Functional Change of NMDA Receptors Related to Enhancement of Susceptibility to Neurotoxicity in the Developing Pontine Nucleus

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The Journal of Neuroscience, October 1, 1998, 18(19):7941-7952

Functional Change of NMDA Receptors Related to Enhancement of Susceptibility to Neurotoxicity in the Developing Pontine Nucleus
Akira Mitani¹, Masahiko Watanabe², and Kiyoshi Kataoka¹
¹ Department of Physiology, School of Medicine, Ehime University, Shigenobu, Onsen-gun, Ehime 791-0295, Japan, and ² Department of Anatomy, Hokkaido University School of Medicine, Sapporo 060-8638, Japan

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The developing neurons have been reported to be extremely susceptible to toxicity of NMDA during a restricted developmentalperiod. Pontosubicular neuronal necrosis is a typical type ofperinatal human brain lesion and often coexists with other formsof cerebral hypoxic and ischemic injuries. To determine whetherfunctional changes of NMDA receptors related to the susceptibilityto NMDA toxicity are involved in developing neurons in the pontinenucleus, we have examined the lesion produced by in vivo directinjection of NMDA into the pontine nucleus of rats at postnataldays 1-30, recorded NMDA-induced whole-cell currents from neuronsin the pontine nucleus in the developing rat brainstem slices,and performed in situ hybridization for NMDA receptor subunitmRNAs in the pontine nucleus. The susceptibility to NMDA neurotoxicitypeaked near postnatal day 15, and the NMDA-induced currents showedprominent reduction of the voltage-dependent block by Mg²⁺ near postnatal day 15. The pontine nucleus near postnatal day15 showed distinct expression of the NMDA receptor subunit NR2CmRNA. These results suggest that the susceptibility to NMDA neurotoxicitythat is enhanced in the rat pontine nucleus near postnatal day15 is mediated by the NMDA receptor channels that are relativelyinsensitive to Mg²⁺ and that the reduction in the sensitivity of NMDA receptors toMg²⁺ correlates with the expression of the NR2C. We present the possibilitythat functional changes in the NMDA receptor channels play a crucialrole in the occurrence of developmentally specific neuronal injury.

Key words: NMDA receptor; pontine nucleus; development; neurotoxicity; slice patch clamp; Mg²⁺ block; in situ hybridization; NR2 subunits

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

NMDA receptors play an important role in neuronal plasticity (Collingridge and Bliss, 1987; Mayer and Westbrook, 1987; Rabacchiet al., 1992; Komuro and Rakic, 1993). Recent molecular biologicalstudies have revealed that marked changes occur in the distributionof mRNAs encoding various NMDA receptor subunits during developmentof the brain (Moriyoshi et al., 1991; Meguro et al., 1992; Watanabeet al., 1992; Yamazaki et al., 1992; Akazawa et al., 1994) andthat the changes result in the appearance of functionally distinctNMDA receptors (Ikeda et al., 1992; Kutsuwada et al., 1992; Moneyet al., 1992, 1994; Ishii et al., 1993; Farrant et al., 1994;Sakimura et al., 1995; Takahashi et al., 1996). The developingbrain has been reported also to be extremely susceptible to neurotoxicityproduced by NMDA during a restricted developmental period (McDonaldet al., 1988; McDonald and Johnston, 1990). These results mayindicate that the functional changes of NMDA receptors underliethe NMDA neurotoxicity enhanced during a restricted developmentalperiod.

Pontosubicular neuronal necrosis is a typical type of perinatal brain lesion (Friede, 1972). It often coexists with otherforms of cerebral hypoxic and ischemic injuries and is found inthe pontine nucleus and the subiculum of the hippocampus in thehuman brain during a restricted developmental period between 30weeks of gestation and the second postnatal month (Friede, 1972;Torvik et al., 1992; Sohma et al., 1995). These clinical reportssuggest the possibility that some functional changes of NMDA receptorsare involved in neurons in the pontine nucleus and the subiculumduring the restricted developmental period. The purpose of thisstudy is to find the functional changes of NMDA receptors thatare related to the susceptibility to NMDA toxicity in neuronsof the pontine nucleus (PN neurons) during development. First,to determine whether changes in the susceptibility to NMDA neurotoxicityis involved in the developing pontine nucleus, we have examinedthe extent of the lesion produced by in vivo direct injectionof NMDA into the developing pontine nucleus of the rat. Second,to determine what functional changes of NMDA receptors mediatethe changes in the susceptibility to NMDA neurotoxicity, we haverecorded whole-cell currents induced by NMDA from PN neurons ofdeveloping rat brainstem slices. Third, to clarify the molecularbasis for the functional changes of NMDA receptors, we have performedin situ hybridization for NMDA receptor subunit mRNA expressionwith ³⁵S-dATP-labeled antisense oligonucleotides in the brainstem includingthe pontine nucleus.

According to histogenetic studies (Rakic and Sidman, 1970; Sidman and Rakic, 1982), mossy fibers of the pontine nucleus makecontact with granule cells of the cerebellar cortex by ~30 weeksof gestation in the human. This stage approximately correspondsto the second postnatal week of the rat in which pontine mossyfibers begin to form synaptic connections with granule cells atpostnatal days 10-12 (Altman, 1972a,b; Shimono et al., 1976).Therefore, in the present study, we have used rats at postnataldays 1-30.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The following experiments were conducted in accordance with the Guideline for Animal Experimentation at Ehime University Schoolof Medicine.

In vivo injection of NMDA. To examine developmental changes in neuronal susceptibility to the toxicity produced by NMDA, weinjected NMDA in the pontine nucleus of Sprague Dawley rats atpostnatal days 5-7 (P5-P7) (n = 18), at P14-P16 (n = 18), at P20-P21(n = 18), and at P28-P30 (n = 18). P1 was designated as the dayof birth. The animals were anesthetized with a mixture of 2.5%halothane in nitrous oxide/oxygen (7:3). Micropipettes (tip diameter,50-60 µm) were pulled from thin-walled glass (105G; Drummond ScientificCompany, Broomall, PA) and equipped with a stainless steel plunger(105P; Drummond Scientific Company) and a micrometer. The micropipetteswere filled with 0.1, 0.5, or 1.0 mM NMDA (Sigma, St. Louis, MO)dissolved in a Ringer's solution, adjusted to pH 7.4. Stereotaxicpressure injections (total volume, 1 µl; 0.04 µl/min for 25 min)were made into the pontine nucleus of rats at P5-P7 (n = 6, 0.1mM NMDA; n = 6, 0.5 mM NMDA; and n = 6, 1.0 mM NMDA), at P14-P16(n = 6, 0.1 mM NMDA; n = 6, 0.5 mM NMDA; and n = 6, 1.0 mM NMDA),at P20-P21 (n = 6, 0.1 mM NMDA; n = 6, 0.5 mM NMDA; and n = 6,1.0 mM NMDA), and at P28-P30 (n = 6, 0.1 mM NMDA; n = 6, 0.5 mMNMDA; and n = 6, 1.0 mM NMDA); injections were 0.2 mm rostralto lambda, 0.5 mm lateral to the midline, and 6.5 mm ventral tothe cortical surface in P5-P7 rats; 0.2 mm rostral to lambda,0.5 mm lateral to the midline, and 9.0 mm ventral to the corticalsurface in P14-P16 rats; 0.1 mm rostral to lambda, 1.0 mm lateralto the midline, and 9.0 mm ventral to the cortical surface inP20-P21 rats; and 0.1 mm rostral to lambda, 1.0 mm lateral tothe midline, and 9.6 mm ventral to the cortical surface in P28-P30rats. Equivalent volumes of a Ringer's solution were injectedinto the pontine nucleus of control animals (n = 2, P5-P7 rats;n = 2, P14-P16 rats; n = 2, P20-P21 rats; and n = 2, P28-P30 rats).After injections, the micropipettes were gently pulled out, andsurgical incisions were carefully sutured. Rats were treated withantibiotics and brought into a comfortable position on a warmingblanket. After awakening, rats at P5-P7 and P14-P16 were returnedto their mothers, and rats at P20-P21 and P28-P30 were returnedto individual cages. After 4 d of survival, the animals were deeplyanesthetized with sodium pentobarbital and transcardially perfusedwith 10% formalin in 0.1 M phosphate buffer, pH 7.4. The brainswere removed and saturated with a solution of 25% sucrose in thesame buffer. Subsequently, frontal frozen sections were made seriallyat 40 µm for Nissl stain. The serial sections of the pontine nucleuswere scanned to determine which section contained the largestlesion, and the longest axis of the lesion was evaluated as theextent of the lesion produced by NMDA neurotoxicity.

In addition, to confirm that the lesion elicited by NMDA injection is attributable to NMDA receptor stimulation, we injected1 mM D-2-amino-5-phosphonopentanoic acid (AP-5), a competitiveantagonist of the NMDA receptor (Tocris Cookson, Bristol, UK),0.1 mM ketamine, a noncompetitive antagonist of the NMDA receptor(Sigma), or 0.5 mM 2,3-dihydroxy-6-nitro-7-sulfamoyl-benzo(F)quinoxaline(NBQX), a non-NMDA receptor antagonist (Tocris Cookson), with0.5 mM NMDA into the pontine nucleus at P14-P16 (for each group,n = 6). Then, by use of the same procedure described above, theextent of the lesion was measured to examine whether it is reducedby the antagonists.

Preparation for whole-cell recording. Rats from P1 to P30 were decapitated under ether anesthesia. After the brainstem includingthe pontine nucleus was isolated, frontal slices (150 µm) werecut using a vibrating slicer (DSK 1000; Dosaka, Kyoto, Japan).Slices were incubated at 36°C for 1 hr and then maintained atroom temperature (23-25 °C) in a standard Ringer's solution containing(in mM): NaCl, 124; KCl, 2; KH₂PO₄, 1.5; NaHCO₃, 26; MgCl₂, 1;CaCl₂, 2; and glucose, 10, pH 7.4, when equilibrated with 95%O₂/5% CO₂. For experiments, slices were transferred into a superfusingchamber (volume, ~0.5 ml) on a stage of an upright microscopeequipped with an epifluorescence system (Axioskop; Zeiss), helddown with a nylon net stretched out on a U-shaped piece of flattenedplatinum wire (Edwards et al., 1989), and perfused with a standardRinger's solution equilibrated with 95% O₂/5% CO₂. Cells in thepontine nucleus were viewed under Nomarski optics with a water-immersion40× objective (Zeiss) at a magnification of 640× and also monitoredusing a CCD camera and television monitor system (XC-77; Sony,Tokyo, Japan) at a magnification of 1000×.

Solutions. Solutions were equilibrated with 95% O₂/5% CO₂. Tetrodotoxin (1 µM) (Wako, Osaka, Japan) and bicuculline (20 µM)(Sigma) were added routinely to a standard Ringer's solution toblock Na⁺ currents and spontaneous synaptic activities mainly mediatedby GABA, respectively; glycine (10 µM) (Wako) was also added tothe solution to ensure a constant, saturating concentration ofglycine for the NMDA receptor (Johnson and Ascher, 1987) (1 mMMg²⁺ Ringer's solution). To release NMDA responses from a Mg²⁺ block (Mayer et al., 1984; Nowak et al., 1984), we reduced Mg²⁺ to 0.1 mM (0.1 mM Mg²⁺ Ringer's solution) or omitted Mg²⁺ from the solution (we defined this solution as a nominally 0mM Mg²⁺ Ringer's solution in the present study). To examine the permeationof Ca²⁺ through NMDA receptor channels in the presence of Mg²⁺, we changed the solution to a Ca²⁺ Ringer's solution in which Na⁺ and K⁺ were replaced with an impermeant cation N-methylglucamine (NMG)(Sigma) (Iino et al., 1990). The Ca²⁺ Ringer's solution contained 135 mM NMG, 10 mM glucose, 10 mMHEPES, 10 mM CaCl₂, 5 mM MgCl₂, 1 µM tetrodotoxin, 20 µM bicuculline,and 10 µM glycine, equilibrated with O₂ and adjusted to pH 7.4with HCl; the osmolarity was ~305 mOsm/l.

Patch pipettes were pulled from thin-walled glass (GC150TF-15; Clark Electromedical Instruments, Pangbourne, UK), coated withSylgard resin, and fire-polished to a final resistance of 8-10M $Omega$ . The pipette solution contained (in mM): Cs gluconate, 110;CsCl, 40; NaCl, 4; HEPES, 10; EGTA, 5; CaCl₂, 0.5; and Mg-ATP,2, adjusted to pH 7.2 with CsOH; the osmolarity was ~295 mOsm/l.

Drug application. NMDA was applied by bath application to examine current responses evoked by a long-lasting high concentrationof extracellular glutamate that is considered to be induced underhypoxic conditions (Benveniste et al., 1984; Hagberg et al., 1985;Globus et al., 1991; Mitani et al., 1992, 1994b) or was appliedby ionophoresis to examine developmental changes in the voltage-dependentMg²⁺ block of NMDA receptor channels at various membrane potentialsand also was applied by ionophoresis to examine the permeationof Ca²⁺ through NMDA receptor channels. For bath application, 50 µM NMDAwas dissolved in a 1 mM Mg²⁺ or a nominally 0 mM Mg²⁺ Ringer's solution. The 50 µM NMDA solution was applied to a slicefor 2 min by switching the superfusion line at the inlet of therecording chamber with magnetic pinch valves. The dead-space timewas ~5 sec. Usually, a single trial of the NMDA bath applicationwas performed in each slice. For ionophoric application, a high-resistance(100 M $Omega$ ) electrode was used. The electrode was filled with 100mM NMDA solution. To dissolve NMDA, we added NMG to the solutionuntil the pH was raised to 7.4 (Iino et al., 1990). The NMDA wasapplied to the soma perfused with a nominally 0, 0.1, or 1 mMMg²⁺ Ringer's solution using 100 msec current pulses of 100-500 nAintensity at a frequency of 0.05 Hz; a retaining current of 1-5nA was used to prevent leakage. All recordings are performed atroom temperature (23-25 °C).

Whole-cell recording. Whole-cell recordings were made from PN neurons using an EPC-9 (List, Germany) amplifier. The seal resistancewas usually >10 G $Omega$ . Holding potentials were corrected for theliquid junction potential between pipette solution and superfusate(approximately +7 mV). The cell capacitance was measured fromtransient currents produced by 10 mV hyperpolarizing-voltage steps.NMDA-induced currents were low-pass filtered at 10 kHz (three-poleBessel filter) and stored on a pulse code modulation data recorderfor later off-line analysis. In addition, by the use of a CCDcamera and television monitor system at a magnification of 1000×,the cell body size of recorded neurons was evaluated by measuringmajor and minor diameters; the major diameter was the longestaxis, and the longest diameter at a right angle to the longestaxis was defined as the minor diameter.

In some experiments, whole-cell recordings were made from retrogradely labeled PN neurons after injection of a fluorescentdye into the cerebellar cortex. The micropipettes (tip diameter,50-60 µm) were filled with 10% rhodamine-B dextran-amine (70,000MW; Molecular Probes, Eugene, OR) dissolved in 0.9% saline (Schmuedet al., 1990), and pressure injections (total volume, 1 µl; 0.04µl/min for 25 min) were accomplished into the cerebellar cortexof rats at P8-P25 with the same procedure that was used for invivo injection of NMDA. After 4-6 d of survival, brainstem slicesthat included the pontine nucleus were made from the rats. Afteridentification of retrogradely labeled pontinecerebellar-projectingPN neurons, whole-cell recordings were made from the labeled PNneurons (Manabe et al., 1991).

In situ hybridization. Rats at P1, P7, P11, P14, P21, and 4 months of age (adult) were deeply anesthetized with pentobarbitaland then killed by decapitation. The brains were fresh frozenin powdered dry ice. Subsequently, frontal sections were cut at20 µm on a cryostat and mounted on glass slides. They were fixedwith 4% paraformaldehyde in 0.1 M phosphate buffer for 10 minand then acetylated with 0.25% acetic anhydride in 0.1 M triethanolamine-HCl,pH 8.0, for 10 min. For isotopic detection of mRNAs for the ratNMDA receptor subunits that have been designated as NR1, NR2A,NR2B, NR2C, and NR2D, 45-mer nonoverlapping antisense oligonucleotideswere synthesized against nucleotide residues 236-280 of the ratNR1 cDNA (Hollmann et al., 1993; accession number L08228),residues 3189-3233 of the rat NR2A cDNA (Money et al., 1992; accessionnumber M91561), residues 3242-4286 of the rat NR2B cDNA (Moneyet al., 1992; accession number M91562), residues 144-188 ofthe rat NR2C cDNA (Money et al., 1992; accession number M91563),and residues 2951-2995 of the rat NR2D (Money et al., 1994; accessionnumber L31611). Oligonucleotides were labeled with ³⁵S-dATP to a specific activity of 0.5 × 10⁹ dpm/µg of DNA by the use of terminal deoxyribonucleotidyl transferase(BRL, Bethesda, MD). After prehybridization at room temperaturefor 1 hr in a hybridization buffer containing 50% formamide, 50mM Tris-HCl, pH 7.5, 0.02% Ficoll, 0.02% polyvinylpyrrolidone,0.02% bovine serum albumin, 0.6 M NaCl, 0.25% sodium dodecyl sulfate,200 µg/ml tRNA, 1 mM EDTA, and 10% dextran sulfate, the hybridizationwas performed at 42°C for 10 hr in the hybridization buffer supplementedwith 10,000 cpm/µl of ³⁵S-labeled oligonucleotide probes and 0.1 M dithiothreitol. Then,the slides were washed twice at 55°C for 40 min in 0.1× SSC (1×SSC, 0.15 M NaCl and 0.015 M sodium citrate) containing 0.1% sarcosyland were exposed for 3 weeks to Hyperfilm $beta$ -max (Amersham, ArlingtonHeights, IL). Other details pertaining to the histological proceduresfor in situ hybridization are described elsewhere (Watanabe etal., 1992, 1993).

Data analysis. Data obtained by whole-cell recordings were analyzed using the data analysis software EP Analysis (version1.1) (Shoshin, Okazaki, Japan) on a Macintosh computer. All valuesin the text are expressed as mean ± SEM. Statistical significancewas assessed using ANOVA with a Bonferroni/Dunn post hoc analysisfor intergroup significance of difference.

  RESULTS

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Abstract
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Materials & Methods
Results
Discussion
References

Susceptibility to NMDA neurotoxicity

The extent of the lesion produced by direct injection of NMDA into the pontine nucleus varied over postnatal development (Figs.1, 2). Injection of 0.1 mM NMDA produced a very small lesion inthe pontine nucleus at any age; the lesion was confined to thetract of micropipettes, and the size did not differ from thatof the injection of a Ringer's solution (Fig. 2). Injection of0.5 mM NMDA produced substantial neuronal loss in the pontinenucleus at P14-P16; extensive lesion with a diameter of ~0.4 mmwas produced (Fig. 1C,D). In contrast, the 0.5 mM NMDA injectiondid not show any obvious neuronal loss in the pontine nucleusat P5-P7, P20-P21, and P28-P30 (Figs. 1A,B,E,F, 2) except foroccasional appearances of reactive glial cells surrounding thetract of micropippetes and the injection site at P20-P21 (datanot shown) and P28-P30 (Fig. 1E,F). Injection of 1.0 mM NMDA producedmore widespread neuronal loss in the pontine nucleus at P14-P16and produced restricted neuronal loss or disruption of the normalcytoarchitecture in the pontine nucleus at P5-P7, P20-P21, andP28-P30 (Fig. 2). Quantitative analysis of the extent of lesiondemonstrated that the pontine nucleus at P14-P16 was most susceptibleto the toxicity of NMDA; post hoc analysis showed that the extentof lesion at P14-P16 was significantly larger than that at P5-P7,P20-P21, and P28-P29 (p < 0.0001, after injections of 0.5 and1.0 mM NMDA) (Fig. 2). Interestingly, some normal-appearing neuronswere observed in the lesion sites produced by NMDA (Fig. 1D).This means that some neurons that are comparatively tolerant tothe toxicity of NMDA intermingle with many neurons that are susceptibleto the toxicity of NMDA in the developing pontine nucleus. Theymay be interneurons in the pontine nucleus.

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Figure 1. Changes in the susceptibility of neurons in the pontine nucleus to NMDA neurotoxicity during postnatal development. Nissl-stained frontal brainstem sections are shown. A unilateral injection of 0.5 mM NMDA (total volume, 1 µl; 0.04 µl/min for 25 min) was made into the developing rat pontine nucleus, and the animals were killed 4 d later. A, C, E, The severity of the brain lesion is maximal at P14; substantial neuronal loss is observed in the pontine nucleus (C). In comparison with that at P14, obvious neuronal loss is not observed at P7 (A) and P28 (E) except for occasional appearances of reactive glial cells surrounding the track of a micropipette and the injection site (E). Arrows indicate traces of the tip of a micropipette for injection. B, D, F, Higher magnifications of the pontine nucleus surrounding the NMDA injection site in A, C, and E, respectively, are shown. Note that some normal-appearing neurons are observed in the lesion (some of them are indicated by arrowheads in D). Scale bars: A, C, E, 0.4 mm; B, D, F, 0.1 mm.

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Figure 2. Dose-response comparison of the maximum extent of NMDA-induced lesion during postnatal development. Animals received a unilateral injection of Ringer's solution or of 0.1, 0.5, or 1.0 mM NMDA (total volume, 1 µl; 0.04 µl/min for 25 min) into the pontine nucleus and were killed 4 d later. The serial sections of the pontine nucleus were scanned to determine which section contained the largest lesion, and the longest axis of the lesion was evaluated as the maximum extent of lesion. Data represent mean ± SEM (bars) (each column for NMDA, n = 6; each column for Ringer's solution, n = 2). After injections of 0.5 or 1.0 mM NMDA, the extent of lesion at P14-P16 (stippled columns) is significantly larger than the corresponding value at P5-P7 (filled columns), P20-P21 (hatched columns), and P28-P30 (open columns). Statistical analysis consisted of one-way ANOVA and Bonferroni/Dunn post hoc tests (*p < 0.0001, compared with values at P5-P7, P20-P21, and P28-P30).

To confirm that the NMDA neurotoxicity elicited is attributable to NMDA receptor stimulation, we examined in the pontine nucleusat P14-P16 whether the lesion produced by the NMDA injection isreduced by NMDA receptor antagonists AP-5 and ketamine but notby the non-NMDA receptor antagonist NBQX. The lesion producedby 0.5 mM NMDA was markedly reduced by 1 mM AP-5 [maximum extentof lesion, 41.8 ± 7.9 µm (n = 6; mean ± SEM)] (data not shown)and 0.1 mM ketamine [maximum extent of lesion, 37.5 ± 5.6 µm (n= 6)] (Fig. 3A) but not by 0.5 mM NBQX [maximum extent of lesion,417.5 ± 47.4 µm (n = 6)] (Fig. 3B).

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Figure 3. Effects of NMDA and non-NMDA receptor antagonists on NMDA neurotoxicity during postnatal development. Nissl-stained frontal brainstem sections are shown. A, Ketamine (0.1 mM), a noncompetitive antagonist of the NMDA receptor, was injected with 0.5 mM NMDA (total volume, 1 µl; 0.04 µl/min for 25 min) into the pontine nucleus at P14. B, NBQX (0.5 mM), a non-NMDA receptor antagonist, was injected with 0.5 mM NMDA into the pontine nucleus at P14. The animals were killed 4 d later. The lesion produced by 0.5 mM NMDA is blocked by 0.1 mM ketamine (A) but not by 0.5 mM NBQX (B); obvious neuronal loss is observed surrounding the injection site in B. Arrows indicate traces of the tip of a micropipette. Scale bar, 0.4 mm.

These results indicate that the susceptibility of neurons in the pontine nucleus to NMDA neurotoxicity markedly changes duringpostnatal development and that the susceptibility peaks near postnatalday 15 in the developing pontine nucleus.

Developing changes in cell body size and capacitance

The cell body size of recorded neurons, which was measured using a CCD camera and television monitor system at a magnificationof 1000×, increased during the first two postnatal weeks; themajor and minor diameters of neurons were 12.1 ± 0.7 and 9.3 ±0.4 µm at P1-P2 (n = 14) and 22.3 ± 0.8 and 16.1 ± 0.6 µm at P15-P16(n = 16; mean ± SEM). After postnatal day 16, there were no significantchanges in cell body size; the major and minor diameters of neuronswere 21.1 ± 0.8 and 15.4 ± 0.6 µm at P29-P30 (n = 14). In addition,the capacitance of PN neurons increased during the first two postnatalweeks from 3.2 ± 0.3 pF at P1-P2 (n = 14) to 13.2 ± 0.6 pF atP15-P16 (n = 37). After postnatal day 16, no significant changesin the capacitance with age were observed; the capacitance atP29-P30 was 14.6 ± 0.7 pF (n = 24). These results indicate thatthe cell membrane surface of PN neurons shows a fourfold increaseand reaches the adult value during the first two postnatal weeks.

Current responses evoked by a long-lasting high concentration of extracellular NMDA

Bath application of NMDA (50 µM) induced small currents in the PN neurons at P1-P2 in a nominally 0 mM Mg²⁺ and also in a 1 mM Mg²⁺ Ringer's solution (Figs. 4a,d, 5). The NMDA-induced currentsin a nominally 0 mM Mg²⁺ Ringer's solution steeply increased during the first two postnatalweeks (Fig. 5A); large NMDA-induced currents were evoked in thePN neurons near postnatal day 15 (Fig. 4b). The currents of P15-P16neurons held at $-$ 80 mV were ~33 times greater than those of P1-P2neurons held at $-$ 80 mV. The NMDA-induced currents in a 1 mM Mg²⁺ Ringer's solution also markedly increased during the first twopostnatal weeks and reached a peak at P15-P16 (Fig. 5B). SubstantialNMDA-induced currents were observed in the PN neurons near postnatalday 15 even in the presence of 1 mM Mg²⁺ (Fig. 4e). The currents of P15-P16 neurons held at $-$ 80 mV were~31 times greater than those of P1-P2 neurons held at $-$ 80 mV.After postnatal day 16, the NMDA-induced currents in a nominally0 mM Mg²⁺ Ringer's solution slightly decreased, and the amplitudes of thecurrents were maintained at comparatively high levels (Fig. 5A);large NMDA-induced currents were evoked in the PN neurons at P29-P30held at $-$ 80 mV in a nominally 0 mM Mg²⁺ Ringer's solution (Fig. 4c). In contrast, the NMDA-induced currentsin a 1 mM Mg²⁺ Ringer's solution markedly declined (Fig. 5B). When the PN neuronsat P29-P30 were perfused with a 1 mM Mg²⁺ Ringer's solution, the amplitudes of the NMDA-induced currentswere markedly reduced (Fig. 4f). This Mg²⁺ block of NMDA-induced currents is a typical feature of NMDA receptors,and this observation is consistent with that in previous studies(Mayer et al., 1984; Nowak et al., 1984). Generally, NMDA receptorchannels are sensitive to voltage-dependent block by Mg²⁺, and the activation of NMDA receptor channels is usually blockedby Mg²⁺ at resting membrane potentials. Therefore, the present NMDA responsesthat are activated at $-$ 80 mV in a 1 mM Mg²⁺ Ringer's solution in the PN neurons near postnatal day 15 areconsidered to be relatively insensitive to Mg²⁺.

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Figure 4. Whole-cell responses to bath application of NMDA (50 µM) during postnatal development. The responses were recorded at $-$ 80 mV in the presence of 0 mM Mg²⁺ (a-c) and 1.0 mM Mg²⁺ (d-f) from neurons in the pontine nucleus at P2 (a, d), P15 (b, e), and P29 (c, f). The paired arrows indicate the duration of NMDA application. Small responses to NMDA are observed in neurons of the pontine nucleus at P2 in a nominally 0 mM Mg²⁺ Ringer's solution (a) and in a 1 mM Mg²⁺ Ringer's solution (d). Large responses to NMDA are observed in neurons of the pontine nucleus at P15 (b) and P29 (c) in a nominally 0 mM Mg²⁺ Ringer's solution. In the presence of 1.0 mM Mg²⁺, the response to NMDA at P29 shows a typical Mg²⁺ block; the NMDA-induced current is markedly reduced (f). In contrast, the degree of Mg²⁺ block at P14 is smaller than that at P29; a substantial NMDA-induced current is induced even in the presence of 1.0 mM Mg²⁺ (e). Solutions contained 1 µM tetrodotoxin, 20 µM bicuculline, and 10 µM glycine.

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Figure 5. Developmental changes in whole-cell responses to bath application of NMDA (50 µM) during postnatal development. Histograms show pooled data of peak amplitudes of NMDA-induced currents (error bars represent SEM; n = 6-20). The responses were recorded from developing neurons in the pontine nucleus at $-$ 80 mV in the presence of 0 mM Mg²⁺ (A) and 1.0 mM Mg²⁺ (B). In a nominally 0 mM Mg²⁺ solution (A), the responses at P13-P14 and P15-P16 are significantly greater than those at P1-P2, P3-P4, P5-P6, P7-P8, and P9-P10 (one-way ANOVA and Bonferroni/Dunn post hoc tests; p < 0.0001). In the presence of 1.0 mM Mg²⁺, the responses at P13-P14 and P15-P16 are significantly greater than those at P1-P2, P3-P4, P5-P6, P7-P8, P9-P10, P19-P20, P21-P22, P23-P24, P25-P26, P27-P28, and P29-P30 (one-way ANOVA and Bonferroni/Dunn post hoc tests; p < 0.0001). Solid circles indicate the peak current amplitudes recorded from retrogradely labeled neurons in the pontine nucleus after injection of a fluorescent dye into the cerebellar cortex (10% rhodamine-B dextran-amine).

Whole-cell recordings from retrogradely labeled PN neurons revealed that labeled PN neurons, which were identified as pontine-cerebellar-projectingPN neurons, showed the same developmental changes in NMDA-inducedcurrents that are described above (Fig. 5, solid circles). Thisresult means that the developmental changes in the NMDA-inducedcurrents observed in the present study represent those of thepontine-cerebellar-projecting PN neurons.

These results indicate that NMDA-induced currents that are relatively insensitive to Mg²⁺ increase and reach a peak in developing PN neurons near postnatalday 15 when PN neurons are most susceptible to NMDA toxicity.

Voltage-dependent Mg²⁺ block

Whole-cell recordings were made from PN neurons at P3-P4 (n = 12), P14-P15 (n = 12), and P28-P29 (n = 12). Ionophoretic applicationsof NMDA were performed to evoke current responses in PN neuronsperfused with a nominally 0, 0.1, or 1 mM Mg²⁺ Ringer's solution. Current-voltage relationships were obtainedfor the current responses to NMDA at P3-P4, P14-P15, and P28-P29.The currents reversed close to 0 mV in all cases. At P3-P4 andP28-P29, the current responses to NMDA in a nominally 0 mM Mg²⁺ Ringer's solution varied nearly linearly with a wide range ofmembrane potentials (Fig. 6Aa,Ac,Ba,Bc, open circles). In thepresence of extracellular Mg²⁺, the current responses showed a typical voltage-dependent blockby Mg²⁺. The addition of extracellular 0.1 mM Mg²⁺ produced little change in the outward currents but markedly reducedthe inward currents (Fig. 6Ad,Af,Ba,Bc, solid circles). The blockingeffect of Mg²⁺ increased as the membrane potential was hyperpolarized. The voltage-dependentMg²⁺ block of the current responses to NMDA was more pronounced in1 mM Mg²⁺ (Fig. 6Ba,Bc, solid triangles). At P14-P15, the current responsesto NMDA in a nominally 0 mM Mg²⁺ Ringer's solution varied nearly linearly with a wide range ofmembrane potentials (Fig. 6Ab,Bb, open circles). In the presenceof extracellular Mg²⁺, the current responses to NMDA at P14-P15 showed resistance tothe voltage-dependent block by Mg²⁺. The addition of extracellular 0.1 mM Mg²⁺ produced little change in the outward currents and induced limitedreductions in inward currents. The degree of voltage-dependentblock by 0.1 mM Mg²⁺ was smaller compared with that at P3-P4 and at P28-P29 (Fig.6Ae,Bb, solid circles). The decrease in the blocking effect ofMg²⁺ was also observed after the addition of extracellular 1 mM Mg²⁺ (Fig. 6Bb, solid triangles). At a holding potential of $-$ 70 mV,the remaining proportion of the peak amplitude of current responsesin 0.1 mM Mg²⁺ was 66.1 ± 5.6% of that in a nominally 0 mM Mg²⁺ Ringer's solution at P14-P15, whereas it was 33.2 ± 2.5% of thatat P3-P4 and 31.4 ± 2.5% of that at P28-P29 (p < 0.0001, Bonferroni/Dunnpost hoc tests) (Fig. 7A). Also the proportion of the currentresponses remaining unblocked in 1 mM Mg²⁺ was 12.4 ± 1.3% of that in a nominally 0 mM Mg²⁺ Ringer's solution at P14-P15, whereas it was 5.5 ± 0.2% of thatat P3-P4 and 5.8 ± 0.7% of that at P28-P29 (p < 0.0001, Bonferroni/Dunnpost hoc tests) (Fig. 7B). These results reinforce that the degreeof voltage-dependent Mg²⁺ block of the current responses to NMDA is prominently reducedin developing PN neurons near postnatal day 15.

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Figure 6. Voltage-dependent Mg²⁺ block of current responses to NMDA during postnatal development. A, Current responses recorded in a nominally 0 mM Mg²⁺ Ringer's solution (a-c) and in a 0.1 mM Mg²⁺ Ringer's solution (d-f) at different holding potentials are superimposed; holding potentials (in mV) are indicated in a-f. Ionophoretic applications of NMDA were performed to evoke current responses of neurons in the pontine nucleus at P3 (a, d), P14 (b, e), and P28 (c, f). B, Current-voltage relationships of the responses to NMDA obtained from neurons in the pontine nucleus at P3-P4 (a), P14-P15 (b), and P28-P29 (c) are shown. Data points are obtained in a nominally 0 mM Mg²⁺ Ringer's solution (open circles) and in the presence of 0.1 mM Mg²⁺ (solid circles) and 1 mM Mg²⁺ (solid triangles). All solutions contained 1 µM tetrodotoxin, 20 µM bicuculline, and 10 µM glycine. The peak amplitudes of the responses to NMDA were normalized to the mean value at +50 mV in each experimental condition. Data are mean ± SEM (n = 12).

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Figure 7. Changes in the Mg²⁺ block of current responses to NMDA in developing neurons in the pontine nucleus. Histograms show pooled data of peak amplitudes of current responses remaining after Mg²⁺ block relative to responses in a nominally 0 mM Mg²⁺ Ringer's solution (error bars represent SEM; each column, n = 12). The data were obtained at $-$ 70 mV in the presence of 0.1 mM Mg²⁺ (A) and 1.0 mM Mg²⁺ (B) from neurons in the pontine nucleus at P3-P4, P14-P15, and P28-P29. The remaining proportions of current responses in the presence of 0.1 and 1.0 mM Mg²⁺ at P14-P15 are significantly larger than the corresponding values at P3-P4 and at P28-P29 (one-way ANOVA and Bonferroni/Dunn post hoc tests, *p < 0.0001).

Permeation of Ca²⁺ through NMDA receptor channels in the presence of Mg²⁺

A decrease in Mg²⁺ block would increase the Ca²⁺ entry particularly at the resting membrane potential. We examined permeationof Ca²⁺ through NMDA receptor channels that are relatively insensitiveto Mg²⁺. Whole-cell recordings were made from PN neurons at P3-P4 (n= 8), P14-P15 (n = 8), and P28-P29 (n = 8). Ionophoretic applicationsof NMDA were performed to evoke Ca²⁺ currents in PN neurons that were perfused with a Ca²⁺ Ringer's solution in which Na⁺ and K⁺ were replaced with an impermeant cation NMG and 10 mM Ca²⁺ and 5 mM Mg²⁺ were added. When PN neurons were held at a more negative membranepotential ( $-$ 100 mV) to eliminate the currents through NMDA receptorchannels that are sensitive to voltage-dependent Mg²⁺ block, the amplitudes of NMDA-induced Ca²⁺ currents at P3-P4 and P28-P29 were very small (Fig. 8a,c), whereassubstantial NMDA-induced Ca²⁺ currents were induced in PN neurons at P14-P15 (Fig. 8b). Ata holding potential of $-$ 100 mV, the amplitudes of Ca²⁺ currents at P14-P15 were significantly larger than those at P3-P4and P28-P29 (p < 0.0001) (Fig. 9). These results indicate thatthe NMDA channels that are relatively insensitive to Mg²⁺ in developing PN neurons near postnatal day 15 are permeableto Ca²⁺ at the resting membrane potential.

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Figure 8. Permeation of Ca²⁺ through NMDA receptor channels in the presence of Mg²⁺ during postnatal development. Neurons in the pontine nucleus at P3 (a), P14 (b), and P28 (c) were perfused with a Ca²⁺ Ringer's solution in which Na⁺ and K⁺ were replaced with an impermeant cation NMG and 10 mM Ca²⁺ and 5 mM Mg²⁺ were added. Ionophoretic applications of NMDA were performed to evoke current responses. Current responses at $-$ 100 mV are shown. Substantial NMDA-induced Ca²⁺ currents are shown at P14.

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Figure 9. Changes in permeation of Ca²⁺ through NMDA receptor channels of developing neurons in the pontine nucleus at $-$ 100 mV in the presence of Mg²⁺. The responses were recorded from neurons in the pontine nucleus at P3-P4, P14-P15, and P28-P29. The amplitude of current responses was normalized to the mean value at +50 mV in each experiment. Histograms show pooled data of peak amplitudes of current responses to NMDA in a Ca²⁺ Ringer's solution. Error bars represent SEM (each column, n = 8). The normalized peak amplitude of current responses to NMDA at P14-P15 is significantly larger than that at P3-P4 and at P28-P29 (one-way ANOVA and Bonferroni/Dunn post hoc tests, *p < 0.0001).

In situ hybridization for NMDA receptor subunit mRNAs

Prominent expression signals for the NR1 mRNA were already expressed in the pontine nucleus and also in other various brainstemnuclei at P1 and were observed at all developmental stages examined(Fig. 10A-E). Few specific signals for the NR2A mRNA were foundin the pontine nucleus at P1. Specific signals for the NR2A mRNAappeared in the pontine nucleus at P7, the signal intensity increasedgradually until P21, and the expression of NR2A mRNA in the pontinenucleus slightly decreased in adult rats (Fig. 10F-J). The NR2BmRNA was intensely expressed in the pontine nucleus and also inother various brainstem nuclei at P1. Then, the signal intensityin the pontine nucleus gradually decreased and was weak in adultrats (Fig. 10K-O). Few specific signals for the NR2C mRNA werefound in the pontine nucleus during the first week after birth(Fig. 10P,Q). Expression signals for the NR2C mRNA appeared inthe pontine nucleus after P7; the signals were distinctly expressedin the pontine nucleus at P11 (data not shown), P14 (Fig. 10R),and also P21 (Fig. 10S). In adult rats, the NR2C mRNA was stillexpressed in the pontine nucleus (Fig. 10T). No specific signalsfor the NR2D mRNA were detected in the pontine nucleus at P1,whereas the signals were intensely expressed in many other brainstemnuclei (Fig. 10U). Slight expression signals for the NR2D mRNAwere detected in the pontine nucleus at P7-P21, especially atP7, but the expression of NR2D mRNA in the pontine nucleus wasgenerally weak at all developmental stages examined (Fig. 10U-Y).When the overall distribution patterns of NMDA receptor subunitmRNAs examined in other brainstem nuclei were applied to parasagittalor horizontal brainstem sections of developing and adult rats,they were generally in accordance with those reported by previousstudies in rats and mice (Moriyoshi et al., 1991; Money et al.,1992; Watanabe et al., 1992, 1993; Akazawa et al., 1994).

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Figure 10. In situ hybridization showing the expression of mRNAs for the five NMDA receptor subunits (NR1, NR2A, NR2B, NR2C, and NR2D) in the developing rat pontine nucleus. A-E, NR1. F-J, NR2A. K-O, NR2B. P-T, NR2C. U-Y, NR2D. Antisense oligonucleotides labeled with ³⁵S-dATP were hybridized to adjacent frontal sections at P1 (A, F, K, P, U), at P7 (B, G, L, Q, V), at P14 (C, H, M, R, W), at P21 (D, I, N, S, X), and in the adult (E, J, O, T, Y) in the same experiment. Arrowheads in A-E indicate the pontine nucleus. Each set of developing brainstem sections was exposed to a single x-ray film, from which photographs were directly printed at the same magnification. Scale bar, 1 mm.

The signals were almost completely abolished when the hybridization was performed in the presence of excess unlabeled oligonucleotides,which indicated the specificity of the present in situ hybridization.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The present in vivo NMDA injection study demonstrated that the pontine nucleus near postnatal day 15 was most susceptibleto the toxicity of NMDA. Furthermore, the whole-cell recordingstudy revealed that NMDA responses that are relatively insensitiveto Mg²⁺ steadily increased in an age-dependent manner during the firsttwo postnatal weeks, reached the maximal level near postnatalday 15, and then decreased after postnatal day 16. The whole-cellrecording study also demonstrated that the NMDA responses thatare relatively insensitive to Mg²⁺ induced Ca²⁺ entry at the resting membrane potential. In the excitotoxic hypothesis(Rothman and Olney, 1986; Choi, 1988; Siesjö and Bengtsson, 1989),large Ca²⁺ entry has been thought to trigger catastrophic enzymatic processesleading to irreversible neuronal injury. The NMDA receptor channelsthat easily permit Ca²⁺ entry at the resting membrane potential could play an importantrole in the development of neuronal death induced by NMDA toxicity.Therefore, the present results suggest that the susceptibilityto NMDA neurotoxicity that is enhanced in the rat pontine nucleusnear postnatal day 15 is mediated by the NMDA responses that arerelatively insensitive to Mg²⁺. The present in situ hybridization study demonstrated that theexpression signals for the NR2C mRNA in the pontine nucleus appearedafter postnatal day 7 and were distinctly expressed at postnatalday 14. This time course of the developmental change in the expressionof the NR2C mRNA in the pontine nucleus until postnatal day 14coincided with that of the developmental change in the NMDA responsesthat are relatively insensitive to Mg²⁺. Previous molecular biological studies have reported that thesensitivity of NMDA receptor channels to Mg²⁺ block is critically determined by the constituting NR2 subunits(Kutsuwada et al., 1992; Ishii et al., 1993; Money et al., 1994);the recombinant NR1-NR2C and NR1-NR2D channels show relativelyweak sensitivity to Mg²⁺ block, whereas the recombinant NR1-NR2A and NR1-NR2B channelsshow strong sensitivity to Mg²⁺ block (Money et al., 1994). Thus, the developmental increasein the NMDA responses that are relatively insensitive to Mg²⁺ in the pontine nucleus until postnatal day 14 may correlate withthe increase in the expression of NR2C. Takahashi et al. (1996)have reported that Mg²⁺ block of NMDA receptor-mediated EPSCs decreases as the expressionof the NR2C ( $epsilon$ 3) is predominantly in developing granule cellsof the mouse cerebellum. The extent of the reduction in the sensitivityof NMDA receptors to Mg²⁺ block observed in the cerebellar granule cells is very similarto that observed in the present study. The present in situ hybridizationstudy also demonstrated that the time course of the developmentalchange in the expression of the NR2C mRNA in the pontine nucleusafter postnatal day 16 did not coincide with that of the developmentalchange in the NMDA responses that are relatively insensitive toMg²⁺. The expression signals for the NR2C mRNA were still high inthe pontine nucleus at postnatal day 21 and in adult rats, whereasthe NMDA responses that are relatively insensitive to Mg²⁺ significantly decreased throughout the stages. This result suggeststhat factors other than NR2C expression reduce the Mg²⁺-insensitive NMDA responses and the susceptibility to NMDA-mediatedneuronal injury in the pontine nucleus after postnatal day 16.It has been reported that native NMDA receptors might be assembledfrom more than two NR2 subunits. Wafford et al. (1993) have shownthat the NR1, NR2A, and NR2C subunits preferentially coassemblein the same NMDA receptor complex when all three subunit cDNAsare present and also have demonstrated that the glutamate affinityof the receptors formed from NR1+NR2A+NR2C is lower than thatof the receptors formed from NR1+NR2C. Incorporation of NR2A orother Mg²⁺-sensitive subunits into the NR1+NR2C receptors may occur progressivelyin the pontine nucleus after postnatal day 16, and it might producereductions in the Mg²⁺-insensitive NMDA responses and in the susceptibility to NMDA-mediatedneuronal injury in spite of high expression of NR2C throughoutthe stages.

Changes in the neuronal susceptibility to NMDA toxicity have been observed in other developing brain regions. NMDA that wasdirectly injected into the striatum at postnatal day 7 induceda maximal lesion involving the striatum and overlying neocortex,whereas the same concentration of NMDA did not induce any apparentlesion at postnatal days 1, 14, and 21 (McDonald et al., 1988;McDonald and Johnston, 1990). The expression of the NMDA receptorchannels that are relatively insensitive to Mg²⁺ may underlie the enhancement of susceptibility to NMDA neurotoxicityin other developing brain regions. Indeed, in immature rat neocorticalneurons, NMDA receptors have been reported to show a reduced Mg²⁺ block (Kato and Yoshimura, 1993). According to electrophysiologicaland histogenetic studies (Shimono et al., 1976; Hámori and Somogyi,1983; Garthwaite and Brodbelt, 1989; D'Angelo et al., 1993), mossyfibers in the rat pontine nucleus begin to make contact with granulecells at postnatal day 10, and the process of the contact is acceleratedand reaches a peak at postnatal day 15 and is complete by postnatalday 21. The time course of the development of mossy fiber-granulecell synaptic contacts coincides with that of the developmentof NMDA currents that are relatively insensitive to Mg²⁺. This coincidence proposes an idea that the NMDA receptor channelsthat are relatively insensitive to Mg²⁺ and easily permit Ca²⁺ entry at the resting membrane potential are essential for developingneurons to perform the neuronal differentiation and the establishmentor elimination of synapses.

In the human brain, it is at ~30 weeks of gestation that mossy fibers make contact with granule cells (Rakic and Sidman, 1970;Sidman and Rakic, 1982). The NMDA receptor channels that are relativelyinsensitive to Mg²⁺ may be expressed in the pontine nucleus of the human at the developingperiod. It is well known that glutamate is excessively releasedwith no regional selectivity in the hypoxic-ischemic brain (Benvenisteet al., 1984; Hagberg et al., 1985; Globus et al., 1991; Mitaniet al., 1992, 1994b), whereas excessive increase in intracellularCa²⁺ is selectively produced in vulnerable brain regions to hypoxiaand ischemia (Mitani et al., 1990, 1994a, 1995). Therefore, theexcessive increase in intracellular Ca²⁺ is thought to play a crucial role in the development of hypoxia-and ischemia-induced neuronal death (Choi, 1995; Mitani, 1996).If the NMDA receptor channels that are relatively insensitiveto Mg²⁺ are expressed in the developing pontine nucleus of the humanas mentioned above, the pontosubicular neuronal necrosis, whichis found in the human brain during a developmental period between30 weeks of gestation and the second postnatal month and oftencoexists with other forms of cerebral hypoxic and ischemic injuries,may be mediated by the NMDA receptor channels that are relativelyinsensitive to Mg²⁺.

  FOOTNOTES

Received Dec. 22, 1997; revised July 17, 1998; accepted July 17, 1998.

This work was supported by research grants from the Mother and Child Health Foundation, the Ministry of Education, Science,and Culture of Japan, and the Ministry of Health and Welfare ofJapan. We thank Dr. Tomoyuki Takahashi (Institute for Brain Research,University of Tokyo), Dr. Seiji Ozawa (Department of Physiology,Gunma University), and Dr. Youngnam Kang (Department of Physiology,Kyoto University) for critical advice. We also thank Mr. TakeoYagi for photographic help and Mr. Manabu Miyoshi for help inthe animal experiments.
Correspondence should be addressed to Dr. Akira Mitani, Department of Physiology, School of Medicine, Ehime University, Shigenobu,Onsen-gun, Ehime 791-0295, Japan.

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Abstract
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Materials & Methods
Results
Discussion
References

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