Lower Sensitivity to Stress and Altered Monoaminergic Neuronal Function in Mice Lacking the NMDA Receptor epsilon 4 Subunit

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The Journal of Neuroscience, March 15, 2002, 22(6):2335-2342

Lower Sensitivity to Stress and Altered Monoaminergic Neuronal Function in Mice Lacking the NMDA Receptor $epsilon$ 4 Subunit
Yoshiaki Miyamoto¹, Kiyofumi Yamada¹, Yukihiro Noda¹, Hisashi Mori², Masayoshi Mishina², and Toshitaka Nabeshima¹
¹ Department of Neuropsychopharmacology and Hospital Pharmacy, Nagoya University Graduate School of Medicine, Showa-ku, Nagoya 466-8560, Japan, and ² Department of Molecular Neurobiology and Pharmacology, School of Medicine, University of Tokyo, Bunkyou-Ku, Tokyo 113-0033, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

NMDA receptors, an ionotropic subtype of glutamate receptors (GluRs), play an important role in excitatory neurotransmission,synaptic plasticity, and brain development. They are composedof the GluR $zeta$ subunit (NR1) combined with any one of four GluR $epsilon$ subunits (GluR $epsilon$ 1-GluR $epsilon$ 4; NR2A-NR2D). Although the GluR $zeta$ subunitexists in the majority of the CNS throughout all stages of development,the GluR $epsilon$ subunits are expressed in distinct temporal and spatialpatterns. In the present study, we investigated neuronal functionsin mice lacking the embryonic GluR $epsilon$ 4 subunit. GluR $epsilon$ 4 mutant miceexhibited reductions of [³H]MK-801 [(+)-5-methyl-10,11-dihydro-5H-dibenzo [a,d] cyclohepten-5,10-iminemaleate] binding and ⁴⁵Ca²⁺ uptake through the NMDA receptors. The expression of GluR $zeta$ subunitprotein, but not GluR $epsilon$ 1 and GluR $epsilon$ 2 subunit proteins, was reducedin the frontal cortex and striatum of the mutant mice. A postmortemexamination in GluR $epsilon$ 4 mutant mice revealed that tissue contentsof norepinephrine, dopamine, serotonin, and their metaboliteswere reduced in the hippocampus and that dopamine, as well asserotonin, metabolism was upregulated in the frontal cortex, striatum,hippocampus, and thalamus. To clarify the phenotypical influencesof the alteration in neuronal functions, performances in variousbehavioral tests were examined. GluR $epsilon$ 4 mutant mice showed reducedspontaneous locomotor activity in a novel environment and lesssensitivity to stress induced by the elevated plus-maze, light-darkbox, and forced swimming tests. These findings suggest that GluR $epsilon$ 4mutant mice have dysfunctional NMDA receptors and altered emotionalbehavior probably caused by changes in monoaminergic neuronalactivities inadulthood.

Key words: NMDA receptor; GluR $epsilon$ 4 subunit; GluR $zeta$ subunit; monoaminergic neuronal systems; locomotor activity; emotional behavior

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glutamate receptors (GluRs) play an important role in excitatory neurotransmission, synaptic plasticity, neuronal development,and neurodegenaration of the CNS. They are divided in two generalgroups: ionotropic GluRs form ligand-gated cation channels andare subdivided into NMDA, AMPA, and kainate receptors, whereasmetabotropic GluRs link G-protein that modulates the productionof intracellular messengers (Hollmann and Heinemann, 1994; Nakanishiand Masu, 1994; Pin and Duvoisin, 1995).

NMDA receptors are thought to be a critical subtype mediating glutamate actions in the CNS. They are coupled with inherenthigh Ca²⁺-permeable channels, which are formed by assembly of the GluR $zeta$ subunit (NR1) and any one of four GluR $epsilon$ subunits (GluR $epsilon$ 1-Glu $epsilon$ R4;NR2A-NR2D). Although the GluR $zeta$ subunit exists in the brain atall developmental stages, the GluR $epsilon$ subunits are expressed indistinct temporal and spatial patterns (Mayer and Westbrook, 1987;Hollmann and Heinemann, 1994; Nakanishi and Masu, 1994). PrenatalNMDA receptors include the GluR $epsilon$ 2 and/or GluR $epsilon$ 4 subunit, whereasthe GluR $epsilon$ 1 and GluR $epsilon$ 3 subunits appear only after birth, the formerbeing expressed predominantly in the forebrain and the lattermainly in the cerebellum (Watanabe et al., 1992; Monyer et al.,1994). Thus, the GluR $epsilon$ subunits provide the molecular diversityin NMDA receptors during development and in various regions ofthebrain.

The physiological significance of NMDA receptor subunits has been demonstrated in knock-out mice. Although disruption of theGluR $epsilon$ 2 subunit caused perinatally death (Kutsuwada et al., 1996),mice lacking the embryonic GluR $epsilon$ 4 subunit are viable and exhibitreduced spontaneous locomotor activity (Ikeda et al., 1995). Theimpairment of spatial and contextual learning was demonstratedin GluR $epsilon$ 1 mutant mice (Sakimura et al., 1995; Kiyama et al., 1998),but no deficits were observed in GluR $epsilon$ 3 mutant mice (Ebralidzeet al., 1996). GluR $zeta$ mutant mice showed a deficit of all NMDAreceptors and perinatal death (Forrest et al., 1994; Li et al.,1994). These findings suggest that the GluR $epsilon$ subunits are majordeterminants of the functional properties of NMDA receptors, whereasthe GluR $zeta$ subunit is an essential molecule in functional NMDAreceptors and in braindevelopment.

Accordingly, we investigated the alteration of neuronal functions in mice lacking NMDA receptor subunits. In GluR $epsilon$ 1 mutantmice, NMDA receptor function was significantly reduced, but thedopaminergic neuronal activity was increased because of disinhibitionof inhibitory GABAergic input. Furthermore, GluR $epsilon$ 1 mutant miceshowed an enhancement of locomotor activity in a novel environment,which is attributed to hyperfunction of dopaminergic neuronalsystem (Miyamoto et al., 2001). In the present study, we investigatedthe alteration of neuronal functions in adult mice lacking theembryonic GluR $epsilon$ 4 subunit. [³H]MK-801 [(+)-5-methyl-10,11-dihydro-5H-dibenzo [a,d] cyclohepten-5,10-iminemaleate] binding and ⁴⁵Ca²⁺ uptake through the NMDA receptors were measured to elucidatethe role of the GluR $epsilon$ 4 subunit in NMDA receptor function. Becausethe functional alteration of NMDA receptors in vivo has been reportedto affect monoaminergic neuronal function and behavior (Hiramatsuet al., 1989; Imperato et al., 1990; Miller and Abercrombie, 1996),monoamine metabolism, locomotor activity, and emotional behaviorin GluR $epsilon$ 4 mutant mice were alsoassessed.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. Mutant mice lacking the GluR $epsilon$ 4 subunit of NMDA receptors were provided by Prof. M. Mishina (Ikeda et al., 1995).The homozygous GluR $epsilon$ 4 mutant ( $-$ / $-$ ; 3 months old) and the wild-type(+/+; 3 months old) mice used in this study were obtained by crossingF11 heterozygous GluR $epsilon$ 4 mutant mice (+/ $-$ ) having a 99.99% pureC57BL/6 genetic background. The genotypes of mice were determinedby Southern blotting analyses of tail DNA as described by Ikedaet al. (1995). The animals were housed in plastic cages and werekept in a regulated environment (24 ± 1°C, 50 ± 5% humidity),with a 12 hr light/dark cycle (lights on at 9:00 A.M.). Food andtap water were available ad libitum. All experiments were performedin accordance with the Guidelines for Animal Experiments of theNagoya University School of Medicine. The procedures involvinganimals and their care were conducted in conformity with the internationalguidelines Principles of Laboratory Animal Care (National Institutesof Health publication 85-23, revised1985).

[³H]MK-801 binding. The GluR $epsilon$ 4 mutant mice and the wild-type mice were killed by decapitation, and brains were quickly removedand placed on an ice-cold glass plate. The forebrain (whole brainminus the cerebellum and brainstem) was rapidly dissected out,frozen, and stored in a deep freezer at $-$ 80°C until assayed. [³H]MK-801 binding was measured as described previously (Yonedaand Ogita, 1989, 1991), with a minor modification (Miyamoto etal., 2001). Briefly, frozen samples were thawed at room temperatureand homogenized in 40 vol of 50 mM Tris-acetate buffer, pH 7.4,containing 1 mM EDTA using a Physcotron homogenizer. All additionalprocedures were performed at 4°C. The homogenates were centrifugedat 40,000 × g for 30 min, and resultant pellets were washed threetimes with the same volume of 50 mM Tris-acetate buffer. The finalpellets were suspended in 30 vol of 0.32 M sucrose, and the suspensionswere frozen at $-$ 80°C for no longer than 1 week until use. On theday of the experiments, the frozen suspensions were thawed atroom temperature and treated with 0.08% Triton X-100 at 4°C (anapproximate protein concentration of 0.32 mg/ml) for 10 min withgentle stirring. The treatment was terminated by centrifugationat 40,000 × g for 30 min, and pellets were washed five times with40 vol of 50 mM Tris-acetate buffer, followed by centrifugationat 40,000 × g for 30 min. For determination of [³H]MK-801 binding, an aliquot (0.3 mg of protein) of the membranepreparations was incubated, in the presence or absence of glutamate(10 µM), glycine (10 µM), and spermidine (1 mM), with 5 nM (+)[3-³H]MK-801 (22.5 Ci/mmol; NEN Life Science Products, Boston, MA)in a total volume of 0.5 ml of 50 mM Tris-acetate buffer at 30°Cfor 16 hr. The incubation was terminated by the addition of 3ml of ice-cold 50 mM Tris-acetate buffer and subsequent filtrationthrough a Whatman GF/B glass filter under a constant vacuum. Thefilter was rinsed with the same volume of ice-cold 50 mM Tris-acetatebuffer three times within 10 sec. The radioactivity retained onthe filter was measured by liquid scintillation spectrophotometry,at a counting efficiency of 57-59%. Nonspecific binding was determinedwith 0.1 mM cold (+)MK-801 (Sigma, St. Louis, MO), and the specificbinding accounted for >60% of the total binding found in the absenceof cold (+)MK-801.

⁴⁵Ca²⁺ uptake. ⁴⁵Ca²⁺ uptake through the NMDA receptors was measured as described by Miyamoto et al. (2001). The GluR $epsilon$ 4 mutant miceand the wild-type mice were killed by decapitation, the brainswere quickly removed, and the forebrain (whole brain minus thecerebellum and brainstem) was dissected out on an ice-cold glassplate. The forebrains were homogenized in 20 vol of ice-cold 0.32M sucrose at 4°C in a Teflon glass homogenizer. All additionalprocedures were performed at 4°C. The homogenates were centrifugedat 1000 × g for 10 min. The supernatants were collected and thendiluted 1:1 with basal buffer of the following composition (inmM): 135 NaCl, 5 KCl, 1 CaCl₂, and 10 HEPES, pH adjusted to 7.4with Tris base, and centrifuged at 10,000 × g for 15 min. Thepellets were resuspended in basal buffer and used for the ⁴⁵Ca²⁺ uptake assay. The synaptosome suspension (0.5 mg of protein)was preincubated in a total volume of 450 µl of basal buffer,in the presence or absence of (+)MK-801 (100 µM), at 37°C for10 min. The ⁴⁵Ca²⁺ uptake assay was initiated by adding 50 µl of prewarmed basalbuffer containing 1 µCi/ml ⁴⁵CaCl₂ (18.1 mCi/mg; NEN Life Science Products), in the presenceor absence of NMDA (100 µM), glycine (10 µM), and spermidine (1mM) or high K⁺ (45 mM; isomolar replacement of NaCl with KCl). The reactionwas terminated after 5 min by adding 3 ml of ice-cold basal buffer.The mixture was rapidly filtered under vacuum over Whatman GF/Bglass filters, and the filters were rinsed twice with 3 ml ofbasal buffer. The radioactivity was determined by liquid scintillationspectrophotometry at a counting efficiency of 90%. Ca²⁺ uptake was defined by subtracting the uptake at 4°C.

Western blot analysis. The GluR $epsilon$ 4 mutant mice and the wild-type mice were killed by decapitation, the brains were quicklyremoved, and the frontal cortex, striatum, hippocampus, and thalamuswere dissected out on an ice-cold glass plate according to themethod of Glowinski and Iversen (1966). Each section was homogenizedwith an ultrasonic processor in 10 vol of buffer (10 mM Tris-Cl,pH 7.2, 5 mM EDTA, 0.32 M sucrose, 1 mM phenylmethylsulfonyl fluoride,and 10 mg/l leupeptin) within 3 min of decapitation. The homogenateswere centrifuged at 1000 × g for 10 min at 4°C to obtain a postnuclearfraction. Protein determinations were made by the method of Lowryet al. (1951). The supernatants of 50 µg of protein were electrophoresedin a 7.5% SDS-polyacrylamide gel, transferred to polyvinylidenedifluoride membrane, and incubated with a 1:1000 dilution of GluR $zeta$ ,GluR $epsilon$ 1, or GluR $epsilon$ 2 polyclonal antibody (Santa Cruz Biotechnology,Santa Cruz, CA). Antibody binding was detected by peroxidase-labeledsecondary antibodies and the ECL detection kit (Amersham Biosciences,Arlington Heights, IL). The films were quantitated with adensitometer.

Contents of monoamines and their metabolites. The GluR $epsilon$ 4 mutant mice and the wild-type mice were killed by focused microwaveirradiation for 1.5 sec at 5 kW, the brains were quickly removed,and the frontal cortex, striatum, hippocampus, and thalamus weredissected out on an ice-cold glass plate according to the methodof Glowinski and Iversen (1966). Each section was rapidly frozenand stored in a deep freezer at $-$ 80°C until assayed. The contentsof monoamines and their metabolites were determined using an HPLCsystem with an electrochemical detector (Eicom, Kyoto, Japan),as described by Noda et al. (1998), with a minor modification(Miyamoto et al., 2001). Briefly, each frozen brain sample wasweighed and homogenized with an ultrasonic processor in 350 µlof 0.2 M perchloric acid containing isoproterenol as an internalstandard. The homogenates were placed on ice for 30 min and centrifugedat 20,000 × g for 15 min at 4°C. The supernatants were mixed with1 M sodium acetate to adjust the pH to 3.0 and injected into anHPLC system equipped with a reversed-phase ODS-column (EicompakMA-5 ODS; 4.6 × 150 mm; Eicom) and an electrochemical detector.The column temperature was maintained at 25°C, and the detectorpotential was set at +750 mV. The mobile phase was 0.1 M citricacid and 0.1 M sodium acetate, pH 3.6, containing 14% methanol,180 mg/l sodium-L-octanesulfonate, and 5 mg/l EDTA, and the flowrate was set at 1 ml/min. The turnover of monoamines was calculatedfrom the concentrations of each monoamine and itsmetabolite.

Behavioral analyses. To measure locomotor activity in a novel environment, a mouse was placed in a transparent acrylic cagewith a black frosting Plexiglas floor (45 × 26 × 40 cm), and locomotionand rearing were measured every 5 min for 30 min using digitalcounters with infrared sensors (Scanet SV-10; Toyo Sangyo Co.Ltd., Toyama,Japan).

The elevated plus-maze consisted of two open (25 × 8 × 0.5 cm) and two closed (25 × 8 × 20 cm) arms emanating from a commoncentral platform (8 × 8 cm) to form a plus shape (Yamada et al.,2000). The entire apparatus was elevated to a height of 50 cmabove floor level. The test was started by placing a mouse onthe central platform of the maze facing an open arm, and a 5 mintest duration was used. Conventional parameters consisted of thefrequency of entry to open and closed arms. These data were usedto calculate the percentage of open arms entries [i.e., (openarms entries/open and closed arms entries) × 100].

The light-dark box consisted of two compartments: a transparent Plexiglas box with a white frosting Plexiglas floor and ablack Plexiglas box with a black frosting Plexiglas floor (both15 × 15 × 15 cm). Each box could be divided by a sliding door(10 × 5 cm high). The test was started by placing a mouse in theblack Plexiglas box. The amounts of time spent in the transparentand black Plexiglas boxes was measured for 10 min using digitalcounters with infrared sensors (Scanet SV-10 LD; Toyo Sangyo Co.Ltd.). These data were used to calculate the percentage of timespent in the light box [i.e., (time spent in transparent Plexiglasbox/time spent in transparent and black Plexiglas boxes) × 100].

In the forced swimming test, a mouse was placed in a transparent glass cylinder (8 cm in diameter × 20 cm high), which containedwater at 25°C to a depth of 8 cm, and was forced to swim for 10min. The duration of immobility was measured every 1 min usingdigital counters with infrared sensors (Scanet MV-10 AQ; ToyoSangyo Co. Ltd.), as described previously (Noda et al., 1995).

Statistical analysis. All data were expressed as the mean ± SEM. Statistical differences between the GluR $epsilon$ 4 mutant mice andthe wild-type mice were determined with Student's t comparisontest. In the analysis of locomotion and rearing curves, statisticaldifferences between the GluR $epsilon$ 4 mutant mice and the wild-type micewere determined by an ANOVA with repeatedmeasures.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Function of NMDA receptors in adult GluR $epsilon$ 4 mutant mice

To demonstrate the functional changes in NMDA receptors of adult GluR $epsilon$ 4 mutant mice, we first measured the binding activityof [³H]MK-801, which is known as a noncompetitive antagonist for NMDAreceptors, in synaptic membranes of the forebrain (whole brainminus the cerebellum and brainstem) treated with Triton X-100to deplete endogenous amino acids (Fig. 1). The specific bindingof [³H]MK-801 in both wild-type and mutant mice was increased whenthe assay was performed in the presence of activators for NMDAreceptors such as glutamate (10 µM), glycine (10 µM), and spermidine(1 mM). In the presence of glutamate, glutamate plus glycine,or glutamate plus glycine plus spermidine, the specific bindingof [³H]MK-801 was significantly lower in GluR $epsilon$ 4 mutant mice than wild-typemice. Treatment with glycine or spermidine alone did not affectthe basal-specific binding of [³H]MK-801 in either of the mice (data not shown).

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Figure 1. [³H]MK-801 binding in forebrain synaptic membranes of adult GluR $epsilon$ 4 mutant mice. Triton X-100-treated forebrain synaptic membranes were incubated with 5 nM [³H]MK-801 at 30°C for 16 hr, in the presence or absence of 10 µM glutamate (Glu), Glu plus 10 µM glycine (Gly), or Glu plus Gly plus 1 mM spermidine (SPD). Each column represents the mean ± SEM (n = 6). *p < 0.05 and **p < 0.01 versus wild-type (+/+).

We next measured NMDA-stimulated ⁴⁵Ca²⁺ uptake into synaptosomes of the forebrain (whole brain minus the cerebellum and brainstem)(Fig. 2). There was no difference in the basal level of ⁴⁵Ca²⁺ uptake between wild-type (12.7 ± 0.1 nmol/mg protein per 5 min)and GluR $epsilon$ 4 mutant (12.8 ± 0.2 nmol/mg protein per 5 min) mice.When the assay was performed in the presence of NMDA (100 µM),NMDA plus glycine (10 µM), or NMDA plus glycine plus spermidine(1 mM), ⁴⁵Ca²⁺ uptake was increased in both groups. However, there was significantlyless ⁴⁵Ca²⁺ uptake in GluR $epsilon$ 4 mutant mice than in wild-type mice under thesestimulated conditions. The NMDA-, glycine-, and/or spermidine-stimulated⁴⁵Ca²⁺ uptake in both groups was antagonized by the pretreatment withMK-801 (100 µM). On the other hand, there was no difference inhigh K⁺ (45 mM)-stimulated ⁴⁵Ca²⁺ uptake between wild-type (6.5 ± 0.2 nmol/mg protein per 5 min)and GluR $epsilon$ 4 mutant (6.8 ± 0.4 nmol/mg protein per 5 min) mice.The results on [³H]MK-801 binding and NMDA-stimulated ⁴⁵Ca²⁺ uptake suggest that the function of NMDA receptors is reducedin adult GluR $epsilon$ 4 mutant mice.

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Figure 2. NMDA-stimulated ⁴⁵Ca²⁺ uptake into forebrain synaptosomes of adult GluR $epsilon$ 4 mutant mice. The forebrain synaptosomes were preincubated at 37°C for 10 min, in the presence or absence of 100 µM MK-801. The assay was initiated by adding prewarmed buffer containing 1 µCi/ml ⁴⁵CaCl₂ for 5 min, in the presence of 100 µM NMDA, NMDA plus 10 µM glycine (Gly), or NMDA plus Gly plus 1 mM spermidine (SPD). Each column represents the mean ± SEM (n = 8 for $-$ MK-801 group; n = 6 for +MK-801 group). *p < 0.05, **p < 0.01, and ***p < 0.001 versus wild-type ( $-$ MK-801).

Expression of NMDA receptor subunit in adult GluR $epsilon$ 4 mutant mice

As demonstrated above, a defect in the embryonic GluR $epsilon$ 4 subunit results in an impairment of NMDA receptor function in adulthood(3 months old). Because the GluR $epsilon$ 4 subunit is expressed predominantlyat the prenatal stage, but not at the postnatal stage, these findingssuggest that disruption of the GluR $epsilon$ 4 subunit affects the expressionof other GluR subunits composing NMDA receptors in adult animals.To test this possibility, the expression of other subunit proteinsforming NMDA receptors was analyzed by Western blotting in adultGluR $epsilon$ 4 mutant mice (Fig. 3). The amount of GluR $zeta$ subunit protein,an essential molecule for functional NMDA receptors in vivo, wasselectively reduced in the frontal cortex and striatum, but notin the hippocampus and thalamus, of GluR $epsilon$ 4 mutant mice (Fig. 3A).There was no significant difference in GluR $epsilon$ 1 and GluR $epsilon$ 2 subunitprotein levels in any region between wild-type and GluR $epsilon$ 4 mutantmice (Fig. 3B,C). These findings indicate that NMDA receptor subunitcomposition or the amount of functional NMDA receptors may bealtered in adult GluR $epsilon$ 4 mutant mice, which results in the malfunctionof NMDA receptors.

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Figure 3. Expression of NMDA receptor subunit proteins in various regions of the adult GluR $epsilon$ 4 mutant mouse brain. The amount of each NMDA receptor subunit was determined by Western blot analysis using antibodies against GluR $zeta$ , GluR $epsilon$ 1, or GluR $epsilon$ 2. The synaptosomal protein samples were prepared from various regions of the adult GluR $epsilon$ 4 mutant mouse brain. FC, Frontal cortex; HIP, hippocampus; STR, striatum; THA, thalamus. Each column represents the mean ± SEM (n = 4). *p < 0.05 versus wild-type (+/+).

Monoaminergic neuronal function in adult GluR $epsilon$ 4 mutant mice

To investigate whether targeted disruption of the embryonic GluR $epsilon$ 4 subunit gene would affect the function of monoaminergicneuronal systems, the tissue contents of monoamines and theirmetabolites in various regions of the adult GluR $epsilon$ 4 mutant mousebrain were measured (Table 1). A marked reduction of norepinephrine(NE), dopamine (DA), and serotonin (5-hydroxytryptamine; 5-HT)contents, being 53, 22, and 50% of that in wild-type mice, respectively,was evident in the hippocampus of the mutant mice. Metabolitelevels were also reduced in this region. In addition, DA in thefrontal cortex and NE in the striatum decreased significantly,whereas 5-HT in the striatum increased in the mutant mice comparedwith the wild-type mice. To address the functional alterationsof monoaminergic neuronal systems, monoamine metabolism was evaluatedby calculating the ratio of the tissue content of the monoaminesto their metabolites (Fig. 4). The ratio of 3,4-dihydroxyphenylaceticacid (DOPAC) to DA and/or of homovanillic acid (HVA) to DA inthe frontal cortex, striatum, hippocampus, and thalamus was significantlyincreased in GluR $epsilon$ 4 mutant mice compared with wild-type mice (Fig.4A-D). In the same regions, the ratio of 5-hydroxyindoleaceticacid (5-HIAA) to 5-HT was also significantly increased in themutant mice (Fig. 4A-D). In contrast, the ratio of 3-methoxy-4-hydroxyphenylglycol(MHPG) to NE decreased in the frontal cortex and hippocampus (Fig.4A,C), but not in the striatum and thalamus (Fig. 4B,D), of GluR $epsilon$ 4mutant mice. These findings suggest that the activities of monoaminergicneuronal systems are altered in adult GluR $epsilon$ 4 mutant mice as aresult of the disruption of the GluR $epsilon$ 4 subunit gene.


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Table 1. Monoamines and their metabolites contents in various regions of the adult GluR $epsilon$ 4 ( $-$ / $-$ ) mutant mouse brain

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Figure 4. Monoamine metabolism in various regions of the adult GluR $epsilon$ 4 mutant mouse brain. The tissue contents of monoamines and their metabolites in various regions were measured by HPLC with an electrochemical detector. a, MHPG/NE; b, DOPAC/DA; c, HVA/DA; d, 5-HIAA/5-HT. Each column represents the mean ± SEM (n = 8). *p < 0.05 and **p < 0.01 versus wild-type (+/+).

Locomotor activity in adult GluR $epsilon$ 4 mutant mice

Monoaminergic neuronal systems, particularly dopaminergic and serotonergic neuronal activities, are thought to regulate locomotoractivity in animals (Geyer, 1996; Giros et al., 1996; Lucki, 1998;Gainetdinov et al., 1999). To clarify the behavioral influencesof altered monoaminergic neuronal function in adult GluR $epsilon$ 4 mutantmice, the locomotor activity in a novel environment was measuredfor 30 min using digital counters with infrared sensors to recordhorizontal (locomotion) (Fig. 5A) and vertical (rearing) (Fig.5B) activity. Although a time course analysis of locomotor activityrevealed no significant difference between wild-type and GluR $epsilon$ 4mutant mice [F_(1,19) = 0.192, p = 0.9651 (locomotion); F_(1,19)= 1.180; p = 0.3253 (rearing)], total counts for both locomotionand rearing during a 30 min observation period were significantlylower in the mutant mice. These results suggest that GluR $epsilon$ 4 mutantmice show reduced locomotor activity in a novel environment.

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Figure 5. Locomotor activity in a novel environment in adult GluR $epsilon$ 4 mutant mice. Locomotor activity and the number of rearing events in a novel environment were measured every 5 min for 30 min. Each column represents the mean ± SEM (n = 10-11). An ANOVA with repeated measures revealed no difference in the time course of locomotion (F_(1,19) = 0.192; p = 0.9651) and rearing (F_(1,19) = 1.180; p = 0.3253). **p < 0.01 versus wild-type (+/+).

Emotional behavior of adult GluR $epsilon$ 4 mutant mice

We examined the performance of adult GluR $epsilon$ 4 mutant mice in three different paradigms, the elevated plus-maze, light-dark box,and forced swimming tests (Fig. 6), because monoaminergic neuronalsystems are also implicated in the regulation of emotional behavior(Schildkraut, 1965; Kim et al., 1997). In the elevated plus-mazetest, GluR $epsilon$ 4 mutant mice spent significantly more time exploringthe open arms (Fig. 6A) and had more entries into the open arms(GluR $epsilon$ 4 mutant mice, 7.0 ± 0.5 entries per 5 min; wild-type mice,9.3 ± 0.6 entries per 5 min) than did wild-type mice. In the light-darkbox test, GluR $epsilon$ 4 mutant mice spent significantly more time inthe light box than wild-type mice (Fig. 6B). The results in theelevated plus-maze and light-dark box tests suggest a reducedpsychological anxiety in GluR $epsilon$ 4 mutant mice. The immobility timein the forced swimming test decreased in GluR $epsilon$ 4 mutant mice comparedwith wild-type mice (Fig. 6C). Because immobility in this testis considered to reflect behavioral despair to escape from water(Porsolt et al., 1977a,b, 1978), GluR $epsilon$ 4 mutant mice may have anincreased motivation or a reduced susceptibility to stress. Itis unlikely that the reduced immobility is attributable to a hyperactivityof the mutant mice because their locomotor activity is ratherreduced in a novel environment. Thus, our findings on emotionalbehavior indicate that GluR $epsilon$ 4 mutant mice may have a reduced susceptibilityto stress and/or reduced psychological anxiety.

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Figure 6. Emotional behavior of adult GluR $epsilon$ 4 mutant mice. A, Elevated plus-maze test; the frequencies of entries to open and closed arms were recorded for 5 min. B, Light-dark box test; the amounts of time spent in the light and dark boxes were measured for 10 min. C, Forced swimming test; the duration of immobility was measured for 10 min. The data represent the mean ± SEM (n = 8-10). **p < 0.01 and ***p < 0.001 versus corresponding wild-type (+/+).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

NMDA receptors are heteromeric assemblies of the GluR $zeta$ and GluR $epsilon$ subunits, which exhibit characteristic differences in activitiesand properties depending on the GluR $epsilon$ subunits involved, suchas affinity for agonists, channel gating kinetics, unitary conductance,and sensitivity to Mg²⁺, Zn²⁺, and antagonist block (Kutsuwada et al., 1992; Monyer et al.,1992; Ishii et al., 1993). Among GluR $epsilon$ / $zeta$ heteromeric NMDA receptors,the GluR $epsilon$ 4/ $zeta$ 1 assembly has the highest apparent affinities forglutamate and glycine (Ikeda et al., 1992), has a very slow channelgating (Monyer et al., 1994), and is less sensitive to Mg²⁺ block than the GluR $epsilon$ 1/ $zeta$ 1 and GluR $epsilon$ 2/ $zeta$ 1 assemblies (Mishina etal., 1993). These findings suggest that the GluR $epsilon$ 4 subunit playsan important role in synaptic transmission in the early stagesof brain development, because this subunit is abundant in theembryonic diencephalon and abruptly disappears in the postnatalforebrain (Watanabe et al., 1992; Monyer et al., 1994). To demonstratethe physiological significance of the GluR $epsilon$ 4 subunit in vivo,Ikeda et al. (1995) generated mutant mice without this subunitby a gene-targeting recombination technique. In the present study,we investigated the altered neuronal functions of the mutant miceinadulthood.

In [³H]MK-801 binding and ⁴⁵Ca²⁺ uptake through the NMDA receptors under various conditions, an impairment of NMDA receptor functionwas demonstrated in the forebrain (whole brain minus the cerebellumand brainstem) of adult GluR $epsilon$ 4 mutant mice. Furthermore, a reductionin GluR $zeta$ subunit protein, but not GluR $epsilon$ 1 and GluR $epsilon$ 2 subunit proteins,in the frontal cortex and striatum of the mutant mice was alsoevident by Western blot analysis. The expression of the GluR $zeta$ subunit did not change, however, in the hippocampus and thalamus.A similar modification of the GluR subunit expression has beendemonstrated in mice lacking the GluR $zeta$ subunit (Forrest et al.,1994) or overexpressing the GluR $epsilon$ 4 subunit (Okabe et al., 1998).Therefore, it is suggested that the impairment of NMDA receptorfunction in adult GluR $epsilon$ 4 mutant mice is associated with an alterationof NMDA receptor subunit composition, that is, a reduction ofGluR $zeta$ subunit expression in the frontal cortex and striatum attributableto the disruption of the embryonic GluR $epsilon$ 4 subunit. Alternatively,because the GluR $zeta$ subunit is an essential molecule for functionalNMDA receptors in vivo, which are composed by assembly of fouror five GluR subunits, including at least two of the GluR $zeta$ subunits(Laube et al., 1998; Hawkins et al., 1999), the reduction of GluR $zeta$ subunit protein might result in fewer functional NMDA receptorsper se, without alterations of subunit composition in the receptors.In addition, our findings suggested that the expression of NMDAreceptor subunits is regulated interdependently during the developmentof the brain in a region-specific manner. Thus, the embryonicGluR $epsilon$ 4 subunit may play a role in the regulation of NMDA receptorfunction in adulthood. To ascertain precisely where in the forebrainthe NMDA receptor function is altered, an autoradiographic analysisof [³H]MK-801 binding is necessary. Moreover, it remains to be determined,however, why the expression of the GluR $zeta$ subunit in GluR $epsilon$ 4 mutantmice was downregulated in the frontal cortex and striatum butnot other regions of thebrain.

In the postmortem brain analysis, GluR $epsilon$ 4 mutant mice showed reduced monoamines and their metabolite contents in the hippocampus.They also showed an increase in both DA and 5-HT metabolism inthe frontal cortex, striatum, hippocampus, and thalamus. The alterationto monoaminergic neuronal systems was greatest in the hippocampusamong the regions examined, including the frontal cortex, striatum,and thalamus. Thus, in monoaminergic neuronal systems of adultGluR $epsilon$ 4 mutant mice, it is likely that the hippocampus is mostseverely influenced by a lack of the embryonic GluR $epsilon$ 4subunit.

The mechanisms responsible for the functional alteration of monoaminergic neuronal systems in adult GluR $epsilon$ 4 mutant mice remainto be determined. It is of interest that rats with neonatal excitotoxiclesions in the ventral hippocampus exhibit hyperfunction of dopaminergicand hypofunction of glutamatergic neuronal systems in adulthood(Schroeder et al., 1999), which resemble the increase of DA metabolismand malfunction of NMDA receptors in adult GluR $epsilon$ 4 mutant mice.It has been proposed that hyperfunction of dopaminergic neuronalsystem in the hippocampus-lesioned rats is attributable to animpairment of neuronal development induced by the loss of synapticconnections between the medial prefrontal cortex and ventral hippocampusas a result of excitotoxic lesions of the hippocampus during theneonatal period (Lipska et al., 1993; Schroeder et al., 1999).In GluR $epsilon$ 4 mutant mice, there are no alteration of NMDA receptorsubunit levels in the hippocampus (present study) and no obvioushistological abnormalities in any region, including the hippocampuson Nissl staining (Ikeda et al., 1995). Therefore, we considerthat there may be an impairment of synapse formation connectingthe hippocampus and other brain regions in GluR $epsilon$ 4 mutant mice,because previous studies have suggested a role of NMDA receptorsin neuronal development (Scheetz and Constantine-Paton, 1994;Contestabile, 2000). Additional study is required to address thispossibility.

Alternatively, it may be attributable to the results of NMDA receptor malfunction in adult GluR $epsilon$ 4 mutant mice, because thepharmacological blockade of NMDA receptors in vivo either directlyor indirectly results in an altered neuronal activity in monoaminergicneuronal systems, particularly dopaminergic and serotonergic neuronalsystems (Hiramatsu et al., 1989; Imperato et al., 1990; Millerand Abercrombie, 1996). Moreover, we provided recently geneticevidence that GluR $epsilon$ 1 mutant mice with reduced NMDA receptor functionexhibit an increase in dopaminergic and serotonergic neuronalactivities in the frontal cortex and striatum (Miyamoto et al.,2001). In fact, an impairment of NMDA receptor function in theforebrain was evident as a significant decrease of [³H]MK-801 binding and ⁴⁵Ca²⁺ uptake through the NMDA receptors in adult GluR $epsilon$ 4 mutantmice.

It has been demonstrated that GluR $epsilon$ 4 mutant mice show a reduction of spontaneous locomotor activity (Ikeda et al., 1995).Consistent with this finding, reduced locomotor activity in themutant mice was observed in the present study. Moreover, we founda change in the emotional behavior of GluR $epsilon$ 4 mutant mice. Themutant mice exhibited less susceptibility to psychological andphysiological stress induced in the elevated plus-maze, light-darkbox, and forced swimming tests. It is considered that locomotoractivity and emotional behavior are regulated by the homeostaticbalance of activity among monoaminergic neuronal systems (Schildkraut,1965; Geyer, 1996; Giros et al., 1996; Kim et al., 1997; Lucki,1998; Gainetdinov et al., 1999). In GluR $epsilon$ 4 mutant mice, a significantincrease in DA and 5-HT metabolism in the frontal cortex, striatum,hippocampus, and thalamus was evident. Thus, the reduction inlocomotor activity and susceptibility to stress may be attributedto the altered monoaminergic, especially dopaminergic and serotonergic,neuronal functions in the mutant mice. However, alteration ofneuronal functions in GABAergic neuronal system must be considered,because agonistic modulators of GABA_A receptors are effectivein reducing emotional behaviors in the elevated plus-maze andlight-dark box tests (Lister, 1987; Dalvi and Rodgers, 1996; Chaouloffet al., 1997).

Interestingly, a previous study demonstrated that the performance of GluR $epsilon$ 4 mutant mice was not different from that of heterozygousmice as control group in the elevated plus-maze and light-darkbox tests (Ikeda et al., 1995). It is possible that significantchanges in emotional behavior could not be detected because homozygousGluR $epsilon$ 4 mutant mice were compared with heterozygous littermates.Alternatively, the inconsistency between the two studies is attributableto the difference in the age of the mutant mice used. We usedGluR $epsilon$ 4 mutant mice at 3 months of age in this study, whereas theprevious study examined mutant mice at postnatal day 26 (P26)or P28. The GluR $epsilon$ 4 subunit mRNA is mainly expressed from embryonicday 13 through P14 in mouse brain (Watanabe et al., 1992). Consideringthat disruption of the GluR $epsilon$ 4 subunit may affect the maturationof brain, the function of the CNS in mutant mice is more stableat 3 months than at 4 weeks, which is just after the weaning period.Because different behavioral effects of the GluR $epsilon$ 4 subunit genedisruption in juvenile and adult mice are of special interest,additional studies are required to examine whether there is acritical age when GluR $epsilon$ 4 mutant mice exhibit less susceptibilityto psychological and physiologicalstress.

In summary, adult mice lacking the embryonic GluR $epsilon$ 4 subunit had dysfunctional NMDA receptors, possibly attributable to changesin the receptor subunit composition or reduction of functionalNMDA receptors without alterations of subunit composition. Themutant mice showed altered emotional behavior, which is probablyattributable to a change in monoaminergic neuronalactivities.

  FOOTNOTES

Received July 31, 2001; revised Nov. 14, 2001; accepted Dec. 18, 2001.

This work was supported in part by Grant-in-Aid for Scientific Research 10044260 from the Ministry of Education, Science,Sports, and Culture of Japan and by Special Coordination Fundsfor Promoting Science and Technology, Target-Oriented Brain ScienceResearch Program from the Ministry of Education, Culture, Sports,Science, and Technology ofJapan.

Correspondence should be addressed to Dr. Toshitaka Nabeshima, Department of Neuropsychopharmacology and Hospital Pharmacy,Nagoya University Graduate School of Medicine, 65 Tsuruma-cho,Showa-ku, Nagoya 466-8560, Japan. E-mail: tnabeshi{at}med.nagoya-u.ac.jp.

Y. Miyamoto's present address: Department of Molecular Genetics, National Institute for Longevity Sciences, Gengo 36-3, Morioka-cho,Oobu, Aichi 474-8522,Japan.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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Lower Sensitivity to Stress and Altered Monoaminergic Neuronal Function in Mice Lacking the NMDA Receptor 4 Subunit

Lower Sensitivity to Stress and Altered Monoaminergic Neuronal Function in Mice Lacking the NMDA Receptor $epsilon$ 4 Subunit