NMDA Receptor and the Tyrosine Phosphorylation of Its 2B Subunit in Taste Learning in the Rat Insular Cortex

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Volume 17, Number 13, Issue of July 1, 1997 pp. 5129-5135
Copyright ©1997 Society for Neuroscience

NMDA Receptor and the Tyrosine Phosphorylation of Its 2B Subunit in Taste Learning in the Rat Insular Cortex

Kobi Rosenblum, Diego E. Berman, Shoshi Hazvi, Raphael Lamprecht, and Yadin Dudai
Department of Neurobiology, The Weizmann Institute of Science, Rehovot 76100, Israel

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

We demonstrate that the NMDA receptor is involved in taste learning in the insular cortex of the behaving rat and describetwo facets of this involvement. Blockage of the NMDA receptorin the insular cortex by the reversible antagonist APV duringtraining in a conditioned taste aversion (CTA) paradigm impairedCTA memory, whereas blockage of the NMDA receptor in an adjacentcortex or before a retrieval test had no effect. When rats sampledan unfamiliar taste and hence learned about it, either incidentallyor in the context of CTA training, the tyrosine phosphorylationof the NMDA receptor subunit 2B (NR2B) in the insular cortex wasspecifically increased. The level of tyrosine phosphorylationon NR2B was a function of the novelty of the taste stimulus andthe quantity of the taste substance consumed, properties thatalso determined the efficacy of the taste stimulus as a conditionedstimulus in CTA; however, blockage of the NMDA receptor by APVduring training did not prevent tyrosine phosphorylation of NR2B.We suggest that tyrosine phosphorylation of NR2B subserves encodingof saliency in the insular cortex during the first hours afteran unfamiliar taste is sampled and that this encoding is independentof another, necessary role of NMDA receptors in triggering experience-dependentmodifications in the insular cortex during taste learning. Becausea substantial fraction of the NR2B protein in the insular cortexseems to be expressed in interneurons, saliency and the tyrosinephosphorylation of NR2B correlated with it may modulate inhibitionin cortex.
Key words: taste learning; conditioned taste aversion; insular cortex; latent inhibition; NMDA receptor subunit 2B; tyrosine phosphorylation

INTRODUCTION

Information about taste in the rat converges on the central gustatory area (GC) in the insular cortex (Finger, 1987; Hettingerand Frank, 1992). Rats lacking GC can still react to gustatoryinput (Braun et al., 1982), but lesions in GC cause marked deficitsin various aspects of taste learning (Braun et al., 1972; Dunnand Everitt, 1988; Bermudez-Rattoni and McGaugh, 1991; Gallo etal., 1992; Kiefer and Orr, 1992). Such results led to the hypothesisthat the gustatory area in the insular cortex plays only a minorrole in fundamental taste detection and reactivity but a majorrole in higher level processing of taste information (Braun etal., 1982).

A convenient paradigm for investigating taste learning is conditioned taste aversion (CTA) (Revusky and Garcia, 1970; Bureset al., 1988; Schafe et al., 1995). In CTA, organisms learn toavoid a novel taste if its ingestion is followed by transientpoisoning. The behavioral manifestations of CTA have been investigatedextensively over the years (Bures et al., 1988), but the neurobiologicalfoundations of this experience-dependent behavior are not yetelucidated (Chambers, 1990; Yamamoto et al., 1994). We have approachedthe role of the insular cortex in taste learning in general, andin CTA in particular, by using local transient metabolic lesionsand by correlating molecular alterations that are unveiled ininsular cortex during learning and afterward with the behavioralchange. Using such methods, we were able to show that taste memoryrequires protein synthesis (Rosenblum et al., 1993) and cholinergicactivity (Naor and Dudai, 1996) in the insular cortex during training,and that sampling a novel taste, either incidentally or in thecontext of CTA training, specifically enhances tyrosine phosphorylationof a set of proteins in that cortex (Rosenblum et al., 1995).

The major protein whose tyrosine phosphorylation is modulated by taste learning in the insular cortex is a postsynaptic density(PSD) constituent of molecular weight (MW) 180 kDa (Rosenblumet al., 1995). The main 180 kDa tyrosine kinase substrate in thePSD is the 2B subunit of the NMDA receptor (NR2B) (Moon et al.,1994; Lau and Huganir, 1995). NR2B, which is expressed throughoutthe embryonic rat brain but becomes restricted to the forebrainin the adult (Mori and Mishina, 1995), is considered to play anessential role in neuronal pattern formation and plasticity (Kutsuwadaet al., 1996). Tyrosine phosphorylation of NR2A or NR2B altersthe NMDA receptor functional properties in vitro (Yu et al., 1997).Tyrosine phosphorylation of NR2B also was implicated recentlyin long-term potentiation (LTP) in the hippocampal formation invivo (Rosenblum et al., 1996b; Rostas et al., 1996). In the presentreport we describe the participation of the NMDA receptor andthe tyrosine phosphorylation of its 2B subunit in taste learningin the insular cortex and propose that cortical NMDA receptorsplay multiple roles in CTA, and specifically that tyrosine phosphorylationof NR2B is related to the encoding of sensory input saliency incortex.

MATERIALS AND METHODS
Animals. Male Wistar rats (~60 d old, 200-250 gm) were used. They were caged individually at 22 ± 2°C in a 12 hr light/darkcycle.

Reagents. Polyclonal antiphosphotyrosine ( $alpha$ PY) and $alpha$ PY-agarose (monoclonal PY20) were from Zymed (San Francisco, CA). Horseradishperoxidase (HRP)-linked protein A and the enhanced chemiluminescence(ECL) kit were from Amersham (Buckinghamshire, UK). Protein A-Sepharosewas from Pharmacia (Uppsala, Sweden), biotinylated goat anti-rabbitand Elite avidin-biotin complex were from Vector (Burlingame,CA), RNase A and diaminobenzidine (DAB) peroxidase substrate (SIGMAFAST)were from Sigma (St. Louis, MO), and MK-801 and APV were fromRBI (Natick, MA). ³⁵S-UTP was from Amersham, and NdeI was from New England Biolabs(Beverly, MA). All other chemicals were of analytical grade orthe highest grade available.

Preparation of anti-NR2B ( $alpha$ NR2B). We have prepared polyclonal antibodies to NR2B using specific peptides as immunogens. Twopolyclonal antibodies were generated: ab971 and ab013. For preparationof the first, three peptides from the C-terminal portion of NR2Bwere synthesized (Biological Services, The Weizmann Instituteof Science): residues 1085-1101 (peptide A, NH₂-YKDSLKKRPASAKSRRE-COOH),1103-1118 (peptide B, NH₂-DEIELAYRRRPPRSPD-COOH), and 1464-1482(peptide C, NH₂-NGSSNGHVYEKLSSIESDV-COOH). The mixture of thethree peptide-KLH conjugates was injected into rabbits in completeFreund's adjuvant, and one of the sera, ab971, was used in thepreliminary set of experiments. Analysis of the binding of ab971to the different peptides and their mixture in an ELISA test showedthat >90% of the response was contributed by peptide B. Subsequently,a second antibody was raised against peptide B alone, ab013, andthis was used throughout the rest of the study. Results obtainedwith ab971 and ab013 were identical. The sequence of peptide Bis specific to NR2B (Ishii et al., 1993). The specificity of theantibodies was established by several tests: the reaction of ab013with the 180 kDa polypeptide was not detected in the preimmuneserum and was completely blocked by peptide B (10 µM). In addition,we expressed the NR2A and NR2B proteins in vitro, using the NR2AcDNA cloned in pCDNA3 and the NR2B cloned in pBluescript KS( $-$ )(kindly provided by S. Nakanishi, Kyoto University) in the TNT-coupledreticulate lysate systems (Promega, Madison, WI); ab971 precipitatedthe NR2B protein (a 162 kDa protein in the reticulate lysate transcriptionand translation system) but not the NR2A protein (data not shown).

Behavioral procedures. CTA was performed as described in Rosenblum et al. (1993), with minor modifications. Unless indicatedotherwise, saccharin (0.1% w/v, sodium salt) was used as the unfamiliartaste in training [i.e., the conditioned stimulus (CS)], and injectionof LiCl (0.15 M, 2% body weight, i.p.) as the malaise-inducingagent [unconditioned stimulus (UCS)]. At the beginning of thebehavioral experiment, the rats were trained for 3 d to get theirdaily water ration once a day for 10 min from two pipettes eachcontaining 10 ml of water. On the conditioning day, they wereallowed to drink the saccharin solution instead of water fromsimilar pipettes for 10 min, and 50 min later were injected withLiCl. Under these conditions, 3 d after training the conditionedrats preferred water to saccharin at a ratio of 9:1 in a multiplechoice test situation (three pipettes with 5 ml of saccharin each,three with 5 ml of water each), whereas nonconditioned rats preferredsaccharin to water. The behavioral data are presented below interms of aversion index, defined as [ml water/(ml water + ml saccharin)]consumed in the test; 0.5 is chance level, and the higher theaversion index, the more the rats prefer water to the conditionedtaste.

In some experiments, a latent inhibition procedure (Lubow, 1989) was combined with CTA to further isolate the effect of tastelearning on cortical molecular mechanisms from the potential confoundingeffects of the UCS and the CS-UCS association. Latent inhibitionis a process by which preexposure to a sensory stimulus diminishesthe ability of that same stimulus to serve as an associated stimulusin subsequent learning. Thus, exposure of rats to an unfamiliartaste several days before this same taste serves as the CS inCTA training, significantly reduces the acquired aversion (Rosenblumet al., 1993). Under such conditions, the degree of aversion afterCTA training is a measure of the memory of saccharin acquiredincidentally (Hebb, 1949) in the pre-CTA trial. In latent inhibitionexperiments, the rats were exposed either to saccharin or water(control) for 10 min, in two pipettes of 10 ml each, 3 d beforeCTA training, as described above, in which saccharin was usedas the CS. Testing was also as described above for the usual CTAprocedure.

Surgery and microinjection. Rats were anesthetized with 5.6 ml/kg Equithesin (2.12% w/v MgSO₄, 10% v/v ethanol, 39.1% v/vpropylene glycol, 0.98% w/v sodium pentobarbitone, 4.2% w/v chloralhydrate), restrained in a stereotaxic apparatus (Kopf), and implantedbilaterally with a guide stainless steel cannula (23 gauge) aimed1.0 mm above the gustatory neocortex [anteroposterior +1.2 mm,lateral ±5.5 mm, ventral 5.5 mm relative to bregma; accordingto Paxinos and Watson (1986)]. The cannulae were positioned inplace with acrylic dental cement and secured by two skull screws.A stylus was placed in the guide cannulae to prevent clogging.Animals were allowed 1 week to recuperate before being subjectedto experimental manipulations. The stylus was removed from theguide cannula, and a 28 gauge injection cannula, extending 1.0mm from the tip of the guide cannula, was inserted. The injectioncannula was connected via PE20 tubing to a Hamilton microsyringedriven by a microinfusion pump (CMA/100, Carnegie Medicin). Microinjectionwas performed bilaterally in a 1 µl vol/hemisphere delivered over1 min. The injection cannula was left in position before withdrawalfor an additional 1 min to minimize dragging of the injected liquidalong the injection tract.

Homogenization and fractionation. Rats were decapitated either 60 min after the completion of the exposure to the unfamiliartaste (taste only groups), 10 min after the completion of CTAtraining (CTA groups), or 10 min after intraperitoneal injectionof LiCl (LiCl only groups). The insular cortex containing theGC, or other brain areas indicated in Results, were dissectedout. For the insular cortex, the crossing of the rhinal fissureand the medial cerebral artery was used as a reference point,and cortical tissue 1.0 mm rostral, 0.5 mm caudal, and 1.5 mmdorsal to it was excised. Two homogenization and processing protocolswere used. In protocol A, the tissue was homogenized in a glass-Teflonhomogenizer in SDS sample buffer containing 10% glycerol, 5% $beta$ -mercaptoethanol,and 2.3% SDS, in 62.5 mM Tris-HCl, pH 6.8. This type of homogenatewas then subjected to SDS-PAGE and immunoblotting with $alpha$ PY or $alpha$ NR2B, as detailed below, for the determination of the level ofprotein tyrosine phosphorylation. Protocol B was used in experimentsin which the level of phosphotyrosine on NR2B was determined andincluded affinity purification of the tyrosine phosphorylatedprotein fraction before SDS-PAGE and immunoblotting with $alpha$ NR2B,as detailed below. In this protocol, the tissue from two to fourrats from the same experimental group was combined and homogenizedin 0.35 M sucrose, 0.5 mM EGTA, 2 mM EDTA, 2 mM Na₃VO₄, and 1mM PMSF, in 10 mM Tris-HCl, pH 7.4. The samples were centrifugedfor 1 min at 2000 × g, the supernatant was collected, the pelletwas recentrifuged as above, and the supernatants were combinedand diluted 1:1 with 2% SDS. The sample was then sonicated for10 min and boiled for 5 min, followed by dilution of 1:10 in 100mM NaCl, 5 mM EDTA, 50 mM NaF, 0.1% SDS, 0.1% Triton X-100, and1 mM Na₃VO₄, in 50 mM Tris-HCl, pH 7.5. The resulting aliquotswere subjected to affinity chromatography on $alpha$ PY-agarose. Afterapplication and equilibration for 2 hr at room temperature, theresin was washed with 100-fold packed resin volume of the applicationbuffer, and the tyrosine phosphorylated protein fraction was theneluted with 40 mM p-nitrophenyl phosphate (PNPP).

Western blot analysis. Aliquots in SDS sample buffer (equal amounts of protein) were subjected to SDS-PAGE (Laemmli, 1970)(7.5% polyacrylamide in the presence of SDS and $beta$ -mercaptoethanol)and Western blot analysis (Burnette, 1981). The amount of proteinin each sample was always determined before loading, and the sameamount of protein (range, 25-50 µg) was loaded in each lane (Lowryet al., 1951). After the run the lanes were also compared by Ponceaustaining. After it was blocked with 1% BSA, the blot was reactedeither overnight at 4°C or for 1 hr at room temperature with either $alpha$ PY or $alpha$ NR2B. The presence of the $alpha$ PY or $alpha$ NR2B was determinedwith HRP-linked protein A and the ECL kit. Quantification wasperformed using a computerized densitometer and image analyzer(Molecular Dynamics, Sunnyvale, CA).

Immunocytochemistry. Rats were anesthetized with Equithesin as above and perfused transcardially with 200 ml PBS at ambienttemperature and then with 2.5% paraformaldehyde in cold PBS containing5% sucrose, pH 7.4. The brain was removed immediately after theperfusion and placed overnight in a fixative containing 1% paraformaldehydein PBS and 30% sucrose. Fifty-micrometer-thick sections were cutusing a freezing microtome and put in 0.01% sodium azide in PBSin a 24-well plate and kept at 4°C until they were used. The sectionswere washed three times, 5 min each, in PBS and then treated with0.9% H₂O₂ in 50% methanol in PBS for 30 min. The sections werewashed five times in PBS as above and immersed for 15 min in 0.15M glycine in PBS, pH 7.4. Then they were blocked with 20% normalgoat serum (NGS) in PBS and 0.5% Triton X-100 for 1-3 hr at 37°C.After they were blocked, the sections were incubated with $alpha$ NR2B(1:500 in 2% NGS in PBS) overnight at room temperature. For control,2% NGS was used in the absence of $alpha$ NR2B. Sections were washedthree times and incubated for 1.5 hr with 1:200 biotinylated goatanti-rabbit in 2% NGS. Then they were washed three times as aboveand incubated for 1.5 hr with avidin-biotin complex. The sectionswere washed once in PBS and twice in 50 mM Tris-Cl, pH 7.4. Antibodybinding was visualized using a DAB peroxidase substrate tabletset. The sections were mounted on gelatinized slides, dried, counterstainedwith hematoxylin, dehydrated in alcohol, and covered with Permount.

In situ hybridization. Levels of NR2B mRNA were examined in brain sections using in situ hybridization of a ³⁵S-labeled cRNA probe complementary to residues 4069-4560 of theC terminal of NR2B mRNA. The antisense cRNA was transcribed froma NdeI-linearized pBluescript KS/NR2B (S. Nakanishi, Kyoto University), with T₇ RNA polymerasein the presence of ³⁵S-UTP. The brain was removed rapidly and frozen on dry ice. Brainsections (30 µm) mounted on gelatinized slides were dried for2 min at 52°C and then fixed in 4% paraformaldehyde for 20 minat room temperature, rinsed in PBS for 5 min, and reacted with0.25% acetic anhydride in 0.1 M triethanolamine for 10 min atroom temperature. The sections were rinsed in PBS and dehydratedby successive rinses in 70%, 80%, 95%, and 100% ethanol. The slideswere then dried for 1 hr at room temperature. The sections werehybridized with the ³⁵S-labeled NR2B cRNA in hybridization solution at 47°C for 12 hr.After hybridization, the sections were incubated in the followingsolutions: 5× SSC, 10 mM DTT at 50°C for 30 min; 50% formamide,2× SSC, 100 mM DTT at 65°C for 20 min and ×3 in washing solution(5 mM EDTA, 0.4 M NaCl in 10 mM Tris-Cl, pH 7.5) at 37°C for 15min each. This was followed by incubation with 20 mg RNase A inwashing solution at 37°C for 30 min, washing solution at 37°Cfor 15 min, then 2× SSC at 37°C for 15 min, and finally 0.1× SSCat 37°C for 15 min. The sections were dehydrated in ethanol/0.3M ammonium acetate series: 30%, 60%, 80%, and 95%. Slides werewashed in 100% ethanol, dried, dipped in Kodak NTB-2 emulsionat 45°C, and stored for 7 d at 4°C in a light-tight box. Developingwas in Kodak D-19 for 2 min, followed by incubation in 1% aceticacid for 1 min, Kodak X-ray fixer (AL4) for 4 min, and water for5 min at 16°C followed by 6 × 5 min at room temperature. The slideswere lightly stained with hematoxylin/eosin as a counterstain.

RESULTS

The effect of taste learning on the tyrosine phosphorylation of NR2B in the insular cortex
In rats sampling an unfamiliar taste and hence learning about it, either incidentally or in the context of CTA, tyrosine phosphorylationof a set of proteins in the insular cortex but not in other brainareas is specifically increased (Rosenblum et al., 1995). Themajor modulated proteins are of MW 100, 115, and 180 kDa (ibid)(Fig. 1A). We now have established that a 180 kDa phosphoprotein,which is the most prominent member of the aforementioned set,is NR2B. This was determined by subjecting rats to taste learningand then quantitatively immunoblotting the tyrosine phosphorylatedfraction, isolated from the insular cortex by affinity chromatographyon an $alpha$ PY-resin, with $alpha$ NR2B (Fig. 1B). Mere intraperitoneal injectionof LiCl, i.e., the UCS used in CTA training, had no effect (Fig.1A-C). The effect of taste experience on the tyrosine phosphorylationof the 180 kDa polypeptide was similar regardless of whether $alpha$ PYor $alpha$ NR2B was used on the blot. In the set of experiments summarizedin Figure 1C, the ratio of tyrosine phosphorylation in saccharin-experiencedrats to that in water-experienced rats (S/W) was 1.60 ± 0.11 (n= 7) using $alpha$ PY and 1.63 ± 0.15 (n = 11) using $alpha$ NR2B. The totallevel of NR2B in the insular homogenate before purification onthe $alpha$ PY affinity resin was not altered by experience: S/W = 1.05± 0.06 (n = 8). Assuming that the $alpha$ PY affinity resin retains tyrosine-phosphorylatedNR2B whether it is phosphorylated on one or more tyrosine residues,one may infer from the above data that the increase in tyrosinephosphorylation is attributable to an increase in the number ofphosphorylated receptor molecules rather than merely an increaseof phosphorylation on already phosphorylated molecules.
Fig. 1. The effect of gustatory experience on the tyrosine phosphorylation of NR2B in the insular cortex. A, Electrophoretogram offractions from the insular cortex of rats subjected to gustatoryand/or visceral experience, eluted from $alpha$ PY affinity resin andimmunoblotted with $alpha$ PY. Eff, Fraction washed from the resin inthe application buffer; Elu, fraction eluted with PNPP; Wash,fraction washed before PNPP elution. For experimental proceduressee Materials and Methods. LiCl, Sample from the insular cortexof rats injected intraperitoneally with LiCl, without previousexposure to a novel taste; Water, rats drinking water (used asfor determining basal level of tyrosine phosphorylation afterdrinking a familiar solution); Sacch, rats drinking an unfamiliartaste, saccharin; CTA, rats trained on CTA using saccharin asthe unfamiliar taste. B, Same as in A but immunoblotted with $alpha$ NR2B;C, summary of data from experiments like those depicted in A (PY)and B (NR2B) above. Open bar, LiCl; black bar, CTA; gray bar,Sacch. Water was used as control. Values are mean ± SEM; n = 3-6each; * p < 0.04.
[View Larger Version of this Image (34K GIF file)]

The effect of the unfamiliar taste on tyrosine phosphorylation was not confined to saccharin. A similar increase in tyrosinephosphorylation of NR2B in the insular cortex was detected aftera drink for the first time of a solution of 0.6% NaCl (1.65-foldincrease in tyrosine phosphorylation of NR2B relative to waterintake, two experiments) or 1.0% monosodium glutamate (1.56-foldincrease, one experiment).

CTA and tyrosine phosphorylation of NR2B as a function of the amount of unfamiliar taste consumed
The effect of experiencing the unfamiliar taste on the tyrosine phosphorylation of NR2B was found to depend on the dose ofthe taste consumed: maximal phosphorylation was obtained aftera consumption of ~5 ml of saccharin (Fig. 2). A similar dose-responsecurve was obtained for the dependence of CTA behavior on the amountof saccharin consumed in training (Fig. 2).
Fig. 2. Tyrosine phosphorylation on NR2B and CTA memory as a function of the amount of saccharin (i.e., the unfamiliar taste) consumedduring CTA training. Open circles, Aversion index; closed circles,fold increase in tyrosine phosphorylation at 10 min after thecompletion of CTA training. A different group of animals was usedfor each data point (n = 6-10 each).
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Tyrosine phosphorylation of NR2B as a function of familiarity with the taste
The question was asked whether familiarity with the taste decreases the effect of drinking it on tyrosine phosphorylation.From behavioral experiments it is known that familiarity witha taste diminishes the ability of that same taste to serve asthe conditioned stimulus in CTA. This is an instance of the moregeneral phenomenon of latent inhibition, in which memory of asensory stimulus diminishes the ability of that same stimulusto serve as associative stimulus in subsequent learning (Lubow,1989). A single preexposure to saccharin indeed significantlydecreased the effectiveness of subsequent CTA training with saccharin;the same preexposure also significantly decreased the effect ofdrinking the saccharin solution on tyrosine phosphorylation ofNR2B in the insular cortex (Fig. 3).
Fig. 3. Tyrosine phosphorylation on NR2B (PY on NR2B) and CTA memory (Aversive behavior) as a function of the familiarity of the tasteconsumed during training. Left, inset, A representative blot ofsamples immunoblotted with $alpha$ NR2B. Water, Rats receiving wateronly; Pre (open bar), rats preexposed once to 15 min of saccharindrinking, 24 hr before the experiment; Saccharin (closed bar),rats sampling saccharin for the first time. Magnitude was theintensity of ECL reaction on the immunoblot; control was drinkingwater instead of saccharin. Values are mean ± SEM; * p < 0.01(n = 5 experiments). Right, Rats were trained on CTA using saccharineither as a novel taste (closed bar) or 24 hr after a 15 min preexposureto it (open bar). Magnitude was the aversion index. Control wassubstitution of saccharin with water on the preexposure day. Valuesare mean ± SEM; * p < 0.01 (n = 4 animals).
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The effect of an NMDA receptor antagonist in the insular cortex
To determine whether the NMDA receptor in the insular cortex is necessary for taste learning, we locally microinjected anNMDA receptor antagonist, APV (Watkins and Olverman, 1987), inthat cortex either before exposure to the novel taste or beforeintraperitoneal injection of the LiCl in CTA training. APV inthe insular cortex during training impaired subsequent CTA memory,without impairing sensory, motivational, or motor abilities requiredfor proper reaction to the taste solution and for expression ofmemory once it has been formed (Fig. 4). Furthermore, the effecton CTA was not observed when the APV was injected 2 mm above theGC (Fig. 4).
Fig. 4. Effect of the NMDA receptor antagonist APV in the insular cortex on CTA memory. The antagonist was microinjected into thecortex as described in Materials and Methods before or in CTAtraining (C) or before testing, 3 d after training (T). Open bar,Microinjection of ACSF as control; black bar, 10 µg APV, 30 minbefore exposure to saccharin; dark shaded bar, 10 µg APV, 30 minbefore LiCl injection in CTA training. Light shaded bar, APV microinjected2 mm above the coordinates used for injection into the insularcortex. Values are mean ± SEM; n = 8; * p < 0.01.
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Although APV in the insular cortex impaired CTA when injected into the insular cortex before and during training as above,it had no effect on the tyrosine phosphorylation of NR2B inducedby the novel taste (S/W = 2.0 ± 0.1 vs 1.8 ± 0.2 in control vsAPV-injected rats, respectively; n = 4 in each of the four groupsof rats used in this comparison).

Localization of NR2B mRNA and protein in the insular cortex
We used an RNA-labeled probe complementary to the C-terminal sequence of the NR2B to identify the anatomical localizationof the NR2B message in cortex. Confirming earlier observations(Monyer et al., 1994), the mRNA was observed all over the cortex,with layers II-III displaying especially heavy staining. A continuumwas observed from the piriform cortex dorsally throughout thecortex, including the insular and taste areas (Fig. 5A). To obtaininformation on the localization of the NR2B-expressed polypeptide,we performed an immunocytochemical analysis. Variability was revealedbetween different cortical regions, with heavier staining in thecingulate, retrosplenial, and motor areas (data not shown). Inthe insular cortex there was a low number of heavily stained neurons,especially in layers II-III (Fig. 5B). Many of these were multipolar,possibly GABAergic interneurons (Fig. 5C), similar to the situationobserved in the hippocampal formation (K. Rosenblum, G. Richter-Levin,and Y. Dudai, unpublished observations). In addition, there wasstaining of large pyramidal cells in layer V, sometimes includingtheir apical dendrites, with the number of these neurons increasingafter moving rostrally from the agranular cortex to the granularinsular cortex (data not shown).
Fig. 5. Localization of NR2B in the insular cortex. A, Dark-field picture of a coronal section showing in situ hybridization withan RNA-labeled probe complementary to a C-terminal sequence ofNR2B. Scale bar, 500 µm. B, A coronal section of the insular corticalarea of rat brain after immunocytochemistry performed with $alpha$ NR2B.In both A and B, the arrow indicates the rhinal fissure. Scalebar, 150 µm. C, A typical multipolar neuron stained for $alpha$ NR2Bin the insular cortex. Scale bar, 20 µm.
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DISCUSSION
In this work we demonstrate that the NMDA receptor is involved in taste learning in the insular cortex of the behaving ratand describe two facets of this involvement. The first is theneed for NMDA receptor activity in CTA learning (but not in retrievalof CTA memory once it has been formed), and the second is thecorrelation of the tyrosine phosphorylation of NR2B with the noveltyof the learned taste stimulus.

Previous authors differ with respect to their conclusions on the role of NMDA receptors in central gustatory plasticity (Welzlet al., 1990; Willner et al., 1992; Aguado et al., 1994; Caramanosand Shapiro, 1994; Fanslow et al., 1994). These studies used eitherintraperitoneal or intracerebroventricular administration of NMDAligands, which are problematic as far as the delineation of thetarget area is concerned, whereas we have used direct, local applicationof the antagonist into the insular cortex. Furthermore, NMDA receptorsare expected to be required for some but not other facets of learning,even within a single paradigm, and hence their unveiled role maydiffer according to the protocol used and the variables measured(Caramanos and Shapiro, 1994; Fanslow et al., 1994; Bannermanet al., 1995). Our data show that the function of the NMDA receptorin the insular cortex is obligatory for taste learning and furthermorethat it may also contribute to a representation of the UCS orto an interaction of the representations of the CS and UCS incortex. An association of the CS and UCS in CTA can happen inthe absence of a functional insular cortex and probably takesplace in subcortical areas (Bures et al., 1988; Yamamoto et al.,1994; Schafe et al., 1995), but this does not contradict the possibilitythat under normal conditions the cortex does foster an effectiveinteraction of the representations of taste and malaise.

The present report extends our previous observation that the sampling of a novel taste, either incidentally or in the contextof CTA training, is correlated with tyrosine phosphorylation inthe insular cortex but not in other brain areas (Rosenblum etal., 1995), and establishes that the major protein so modulatedis NR2B. Furthermore, our results demonstrate that tyrosine phosphorylationof NR2B is a function of the novelty and intensity, hence saliency,of the taste stimulus, properties that also determine the efficacyof a taste stimulus as a conditioned stimulus in CTA. NR2B haspreviously been shown to undergo tyrosine phosphorylation (Moonet al., 1994; Lau and Huganir, 1995). Our data thus establishthat this post-translational modification takes place in brainin vivo, in the behaving rat, in response to a physiological stimuluswithin the context of a natural learning situation, in a corticalarea that is expected to process the relevant sensory stimulusand subserve its storage.

Protein tyrosine phosphorylation has been implicated in short-term neuronal plasticity (O'Dell et al., 1991; Grant et al.,1992; Abe and Saito, 1993). The enhancement in tyrosine phosphorylationinduced by taste in the insular cortex was previously shown byus to occur within minutes and last for hours (Rosenblum et al.,1995); it is hence a candidate molecular mechanism for short-termmemory and for processes that subserve consolidation of short-into long-term taste memory (Dudai, 1996). This mechanism is apparentlyrelated to the memory of taste but not of the taste-malaise association,because the UCS did not significantly augment the tyrosine phosphorylationafter the CS. Hippocampal LTP, a candidate cellular plasticitymechanism in the CNS, is also correlated with an increase of tyrosinephosphorylation of NR2B that lasts for several hours and may subserveshort and intermediate maintenance of LTP (Rosenblum et al., 1996b;Rostas et al., 1996). Therefore it is tempting to suggest thatmechanisms similar to those operating in LTP also take place inthe insular cortex in response to a novel taste stimulus.

In cultured mammalian neurons, the function of the NMDA receptor channel is regulated by protein tyrosine kinases (Wang andSalter, 1994), e.g., src (Yu et al., 1997), and by protein phosphatases(Wang et al., 1994; Tong et al., 1995). Köhr and Seeburg (1996)suggest that the increase in glutamate-activated currents inducedby src and fyn kinases in cultured HEK 293 embryonic kidney cellsis mediated via tyrosine phosphorylation of NR2A and not NR2B,but even if this proves to hold for cortical neurons in vivo,the possibility should be considered that the effect of tyrosinephosphorylation of NR2B is not necessarily reflected in channelproperties, but rather in altered function of an intracellularsignal transduction machinery interfacing with the receptor (e.g.,Niethammer et al., 1996; see discussion in Rosenblum et al., 1996b).Altered interaction with other PSD proteins may play a role insuch regulation (Kornau et al., 1995; Gomperts, 1996; Muller etal., 1996; Niethammer et al., 1996). Some of the components ofsuch multiprotein functional conglomerates may be the 100 and115 kDa polypeptides, whose tyrosine phosphorylation is modulatedin cortex and hippocampus together with that of NR2B (Rosenblumet al., 1995, 1996b).

Although the NMDA receptor in the insular cortex was found necessary for taste learning, its function was not obligatory forthe tyrosine phosphorylation of the 2B subunit. On the basis ofthis functional dissociation, the correlation between noveltyand amount of taste and the tyrosine phosphorylation of NR2B,and the time course of the effect (Rosenblum et al., 1995), wepropose that tyrosine phosphorylation of NR2B is related to theencoding of saliency in the cortex during the first hours afteran unfamiliar taste is sampled and that this encoding is independentof another, necessary role of NMDA receptors, probably relianton receptor-mediated channel activity, in triggering experience-dependentmodifications in the insular cortex during taste learning. Thesaliency or contextual encoding is expected to involve non-NMDAglutamatergic receptors or other neuromodulatory receptors. Appealingcandidates are cholinergic receptors in cortex, because transientimpairment of cholinergic function in the insular cortex disruptsthe encoding of information on novel tastes (Naor and Dudai, 1996),and microinjection of carbachol into the insular cortex enhancestyrosine phosphorylation of NR2B (Rosenblum et al., 1996a). Aplausible model is thus that activation of the cholinergic systemby contextual saliency leads to acetylcholine receptor-inducedincrease in Ca²⁺ influx in cortical neurons (Cox et al., 1994; Lev et al., 1995),resulting in activation of protein kinase(s) such as members ofthe src family mentioned above (Kohr and Seeburg, 1996) or thefak family (Lev et al., 1995), and culminating in enhanced phosphorylationof a set of substrates, including NR2B. This might be a molecularmanifestation of the cross-talk of the glutamatergic and cholinergicsystems in cortex, a cross-talk that is proposed to play a prominentfunction in learning and attention (Aigner, 1995).

It is not unlikely that the two roles of NMDA receptor in CTA described in the present report involve two subtypes of receptor,only one of which may contain the post-translationally modifiedNR2B. In this respect it is of interest to note that our immunocytochemicalanalysis unveils the presence of NR2B in cortical interneuronsand that in the dentate gyrus, the NR2B protein is preferentiallylocated in GABAergic interneurons and may play a role in modulatinglocal circuit inhibition (K. Rosenblum, G. Richter-Levin, andY. Dudai, unpublished observations). A previous immunocytochemicalanalysis of the distribution of the NMDA receptor protein in therat brain identified the NR2B in cortex, especially in outer layers,but no information was provided on higher resolution of corticaltissue and on the identity of stained cells (Wenzel et al., 1995).The issue of discrepancies between NR2B mRNA and NR2B proteinlocalization in the brain (Wenzel et al., 1995) (K. Rosenblum,D. E. Berman, and Y. Dudai, unpublished observations), and thepossibility of post-transcriptional regulation of expression suchas that suggested for NR2A (Wood et al., 1996), await furtherinvestigation. Nevertheless, if experience-dependent tyrosinephosphorylation of NR2B in insular cortex takes place on interneurons,the possibility arises that saliency may regulate inhibition ofcortical circuits.

FOOTNOTES

Received Feb. 26, 1997; revised April 8, 1997; accepted April 11, 1997.

The support of the Carl Dominic Center for Brain Research is gratefully acknowledged. We thank E. Soriano for advice on theimmunocytochemical analysis and T. V. P. Bliss for helpful commentson this manuscript.

Correspondence should be addressed to Dr. Yadin Dudai, Department of Neurobiology, The Weizmann Institute of Science, Rehovot76100, Israel.

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