Immunohistochemical Evidence of Seizure-Induced Activation of trkB Receptors in the Mossy Fiber Pathway of Adult Mouse Hippocampus

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The Journal of Neuroscience, September 1, 2002, 22(17):7502-7508

Immunohistochemical Evidence of Seizure-Induced Activation of trkB Receptors in the Mossy Fiber Pathway of Adult Mouse Hippocampus
Xiao-Ping He¹, Liliana Minichiello⁴, Rüdiger Klein⁵, and James O. McNamara¹^,²^,³
Departments of ¹ Medicine (Neurology), ² Neurobiology, and ³ Pharmacology and Molecular Cancer Biology, Duke University Medical Center, Durham, North Carolina 27710, ⁴ European Molecular Biology Laboratory, 00016 Monterotondo, Italy, and ⁵ Max-Planck-Institute of Neurobiology, D-82152 Martinsried, Germany

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Genetic and pharmacological perturbations suggest that tyrosine receptor kinase B (trkB) receptor activation promotes limbicepileptogenesis, but whether or where trkB activation occurs duringepileptogenesis is uncertain. Because activation of trk receptorsinvolves phosphorylation of specific tyrosine residues (Segalet al., 1996), the availability of antibodies that selectivelyrecognize the phosphorylated form of trk receptors at the Shcsite permits an immunohistochemical assessment of trk receptoractivation. We reported previously increased phospho-specifictrk (p-trk) immunoreactivity in the mossy fiber pathway of thehippocampus during epileptogenesis in rats (Binder et al., 1999b).Because the p-trk antibody does not distinguish among trkA, trkB,and trkC, the identity of the neurotrophin receptor(s) undergoingphosphorylation was uncertain. The development of mice carryinga point mutation of the Shc binding site (Y515F) in the trkB gene(trkB^shc) provided an opportunity to test the hypothesis that trkB isthe neurotrophin receptor undergoing phosphorylation. Epileptogenesisin wild-type (WT) mice was associated with increased p-trk immunoreactivityin both the mossy fiber pathway and CA3 stratum oriens of hippocampus.In contrast, the epileptogenesis-associated increase of p-trkimmunoreactivity was reduced in trkB^shc mutant mice. The development of epileptogenesis as measured byelectrophysiological and behavioral indices did not differ betweentrkB^shc mutant and WT mice. These data demonstrate that the neurotrophinreceptor trkB undergoes phosphorylation in the mossy fiber pathwayand CA3 stratum oriens of the hippocampus during limbic epileptogenesis.In addition, the signaling pathways activated by the Shc siteof trkB exert no detectable regulatory effects on limbicepileptogenesis.

Key words: epileptogenesis; kindling; seizures; neurotrophin; trkB receptor; Shc; hippocampus; phosphorylation

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Elucidating the mechanisms of limbic epileptogenesis in cellular and molecular terms may provide novel therapeutic approachesto prevent the disease. In the kindling model, repeated inductionof brief, focal seizures by application of initially subconvulsiveelectrical stimuli eventually results in intense focal and tonic-clonicseizures (Goddard et al., 1969). Once established, the enhancedsensitivity to electrical stimulation is lifelong. The cellularand molecular events by which seizures beget more intense seizuresare incompletely understood. The idea emerged that extracellularsignaling molecules might be pivotal in the transduction process.Two criteria for candidate signals emerged: that seizure activityregulates the production and release of the molecules and thatthe molecules effect structural and functional changes that couldresult in hyperexcitability. One class of molecules that met thesecriteria was the neurotrophins, in particular brain-derived neurotrophicfactor (BDNF) and its cognate tyrosine kinase receptor trkB. Limbicseizures increase the mRNA content of BDNF in multiple neuronalpopulations of forebrain (Isackson et al., 1991). The developmentof kindling is inhibited in mice heterozygous for BDNF (Kokaiaet al., 1995). Intraventricular infusion of trk receptor bodiessequester and limit the action of distinct neurotrophins; infusionof trkB-Fc inhibited epileptogenesis, whereas infusion of trkA-Fcor trkC-Fc did not (Binder et al., 1999a). The occurrence of epileptiformspiking on electroencephalogram (EEG) long after kainate-inducedstatus epilepticus is impaired in transgenic mice overexpressingtruncated trkB, presumably by limiting activation of trkB (Lähteinenet al., 2002). Finally, although conflicting results emerged fromintracerebral infusions of BDNF (Larmet et al., 1995; Scharfmanet al., 2002), transgenic mice overexpressing BDNF exhibit anenhanced response to epileptogenic stimuli (Croll et al., 1999).

Together with the seizure-induced expression of BDNF, these findings led to the hypothesis that enhanced activation of trkBoccurs in the hippocampus during limbic epileptogenesis. Becauseactivation of trk receptors involves phosphorylation of specifictyrosine residues (Schlessinger and Ullrich, 1992; Segal and Greenberg,1996), the availability of antibodies that selectively recognizethe phosphorylated form of trk receptors (Segal et al., 1996)permits immunohistochemical assessment of trk receptor activation.We reported increased phospho-specific trk immunoreactivity (p-trkIR) in the hippocampal mossy fiber pathway during epileptogenesisin rats (Binder et al., 1999b). Because the p-trk antibody doesnot distinguish among trkA, trkB, and trkC, the precise neurotrophinreceptor(s) undergoing phosphorylation was uncertain. The temporaland spatial concordance of seizure-induced increases of p-trkimmunoreactivity and BDNF protein suggested that increased phosphorylationof trkB was responsible for the increased p-trk immunoreactivity.The development of mice carrying a point mutation of the Shc bindingsite in the trkB gene (trkB^shc mutant mice) permitted testing this hypothesis. That is, substitutionof phenylalanine for tyrosine at residue 515 of trkB (Y515F) eliminatesthe binding site for the phospho-trk antibody in trkB but nottrkA or trkC. This mutation of trkB disrupts the binding of Shcadaptor protein to trkB and abolishes Shc site-mediated downstreamsignaling events (Minichiello et al., 1998). If our hypothesisis correct, induction of epileptogenesis should produce increasedphospho-trk immunoreactivity in the mossy fiber pathway of wild-type(WT) but not trkB^shc mutantmice.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mice. trkB^shc mutant mice were generated as described previously (Minichiello et al., 1998). In brief, PCR-aided mutagenesiswas used to introduce a single point mutation (A to T, position2055) in trkB receptor that resulted in a change of tyrosine 515into phenylalanine (Y515F). Nonphosphorylatable F515 disruptedthe binding of adaptor proteins to the Shc site in trkB and abolishedShc site-mediated down-stream signaling events. The amount ofautophosphorylated trkB was reduced in trkB^shc/shc neurons after BDNF or neurotrophin-4 (NT-4) stimulation. In thepresent study, the genotype of each animal was assessed twiceusing PCR of genomic DNA isolated from tail (before experiment)and liver (after being killed). Nine wild-type (+/+), 14 heterozygous(+/ $-$ ), and 13 homozygous ( $-$ / $-$ ) trkB^shc mice (20-35 gm) were used in thisexperiment.

Antibody. A peptide affinity-purified polyclonal trk antibody (pY490) (New England Biolabs, Beverly, MA) directed againsta synthetic phospho-tyr 490 peptide corresponding to residues485-493 (IENPQY*FSD) of human trkA was used for immunohistochemistryas we described previously (Binder et al., 1999b). The sequenceof this peptide is highly conserved among trkA, trkB, and trkCreceptors and also among human, rat, and mouse. Antibody pY490is phospho-specific, recognizing the phosphorylated but not thenonphosphorylated form of peptide 490. Additionally, pY490 isphosphorylation site specific, recognizing phosphorylated 490but not a trk peptide phosphorylated at residues 674/675 (Binderet al., 1999b).

Surgery and kindling. Under pentobarbital anesthesia (60 mg/kg, i.p.), a stimulation-recording bipolar electrode was stereotacticallyimplanted in the right amygdala using the following coordinates,with bregma as the reference: 1.0 mm posterior, 2.9 mm lateral,and 4.6 mm below dura. A wire secured to the skull overlying theleft frontal cortex was used as the ground electrode. After apostoperative recovery period of at least 1 week, the electrographicseizure threshold (EST) was determined by application of 1 sectrain of 1 msec biphasic rectangular pulses at 60 Hz beginningat 60 µA; additional stimulations increasing by 20 µA were administeredat 1 min intervals until an electrographic seizure lasting atleast 5 sec was detected on the EEG recorded from the amygdala.Subsequently, experimental animals were stimulated twice eachday at a stimulus intensity 100 µA above the EST, with an interstimulusinterval of at least 4 hr until three consecutive seizures ofclass 4 or greater with limb clonus and/or tonus lasting at least12 sec were evoked. The behavioral manifestations of seizureswere classified according to a modification of Racine's classification(Racine, 1972): 1, facial clonus; 2, head nodding; 3, unilateralforelimb clonus; 4, rearing with bilateral forelimb clonus; 5,rearing and falling (loss of postural control); 6, running orbouncing seizures; and 7, tonic hindlimb extension. The surgeryand kindling procedures were performed by an individual blindedto genotype of the animals. Control animals included unimplantedas well as implanted but unstimulatedmice.

Perfusion and histology. After completion of kindling and a subsequent stimulation-free period of 2 weeks, the persistenceof the hyperexcitability was determined by administration of anadditional stimulation of the same intensity used in kindlingprocedure. Twenty-four hours after stimulation, the experimentaland control animals were perfused transcardially under pentobarbitalanesthesia with ice-cold 4% paraformaldehyde in 1× PBS containing1 mM sodium orthovanadate (PBSV) for 5 min at a flow rate 7.5ml/min. The brains were removed, postfixed in the same solutionovernight at 4°C, and cryoprotected in 20% sucrose in 1× PBSVuntil they sank. Coronal sections of 40 µm were cut in a cryostatat $-$ 20°C, and two sections per slide were mounted in PBSV on slides,air dried, frozen, and stored at $-$ 70°C until use. The sectionswere stained with methyl green pyronine-Y for determination ofelectrode placement. Only animals with correct electrode placementin the amygdaloid complex were included in the statisticalanalysis.

Phospho-trk immunohistochemistry. To facilitate quantitative comparisons, slide-mounted sections isolated from stimulatedand unstimulated animals of all three genotypes (WT, heterozygotes,and homozygotes) were processed in batches using the identicalsolutions and durations of incubations, washes, etc. AntibodypY490 was used to detect the phosphorylated form of trk receptorusing the protocol described in detail previously (Binder et al.,1999b). Briefly, after quenching of endogenous peroxidase activitywith 0.3% H₂O₂/MeOH for 30 min, sections were blocked and permeabilizedin 5% normal goat serum (NGS) and 0.5% NP-40 in 1× PBSV for 1hr. The primary antibody, pY490 (1:10 in 1× PBSV and 5% NGS),was incubated with sections and covered by coverslips in a humidifiedchamber at room temperature for 1 hr. The sections were subsequentlyincubated in biotin-conjugated goat anti-rabbit IgG (1:100 inPBSV and 5% NGS; Jackson ImmunoResearch, West Grove, PA) for 1hr. The ABC method (1:100 in PBSV with 5% NGS, applied twice;Vectastain Elite; Vector Laboratories, Burlingame, CA) was usedfor detection of immunoreactivity. Biotinyl tyramide (1:100 inPBSV with 5% NGS, applied between two ABC incubations; Bio-Rad,Richmond, CA) was used to enhance detection of the immunoreactivity.The sections were preincubated with DAB solution (Sigma Fast;Sigma, St. Louis, MO) containing 0.04% nickel ammonium sulfatefor 15 min and then developed for 10-30 min in the same DAB solutionbut also containing 0.03% H₂O₂. The slides were rinsed in PBS,dehydrated in ethanol, cleared in xylene, and coverslipped. Theslides were subsequently coded and analyzedblinded.

Peptide competition. The immunogen of antibody pY490 (phosphopeptide 490) and the unphosphorylated form of the same peptidewere used for peptide competition. For other controls, four additionalpeptides of trkA, the phospho- and unphospho-peptides of sites674/675 and 785, respectively (New England Biolabs), were includedin the experiments. Each peptide used at 300 nM was incubatedat room temperature with the primary antibody solution (1:10 inPBSV with 5% NGS) for 30 min to 1 hr. After slides were quenched,blocked, and permeabilized, the primary antibody solution coincubatedwith the relevant peptide was applied to the sections. The remainingsteps followed the standard protocol of phospho-trkimmunohistochemistry.

Densitometry quantification. Images of the immunoreactivity in the CA3 and dentate gyrus (DG) of hippocampus were capturedusing a high-resolution CCD camera interfaced with a light microscope(Axiovert 135; Zeiss, Oberkochen, Germany) and measured usinga computer-assisted image analyzer (MetaMorph 3D; Universal Imaging,West Chester, PA). For densitometric analysis, a square box offixed size was placed in distinct regions within CA3 and dentategyrus to measure the average gray value for each location. ForCA3, the gray value was measured in three locations: strata radiatum,lucidum, and oriens. For dentate gyrus, gray values were measuredin five locations: outer molecular layer (OML), middle molecularlayer (MML), inner molecular layer (IML), hilar border with granulecell layer (hilus-GCL border), and deep hilus at the midpointof granule cell layer (see Fig. 3). Because the corpus callosumhad less variation and a higher gray value reflecting less immunoreactivity,it was chosen as the reference. The results from measured locationsare presented as the percentage of reduction in gray value comparedwith corpus callosum, a greater reduction in gray value reflectingmore phospho-trk immunoreactivity. The data for each animal areexpressed as the average from four hippocampi (one slide per animalcontaining two sections, each with two hippocampi). All resultswere analyzed by one-wayANOVA.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Increased p-trk IR in WT mice after kindling

Our recent studies provided immunohistochemical evidence that trk receptors undergo phosphorylation in a spatially specificpattern in the hippocampus during the development of kindlingof rats (Binder et al., 1999b). To determine whether trk receptorphosphorylation also occurs in mice, p-trk immunohistochemistrywas performed in wild-type mice killed 24 hr after the last seizureevoked by stimulation of the right amygdala. A spatially selectiveincrease of p-trk IR in the hippocampal formation was detectedin each of the four stimulated WT mice compared with unstimulatedWT mice (Fig. 1, compare A, B, arrows). The increased immunoreactivitywas evident in the hippocampal formation bilaterally, mainly inthe mossy fiber pathway. In addition, a moderately high levelbut more diffuse pattern of p-trk IR was apparent throughout stratumoriens of CA3. In contrast, no overt changes of p-trk IR wereevident in CA1, in stratum radiatum of CA3, or in the molecularlayer of the dentate gyrus. Quantitative analyses of these dataare presented below. Importantly, omission of the primary antibodyeliminated immunoreactivity in these WT animals (data not shown).

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Figure 1. Reduction of seizure-induced increase of p-trk immunoreactivity in trkB^shc mutant mice. A, C, E, p-trk immunoreactivity in unstimulated +/+, +/ $-$ , and $-$ / $-$ mice. Note the absence of detectable immunoreactivity in dentate hilus and CA3 stratum lucidum of hippocampus. B, D, F, p-trk immunoreactivity in +/+, +/ $-$ , and $-$ / $-$ mice 24 hr after a seizure evoked by stimulation of right amygdala. Arrows denote immunoreactivity in dentate hilus and stratum lucidum in stimulated +/+ and +/ $-$ mice. Despite some differences in background among individual animals, no systematic variation in background attributable to genotype or stimulation status was present (data not shown). Note that quantitation was controlled for individual differences in background by use of a control region (corpus callosum) intrinsic to each section. Scale bar, 650 µm.

To verify the specificity of p-trk IR in kindled mice, peptide competition experiments were performed. Preincubation of pY490antibody with its phosphopeptide immunogen (300 nM) eliminatedp-trk IR in sections from kindled mice (Fig. 2, compare A, C)and unstimulated controls (data not shown). Importantly, preincubationwith the unphosphorylated form of peptide 490 had no effect onthe immunoreactivity (Fig. 2, compare A, B). Moreover, preincubationof pY490 antibody with either phospho- or unphospho-peptides fromother sites of the trk receptor, 674/675 and 785, did not reducep-trk IR (data not shown). Together, the results from these competitionexperiments support the assertion that the p-trk IR detected byantibody pY490 in wild-type mice reflects the phosphorylated formof a trk receptor at a tyrosine residue within a sequence similarto that of pY490 of human trkA.

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Figure 2. Reduction of p-trk immunoreactivity by phosphopeptide but not by nonphosphopeptide. Immunoreactivity to p-trk is shown in representative coronal sections of hippocampus from a WT mouse killed 24 hr after a kindled seizure in which pY490 antibody is coincubated with the following: A, no peptide; B, 300 nM nonphosphorylated form of peptide 490; C, 300 nM phosphorylated form of peptide 490. Scale bar, 650 µm.

Analyses of brain regions outside the hippocampal formation in unstimulated controls disclosed p-trk immunoreactivity in multipleareas of forebrain, including neocortex, lateral habenula, andsome hypothalamic nuclei (data not shown). In contrast to thehippocampal formation, no marked increases were noticed in anyof these regions after seizures evoked in WT mice. Thus, subsequentanalyses were confined to the hippocampal formation in thesestudies.

Reduction of seizure-induced increased phospho-trk immunoreactivity in trkB^shc mutant mice

Because the pY490 antibody can detect the phosphorylated tyrosine residue in trkA, trkB, or trkC (Segal et al., 1996), theprecise trk receptor undergoing phosphorylation in the hippocampusduring epileptogenesis is uncertain. To determine whether phosphorylationof trkB in particular accounts for the increased immunoreactivityin the hippocampus during epileptogenesis, p-trk immunohistochemistrywas performed in WT and trkB^shc mice, which were either not stimulated or were killed 1 d aftera stimulation-evoked seizure. As described in the preceding section,a marked increase of p-trk IR was evident in stratum lucidum anddentate hilus with a moderate increase in stratum oriens of CA3after a seizure evoked in WT mice (Fig. 1, compare A, B). ThetrkB^shc mutation reduced the seizure-evoked increase of immunoreactivity.That is, seizures evoked in trkB^shc null mice triggered no significant increase of immunoreactivityin stratum lucidum, dentate hilus, or stratum oriens of CA3 (Fig.1, compare B, F). Results with heterozygous trkB^shc were intermediate between the WT and trkB^shc nulls (Fig. 1, compare B, D, F, in lucidum, dentate hilus, andstratum oriens ofCA3).

The immunoreactivity within hippocampus was quantified in distinct subregions (Fig. 3) and confirmed the findings evidentby visual inspection. First, analyses of WT mice confirmed thespatially selective, twofold to threefold increase of phospho-trkimmunoreactivity in stratum lucidum, the dentate hilus, and hilusborder after a seizure compared with unstimulated controls (Fig.4A,B). Significant (p < 0.05; ANOVA) increases of a smaller magnitudewere also evident in stratum oriens of CA3 (Fig. 4A). In contrast,comparison of stimulated with unstimulated trkB^shc null mutants disclosed no significant seizure-induced increasesof immunoreactivity in stratum lucidum, the dentate hilus or hilusborder, or CA3 stratum oriens (Fig. 4A,B). In addition to theabove comparisons of unstimulated versus stimulated mice of agiven genotype, comparisons of seizure-treated mice of distinctgenotypes revealed significant increases of immunoreactivity inthe mossy fiber pathway and stratum oriens of CA3 in WT comparedwith trkB^shc null mutants (Fig. 4A,B). Similar analyses of trkB^shc heterozygotes disclosed results intermediate between wild-typeand null mutants, but no significant increases of immunoreactivitywere detected in the mossy fiber pathway and stratum oriens ofCA3 after a kindled seizure compared with unstimulated controlsof the same genotype (Fig. 4A,B). Interestingly, the increasesof p-trk IR after seizures exhibited striking heterogeneity amongthe trkB^shc heterozygotes (data described but not shown). Robust stainingwas seen in three of nine heterozygous mice after a seizure withintensity and distribution similar to WT mice after a seizure.However, no detectable increase was evident in four heterozygousmice and a slight increase in the remaining two mice. Together,these quantitative analyses demonstrate that substitution of phenylalaninefor tyrosine at residue 515 of trkB reduces the increased p-trkIR after limbic seizures.

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Figure 3. Locations at which densitometric measures of p-trk immunoreactivity were performed: 1, strata radiatum; 2, lucidum; 3, oriens; 4, deep hilus; 5, hilus-GCL border; 6, IML; 7, MML; 8, OML.

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Figure 4. Quantitative analyses of p-trk immunoreactivity in hippocampal subregions of stimulated and unstimulated WT, heterozygous, and null (trkB^shc) mutant mice. The data are the mean ± SEM of the percentage reduction in gray value in the given subregions compared with corpus callosum (see Materials and Methods); high values reflect more intense immunoreactivity. *p < 0.05 compared with unstimulated WT mice; $phi$ p < 0.05 compared with kindled and stimulated WT mice (one-way ANOVA with post hoc Bonferroni's test).

Development and persistence of kindling in trkB^shc mutant mice

No significant differences in the development of kindling were detected among WT (+/+), heterozygous, and null trkB^shc mutants, as evident in the following observations. First, thecurrent required to evoke an afterdischarge (i.e., EST) was similarin the three groups (180.0 ± 40.1 µA for +/+, n = 4; 151.1 ± 22.6µA for +/ $-$ , n = 9; 180 ± 24.8 µA for $-$ / $-$ , n = 8; mean ± SEM; p> 0.05; one-way ANOVA). Second, no significant differences weredetected in the numbers of stimulations required to evoke theinitial clonic motor seizures (class 4 or greater) in WT (5.5± 0.9 stimulations) compared with heterozygous (6.4 ± 0.5) ornull (6.8 ± 0.7) mutants. Third, no significant differences werefound in the numbers of stimulations required to evoke three consecutiveclass 4 (or greater) seizures, the numbers of stimulations being9.8 ± 1.5, 10.3 ± 0.5, and 10.8 ± 0.9 in WT, heterozygous, andnull mutants, respectively (Fig. 5A). Finally, no significantdifferences were noted in the duration of electrographic seizuresduring kindling development among the three experimental groups(Fig. 5B). In summary, kindling development appears to proceednormally in trkB^shc mutants.

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Figure 5. Behavioral (A) and electrographic seizure (B) measures of kindling development in WT and trkB^shc mutant mice. Kindling development is presented as behavioral seizure class (A) and electrographic seizure duration as a function of the number of stimulations that evoked electrographic seizures (y-axis). Wild type (+/+; n = 4), heterozygous (+/ $-$ ; n = 9), and homozygous ( $-$ / $-$ ; n = 8) mutant mice. ADD# (x-axis) refers to the number of stimulations that evoked an afterdischarge with duration of at least 5 sec. Data are mean ± SEM. Note that neither seizure class nor electrographic seizure duration was significantly different among the three groups (one-way ANOVA).

To determine whether the Shc binding site of the trkB receptor influenced the persistence of the hyperexcitability after completionof kindling, WT and trkB^shc mutants were maintained for a stimulation-free period of 2 weeksafter kindling and then subjected to a single stimulation. Thestimulation evoked a generalized seizure in all animals from eachof the three groups (+/+, +/ $-$ , and $-$ / $-$ ). There was no significantdifference among the groups in duration of electrographic seizure(41.5 ± 8.1, 41.4 ± 4.0, and 35.4 ± 2.1 sec, respectively) orseizure class (5.5 ± 0.5, 5.8 ± 0.2, and 5.3 ± 0.2, respectively;p > 0.05; one-way ANOVA). Thus, the persistence of kindling wasunaffected in the trkB^shc mutantmice.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Our previous ex vivo analyses of limbic epileptogenesis in rats demonstrated increased pY490 immunoreactivity in the hippocampalmossy fiber pathway, providing immunohistochemical evidence foractivation of trk receptor tyrosine kinase. Which trk receptor(s)in particular accounted for the immunoreactivity was unclear.To test the hypothesis that phosphorylation of trkB contributedto the increased immunoreactivity, we studied mutant mice (trkB^shc) in which phenylalanine was substituted for tyrosine at residue515 of trkB, a site homologous to residue 490 of human trkA. Threeprincipal findings emerge. First, the previous results in ratswere confirmed and extended by the studies of mice. A single,brief seizure induced by stimulation of the right amygdala ina kindled mouse in a WT background induced increased pY490 immunoreactivitybilaterally in the hippocampal mossy fiber pathway. In addition,increased pY490 immunoreactivity was evident in stratum oriensof CA3 bilaterally. Second, in contrast to WT mice, seizures evokedin null mutant (trkB^shc) mice induced no significant increase of pY490 immunoreactivityin either the mossy fiber pathway or CA3 stratum oriens. Third,despite the reduction of the seizure-induced increase of pY490immunoreactivity, the development and persistence of kindlingas measured by electrophysiological and behavioral indices didnot differ between trkB^shc mutant and WT mice. These data demonstrate that the neurotrophinreceptor trkB undergoes phosphorylation in the mossy fiber pathwayand CA3 stratum oriens of the hippocampus during limbic epileptogenesis.In addition, the signaling pathways activated by the Shc siteof trkB exert no detectable regulatory effects on limbicepileptogenesis.

The present study revealed that the increased p-trk immunoreactivity evident in the hippocampus during limbic epileptogenesiswas reduced in trkB^shc mutant mice, implying that phosphorylation of trkB underliesthe increased p-trk immunoreactivity. Whether the increased p-trkBimmunoreactivity is attributable to a post-translational modificationof a fixed number of constitutively expressed trkB molecules,to post-translational modification of increased numbers of trkBmolecules, or some combination of the two is uncertain. The presenceof the increased p-trk immunoreactivity in WT mice adds to previousfindings in rats and demonstrates that trkB activation occursduring limbic epileptogenesis in multiple species. Moreover, theinduction of the immunoreactivity by a single, brief seizure evokedin a kindled mouse extends the previous studies using chemoconvulsant-inducedstatus epilepticus or massed electrical stimulations and demonstratesthat activation of trkB is common to limbic epileptogenesis inducedby diverse methods. In light of evidence implicating a causalrole for trkB activation in limbic epileptogenesis (Kokaia etal., 1995; Binder et al., 1999a; Croll et al., 1999; Lähteinenet al., 2002), knowing where and when trkB activation occurs willfacilitate elucidating its structural and functional consequencesand, in turn, provide insight into mechanisms of limbicepileptogenesis.

The light microscopic distribution provides a clue to the cellular localization of the increased p-trkB immunoreactivity.Its presence in the dentate hilus and stratum lucidum of CA3 correspondsto the mossy fiber axons of the dentate granule cells, providingthe most parsimonious explanation for its cellular localization.Whereas our studies of rats disclosed increased p-trk immunoreactivityconfined to the mossy fiber pathway (Binder et al., 1999b), thepresent study revealed increased p-trkB immunoreactivity not onlyin the mossy fiber pathway but also throughout stratum oriensof CA3 extending to the junction with CA2 (Fig. 1B). Whether thisp-trkB immunoreactivity is localized to an infrapyramidal projectionof mossy fibers, axons of CA3 pyramidal cells, and/or postsynaptictargets such as interneurons or basilar dendrites of CA3 pyramidalcells is uncertain. Ultrastructural studies will be required toestablish the cellular locale of the p-trkB immunoreactivity inboth the mossy fiber pathway and stratum oriens ofCA3.

Circumstantial evidence implicates increased release of BDNF as the proximate cause for the increased p-trkB immunoreactivityduring limbic epileptogenesis. The binding of neurotrophin tothe trk receptor induces dimerization and trans-autophosphorylationof a subset of tyrosine residues (Schlessinger and Ullrich, 1992;Guiton et al., 1994), thereby suggesting that the binding of aneurotrophin to trkB underlies its increased phosphorylation.The occurrence of the increased p-trkB immunoreactivity afterseizures suggests the possibility that seizures induced increasedexpression of a neurotrophin that is translated, transported,released, and thereby activates trkB. Analysis of the temporaland spatial patterns of seizure-mediated regulation of neurotrophinssupports the candidacy of BDNF. The seizure-induced increase ofBDNF protein peaks at ~24 hr, the time point corresponding toincreased p-trkB immunoreactivity (Nawa et al., 1995; Elmér etal., 1998; Rudge et al., 1998; Binder et al., 1999b). Concordanceof the anatomic distribution of seizure-induced increases of BDNFand the p-trkB immunoreactivity further implicate BDNF; that is,immunohistochemical studies disclosed increased BDNF in the granulecell soma within 2 hr after seizures and in the mossy fiber pathway1 to 2 d thereafter (Yan et al., 1997; Vezzani et al., 1999).We favor the idea that BDNF is anterogradely transported to themossy fiber axons (Conner et al., 1997; Smith et al., 1997), fromwhich it is released and activates trkB on the mossy fibers bya paracrine or autocrine mechanism. Concordance of the anatomicdistribution of seizure-induced BDNF (Yan et al., 1997, theirFig. 7D) and p-trkB immunoreactivity in stratum oriens of CA3implicates BDNF in this site as well. Together with persistenceof seizure-induced p-trk immunoreactivity in NT-4 null mutants(He et al., 1999), this circumstantial evidence favors BDNF asthe neurotrophin activating p-trkB inhippocampus.

What consequence(s) of trkB activation, presumably by BDNF, might contribute to the increased excitability evident as limbicepileptogenesis? The fact that at least part of the increasedp-trkB immunoreactivity may reside in dentate granule cells refinesthe question: what functional and structural consequences of enhancedactivation of trkB in granule cells by BDNF might promote increasedhippocampal excitability? The fact that activation of trkB byBDNF can enhance excitatory synaptic transmission (Lohof et al.,1993; Kang and Schuman, 1995; Levine et al., 1995, Stoop and Poo,1996) and reduce inhibitory synaptic transmission (Tanaka et al.,1997) in hippocampus raises the interesting possibility that enhancedsynaptic activation of CA3 pyramidal cells by mossy fibers, eitherdirectly or indirectly by disinhibition of the mossy fiber-interneuron-CA3pyramidal cell circuit is one consequence of trkB activation.The increased excitability of CA3 pyramidal cells in kindled animalsas detected by increased epileptiform bursting induced by elevatedK⁺ or lowered Mg²⁺ in isolated hippocampal slices (King et al., 1985; Behr et al.,1998) is consistent with this idea. Another possibility relatesto the increased recurrent excitatory synapses that have beenidentified among dentate granule cells in the epileptic brain,synapses that would be expected to promote repetitive firing ofthe granule cells in response to an isolated excitatory synapticinput (Wuarin and Dudek, 2001). Two distinct morphological plasticitiesof the granule cells have been identified in the epileptic brain,either of which could underlie increased recurrent excitatorysynapses: sprouting of the mossy fiber axons and formation ofbasal dendrites (Nadler et al., 1980; Spigelman et al., 1998).We found that particle-mediated gene transfer of BDNF, but notNGF, into the dentate granule cells in hippocampal explant culturesis sufficient to induce increases in both axonal branching andbasilar dendrite number (Danzer et al., 2001). Whether BDNF-mediatedactivation of trkB during limbic epileptogenesis in vivo mediatesthese functional and/or structural effects remains to beelucidated.

Despite the evidence that trkB activation promotes limbic epileptogenesis, the signaling pathways mediating the epileptogenicconsequences of trkB activation are obscure. After binding a ligand,trk receptors autophosphorylate on cytoplasmic tyrosine residues,which themselves become docking sites for intracellular signalingproteins. Shc adaptor proteins associate directly with a specificsite in trk receptors and activate a signaling pathway involvingRas, Raf, MAPK1 [for mitogen-activated protein (MAP) kinase 1],MAPK2, Mek 1 (for MAP kinase kinase 1), and Mek 2, one consequenceof which is activation of transcription factors and regulationof gene expression. The present studies reveal that introductionof the Y515F mutation into the germline of the trkB^shc/shc mice did not modify either electrophysiological or behavioralindices of epileptogenesis, despite previous evidence that BDNF-and NT-4-mediated activation of ERKs (for extracellular signal-regulatedkinase) were attenuated in neurons isolated from Shc mutant mice(Minichiello et al., 1998). These results imply that trkB-mediatedactivation of the Ras/ERK pathway does not mediate epileptogenesisor that this pathway is redundant with other pathways, such asphospholipase C $gamma$ pathway. The absence of detectable differencesin epileptogenesis between WT and trkB^shc/shc is reminiscent of the absence of detectable differences in long-termpotentiation between WT and trkB^shc/shc mice (Korte et al., 2000), despite defects in long-term potentiationin BDNF and trkB null mutant mice (Korte et al., 1995; Minichielloet al., 1999; Xu et al., 2000). The trkB signaling pathways mediatingepileptogenesis remain elusive, and solving this question willrequire the generation of additional signaling alleles of thetrkBgene.

  FOOTNOTES

Received Feb. 7, 2002; revised May 9, 2002; accepted May 20, 2002.

This work was supported by National Institutes of Health Grant NS17771 (J.O.M.).

Correspondence should be addressed to Dr. James O. McNamara, 401 Bryan Research Building, Durham, NC 27705. E-mail: jmc{at}neuro.duke.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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