Degeneration of the Amygdala/Piriform Cortex and Enhanced Fear/Anxiety Behaviors in Sodium Pump {alpha}2 Subunit (Atp1a2)-Deficient Mice

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The Journal of Neuroscience, June 1, 2003, 23(11):4667-4676

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Degeneration of the Amygdala/Piriform Cortex and Enhanced Fear/Anxiety Behaviors in Sodium Pump ${alpha}$ 2 Subunit (Atp1a2)-Deficient Mice
Keiko Ikeda,¹ Tatsushi Onaka,² Makoto Yamakado,³ Junichi Nakai,⁴ Tomo-o Ishikawa,⁵^,6 Makoto M. Taketo,⁵^,6 and Kiyoshi Kawakami¹
¹ Department of Biology Jichi Medical School, Kawachi, Tochigi 329-0498, Japan, ² Department of Physiology Jichi Medical School, Kawachi, Tochigi 329-0498, Japan, ³ Department of Anatomy, Jichi Medical School, Kawachi, Tochigi 329-0498, Japan, ⁴ Department of Information Physiology, National Institute for Physiological Science, Okazaki 444-8585, Japan, ⁵ Department of Pharmacology, Graduate School of Medicine, Kyoto University, Sakyo, Kyoto 606-8501, Japan, and ⁶ Banyu Tsukuba Research Institute (Merck), Tsukuba 300-2611, Japan

   Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

The sodium pump is the enzyme responsible for the maintenanceof Na⁺ and K⁺ gradients across the cell membrane. Four isoformsof the catalytic ${alpha}$ subunit have been identified, but their individualroles remain essentially unknown. To investigate the necessary functions of the ${alpha}$ 2 subunit in vivo, we generated and analyzed mice defective in the ${alpha}$ 2 subunit gene. Mice homozygous for the ${alpha}$ 2 mutation died just after birth and displayed selective neuronalapoptosis in the amygdala and piriform cortex. In these regions,high expression of c-Fos before apoptosis indicated neuralhyperactivity, and re-uptake of glutamic acid and GABA intoP₂ fraction containing crude synaptosome was impaired. Theseresults indicate that the ${alpha}$ 2 subunit plays a critical role regulatingneural activity in the developing amygdala and piriform cortex.Further supporting a role of the ${alpha}$ 2 subunit in the function of the amygdala, heterozygous adult mice showed augmented fear/anxietybehaviors and enhanced neuronal activity in the amygdala andpiriform cortex after conditioned fear stimuli.

Key words: amygdala; piriform cortex; knock-out mice; Na,K-ATPase; neurotransmitter uptake; fear-anxiety behavior

   Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

The sodium pump (Na ⁺,K ⁺-ATPase, EC 3.6.1.3 [EC] ) is an integralplasma membrane protein responsible for the ATP-dependent transport of Na⁺ and K⁺ across the membrane. This transport producesthe ion gradients that are critical to maintain a resting membrane potential, osmotic balance, and cytosolic pH, and for Na⁺-coupled transport of various ions, glucose, and amino acids across themembrane. The pump consists of ${alpha}$ and ${beta}$ subunits. The catalytic ${alpha}$ subunit contains the binding sites for the cations, ATP, andcardiac glycosides (Lingrel and Kuntzweiler, 1994), whereas ${beta}$ subunit is required for the structural and functional maturationof the ${alpha}$ subunit (for review, see Geering, 2001). Genes encoding four ${alpha}$ and three ${beta}$ isoforms have been identified, yet the specific role of each isoform remains essentially unknown. Tissue-restrictedexpression of some isoforms suggests isoform-specific rolesin cell physiology. In adult rats, the ${alpha}$ 1 subunit is ubiquitouslyexpressed; the ${alpha}$ 2 subunit is expressed mainly in excitable tissues,i.e., brain, skeletal muscle, and heart; and the ${alpha}$ 3 subunitis expressed solely in neural and cardiac tissues (Shull etal., 1986; Orlowski and Lingrel, 1988; Sweadner, 1989; Lingrelet al., 1990; Shamraj and Lingrel, 1994). Both the ${alpha}$ 2 and ${alpha}$ 1subunits are broadly expressed in the mouse brain during earlydevelopment [embryonic day (E) 9.5–10.5] and subsequentlybecome expressed in more restricted regions of the brain, suchas meninges, the neopallial cortex, and the intermediate ventricularzones of the cerebral cortex (Herrera et al., 1994).
A recent study suggested a specific role of the ${alpha}$ 2 subunit in regulating Ca ²⁺ concentrations in cardiac myocytes of micewith a heterozygous disruption of this gene (James et al.,1999). We independently sought to examine a specific role ofthis molecule and constructed mice defective in the Na⁺, K⁺-ATPase ${alpha}$ 2 subunit gene (Atp1a2) to study the function of the ${alpha}$ 2 subunitin vivo. Here we show that the homozygous mutant embryos had impaired re-uptake of neurotransmitters, enhanced neural excitation,and cell death specifically in the amygdala and piriform cortex.Furthermore, heterozygous adult mice showed augmented fear/anxietybehaviors and enhanced neuronal activity in the amygdala andpiriform cortex after conditioned fear stimuli, supportinga role for the ${alpha}$ 2 subunit in regulating neural activity.

   Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Construction of Atp1a2 targeting vector and generation of mutant mice
Mouse genomic DNA containing exons 21 and 22 of the Atp1a2 was isolated by screening a 129/Sv mouse genomic ${lambda}$ FIXII library (Stratagene, La Jolla, CA) using a rat Atp1a2 cDNA probe [nucleotide positions 2381–3158 according to Shull et al. (1986)].A 6.5 kb KpnI–SacI fragment containing exons 21 and 22and another downstream fragment of $~$ 1 kb (SacI–SacI) were isolated and subcloned in pBlueScript KS (Stratagene).A PGKneobpA cassette (see neo in Fig. 1A) was inserted intoan XhoI site, which was introduced in exon 21. The bacterialdiphtheria toxin ${alpha}$ subunit gene (see DTA in Fig.1A) drivenby the phosphoglycerate kinase I gene promoter was insertedat an upstream KpnI site. Embryonic stem (ES) cells (RW4 EScell line) were electroporated with the linearized targetingvector as described (Oshima et al., 1995). G418-resistantES clones were screened by PCR using primers 5'-GGTTTGTAGGCCATCCATTTCAACCCAGC-3'and 5'-GCCTGCTTGCCGAATATCATGGTGGAAAAT-3'. Homologous recombinant candidates were verified by Southern hybridization using a probeshown in Figure 1A. Chimeras were generated by injecting therecombinant ES cells into C57BL/6J blastocysts and transferredto multi-cross hybrid (CLEA Japan, Inc., Tokyo, Japan) foster mothers. Atp1a2⁺^/^- was backcrossed five to seven generationsto the C57BL/6J. In every experiment, mice from each genotypewere littermates and of isogenic genetic background. We also backcrossed the Atp1a2 knock-out mice to the 129/Sv strain and observed a similar phenotype. Microsomal fractions were preparedas described (Guillaume et al., 1989). McB2 (anti- ${alpha}$ 2 antibodyused in Fig. 1D) was kindly provided by K. Sweadner (Massachusetts General Hospital) (Urayama et al., 1989), and an anti- ${alpha}$ 1 antibodywas purchased from Upstate Biotechnology (Waltham, MA). AnotherAtp1a2 targeted mouse in which a PGKneobpA cassette was insertedjust after the initiation codon showed similar phenotype ofdeath soon after birth and overexpression of c-Fos in the amygdalaand piriform cortex (data not shown).

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Figure 1. Targeting strategy for mutating the Na ⁺,K ⁺-ATPase ${alpha}$ 2 subunit gene (Atp1a2) and analyses of genomic DNA, mRNA, and protein in wild-type, heterozygous, and homozygous mutant mice. A, A neomycin-resistant gene cassette (neo) was inserted in exon 21, and a DTA gene was inserted in the opposite orientation for negative selection. The targeted allele was verified by PCR (data not shown) and Southern hybridization (B) with the indicated probe. Positions of BamHI DNA fragments from the wild-type (6.0 kb) and targeted (7.2 kb) alleles are shown. C, Total RNA was isolated from the E18.5 brain, and 40 µg of RNA was analyzed by Northern blotting with a ScaI–NheI fragment of the rat Atp1a2 cDNA (Hara et al., 1987) (covering position 121–497 of its cDNA, which corresponds to exons 2–5).As a control, the expression of the Atp1a1 (Na ⁺,K ⁺-ATPase ${alpha}$ 1 subunit) gene is shown in a Northern blot using an NcoI fragment as a probe (Hara et al., 1987) (covering position 236–2435 of its cDNA). D, A microsomal fraction was prepared from the brains of E18.5 embryos, and 40 µg of protein was analyzed by Western blotting with either an anti- ${alpha}$ 2 antibody (1:100, McB2) or an anti- ${alpha}$ 1 antibody (1:2000). The asterisk shows a nonspecific band.

Analysis of spontaneous body movement in fetuses
Immediately after cervical dislocation of the pregnant femalemice, the uterus was taken out and placed onto a thermostaticallycontrolled hot plate (37°C). Fetus spontaneous body movementsin the uterus (twitching of the trunk, forelimb or hindlimbmovement, and head movement) were observed for 3 min. For nociceptiveresponse, the cesarean-delivered fetus was placed onto a thermostaticallycontrolled hot plate (37°C) and pricked on the trunk with a 26 gauge needle, and trunk movements were observed.
Diaphragm muscle membrane potential
Phrenic–diaphragmatic nerve–muscle preparationswere isolated from E18.5 ether-anesthetized embryos. Preparationswere placed under a stereomicroscope (SZX12, Olympus Optical,Tokyo, Japan) equipped with a video-rate charged coupled device(CCD) camera (CCD72, MTI Instruments, Albany, NY) and bathedin Krebs' solution containing (in mM): 137 NaCl, 2 KCl, 5 CaCl₂,2 MgCl₂, 0.25 NaH₂PO₄, 1 HEPES, and 10 glucose, pH 7.4 withNaOH, bubbled with a 95% O₂/5% CO₂ gas mixture at 26°C. Membrane potentials of diaphragmatic muscle were measured usingan intracellular microelectrode filled with 3 M KCl (resistance 10–15 M ${Omega}$ ). The electric signals were filtered by usingHum Bug (Quest Scientific, North Vancouver, BC), amplifiedby using Axoclamp-2A (Axon Instruments, Union City, CA) anda laboratory-made amplifier, and recorded with a data recorder(VR-10B; Instrutech, Port Washington, NY). The resting membranepotentials described in Results are the means of those of 15–20 muscle fibers from each mouse (n = 4 for the wild-type and the homozygote; n = 5 for the heterozygote).
Histological examination
Embryos were obtained from timed pregnancies, with noon of theplug date defined as E0.5. Brains were fixed in 4% paraformaldehyde/0.1M PBS. Paraffin-embedded sections (10 µm thick) werestained with Carazzi's hematoxylin and eosin (see Fig. 2 A–F).Electron microscopy was performed using tissues fixed in 2%glutaraldehyde in 0.1 M cacodylate buffer, pH 7.4, incubatedin 2% OsO₄/PBS, dehydrated, and embedded in Epon. Ultrathinsections were analyzed at 100 kV in a JEM-2000EX microscope(JEOL, Peabody, MA) as described previously (Hanaichi et al.,1986). Terminal deoxynucleotidyl transferase-mediated biotinylatedUTP nick end labeling (TUNEL) analysis was performed accordingto the protocol provided by the manufacturer (NeuroTacs, Trevigen,Inc., Gaithersburg, MD). Immunohistochemistry for c-Fos proteinwas performed as described previously (Onaka and Yagi, 2001). c-Fos-positive cells in the "adult brain" were quantified as follows. At the level of bregma -0.8 to -0.9 mm, the amygdalaand piriform were outlined as oval (0.5 mm ²) and rectangular(0.5 mm ²) regions, respectively, and the number of c-Fos-positivecells in these areas was counted. Data described in the legendfor Figure 8 are the mean number of c-Fos-positive cells persection counted on three successive sections (30 µm thick).Quantification of c-Fos-positive cells in the "embryonic brain"was described in the legend of Table 2. For the preparationof the ${alpha}$ 2-specific subunit peptide antibody used for immunohistochemistry, a peptide (GREYSPAATTAENGGGKKKQ), which covers amino acids 6–25of the mouse ${alpha}$ 2 subunit protein, was synthesized and used forimmunization of rabbits. Affinity purification of antibodieswas performed by absorption on covalently linked peptide columns.Immunohistochemistry for the ${alpha}$ 2 subunit was performed with paraffin-embeddedbrain sections using an antigen retrieval method, as describedby the manufacturer (DakoCytomation, Glostrup, Denmark) usingaffinity-purified ${alpha}$ 2 peptide antibody (1:400). As a control,we used rabbit IgG (equivalent protein concentration, 400 ng/ml), which was purified by affinity chromatography on Protein A-SepharoseCL-4B (Amersham Biosciences, Uppsala, Sweden).

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Figure 2. Histopathology of mouse brains defective for the Atp1a2gene.A–C, Sagittal sections of E18.5–P0 fetal brains of wild-type (+/+), heterozygous (+/-), and homozygous (-/-) mutant mice. Representative photographs are shown from multiple brains analyzed of wild-type (n=7), heterozygous (n=7), and homozygous (n=13) mice. Note the decreased cellular density in the homozygous mice (C) that is limited to the amygdala (asterisks), with the exception of the nucleus of the lateral olfactory tract (LOT). Scale bar, 1 mm. D–F, Higher magnification of the amygdala regions shown in A–C, respectively. In the homozygous mutant, the decreased cellular density in the amygdala was bordered by regions of normal cellular density (F, arrowheads). Scale bar, 250 µm. G–I, Increased apoptosis in the brain of homozygous mutant mice. Frontal sections of the brain at E18.5–P0 were stained by TUNEL. The numbers of TUNEL-positive cells in the amygdala and piriform cortex (arrows) were higher in the homozygous brain than in the heterozygous or wild-type brains. In the same sections counterstained with Hoechst 33258, the TUNEL-positive cells had pyknotic nuclei (data not shown). Scale bar, 1 mm. J–L, Electron micrographs of cells in the amygdala (E18.5–P0).Condensed chromatin (K, arrows) typical of apoptotic cells was observed in the homozygous mutant (K,L) but not in the wild-type (J) or heterozygous mutant (data not shown). Two littermates of the wild-type and three of the homozygous were examined. Scale bars: J, K,5 µm; L,2 µm.

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Figure 8. Increased c-Fos expression in adult male heterozygous mutant mice under conditioned fear stimuli. Production of c-Fos protein was detected by an anti-c-Fos antibody and appears as black spots in the expressing nuclei. A, B, Representative photographs are shown from four sets of trials for each genotype under conditioned fear stimuli for wild-type (A) and heterozygous (B) mice. The mean numbers of c-Fos-positive cells were 95 per section (+/+) and 449 per section (+/-) for the piriform cortex and 120 per section (+/+) and 399 (+/-) for the amygdala. C, D, Little c-Fos expression was detected in these regions of the adult brain in either genotype when mice were kept in their home cages. The mean number of c-Fos-positive cells was 23 per section (+/+) and 20 per section (+/-) for the piriform cortex and 19 per section (+/+) and 31 (+/-) for the amygdala. Representative photographs are shown from four sets of each genotype in its home cage. The amygdala (amy) and piriform cortex (pir) are indicated. Scale bar, 1 mm.

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Table 2 . Number of c-Fos-positive cells in E17.5-18.5 embryo brains

Measurements of neurotransmitter contents in the whole brain
Pregnant mice were killed by cervical dislocation, and E17.5–18.0 embryos were obtained by cesarean delivery. The brain was immediatelyremoved from the decapitated embryo and sonicated in 500 µlof a solution of 0.2 M perchloric acid and 100 µM EDTA.The homogenate was centrifuged at 20,000 x g for 15 min at0°C. The supernatant was diluted to 500-fold by 0.1 M K₂CO₃-HCl, pH 9.5, and filtered on a disposable syringe filter(cellulose acetate, 0.45 µm; DISMIC-3CP, Advantec, Tokyo,Japan). Glutamic acid and GABA content of the filtrate weremeasured by reversed-phase HPLC and fluorimetric detectionafter derivatization with o-phthaldialdehyde as described previously (Leng et al., 2001).
Preparation of P₂ fraction and assay of neurotransmitter uptake
The brain was immediately removed from the decapitated embryoand homogenized in an ice-cold sucrose buffer (0.32 M sucrose,5 mM HEPES-NaOH, and 0.1 mM EDTA, pH 7.6) using a Potter glasshomogenizer plus Teflon pestle by 15 strokes at 300 rpm. Thecrude homogenate was centrifuged at 1500 x g for 10 min at4°C. The supernatant was then centrifuged at 12,000 x gfor 30 min at 4°C. The membrane pellets (P₂) (Gray andWhittaker, 1962) were resuspended in artificial CSF (aCSF)containing (in mM): 132 NaCl, 3 KCl, 2 CaCl₂, 2 MgSO₄, 1.2 NaH₂PO₄, 10 HEPES-NaOH, and 10 glucose, pH 7.4, bubbled with95% O₂/5% CO₂ gas mixture and used promptly. Uptake reactionwas initiated after 5 min preincubation at 26°C in aCSFby adding 100 µl of reaction mixture to 100 µlof P₂ fraction at a final concentration of 5 µM [³H]glutamicacid (Amersham Biosciences) or 1 µM [³H]GABA (Amersham Biosciences). Samples were incubated for 3 min at 26°C,and the reaction was terminated by filtration using GF/C filters(Whatman, Kent, UK). Filters were washed three times with 1ml of ice-cold aCSF, and the radioactivity of filters was quantifiedby a Beckman LS1800 scintillation counter (Beckman Coulter,Fullerton, CA). Uptake was normalized for protein content thatwas determined by protein assay kit (Bio-Rad, Hercules, CA).The mean protein concentration of the P₂ fraction was 0.97± 0.24 mg/ml (n = 5) for wild-type, 0.96 ± 0.28mg/ml (n = 5) for homozygous, and 1.01 ± 0.29 mg/ml(n = 5) for heterozygous mice. Nonspecific uptake was estimatedin parallel samples containing specific neurotransmitter transporterblockers: 30 µM L-trans-2,4-pyrrolidine-dicarboxylicacid (PDC) (Tocris Cookson, Ellisville, MO) for glutamic aciduptake and 100 µM N-(4,4-diphenyl-3-butenyl)-3-piperidinecarboxylic acid (SKF 89976A) (Tocris Cookson) for GABA uptake.Nonspecific uptake was similar when determined using "modifiedaCSF" composed of choline chloride instead of sodium chloride.Specific uptake was obtained from total uptake (in the absenceof the specific transporter blocker) minus nonspecific uptake(in the presence of the specific transporter blocker). Inhibitionof specific uptake by 1 mM ouabain (Sigma, St. Louis, MO) wasalso monitored in parallel samples. "Relative uptake" was calculatedas relative percentage of specific uptake of the wild-typemice in each set of experiments, which was set as 100. Littermatesfrom five different mother mice for glutamic acid (n = 5) andsix different mother mice for GABA (n = 6) were examined.
PDC is a glutamate transporter blocker that inhibits three different glutamate transporters of GLT-1, EAAC1, and less efficiently,GLAST. GLT-1 is expressed in glial cells and developing neurons.PDC inhibits the transport activity in cultured neurons preparedfrom embryonic rats, in cortical synaptosomes prepared fromneonatal rats, and cultured astrocytes prepared from adultrats (for review, see Danbolt, 2001). SKF89976A, a derivativeof nipecotic acid, is a potent and specific inhibitor of GABAtransporter 1(GAT-1). GAT-1 is expressed both in neurons andglia in adult rats, as well as in the developing rat brain (for review, see Borden, 1996; Jursky and Nelson, 1996).
Preparation of cultured astrocyte, immunostaining, Western blot, and assay of neurotransmitter uptake into astrocytes
Primary cortical astrocytes cultures were prepared from brainsof E16.5–17.5 embryos as described (Kawakami et al.,1993). The secondary cultures on 24-well tissue culture plateswere grown in Minimum Essential Medium (Sigma) with 10% fetalbovine serum for 1–3 d and used for uptake assays. Thecells on the plates consisted of >95% flat polygonal astrocytesas confirmed by positive immunostaining with anti-glial fibrillary acidic protein (GFAP) antibody (DakoCytomation) (see Fig. 6 A).The 30 µg astrocyte microsomal fractions were subjectedto immunoblot using anti- ${alpha}$ 2 subunit peptide antibody (1:2000)or anti- ${alpha}$ 1 antibody (1:2000). Glutamic acid and GABA uptakewere measured as follows. Cells were washed twice with an assaybuffer containing (in mM): 124 NaCl, 4.6 KCl, 1.2 CaCl₂, 1.3MgCl₂, 0.42 KH₂PO₄, 26.7 NaHCO₃, 10 glucose, pH 7.4, and incubatedin the assay buffer for 30 min at 26°C. Then, each culturewell received 0.5 µCi/ml L-[³H]glutamic acid (Amersham Biosciences) plus 40 µM unlabeled glutamic acid or 0.5µCi/ml L-[³H]GABA (Amersham Biosciences) plus 40 nM unlabeled GABA. Uptake was terminated by washing twice withice-cold assay buffer after 3 min incubation and followed immediatelyby cell lysis in 0.5N NaOH/0.05% sodium lauryl sulfate. Aliquotswere taken for scintillation counting and for protein assay(BCA protein assay kit; Pierce, Rockford, IL) using bovineserum albumin standards. Assays were performed with and without specific blocker, i.e., 30 µM PDC for glutamic acid uptakeand 30 µM SKF 89976A for GABA uptake, and the blocker-inhibitable uptake was shown as specific uptake after normalization to theprotein concentration. All experiments were performed in duplicatein the presence or absence of 1 mM ouabain (glutamic acid,n = 5 for each genotype; GABA, n = 4 for each genotype).

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Figure 6. Glutamic acid and GABA uptake in cultured astrocytes prepared from wild-type, heterozygous, and homozygous mice.A, Representative immunostaining of GFAP or control IgG in cultured astrocytes prepared from a homozygous mutant used in these assays. Phase-contrast images are shown. Scale bar, 100 µm. B, Immunoblot showing the amount of the ${alpha}$ 2 subunit and the ${alpha}$ 1 subunit in microsomal fractions prepared from cultured astrocytes from wild-type (+/+), heterozygous (+/-), and homozygous (-/-) mice. C, D, Specific uptake of [³H]glutamic acid and [³H]GABA into astrocytes in a 3 min incubation at 26°C, for which period specific uptake was correlated linearly with incubation time. The specific uptake activity was almost the same among wild-type, heterozygous, and homozygous mice and in each case was significantly inhibited by the addition of 1 mM ouabain. Error bars indicate SEM. ^**p < 0.01.

Behavioral analysis
Wild-type and heterozygous male mice (70–100 d old) wereused in these studies. Mice lived in a 12 hr light/dark cycle(lights on between 7:30 A.M. and 7:30 P.M.); all behavioralobservations were made during the dark phase (9:30 P.M.–2:00A.M.). Room temperature was 23°C. Food and water were availablead libitum. Mice were housed singly for 1 week before the behavioralexperiments started.
Light/dark test. The light/dark box consisted of two compartments: an open box with a white frosted plastic floor (light) and aclosed black box with a black frosted plastic floor (dark)(30 x 15 x 15 cm each). The test commenced by placing the mousein the black box. The time spent in the light and dark boxeswas measured over a period of 10 min (n = 11 for each genotype).
Open field test. To measure locomotor activity in a new environment,the mouse was placed in the center of a white acrylic cage (50 x 50 x 40 cm), and locomotion activity was measured automatically over a period of 10 min using NIH Image software (n = 16 foreach genotype).
Elevated-plus maze. The elevated-plus maze consisted of twoopen (25 x 5 cm) and two enclosed arms of the same size with15-cm-high transparent walls. The arms and central square wereconstructed of white plastic plates and elevated to a heightof 50 cm above the floor. The mouse was placed on the centralplatform of the maze with its head facing the open arm. Thefrequency of entry to open and closed arms and the time spentin open arms were recorded during the 10 min test (n = 11 foreach genotype).
Contextual fear conditioning. Each mouse was placed in a test chamber (15 x 15 x 40 cm) and allowed to explore freely for5 min. A mild (1 sec, 0.5 mA) foot shock (denoted "F" in Fig.7H) or no foot shock as a control (denoted "C"), was appliedfive times at an interval of 30 sec. Testing was conducted24 hr after conditioning in the same chamber. The test durationwas 10 min for behavioral experiments and 30 min for c-Fosimmunohistochemistry. Data acquisition, control of shocks, anddata analysis were performed automatically. Images were capturedat two frames per second. For each pair of successive frames,the amount of area (pixels) within which the mouse moved wasmeasured. When this area was below a certain threshold (i.e.,10 pixels), the behavior was judged as "freezing." The optimalthreshold (amount of pixels) used to judge freezing was determinedby adjusting it to the amount of freezing measured by humanobservation. Freezing that lasted less than the defined timethreshold (i.e., 1 sec) was not included in the analysis (n= 8 for each genotype). Sensitivity to foot shock was determinedby placing each genotype of mice into the conditioning chamberand giving foot shocks of increasing amplitude (0.1, 0.15,0.2, 0.25, 0.3, 0.4, and 0.5 mA). Thresholds for flinch, jump,and vocalization were not significantly different between wild-typeand heterozygous mice (n = 4 for each genotype). Blood sampleswere obtained by decapitation immediately after conditionedfear stimuli. For c-Fos immunohistochemistry, mice were anesthetizedwith sodium pentobarbital (0.25 gm/kg body weight) and transcardiallyperfused with 4% paraformaldehyde in PBS at 90 min after conditionedfear stimuli.

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Figure 7. Enhanced anxiety-like behaviors in heterozygous adult mice. A–D, Light/dark test. A, Total path length in the light compartment (white) in the light/dark test.B, Total length of time spent in the light compartment of the light/dark test.C, Latency to first entry to the light compartment in the light/dark test. D, Number of transitions between the light and dark compartments in the light/dark test. A–D, n = 11 for each genotype. E, Total path length in the open-field test (n = 16 for each genotype). F, G, Elevated-plus maze. F, Percentage of time in the open arms of the elevated-plus maze. G, Percentage entries into the open arms of the elevated-plus maze. F, G, n = 11 for each genotype. H, Freezing time in conditioned fear paradigms (n = 8 for each genotype and treatment). C, Control mice without foot shock; F, mice that received foot shock during conditioning. Solid bar represents wild-type mice; hatched bar represents heterozygous mice. Error bars indicate SEM. NS, Not significant. ^*p < 0.05; ^**p < 0.01.

Rota-rod test. The apparatus consisted of a bar (3 cm in diameter) that was subdivided into five compartments by disks (Rota-rodtreadmill for mice 7650; Ugo basile, Varese, Italy). Five micewere tested simultaneously on the apparatus. The bar startedto rotate at a speed of 4 rpm. The rotating speed was increasedstepwise every 30 sec at 8, 12, 16, 20, 24, 28, 32, and 40 rpm. The integrity of motor coordination was assessed by thetime to fall from the rod. Mice were habituated to the apparatusonce per day for 4 d before testing [n = 6 (wild-type mice)and n = 8 (heterozygous mice)].
Measurement of spontaneous motor activity. Spontaneous motor activity in the home cage was monitored for 48 hr by using the"Activity Sensor Unit for mouse system" (AS-TIME/Ver.1, O'Hara& Co., Tokyo, Japan), which detects heat radiation fromthe mouse body.
Statistical analysis
Data are expressed as mean ± SEM. Differences betweengroups were examined for statistical significance using one-ortwo-way ANOVA followed by Fisher's PLSD test in the experimentsshown in Figures 5A–D, 6, C and D, and 7H. Data of behavioral analyses shown in Figure 7A–G were comparedby the Student's t test. p < 0.05 denoted the presence ofa statistically significant difference.

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Figure 5. Glutamic acid and GABA content in the brain and uptake of these neurotransmitters into the P₂ fraction. A, B, Glutamic acid and GABA content were significantly higher in the brains of the homozygous mutant mice than in the wild-type mice. The values shown were normalized for protein content. The mean values of glutamic acid (A) and GABA (B) for the wild-type(+/+;n=11), heterozygous(+/-;n=14), and homozygous mice (-/-;n= 6) are shown. ^**p < 0.01. C, D, Uptake of [³H]glutamic acid and [³H]GABA into the P₂ fraction in a 3 min incubation at 26°C, for which period specific uptake was correlated linearly with incubation time. In each experiment, the specific uptake in the wild-type mice was set to 100, and the relative uptake in heterozygous and homozygous mutant mice is shown. Note the significantly lower uptake in the homozygous brain compared with the wild-type and heterozygous (compare columns 1 and 5 and columns 3 and 5). The specific uptake activity was significantly decreased by the addition of 1 mM ouabain to fractions from the wild-type or heterozygous mice (columns 1 and 2 or columns 3 and 4), but not the homozygous mice (columns 5 and 6). Littermates from five different mother mice for glutamic acid (n = 5) and six different mother mice for GABA (n = 6) were examined. Solid bars represent wild-type mice; hatched bars represent heterozygous mice; open bars represent homozygous mice. Error bars indicate SEM. ^*p < 0.05; ^**p < 0.01.

   Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Generation of Atp1a2-deficient mice
To study the function of the sodium pump ${alpha}$ 2 subunit during embryonic development and in adult mice, we generated mice with a mutant ${alpha}$ 2 subunit gene (Fig. 1). A neomycin-resistant gene cassette(neo) was inserted in exon 21, and the targeted allele wasverified by PCR (data not shown) and Southern hybridization(Fig. 1B). We confirmed the lack of ${alpha}$ 2 subunit mRNA in thebrain and lack of the protein in microsomal fractions of thebrain prepared from homozygous E18.5 embryos (Fig. 1C,D).The homozygous mutant mice survived until birth but died soonafter. No gross morphological defects were observed in thehomozygous embryos, and there were no apparent histologicalanomalies in either skeletal or heart muscle (data not shown).The E18.5 embryos showed no spontaneous movement and lackeda nociceptive response, but diaphragmatic muscle contractionwas observed when the phrenic nerve was stimulated (data notshown), and we did not observe any significant differencesof the resting membrane potential of the diaphragm muscle fibers[wild type: -65.4 ± 1.9 mV (n = 4); heterozygote: -65.7± 2.8 mV (n = 5); homozygote, -63.9 ± 2.2 mV(n = 4)]. Therefore, we focused our analyses on the CNS.
Apoptosis of neurons in the amygdala and piriform cortex in the homozygous mutant embryos
Histological examination of the homozygous brain at E18.5–postnatal day 0 (P0) showed extensive neuronal cell loss in the amygdalaand piriform cortex (Fig. 2C,F, Table 1), and abundant apoptoticneurons were found in these regions as determined by TUNEL (Fig. 2G–I) and electron microscopy (Fig. 2J–L).At this stage, the entire amygdaloid complex, including "thebasolateral complex" and "the central and medial division" (Valverde, 1965), was severely damaged in the homozygous mice,whereas the nucleus of the lateral olfactory tract was spared(Fig. 2C). The hippocampal and cingulate cortices also appeared to be unaffected (Fig. 2G–I) (data not shown). The degenerativechanges in the amygdala and piriform cortex could be detectedas early as E17.5–18 in the homozygous embryos (datanot shown). To our knowledge, selective damage of the amygdalaand piriform cortex has not been reported previously in any other gene disruption study in mice. Therefore, our result suggestsa specific role of the ${alpha}$ 2 subunit in the survival of this setof neurons late in embryogenesis.

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Table 1. Histopathological analysis of E18.5-PO embryo brains

We reasoned that the selective degeneration of this subset ofneurons might reflect a restricted expression pattern of the ${alpha}$ 2 subunit in this region. To test this possibility, we examinedthe distribution of the ${alpha}$ 2 subunit in the brain of wild-typeE17.5 embryos by immunostaining. The use of affinity-purifiedpeptide antibody against the N-terminal portion specific to the ${alpha}$ 2 subunit showed strong staining in the meninges, wherethe ${alpha}$ 2 subunit mRNA has been reported to be abundant (Fig.3B, arrowheads) (Herrera et al., 1994). In the brain, the ${alpha}$ 2 subunit was distributed throughout the cerebral cortex and subcortical nuclear regions, including the piriform cortex andamygdala (Fig. 3B). The ${alpha}$ 2 subunit was detected in neuronalcell bodies and in the neuropil (a mixture of neuronal andglial cell processes) in the amygdala (Fig. 3D) and piriform cortex (Fig. 3F), as well as other regions of the cerebralcortex and subcortical nuclear regions (data not shown), indicatingthat the ${alpha}$ 2 subunit resides in both neuronal and glial cells.These results are consistent with the report that the ${alpha}$ 2 subunitis expressed in neurons and glia throughout the brain of E18.5embryo (Moseley et al., 2002). We conclude that the selectivedegeneration of this region is not caused by the restricteddistribution of the ${alpha}$ 2 subunit.

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Figure 3. Photomicrographs showing the expression of the ${alpha}$ 2 subunit in the amygdala and piriform cortex of wild-type E17.5 embryos. Immunoreactive cells using an affinity-purified ${alpha}$ 2 subunit peptide antibody (B, D, F) and a control IgG (A, C, E) are shown. Sections of embryonic mouse brain (C57BL/6J) at lower magnification (A, B) and higher magnification (C–F) of the amygdala (C, D) and the piriform cortex (E, F). The reddish-brown colored reaction product is observed in the meninges (B, arrowheads) and distributed throughout the cerebral cortex and subcortical nuclear regions (B). The product is detected in neuronal cell bodies and in the neuropil (D, F). Note that some neuronal cells do not show immunoreaction with the ${alpha}$ 2 subunit antibody (D, F). All sections were counterstained with hematoxylin. amy, Amygdala; pir, piriform cortex; LOT, nucleus of the lateral olfactory tract. Frontal sections are shown. Scale bars: A, B, 200 µm; C–F, 20 µm.

Overexpression of c-Fos in the amygdala and piriform cortex in the homozygous mutant embryos
Excitatory amino acids, such as glutamic acid, are known tobecome "excitotoxins" when their concentration in the extracellularspace of the brain is high (for review, see Rothman and Olney,1987; Coyle and Puttfarcken, 1993). Disruption of the ${alpha}$ 2 subunitmight alter the transport or re-uptake of excitatory aminoacids; therefore, it is plausible that the selective damage in the homozygote might reflect toxicity from spontaneous neuralactivity during embryonic development. To test this hypothesis,we examined neural activity by c-Fos immunostaining (Hunt et al., 1987). In the wild-type embryos at E17.5–18.5, c-Fos-positivecells were detected in the amygdala and piriform cortex butnot in the hippocampus, neocortex, or cerebellar cortex (Fig.4A, Table 2) (data not shown), indicating spontaneous neuralactivity in the amygdala and piriform cortex at this embryonicstage. A significantly higher number of c-Fos-positive cells were found in the amygdala and piriform cortex in the homozygousmutant embryos compared with the wild-type and heterozygousembryos (Fig. 4A–C, Table 2). Furthermore, both c-Fos-positivecells and degenerating neurons were observed in these regions of the homozygous brains just before birth (Fig. 4D–I). These observations suggest enhanced neural activity in the amygdalaand piriform cortex of the homozygous mutants and suggest thatexcitotoxic damage causes the neural degeneration in thesespecific regions.

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Figure 4. Augmented c-Fos expression and increased numbers of degenerating cells in the amygdala and piriform cortex of homozygous mutant mouse embryos. Production of c-Fos protein was detected by immunostaining with an anti-c-Fos antibody (indicated as black dots). A–C, Representative photographs are shown from five sets of E17.5–18.5 littermates: a wild-type embryo (A), a heterozygous embryo (B), and a homozygous embryo (C). Scale bar, 500 µm. D–F, c-Fos-immunostained sections are counterstained with cresyl violet. Several c-Fos-positive cells were observed in the amygdala and piriform cortex of the wild-type and heterozygous mice (black dots), but few degenerating cells (D, E) were noted. F, Mixed pattern of c-Fos-positive cells and degenerating cells seen in the homozygous mutants. Representative photographs are shown from three sets of embryos just before birth. G–I, Higher magnification of D–F, respectively. I, c-Fos-positive cells (their nuclei are stained dark gray) and degenerating cells (pyknotic nuclei are stained round black, indicated by arrows) in the homozygous mutants. Frontal sections are shown. Scale bars: D–F, 100 µm; G–I, 25 µm. amy, Amygdala; pir, piriform cortex.

Impaired uptake of neurotransmitters into P₂ fraction of the homozygous mutants
Glutamic acid and GABA are the principal neurotransmitters inthe amygdala (Davis et al., 1994). At E17.5–18.0, thewhole-brain levels of both neurotransmitters were higher inthe homozygous mutants than in heterozygous or wild-type mice (Fig. 5A,B). A transporter specific to each neurotransmittermediates its uptake into nerve terminals and adjacent glialcells, maintaining the extracellular neurotransmitter concentrationsat low levels in the CNS (Borden, 1996; Danbolt, 2001). Na ⁺,K ⁺-ATPase generates a sodium gradient used by the transportersto drive the "uphill" transport of the neurotransmitters (Kannerand Schuldiner, 1987). Because the ${alpha}$ 2 subunit was expressedboth in glial cells and in neurons (Fig. 3), we investigatedwhether the ${alpha}$ 2 subunit is involved in the neurotransmitter uptakeby astrocytes and/or nerve terminals.
First, we examined the uptake of the neurotransmitters intoP₂ fraction, which contains nerve-ending particles, preparedfrom whole embryonic brain at E16.5-17.5, when severe apoptosishad not yet occurred in the amygdala and piriform cortex ofthe homozygous mutant. To perform uptake assays, it was necessaryto use fresh samples from each fetal brain before confirmingthe genotype. It was difficult to isolate a sufficient amountof an enriched synaptosomal fraction from a single embryonicbrain by using a Ficoll or Percoll gradient centrifugationmethod; thus we used a P₂ fraction in the following experiments.The P₂ fraction of homozygous mutant mice showed lower neurotransmitteruptake activity for both glutamic acid and GABA (69 and 68%of the wild type, respectively) [Fig. 5C, columns 1, 3, 5(n = 5); D, columns 1, 3, 5 (n = 6)]. These uptake activitieswere inhibited 21–29% by ouabain in wild-type and heterozygousmutant samples (compare columns 1 and 2 and columns 3 and 4).On the contrary, the neurotransmitter uptake of the homozygousmutant was not significantly inhibited by ouabain (comparecolumns 5 and 6). These results indicate that the ouabain-sensitiveuptake of glutamic acid and GABA into the P₂ fraction at E16.5–17.5was mostly dependent on the function of the ${alpha}$ 2 subunit.
The P₂ fraction contains both presynaptic terminals and other membrane-bound particles, including glial cell membranes (Kanervaet al., 1978). To determine the role of glial transmitter uptakein the ${alpha}$ 2 mutant, we next examined the uptake of [³H]glutamicacid and [³H]GABA into cultured astrocytes. We prepared astrocytecultures from the brains of E16.5–17.5 wild-type, heterozygous,and homozygous embryos and confirmed the expression of GFAPby immunostaining (astrocytes prepared from a homozygous mutantare shown in Fig. 6A). The ${alpha}$ 2 subunit was expressed in the wild-type astrocytes (Fig. 6B), consistent with a previous report (Penget al., 1998). The amount of the ${alpha}$ 2 subunit protein was decreased $~$ 50% in the heterozygous mutant and was not detected in the homozygous mutant. In contrast, the uptake of glutamic acidor GABA was almost the same among the wild-type, heterozygous,and homozygous cells and was significantly inhibited by ouabainin all of the genotypes (Fig. 6C,D). Together, these resultsdemonstrate that the ouabain-sensitive uptake of neurotransmittersby glial cells was not dependent on the ${alpha}$ 2 subunit, whereasthis uptake by the P₂ fraction containing both neuronal and glial elements was partly dependent on the ${alpha}$ 2 subunit. We therefore conclude that the uptake of glutamic acid and GABA by neuronalterminals is impaired in the homozygous mutant, although wecannot entirely rule out the involvement of glial cells.
Enhanced fear and anxiety behavior in the heterozygous mutant
The amygdala and temporal lobe structures have critical rolesin emotional behavior (Swanson and Petrovich, 1998; Fendtand Fanselow, 1999; LeDoux, 2000; Maren, 2001; Davis, 2002).Although we could not document significant cell loss in theseregions in the heterozygous mutant brains (data not shown),we hypothesized that there might be a functional anomaly. Accordingly,we investigated the heterozygous mice for behavioral and neuralactivities. We performed the light/dark test (Fig. 7A–D) (n = 11 for each genotype), open field test (Fig. 7E) (n =16 for each genotype), and elevated-plus maze test (Fig. 7F,G) (n = 11 for each genotype) using adult male heterozygousmice and their wild-type littermate controls. In all of thesetests, the heterozygous mutant mice showed increased fear/anxietybehaviors compared with the wild-type mice. In contrast, generallocomotion activity, as measured by home-cage activity monitoring(Table 3, left column), and motor coordination, as measuredby rota-rod testing (Table 3, right column), were not significantlydifferent between the heterozygous and wild-type mice.

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Table 3. Spontaneous motor activity in the home cage and motor coordination (rota-rod test) of the adult wild-type and heterozygous mice

Finally, we investigated their response to conditioned fearstimuli (n = 8 for each genotype and treatment). The heterozygousmutant mice showed exaggerated freezing behaviors (Fig. 7H)compared with the wild-type mice after conditioned fear stimuli.These results strongly suggest that the heterozygous mutantmice have a functional anomaly in the amygdala and piriformcortex. To determine whether neural activity in the amygdalaor piriform cortex was abnormally increased in the heterozygousmutant mice under conditioned fear stimuli, we examined c-Fosexpression in these regions. After conditioned fear stimulus, the numbers of c-Fos-positive cells in the amygdala and piriformcortex were higher in the heterozygous mutant mice than inwild-type mice (Fig. 8A,B). In contrast, few c-Fos-positivecells were found in the amygdala and piriform cortex in theheterozygous or wild-type mice kept in the home cages (Fig.8C,D). These results indicate that the heterozygous mutantmice have abnormally enhanced neural activity in response toconditions that induce fear or anxiety.

   Discussion

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Selective damage of the amygdala and piriform cortex in Atp1a2 mutant mice
Maintenance of a membrane potential in electrically excitablecells is dependent on Na⁺ and K⁺ gradients that are generatedby the sodium pump. Inhibition of Na ⁺,K ⁺-ATPase enzyme activityby ouabain results in depolarization of neurons and glia. However,a low concentration of ouabain, which supposedly inhibits theactivity of ${alpha}$ 2 and ${alpha}$ 3 subunits but not ${alpha}$ 1, does not alter theresting membrane potential in rat brain slices (Calabresiet al., 1995), suggesting alternative roles of ${alpha}$ 2 and ${alpha}$ 3 subunitsother than the maintenance of the electrochemical gradientsof Na⁺ and K⁺ in brain. In our embryos with a homozygous mutationof the ${alpha}$ 2 subunit, the uptake of glutamic acid and GABA intothe P₂ fraction was significantly reduced. Interestingly, ouabaindecreased the uptake of these neurotransmitters into the P₂fraction from wild-type and heterozygous mice to the levelof the homozygous mutant, suggesting that ouabain-sensitiveuptake into the P₂ fraction of the embryonic brain is dependenton the ${alpha}$ 2 subunit. In contrast, cultured astrocytes from homozygousmutant embryos did not show any impairment of neurotransmitteruptake compared with wild-type and heterozygous mutant embryos.Therefore, we propose that the ${alpha}$ 2 subunit in neurons contributesto the clearance of neurotransmitters at this stage of development.This function is important to protect neurons from the continued activity of neurotransmitters. Figure 4A–C and Table 2demonstrate the presence of spontaneous neural activity inthe amygdala and piriform cortex in wild-type mice before birthand increased neural activity in these regions in the homozygousmutant mice. Although the physiological role of spontaneousneural activity in these regions during normal embryonic developmentis unknown, accumulation of glutamic acid in the extracellularspace may induce neural hyperactivity and eventually resultin neuronal apoptosis (Choi, 1988; Coyle and Puttfarcken,1993). GABA also acts as an excitatory neurotransmitter duringembryonic development, and GABA-mediated excitation can triggerCa ²⁺ influx (Ganguly et al., 2001). In addition, the amygdalaand piriform cortex are reported to be vulnerable to excitotoxicity(Candelario-Jalil et al., 2001). Accordingly, decreased neurotransmitteruptake in the homozygous mutant mice might enhance spontaneousneural activity and cause excitotoxic neuronal apoptosis, leadingto selective damage of these regions. Neuronal cell death inthe amygdala and piriform cortex, however, may not be the directcause of lethality in the homozygous mutant mice. Very recently, another mutation of the ${alpha}$ 2 subunit was established in mice bya different targeting strategy, and these mice are reportedto have a respiratory defect caused by a CNS impairment (Moseleyet al., 2002). It may be possible that our homozygous mutantmice also die because of defects in the regulation of the respiratorycircuits in the brain.
Impaired uptake of glutamic acid and GABA into P₂ fraction of homozygous mutant mice
Re-uptake of neurotransmitters, such as glutamic acid and GABA,is known to occur through their respective transporters. Afunctional link between the Na ⁺,K ⁺-ATPase and such transportershas been suggested by ouabain inhibition experiments (Kannerand Schuldiner, 1987; Wonnemann et al., 2000). Reduced uptakeof glutamic acid and GABA into the P₂ fraction in our homozygousmutant mice indicates that the ${alpha}$ 2 subunit of the Na ⁺,K ⁺-ATPaseis partially responsible for the re-uptake process. The activetransport of Na⁺ and K⁺ in the resting membrane is mediatedby the ${alpha}$ 1 subunit. The ${alpha}$ 2 subunit shows lower affinity for K⁺than ${alpha}$ 1 (Blanco et al., 1995) and functions less efficientlyin the resting condition. During neural excitation, however,the ${alpha}$ 2 subunit is activated by the higher K⁺ concentration inthe extracellular space. Therefore, the contribution of the ${alpha}$ 2 subunit to neurotransmitter re-uptake could be critical during neuronal activity. The functional coupling between the ${alpha}$ 2 subunitand transporters would be facilitated if the ${alpha}$ 2 subunit residesin close proximity with the neurotransmitter transporters.In this context, the model has been proposed that the colocalizationof the ${alpha}$ 2 subunit and the Na⁺/Ca ²⁺ exchanger allows an ${alpha}$ 2 isoform-specificfunction in the regulation of intracellular Ca ²⁺ concentrationsand cardiac contractility (Juhaszova and Blaustein, 1997;James et al., 1999). Although colocalization of the ${alpha}$ 2 subunitand amino acid transporters remains to be examined, the specificfunctions of the ${alpha}$ 2 subunit might be based on structural andfunctional coupling with Na⁺-dependent transporters.
Enhanced fear/anxiety behaviors in heterozygous mutant mice
The heterozygous mutant mice did not have any apparent anatomicalanomaly or enhanced neuronal degeneration in the amygdala andpiriform cortex during embryonic development (Figs. 2, 4)or in the adult (data not shown). However, the heterozygousmutant mice had enhanced fear/anxiety behaviors and increasedc-Fos expression in the amygdala and piriform cortex afterconditioned fear stimuli. Electrical or chemical stimulationof the amygdala produces a pattern of behavioral and autonomicchanges that resembles a state of fear (Davis, 2002). Thus,neuronal hyperactivity in these regions of the heterozygousmice may be a cause of the increased fear/anxiety behavior.In this regard, it is interesting that decreased expressionof the ${alpha}$ 2 subunit was reported in the temporal cortex of bipolarpatients (Rose et al., 1998). The enhanced fear/anxiety behaviorsof our adult heterozygous mutant mice could provide clues tothe pathophysiology of human affective disorders. In conclusion,our mutation of the Atp1a2 gene in mice reveals, for the firsttime, the functional significance of the ${alpha}$ 2 subunit in the developmentof the amygdala and piriform cortex and in emotional behaviorsin adult.

   Footnotes

Received Jan. 29, 2003; revised Mar. 11, 2003; accepted Mar. 17, 2003.
This work was supported by a grant from Takeda Science Foundation(K.I.), in part by grants from the Ministry of Education, Culture,Sports, Science and Technology, and Organization for PharmaceuticalSafety and Research, Japan (M.M.T.), and in part by the ResearchGrant for Cardiovascular Diseases (12C-5) (K.K.) from the Ministryof Health, Labor and Welfare. We thank Dr. K. Sweadner foranti- ${alpha}$ 2 antibody, Dr. S. J. Tapscott for critical reading ofthis manuscript, Dr. M. Mishina and Dr. K. Imoto for the helpful discussions, and S. Kamada, Y. Watanabe, M. Takiguchi, and H.Ohto for technical assistance. We also thank the anonymousreviewer for valuable comments to improve this manuscript.
Correspondence should be addressed to Dr. Kiyoshi Kawakami,Department of Biology, Jichi Medical School, Kawachi, Tochigi329-0498, Japan. E-mail: kkawakam{at}jichi.ac.jp.
M. M. Taketo's and T. Ishikawa's present address: Departmentof Pharmacology, Graduate School of Medicine, Kyoto University,Sakyo, Kyoto 606-8501, Japan.
Copyright © 2003 Society for Neuroscience 0270-6474/03/234667-10$15.00/0

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