the stimulus artifact and the peak of the EPSC. PPF(see Fig. 5) is calculated as [(EPSC2 - EPSC1)/EPSC1] × 100 (seeMcKernan and Shinnick-Gallagher, 1997). If a drug increases neurotransmitterrelease, PPF is reduced, whereas enhanced PPF would indicate decreasedneurotransmitter release. Any alterations in PPF suggest a presynapticsite of action. PPF was tested before and during application ofmGluRagonists.
Drugs. The following drugs were used: 2-amino-5-phosphonopentanoic acid (AP-5), 2-chloro-5-hydroxyphenyl-glycine (CHPG), 6-cyano-7-nitroquinoxaline-2,3-dione(CNQX), 7-(hydroxyimino)cyclopropa[b]chromen-1a-carboxylate ethylester (CPCCOEt), (S)-3,5-dihydroxyphenylglycine (DHPG), and 2-methyl-6-(phenylethynyl)pyridine(MPEP); these were purchased from Tocris Cookson (Bristol, UK).All drugs were applied by gravity-driven superfusion in the ACSF.Solution flow into the recording chamber (1 ml volume) was controlledwith a three-way stopcock. Drug applications were for at least8-10 min (agonists) and 10-15 min (antagonists) in duration toestablish equilibrium in thetissue.

Quantitative immunoblotting
Two to three 500 µm amygdala slices from control or arthritic rats (6-8 hr after induction) were homogenized in 1 ml of homogenizationbuffer (in mM: 320 sucrose, 10 HEPES-Na, pH 7.5, and 1 EDTA-Na,pH 8) using eight strokes of a glass-Teflon motorized homogenizer.The homogenate was centrifuged at 1500 × g for 5 min to removenuclei and debris and then centrifuged at 100,000 × g for 30 minin a TLA100.2 rotor to pellet postnuclear membranes. The pelletwas resuspended in homogenization buffer and solubilized withan equal volume of either 2× sample buffer (100 mM Tris-Cl, pH6.8, 4% SDS, 20% glycerol, and 0.02% bromophenol blue) for SDS-PAGEor 4% SDS for protein quantitation. A BCA assay (Pierce, Rockford,IL) using bovine serum albumin as a standard was used to determineproteinconcentration.
Ten micrograms of membrane protein were loaded onto a polyacrylamide gel and transferred to a nitrocellulose membrane usinga semidry transfer apparatus. The blots were blocked in Tris-bufferedsaline with Tween 20 (TBST; 150 mM NaCl, 50 mM Tris-Cl, pH 7.5,and 0.05% Tween 20) and 5% milk for 1 hr at room temperature,incubated for 1 hr in either mGluR1a antibody (1:1000; UpstateBiotechnology, Lake Placid, NY) or mGluR5 antibody (1:2000; UpstateBiotechnology) diluted in TBST and 5% nonfat dry milk, washedfour times with TBST, incubated for 1 hr in ¹²⁵I-coupled donkey anti-rabbit secondary antibody (0.2 µCi/ml; AmershamBiosciences, Piscataway, NJ) diluted in TBST and 5% milk, andfinally washed four times withTBST.
Signals were detected and densitized using a Cyclone phosphorimager and Optiquant acquisition and analysis software (PackardInstrument Co., Meriden, CT). All statistical comparisons weredone using a log transformation of immunoreactivity to yield ratioswith normal distributions for parametric statistics (Robakiewiczand Ryder, 2000).

Data analysis
Electrophysiology. Membrane properties, EPSC threshold, spike threshold, input-output relationships, and drug effects weremeasured in neurons from control rats and neurons from arthriticrats. The Mann-Whitney U test (GraphPad Prism 3.0) was used tocompare membrane properties. Differences in EPSC and spike thresholdswere evaluated for statistical significance using an unpairedt test (GraphPad Prism 3.0). Input-output relationships, drugeffects on paired pulse facilitation, and concentration-responserelationships of drug effects were analyzed using a two-way ANOVAfollowed by Bonferroni post-tests (GraphPad Prism 3.0). EC₅₀ valueswere calculated from sigmoid curves fitted to the cumulative concentration-responsedata by nonlinear regression using the following formula: y =A + (B - A)/[1 + (10^C/10^X)^D], where A is bottom plateau, B is top plateau, C is log(EC₅₀),and D is slope coefficient (GraphPad Prism 3.0). Effects of individualdrug concentrations were compared between control and arthritisusing unpaired t tests. Using the linear curve fit function ofpCLAMP8 software (Axon Instruments), slope conductance (in nanosiemens)in the absence and presence of drugs was calculated from the linearportion of the I-V relationships recorded in voltage-clamp mode.Concentration-dependent drug-related changes of slope conductancein neurons from arthritic rats and in control neurons were analyzedusing post hoc t tests after repeated measures ANOVA (GraphPadPrism 3.0). All averaged values are given as mean ± SEM. Statisticalsignificance was accepted at the p < 0.05.
Quantitative Western blotting. Densitometry of mGluR1a and mGluR5 immunoreactivity in arthritic rats was compared with thatof control rats using a one-sample t test. Ipsilateral and contralateralsides were compared with a paired t test. All averaged valuesare given as mean ± SEM. Statistical significance was acceptedat p < 0.05.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Kaolin- and carrageenan-induced monoarthritis caused swelling of the injected but not the contralateral knee joint within1-3 hr. The inflammation reached a maximum plateau after 4-6 hrand lasted for at least 24 hr (Fig. 1). Intra-articular salineinjections caused only a temporary swelling of the knee, whichdid not last >2 hr (Fig. 1). This monoarthritis resulted in significantlydecreased hindlimb withdrawal and vocalization thresholds to mechanicalstimuli (n = 10) and was associated with reduced exploratory behavior(n = 13) compared with control rats (n = 13).

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Figure 1. Experimental setup, design of electrophysiological studies, and time course of arthritis pain model. Coronal brain slices containing the amygdala were obtained from control (untreated normal and saline-injected sham) rats and from arthritic rats 6-8 hr after injections of kaolin and carrageenan (K/C) into one knee joint. Under microscopic control, the patch-clamp electrode was positioned in the "nociceptive amygdala," which is the lateral capsular part (CeC) of the CeA contralateral to the arthritis (cf. Bourgeais et al., 2001; Neugebauer and Li, 2002). Two stimulation electrodes were arranged for synaptic stimulation of afferent fibers from the pontine PB area providing nociceptive information to the CeA (left; Bernard et al., 1993) and inputs from the lateral-basolateral amygdala (right) providing polymodal information to the CeA from thalamic and cortical areas (part of the netting below the slice can be seen). Individual amygdala neurons were visualized and patched using DIC-enhanced infrared IR videomicroscopy (inset, CeA neurons and "dimple" caused by the patch electrode approaching from the bottom right). CeM, CeL, Medial and lateral subdivisions of the CeA, respectively. Intra-articular injections of kaolin and carrageenan cause the progressive, persistent swelling of the injected knee joint but not the uninjected contralateral knee joint (n = 35; graph on bottom left). Intra-articular saline injections produce only a temporary swelling of the injected knee (n = 12; graph on bottom right).

Synaptic plasticity and altered membrane properties in CeA neurons in the arthritis pain model

Whole-cell voltage-clamp recordings of CeA neurons were made in brain slices from control rats (untreated normal rats or saline-injectedshams) and from rats in which the arthritis had been induced inone knee joint by intra-articular injections of kaolin and carrageenan6-8 hr before. Because no obvious differences in membrane properties,synaptic transmission, and effects of mGluR agonists and antagonistswere measured between neurons from untreated rats and neuronsfrom saline-injected shams, the data were pooled and termed "controls."

Synaptic plasticity in the amygdala has been shown to underlie a number of long-term behavioral modifications in the kindlingmodel of epilepsy, chronic cocaine model of drug addiction, andmodels of conditioned fear and associative learning [lateral amygdala(LA)-BLA: LeDoux et al., 1990; Rainnie et al., 1992; McKernanand Shinnick-Gallagher, 1997; Neugebauer et al., 1997a; Wang andGean, 1999; Lin et al., 2000, Bauer et al., 2001; Blair et al.,2001; Lin et al., 2001] (CeA: Neugebauer et al., 2000; Nader etal., 2001). To test whether the arthritic pain behavior is associatedwith synaptic plasticity in the "nociceptive amygdala" (Bourgeaiset al., 2001; Neugebauer and Li, 2002), we performed whole-cellpatch-clamp recordings of membrane properties and synaptic transmissionin CeA neurons recorded in brain slices obtained from control(normal and sham) rats and arthriticrats.

CeA neurons from arthritic animals (6-8 hr after induction) showed several characteristics that distinguished them from neuronsin brain slices from control animals (Table 1, Fig. 2). The restingmembrane potential of CeA neurons was, on average, significantlydepolarized (Table 1; p < 0.001; Mann-Whitney U test). Comparedwith control neurons, neurons from arthritic rats also had a lowerthreshold and higher frequency of action potentials generatedby direct depolarizing current pulses injected via the recordingelectrode in current-clamp mode (see individual examples in Fig.2A,B). Increased action potential firing rate (Fig. 2C; p < 0.0001;F_(1,448) = 34.25; two-way ANOVA) and membrane potentials at whichaction potentials were evoked by intracellular current injections(Table 1; p < 0.05; Mann-Whitney U test) were significantly different.Current-clamp recordings showed that the input resistance of CeAneurons from arthritic rats was significantly decreased comparedwith control neurons (p < 0.001; Mann-Whitney U test; Table 1).Input resistance was calculated from the slope of the linear portionof the I-V curve. Transient current pulses (500 msec) were injectedvia the recording electrode in 50 pA increments from a holdingpotential of $-$ 60 mV. I-V curves (Fig. 2F) were obtained by plottingsteady-state voltage changes against the amplitudes of currentinjections (see individual examples in Fig. 2D,E). Accordingly,voltage-clamp data showed that the average slope conductance calculatedfrom the linear portion of the I-V relationship was greater inneurons from arthritic animals than in control neurons from normalanimals (Table 1; p < 0.001; Mann-Whitney U test). These datasuggest altered intrinsic membrane properties of CeA neurons inthe arthritis pain model.


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Table 1. Altered membrane properties and synaptic transmission in CeA neurons in the arthritis model of prolonged pain

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Figure 2. Enhanced action potential firing rate, lower spike threshold, and increased input resistance recorded in CeA neurons in the arthritis pain model compared with control neurons. A, B, Current-clamp recordings of depolarizations and action potentials (top traces) generated by direct current pulses of increasing magnitude (200 pA steps, 500 msec duration; bottom traces) injected via the recording electrode in a CeA neuron from a normal rat (A) and in a CeA neuron from an arthritic rat 6 hr after induction of arthritis (B). C, The action potential firing rate in CeA neurons in the arthritis pain model (n = 21) was significantly (p < 0.0001; F_(1,448) = 34.25; two-way ANOVA) increased compared with control CeA neurons (n = 45). **p < 0.01; ***p < 0.001; Bonferroni post-tests after the two-way ANOVA. D-F, Calculation of neuronal input resistance in the current-clamp mode. CeA neurons from arthritic rats (E, F, filled circles) had a lower input resistance than control CeA neurons (D, F, open circles). Input resistance was calculated from the slope of the linear portion of the I-V curve (F). I-V curves were obtained by plotting steady-state voltage changes against the amplitudes of transient current pulses (500 msec) injected via the recording electrode in 50 pA increments from a holding potential of $-$ 60 mV (D, E).

In addition to the enhanced excitability of CeA neurons in the arthritis pain model, we also observed enhanced synaptic transmissionat the nociceptive PB $right-arrow$ CeA synapse and the polymodal BLA $right-arrow$ CeA synapse(see introductory remarks) in CeA neurons from arthritic ratscompared with control CeA neurons (Fig. 3). Monosynaptic EPSCswith progressively larger amplitudes were evoked by electricalstimulation with increasing intensities (BLA $right-arrow$ CeA synapse, Fig.3A,C,E; PB $right-arrow$ CeA synapse, Fig. 3B,D,F). Compared with control neurons(Fig. 3A,B), synaptic transmission was enhanced in CeA neuronsrecorded in brain slices from arthritic rats (6-8 hr after inductionof arthritis) (Fig. 3C,D). In arthritis, evoked monosynaptic EPSCshad larger amplitudes, and the threshold for orthodromic spikegeneration was lower at both synapses, whereas a lower EPSC thresholdwas recorded only at the BLA $right-arrow$ CeA synapse (Table 1). Consistentwith the PB $right-arrow$ CeA synapse providing high-threshold nociceptive PBinput (see introductory remarks), the major change of synaptictransmission was with high-intensity stimulation, whereas synaptictransmission at the polymodal BLA $right-arrow$ CeA synapse was enhanced overa wide range of low- and high-intensity stimulation. The fastmonosynaptic EPSCs at both the BLA $right-arrow$ CeA synapse and the PB $right-arrow$ CeAsynapse were completely blocked in the presence of NMDA and non-NMDAreceptor antagonists (AP-5, 50 µM; CNQX, 30 µM, respectively)in CeA neurons from control animals (n = 12) and in the arthritispain model (n = 8), suggesting that basal synaptic transmissionat these synapses is mediated entirely by ionotropic glutamatereceptors.

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Figure 3. Enhanced synaptic transmission in the CeA in the arthritis pain model. Coronal brain slices containing the CeA were obtained from control (uninjected normal and saline-injected sham) rats and from rats with arthritis in the left knee (6-8 hr after injection of kaolin/carrageenan). Whole-cell voltage-clamp recordings were made from neurons in the lateral capsular part of the CeA. Synaptic transmission was studied at two synaptic pathways in the CeA, using electrical stimulation of afferent fibers from the parabrachial area (PB $right-arrow$ CeA synapse) and from the basolateral amygdala (BLA $right-arrow$ CeA synapse). Monosynaptic EPSCs were recorded, and input-output relationships were obtained by increasing the stimulus intensity in 50 µA steps and measuring the peak amplitudes of evoked EPSCs. A-D, Individual examples of one CeA neuron recorded in the brain slice from a normal rat (A, B) and another CeA neuron from an arthritic rat (C, D; 6 hr after induction). A, C, At the BLA $right-arrow$ CeA synapse, lower thresholds for EPSCs and orthodromic spike generation were recorded in arthritis. B, D, EPSCs evoked at the PB $right-arrow$ CeA synapse in arthritis had lower spike thresholds. E, F, Significantly altered input-output relationships in neurons from arthritic animals (n = 20) compared with control neurons (n = 36; normal uninjected rats, n = 26; saline-injected shams, n = 10), suggesting enhanced synaptic transmission at both the BLA $right-arrow$ CeA (E) and PB $right-arrow$ CeA (F) synapses (two-way ANOVA followed by Bonferroni post-tests). *p < 0.05; **p < 0.01; ***p < 0.001. Neurons were held at $-$ 60 mV.

Input-output relationships were obtained by measuring EPSC peak amplitude (picoamperes) as a function of afferent fiber stimulusintensity (microamperes) for each neuron (see examples in Fig.3A-D). The comparison of input-output relationships between neuronsfrom control rats (n = 36; normal uninjected rats, n = 26; saline-injectedshams, n = 10) and neurons from arthritic rats (n = 20) showedsignificant differences in synaptic transmission in arthritisat both synapses (Fig. 3E,F; two-way ANOVA followed by Bonferronipost-tests). At the BLA $right-arrow$ CeA synapse, the arthritis led to a significantleftward shift of the curves (Fig. 3E) and also lowered the thresholdsfor evoked EPSCs and orthodromic spike generation (Table 1).The input-output relationship measured at the PB $right-arrow$ CeA synapse hada steeper slope, resulting in an upward shift at higher stimulusintensities in CeA neurons from arthritic rats compared with controlneurons (Fig. 3F). The spike threshold, but not the EPSC threshold,was also altered at the PB $right-arrow$ CeA synapse (Table 1).

Differential roles of mGluR1 and mGluR5 in synaptic plasticity in the arthritis pain model

Group I mGluRs, which consist of mGluR1 and mGluR5 subtypes, play important roles in nociceptive plasticity in the peripheralnervous system and the spinal cord and have been proposed as noveltargets for pain relief (Fundytus, 2001; Karim et al., 2001; Neugebauer,2001a,b; Gasparini et al., 2002; Neugebauer, 2002; Neugebauerand Carlton, 2002; Varney and Gereau, 2002). The role of mGluRsin the brain, however, in prolonged, and chronic pain states arefor the most part unknown. Accumulating evidence suggests a roleof mGluRs in the amygdala in synaptic plasticity associated withbehavioral modifications (Holmes et al., 1996; Neugebauer et al.,1997a,b, 2000; Masugi et al., 1999; Keele et al., 2000; Lin etal., 2000). Thus, it is conceivable that mGluRs also contributeto pain-related synaptic plasticity in the amygdala. We testedthis hypothesis using selective group I agonists and antagoniststo analyze changes of receptor function in the arthritis painmodel.

Agonists
We tested whether group I mGluR receptor sensitivity was altered in CeA neurons from arthritic rats compared with controlneurons from normal and saline-injected sham rats. In controlneurons, a group I mGluR agonist, DHPG, which can activate bothmGluR1 and mGluR5 subtypes, potentiated the peak amplitude ofmonosynaptic EPSCs evoked at the PB $right-arrow$ CeA and BLA $right-arrow$ CeA synapses.This effect was mimicked by a selective mGluR5 agonist, CHPG,which produced similar maximum effects. Figure 4A shows the effectsof the group I agonists on EPSCs evoked at the PB $right-arrow$ CeA synapsein one CeA neuron in a brain slice from a normal animal. In CeAneurons from arthritic animals, DHPG more potently potentiatedevoked EPSCs, whereas the effects of CHPG were unchanged. Figure4B shows the effects of DHPG and CHPG at the PB $right-arrow$ CeA synapse inone CeA neuron recorded in a brain slice from an arthritic rat.Drug effects started after superfusing the brain slices for 2-3min and increased further until a plateau effect was observedat 6-10 min of drug application. Drug effects reported in thisstudy were measured at 8-10 min.

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Figure 4. Group I mGluR agonists facilitate synaptic transmission in the amygdala. A, In one CeA neuron recorded in a brain slice from a normal rat, DHPG (1 µM; mGluR1 and mGluR5 agonist) and CHPG (100 µM; mGluR5 agonist) enhanced monosynaptic EPSCs at the PB $right-arrow$ CeA synapse, suggesting the involvement of mGluR5 in group I mGluR effects on normal transmission. B, In a CeA neuron recorded in a slice from an arthritic rat (7 hr after induction), DHPG (100 nM; note lower concentration than in A) but not CHPG became more potent in enhancing EPSCs. Each trace is the average of 8-10 EPSCs recorded at -60 mV. Drugs were applied by superfusion of the slice in ACSF for 8-10 min. Data shown were recorded at 8-10 min. C, D, Cumulative concentration-response relationships (see Materials and Methods) show the increased potency of DHPG but not CHPG on transmission at the PB $right-arrow$ CeA synapse in arthritis 6-8 hr after induction (DHPG, n = 11; CHPG, n = 8) compared with neurons from control rats (DHPG, n = 12; CHPG, n = 9), suggesting a change of mGluR1 rather than mGluR5 receptor sensitivity and function.

Analysis of the cumulative concentration-response relationships in CeA neurons from control and arthritic animals revealedthat DHPG was more potent in arthritis (EC₅₀, 3.4 nM; n = 11)(Fig. 4C, filled circles) than under normal conditions (EC₅₀,25.9 nM; n = 12) (Fig. 4C, open circles), whereas the potencyof CHPG did not change significantly (normal: EC₅₀, 1.2 µM; n= 9; Fig. 4D, open symbols; arthritis: EC₅₀, 0.9 µM; n = 8; Fig.4D, filled symbols; p > 0.05; F_(1,75) = 0.64; two-way ANOVA).Concentration-response relationships for DHPG in CeA neurons fromcontrol and arthritic rats were significantly different (p < 0.05;F_(1,84) = 4.09; two-way ANOVA). These data suggest that undernormal conditions, the potentiating effects of group I mGluR activationare mediated through mGluR5, whereas the enhanced effects of groupI mGluR activation in arthritis involve recruitment or enhancedreceptor sensitivity ofmGluR1.
The potentiating effects of DHPG (100 nM) in control neurons were mostly blocked by a selective mGluR5 antagonist (MPEP, 1µM; n = 4), whereas a selective mGluR1 antagonist (CPCCOEt, 10µM) had only a little effect (n = 4). In the arthritis pain model,however, both CPCCOEt (10 µM; n = 3) and MPEP (1 µM; n = 3) stronglyreduced the potentiation by DHPG (100 nM), suggesting a changeof mGluR1 involvement in group I mGluR function in the arthritispainmodel.
Similar but less pronounced changes of DHPG effects in arthritis were measured at the BLA $right-arrow$ CeA synapse (control: EC₅₀, 7.9nM; n = 12; arthritis: EC₅₀, 3.7 nM; n = 11; p < 0.05; F_(1.84)= 4.23; two-way ANOVA; data not shown), suggesting a closer associationof mGluR1 with arthritis-related changes at the nociceptive PB $right-arrow$ CeAsynapse than the polymodal BLA $right-arrow$ CeA synapse. The potency of CHPGat the BLA $right-arrow$ CeA synapse remained mostly unchanged in the arthritispain model (normal: EC₅₀, 0.4 µM; n = 6; arthritis: EC₅₀, 0.5µM; n = 5; data notshown).
To examine whether enhanced presynaptic transmitter release contributed to the synaptic potentiation by group I mGluR agonists,we analyzed the effect of DHPG on PPF (see Materials and Methods)in CeA neurons. PPF refers to the phenomenon that the amplitudeof the second of two EPSCs evoked by synaptic stimulation of equalmagnitude is usually larger than the initial EPSC if the interstimulusinterval is sufficiently small. If a drug increases neurotransmitterrelease, PPF is reduced, whereas enhanced PPF would indicate decreasedneurotransmitter release. Any alterations in PPF suggest a presynapticsite of action (see McKernan and Shinnick-Gallagher, 1997). Figure5 shows that DHPG (100 nM; thick lines) reduced PPF (50 msec interstimulusintervals) in a CeA neuron from a normal rat (Fig. 5A) and inanother CeA neuron from an arthritic rat (Fig. 5B). The initialEPSC were potentiated by DHPG in both neurons as shown before(Fig. 4). The reduction of PPF by DHPG was statistically significantin CeA neurons from normal rats (Fig. 5C; n = 6; p < 0.0001; F_(1,80)= 62.23; two-way ANOVA) and in CeA neurons from arthritic rats(Fig. 5D; n = 5; p < 0.0001; F_(1,64) = 90.84; two-way ANOVA).

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Figure 5. A group I mGluR agonist (DHPG) reduced PPF, indicating that enhanced presynaptic transmitter release contributed to the synaptic potentiation by DHPG. PPF (see Materials and Methods) was studied at the PB $right-arrow$ CeA synapse before and during application of DHPG. A, B, DHPG (100 nM; thick lines) reduced PPF in a control CeA neuron (A) and in a CeA neuron from an arthritic rat (B), whereas the amplitudes of the initial EPSCs were potentiated by DHPG as described before (Fig. 4). Neurons were recorded in the whole-cell voltage-clamp mode and held at $-$ 60 mV. Each trace is the average of 8-10 EPSCs. DHPG was applied by superfusion of the slice in ACSF for 10 min. Data shown were recorded at 8-10 min. C, D, PPF at the PB $right-arrow$ CeA synapse is significantly reduced in the presence of DHPG in CeA neurons from normal rats (n = 6) and in CeA neurons from arthritic rats (n = 5). Peak amplitudes were measured as the difference between the current level before the stimulus artifact and the peak of the EPSC. PPF was calculated as [(EPSC2 - EPSC1)/EPSC1] × 100. Paired pulse EPSCs were evoked at a frequency of 0.1 Hz. **p < 0.01; ***p < 0.001, Bonferroni post-tests after two-way ANOVA.

Consistent with our PPF studies suggesting presynaptic mechanism(s) of group I mGluR-mediated synaptic potentiation, we didnot find any evidence that the effects of DHPG and CHPG on synaptictransmission were attributable to postsynaptic alterations ofintrinsic membrane properties by these agents. Concentrationsof DHPG and CHPG that potentiated synaptic transmission did notaffect I-V relationships of CeA neurons. Neither a parallel shiftnor a change of slope conductance of the I-V curves was measuredin CeA neurons (Fig. 6A,B). At high concentrations, however, DHPGand CHPG decreased the slope conductance significantly both inCeA neurons from arthritic rats and in control neurons (for details,see Fig. 6A,B). These data show that we were able to detect drugeffects on membrane properties with the experimental approachwe used in this study.

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Figure 6. Low concentrations of the group I mGluR agonists DHPG (A) and CHPG (B) do not produce postsynaptic membrane effects on slope conductance in CeA neurons from arthritic rats (DHPG, n = 11; CHPG, n = 8) and in CeA neurons from control rats (DHPG, n = 12; CHPG, n = 9). At higher concentrations, however, DHPG (1 µM) and CHPG (100 µM) significantly decreased the slope conductance both in CeA neurons from arthritic rats and in control neurons. Group I mGluR antagonists CPCCOEt (C) and MPEP (D) did not have postsynaptic membrane effects on slope conductance in control CeA neurons (CPCCOEt, n = 11; MPEP, n = 10) and in CeA neurons from arthritic animals (CPCCOEt, n = 9; MPEP, n = 9). For each neuron, the slope conductance was calculated from the I-V relationships in the presence and absence of the different drug concentrations. I-V curves were constructed by plotting steady-state currents from voltage-clamp recordings against membrane potential in the absence and presence of a particular drug. Whole-cell currents were elicited by a series of 400 msec voltage steps ( $-$ 110 to $-$ 40 mV) from a holding potential of $-$ 60 mV in control ACSF and during drug application (after 11 min). *p < 0.05, post hoc t test after repeated measures ANOVA.

Antagonists
The results with mGluR1 and mGluR5 agonists suggest that the receptor sensitivity of mGluR1 is increased in arthritic animals.We next examined whether these receptors are involved in tonicregulation of synaptic transmission in CeA neurons under normalconditions and whether this modulation is enhanced in arthritis.In CeA neurons recorded in brain slices from normal rats (seeindividual neuron in Fig. 7A), a selective mGluR5 antagonist,MPEP, inhibited monosynaptic EPSCs evoked at the PB $right-arrow$ CeA and BLA $right-arrow$ CeAsynapses, whereas a selective mGluR1 antagonist, CPCCOEt, hadno effect. In CeA neurons from arthritic animals, however, blockof mGluR1 with CPCCOEt inhibited synaptic transmission (see individualexample in Fig. 7B). Analysis of the concentration-response relationshipsshowed that CPCCOEt (mGluR1 antagonist) (Fig. 7C) inhibited synaptictransmission at the PB $right-arrow$ CeA synapse in the arthritis pain model(EC₅₀, 94 nM; n = 9 neurons) (Fig. 7C, filled circles), whereasCPCCOEt had no significant effect on synaptic transmission undernormal conditions; i.e., the slope of the concentration-responsecurve was not significantly different from zero (p > 0.05; F_(1,3)= 6.482; n = 11; linear regression analysis, Prism 3.0, GraphPadsoftware) (Fig. 7C, open circles). A similar change of CPCCOEteffects was observed at the BLA $right-arrow$ CeA synapse, although the antagonistwas less potent (EC₅₀, 179 nM; n = 9 neurons) than at the PB $right-arrow$ CeAsynapse (see above). The analysis of the raw data showed thatblock of mGluR1 by CPCCOEt reduced the increased EPSC amplitudein CeA neurons from arthritic rats to control levels measuredin neurons from nonarthritic rats (Fig. 7D), suggesting that theincreased EPSC component in enhanced synaptic transmission inthe arthritis pain model involves mGluR1.

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Figure 7. Differential changes of mGluR1- and mGluR5-mediated effects in the arthritis pain model. A, In a CeA neuron recorded in a brain slice from a normal rat, MPEP (1 µM; mGluR5 antagonist) inhibited synaptic transmission, whereas CPCCOEt (10 µM; mGluR1 antagonist) had no effect. B, In a CeA neuron from an arthritic rat (6 hr after induction), both CPCCOEt and MPEP inhibited synaptic transmission, suggesting a change in the endogenous activation of mGluR1 in the arthritis pain model. Each trace is the average of 8-10 monosynaptic EPSCs recorded at -60 mV. Drugs were applied by superfusion of the slice in ACSF for at least 10 min. Data shown were recorded at 10-12 min. C, CPCCOEt inhibited synaptic transmission in neurons from arthritic rats (EC₅₀, 94 nM; n = 9) but not in neurons from normal rats (n = 11), suggesting a change in the activation state of mGluR1 in the arthritis pain model. D, Analysis of the raw data (EPSC peak amplitude in picoamperes) shows that blocking of mGluR1 by CPCCOEt significantly reduced the increased EPSC amplitude in CeA neurons from arthritic rats to control levels measured in neurons from nonarthritic rats. E, The inhibitory effects of MPEP on synaptic transmission in CeA neurons were not significantly different in normal rats (EC₅₀, 28.3 nM; n = 10) and in arthritis (EC₅₀, 27.7 nM; n = 9; p > 0.05; two-way ANOVA). F, Analysis of the raw data (picoamperes) shows that MPEP reduced a larger portion of the increased EPSC in arthritis than in control neurons; however, the MPEP-insensitive component of the EPSC also increased in arthritis. ***p < 0.001; unpaired t test.

The comparison of the concentration-response relationships for MPEP (mGluR5 antagonist) (Fig. 7E) in normal and arthriticanimals showed the concentration-dependent inhibition of synaptictransmission at the PB $right-arrow$ CeA synapse in both experimental conditionswithout a significant change in potency or efficacy (p > 0.05;F_(4,76) = 0.10; two-way ANOVA). The EC₅₀ values for inhibitoryeffects of MPEP at the PB $right-arrow$ CeA synapse were 28.3 nM in controlneurons (n = 10) and 27.7 nM in arthritis (n = 9). MPEP was morepotent at the BLA $right-arrow$ CeA synapse in control neurons (EC₅₀, 11.4 nM;n = 10) as well as in arthritis (EC₅₀, 10.1 nM; n = 9). The analysisof the raw data showed that the mGluR5 antagonist MPEP reduceda larger portion of the increased EPSC in arthritis than in controlneurons; however, the MPEP-insensitive component of the EPSC alsoincreased in arthritis (Fig. 7F). The overall consequence is thatthe mGluR5-dependent component of synaptic transmission remainsunchanged in the arthritis painmodel.
Neither antagonist had any significant postsynaptic effects on intrinsic membrane properties such as current-voltage relationships.There was no drug-induced change in slope conductance in CeA neuronsfrom arthritic rats and in control CeA neurons (Fig. 6C,D).
These data suggest the intrinsic activation of mGluR5, but not mGluR1, in normal synaptic transmission and the additionalinvolvement of mGluR1 in enhanced synaptic transmission in thearthritis pain model. This observation is consistent with theagonist studies (see above) that suggest the increased functionof mGluR1 rather than mGluR5 in the arthritis painmodel.

Upregulation of mGluR1 and mGluR5 protein expression in the arthritis pain model

The enhanced effects of mGluR1 agonists and antagonists in arthritis could be mediated by increased expression of mGluR1,increased sensitivity and activity of existent receptors, or both.To test whether arthritis caused increased expression of mGluR1protein in the CeA, we performed quantitative Western blot analysisof mGluR1 and mGluR5 protein expression in the CeA. We detectedhigh levels of mGluR5 but little mGluR1 under normal conditions(Fig. 8). In the CeA from arthritic animals (6-8 hr after induction),however, significantly more expression of mGluR1 was detectedas well as an increased expression of mGluR5. Densitometric analysisof mGluR1a and mGluR5 immunoreactivity showed a significant increaseof mGluR1 and mGluR5 expression in the contralateral CeA of arthriticrats and a significant increase in mGluR1, but not mGluR5, inthe ipsilateral CeA (Fig. 8B; n = 3 in duplicate; *p < 0.05, arthritiscompared with normal control using a one-sample t test; ⁺p < 0.05, contralateral CeA compared with the ipsilateral sidein arthritis with paired t test). These results strongly suggestthat the increased effects of mGluR1 agonists in arthritis isattributable to increased expression of mGluR1 protein in theCeA.

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Figure 8. Upregulation of mGluR1 and mGluR5 in the amygdala in the arthritis pain model. Group I mGluR1 and mGluR5 expression increased in the amygdala 5-6 hr after kaolin/carrageenan-induced arthritis in the knee. A, Top panel, mGluR1a immunoblot of amygdala (CeA) membranes from normal and arthritic rats; the ~150 kDa band is mGluR1a, whereas the bottom band probably represents a proteolytic fragment or cross-reactive protein. Bottom panel, mGluR5 immunoblot of amygdala (CeA) membranes from normal and arthritic rats; the ~150 kDa band represents mGluR5 immunoreactivity. B, Densitometry of mGluR1a and mGluR5 immunoreactivity suggests an increase in group I mGluR expression in arthritic rats with a greater increase in the contralateral amygdala (n = 3 in duplicate; ⁺p < 0.05 when compared with the ipsilateral side with paired t test; *p < 0.05 when compared with normal rats using a one-sample t test).

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

This study is the first to analyze synaptic plasticity and underlying mechanisms in the amygdala in a model of prolonged pain.We show that the amygdala undergoes dramatic neuroplastic changesin a well established model of arthritic pain arising from a localizedinflammation of one knee joint (Neugebauer et al., 1993, 1994,1995, 1996). Neuroplasticity is manifested as altered excitabilityand enhanced synaptic transmission in CeA neurons recorded inbrain slices in vitro in the arthritis pain state induced in vivo.We also demonstrate the contribution of enhanced function andexpression of presynaptic mGluR1 within the CeA to thisplasticity.

Synaptic plasticity in the amygdala, particularly the lateral and basolateral nuclei (LA and BLA), is involved in a varietyof behavioral modifications and disorders, including models ofepilepsy, drug addiction, conditioned fear, and associative learning(Rainnie et al., 1992; McKernan and Shinnick-Gallagher, 1997;Neugebauer et al., 1997a; Davis, 1998; Huang and Kandel, 1998;Post et al., 1998; Maren, 1999; LeDoux, 2000; Lin et al., 2000,2001; Rolls, 2000; Bauer et al., 2001; Blair et al., 2001). Therole of the amygdala in persistent and chronic pain is not clear.A behavioral study was unable to show a significant reductionof pain responses in the formalin test (Manning, 1998), but long-termincreases of regional blood flow were detected in the amygdalain a neuropathic pain model (Paulson et al., 2002).

We found several long-lasting physiological changes in the CeA in the arthritis pain model. The nociceptive-specific inputsfrom the pontine PB area were potentiated in CeA neurons fromarthritic rats compared with controls. Thus, incoming nociceptivesignals would generate enhanced responses in the amygdala. Inaddition, we also observed significant enhancement of synaptictransmission at the BLA $right-arrow$ CeA synapse, which provides highly processedpolymodal information. This is consistent with the integrativerole of the amygdala in the complex emotional behavior in responseto aversive events (pain). The enhanced transmission was accompaniedby changes in membrane properties of CeA neurons (decreased inputresistance and increased slope conductance), suggesting tonicactivation of ion channels during prolonged pain. The overallenhanced excitability of CeA neurons in the arthritic pain modelis also reflected in the lower threshold for action potentialsgenerated by intracellular currentinjections.

Importantly, changes in synaptic transmission and intrinsic membrane properties of CeA neurons in the arthritis pain modeldiffer from those observed in other models of amygdala plasticity.In a model of drug addiction, chronic cocaine treatment in vivoalso enhanced CeA excitatory synaptic transmission but alteredthe gain of CeA synapses differently than in the present study(Neugebauer et al., 2000). Furthermore, membrane properties ofCeA neurons were altered differently in the chronic cocaine modelthan in our arthritis pain model in that the lower input resistanceand increased slope conductance resulted in a hyperpolarized membranepotential (Neugebauer et al., 2000) rather than a depolarizationas observed here, suggesting that different ionic mechanisms underliethe excitability changes. In contrast to the arthritis pain andchronic cocaine models, enhanced synaptic transmission in thekindling model of epilepsy was not accompanied by intrinsic membraneproperty changes of CeA and BLA neurons (Neugebauer et al., 1997a,2000). Similarly, in the fear-conditioning model, synaptic transmissionin LA neurons was enhanced in the absence of intrinsic membraneproperty changes (McKernan and Shinnick-Gallagher, 1997). Thesedifferential plastic changes in the amygdala suggest specificityin different models of behavioralplasticity.

Our results show that both input to and output from the CeA are enhanced during arthritis-induced prolonged pain. The alteredinput to CeA neurons is reflected in the enhancement of synaptictransmission, and the increased output will result from the enhancedexcitability of CeA neurons in arthritis. As the output nucleusfor major amygdala functions, the CeA with its laterocapsulardivision, also termed the "nociceptive amygdala" because of itshigh content of nociceptive neurons (Bourgeais et al., 2001; Neugebauerand Li, 2002), is well positioned to contribute to aversive andanxiogenic reactions to noxious stimuli, to participate in autonomicand endocrine aspects of emotional pain behavior, and to influencecortical sensory processing and forebrain mechanisms of pain modulation(Willis, 1991; Casey, 1999; Gallagher and Schoenbaum, 1999; Fields,2000; LeDoux, 2000; Bourgeais et al., 2001).

The electrophysiological changes of CeA neurons were closely paralleled by changes in the sensitivity of these cells to thegroup I mGluR agonist DHPG. DHPG potentiated synaptic transmissionat the PB $right-arrow$ CeA synapse, and arthritis produced a significant increasein the potency of DHPG. Interestingly, the effects of the selectivemGluR5 agonist CHPG were unaltered. These data suggest that, undernormal conditions, the facilitation of synaptic transmission bygroup I mGluR agonists is mediated through mGluR5, whereas theenhanced effects of group I mGluR activation in arthritis involverecruitment or enhanced coupling of mGluR1. Similar but less pronouncedchanges of DHPG effects in arthritis were measured at the BLA $right-arrow$ CeAsynapse, suggesting a closer association of mGluR1 with the nociceptivePB $right-arrow$ CeA synapse than with the polymodal BLA $right-arrow$ CeA synapse. Our studyis the first to analyze the role of group I mGluR subtypes onsynaptic transmission at the PB $right-arrow$ CeA and BLA $right-arrow$ CeA synapses in theamygdala. Although previous studies reported inhibition of synaptictransmission by DHPG, there is also good evidence for enhancedtransmitter release by group I mGluRs and facilitation of fastsynaptic transmission by mGluRs (Anwyl 1999; Cartmell and Schoepp,2000). The effects of group I mGluR activation can differ withdifferent brain areas, synapses, systems, and pathways studiedand therefore need to be analyzed in each instance. Importantly,synaptic potentiation by group I mGluRs in the CeA involves enhancedpresynaptic transmitter release, as evidenced by our PPF data(Fig. 5) and the lack of drug effects on intrinsic membrane properties(Fig. 6). PPF has been used in the amygdala before to analyzepresynaptic mechanisms of synaptic plasticity in the fear-conditioningmodel (McKernan and Shinnick-Gallagher, 1997).

Our studies using selective antagonists suggest increased mGluR1 function in the arthritis pain model. Under normal conditions,fast synaptic transmission was partially inhibited by the selectivemGluR5 antagonist MPEP, whereas CPCCOEt, a selective mGluR1 antagonist,had no effect at the concentrations used in this study. However,in neurons from arthritic animals, the mGluR1 antagonist significantlyreduced fast synaptic transmission. Importantly, CPCCOEt reducedthe increased EPSC amplitude in neurons from arthritic animalsto the level of control neurons. Although MPEP reduced a largerportion of the increased EPSC in arthritis than in control neurons,the MPEP-insensitive component of the EPSC also increased in arthritis;therefore, the mGluR5-dependent proportion of synaptic transmissionwould remain unchanged in the arthritis painmodel.

These results suggest that synaptic transmission in the arthritis pain model involves mGluR1 activation. Alternatively, basalextracellular levels of glutamate may increase in arthritis toa concentration sufficient to activate mGluRs, allowing antagoniststo reduce transmission. In other brain regions, activation ofgroup I mGluRs can depolarize cells by activation of a varietyof Ca²⁺-dependent and -independent nonselective inward cationic currents(Conn and Pin, 1997; Anwyl, 1999; Neugebauer, 2001a). This couldexplain the decrease in input resistance, increased slope conductance,and depolarization we observed in CeA neurons from arthritic animals.In the present study, however, mGluR effects were attributableto presynaptic mechanisms in CeA neurons from control or arthriticanimals, suggesting that tonic activation of these mGluRs by ambientglutamate cannot directly account for the alterations in membraneproperties. These data also suggest that synaptic plasticity occurs,at least in part, independently of intrinsic membrane propertychanges.

In addition to enhanced endogenous activation, the following mechanisms could explain the enhanced mGluR1 function in CeAneurons in the arthritis pain model: increased receptor expression,enhanced receptor sensitivity, decreased desensitization, andaltered coupling to signal transduction pathways. We found thatmGluR1 protein expression was significantly increased in the CeAin arthritic animals compared with controls, suggesting that theenhanced mGluR1 function reflects either increased productionof mGluR1 mRNA or protein or increased stability of the protein.We also observed a significant increase in mGluR5 levels in arthriticanimals, but our electrophysiological and pharmacological datasuggest that the proportion of mGluR5-dependent enhanced synaptictransmission is not changed from that in the arthritis pain model.The reason why the increase of mGluR5 does not seem to translateinto functional significance is not clear, but it is possiblethat the maximum contribution of mGluR5 to synaptic transmissionis accomplished with the levels of receptor expression measuredunder normal conditions, and the increase in arthritis would nottranslate into functional changes ("ceiling effect"). Alternatively,the increase in mGluR5 levels may occur in cells other than thoseinvolved in ourrecordings.

In summary, this study is the first to analyze electrophysiological, pharmacological, and biochemical changes in the amygdalain a model of persistent pain arising from a monoarthritic lesion.We demonstrate here that the potentiation of synaptic transmissionand enhanced neuronal excitability in the amygdala is preservedin an in vitro preparation that is disconnected from the siteof arthritic injury induced in vivo, suggesting that this plasticityis maintained independent of continuous afferent inputs. Thisplasticity involves increased presynaptic group I mGluR function,which reflects an underlying increase in mGluR1 expression intheCeA.

  FOOTNOTES

Received April 10, 2002; revised Oct. 9, 2002; accepted Oct. 14, 2002.

This work was supported by John Sealy Memorial Endowment Fund for Biomedical Research 2528-99 (V.N.) and National Institutesof Health Grants NS38261 (V.N.) and MH60230 (R.W.G.). G.B. isa McNair scholar of the Baylor College of Medicine Medical ScientistTraining Program. We thank Dr. William D. Willis for continuedgenerous support and critical reading of and helpful commentson this manuscript. We also thank Vicki Wilson for superb secretarialassistance.

Correspondence should be addressed to Dr. Volker Neugebauer, Department of Anatomy and Neurosciences and Marine BiomedicalInstitute, The University of Texas Medical Branch, 301 UniversityBoulevard, Galveston, TX 77555-1069. E-mail: voneugeb{at}utmb.edu.

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Results
Discussion
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