Cellular Mechanisms Regulating Activity-Dependent Release of Native Brain-Derived Neurotrophic Factor from Hippocampal Neurons

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The Journal of Neuroscience, December 1, 2002, 22(23):10399-10407

Cellular Mechanisms Regulating Activity-Dependent Release of Native Brain-Derived Neurotrophic Factor from Hippocampal Neurons
Agnieszka Balkowiec and David M. Katz
Department of Neurosciences, Case Western Reserve University School of Medicine, Cleveland, Ohio 44106

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Brain-derived neurotrophic factor (BDNF) plays a critical role in activity-dependent modifications of neuronal connectivityand synaptic strength, including establishment of hippocampallong-term potentiation (LTP). To shed light on mechanisms underlyingBDNF-dependent synaptic plasticity, the present study was undertakento characterize release of native BDNF from newborn rat hippocampalneurons in response to physiologically relevant patterns of electricalfield stimulation in culture, including tonic stimulation at 5Hz, bursting stimulation at 25 and 100 Hz, and theta-burst stimulation(TBS). Release was measured using the ELISA in situ technique,developed in our laboratory to quantify secretion of native BDNFwithout the need to first overexpress the protein to nonphysiologicallevels. Each stimulation protocol resulted in a significant increasein BDNF release that was tetrodotoxin sensitive and occurred inthe absence of glutamate receptor activation. However, 100 Hztetanus and TBS, stimulus patterns that are most effective ininducing hippocampal LTP, were significantly more effective inreleasing native BDNF than lower-frequency stimulation. For allstimulation protocols tested, removal of extracellular calcium,or blockade of N-type calcium channels, prevented BDNF release.Similarly, depletion of intracellular calcium stores with thapsigarginand treatment with dantrolene, an inhibitor of calcium releasefrom caffeine-ryanodine-sensitive stores, markedly inhibited activity-dependentBDNF release. Our results indicate that BDNF release can encodetemporal features of hippocampal neuronal activity. The dual requirementfor calcium influx through N-type calcium channels and calciummobilization from intracellular stores strongly implicates a rolefor calcium-induced calcium release in activity-dependent BDNFsecretion.

Key words: activity; BDNF; caffeine; calcium channels; calcium-induced calcium release; electrical field stimulation; ELISA in situ; hippocampus; intracellular calcium stores; LTP; neurotrophins; patterned stimulation; ryanodine-sensitive stores; synaptic plasticity

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Brain-derived neurotrophic factor (BDNF) plays a critical role in activity-dependent modulation of synaptic strength and neuronalconnectivity at cortical and hippocampal synapses (Katz and Shatz,1996; Black, 1999; McAllister et al., 1999; Lu and Gottschalk,2000; Poo, 2001). For example, BDNF is required for activity-dependentsynaptic competition and formation of ocular dominance columnsin developing visual cortex (Cabelli et al., 1995) and can alsoregulate short- and long-term changes in synaptic strength. Specifically,exogenous BDNF can directly potentiate synaptic transmission inthe hippocampus and cortex (Kang and Schuman, 1995; Akaneya etal., 1997), and endogenous BDNF is necessary for establishmentof long-term potentiation (LTP) (Korte et al., 1995; Figurov etal., 1996; Patterson et al., 1996; Kang et al., 1997). However,despite these findings, relatively little is known about the cellularmechanisms regulating activity-dependent BDNF release from corticaland hippocampalneurons.

Most information about BDNF release from hippocampal neurons has been derived from studies using adenoviral gene-transfertechniques to overexpress BDNF to high concentrations (Goodmanet al., 1996; Griesbeck et al., 1999; Gärtner and Staiger, 2002),or cells transfected with BDNF-green fluorescent protein (GFP)expression plasmids (Hartmann et al., 2001; Kohara et al., 2001).It is unclear, however, whether mechanisms governing sorting andrelease of BDNF in these artificial systems are the same or differentfrom those governing sorting and release of native BDNF (Fawcettet al., 1997). In addition, most previous studies of BDNF releaseused continuous membrane depolarization to model neuronal activity(Goodman et al., 1996; Griesbeck et al., 1999). However, we showedpreviously, using primary sensory neurons, that patterned electricalstimulation, which more closely mimics neuronal activity in vivo,is much more effective at releasing native BDNF than continuousKCl depolarization (Balkowiec and Katz, 2000). Moreover, Hartmannet al. (2001) found that different mechanisms regulate releaseof BDNF-GFP in response to high-frequency presynaptic stimulationand continuous KCl depolarization, respectively. Finally, studiesfrom this and other laboratories demonstrated that release ofnative BDNF from sensory neurons (Balkowiec and Katz, 2000; Leveret al., 2001) or of adenovirally overexpressed BDNF (AdVBDNF)from hippocampal neurons (Gärtner and Staiger, 2002) can be regulatedby the frequency and pattern of stimulation. However, mechanismsunderlying activity-dependent secretion of native BDNF from hippocampalneurons have not beendefined.

To address this issue, the present study characterized mechanisms of native BDNF release from hippocampal neurons in responseto physiologically relevant patterns of stimulation. To measurerelease of native BDNF, we developed an in vitro model using dissociatedneuron cultures and a modified ELISA, termed ELISA in situ (Balkowiecand Katz, 2000). Our findings demonstrate that release of nativeBDNF from hippocampal neurons can be evoked directly by patternedelectrical stimulation via activation of tetrodotoxin-sensitivesodium channels and calcium influx through N-type channels, inthe absence of synaptic activity. Moreover, this release requiresintact intracellular calcium stores, suggesting that calcium-inducedcalcium release (CICR) plays a role in activity-dependent secretionof native BDNF from hippocampalneurons.

Parts of this paper have been published previously in abstract form (Balkowiec and Katz; 2001; Katz and Balkowiec, 2001).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation of hippocampal cultures. Newborn rats (Sprague Dawley strain; Zivic-Miller, Zelienople, PA) were deeply anesthetizedby hypothermia and decapitated. Hippocampi were rapidly and asepticallydissected from each brain in ice-cold Ca²⁺/Mg²⁺-free Dulbecco's phosphate-buffered salt solution (Mediatech,Herndon, VA), followed by removal of meninges and mincing to smallpieces. The hippocampal tissue was next digested in 0.1% crystallizedtrypsin-3X (Worthington Biochemical, Lakewood, NJ) with 0.01%Deoxyribonuclease I (Sigma, St. Louis, MO) dissolved in Ca²⁺/Mg²⁺-free HBSS (Mediatech) for 15 min at 37°C in a humidified atmosphereof 5%CO₂ and 95% air. After the enzymatic treatment, hippocampaltissue was rinsed twice: first in 0.1% soybean trypsin inhibitor(Worthington Biochemical) dissolved in Ca²⁺/Mg²⁺-containing Dulbecco's phosphate-buffered salt solution (Mediatech)and next in culture medium containing 10% fetal bovine serum (HyClone,Logan, UT). The tissue was next transferred to chilled Ca²⁺/Mg²⁺-free HBSS and triturated through siliconized fire-polished Pasteurpipettes. After trituration, undissociated tissue fragments wereallowed to settle for 5 min, and the supernatant was transferredto a new tube and centrifuged at 200 × g for 1 min to form a cellpellet. The resulting supernatant was discarded, and the cellswere gently resuspended in culture medium. Dissociated hippocampalcells were plated in UV-sterilized, 96-well flat-bottomed ELISAplates (MaxiSorp; Nalge Nunc, Naperville, IL) coated with poly-D-lysine(Sigma) and anti-BDNF capture antibody (BDNF E_max ImmunoAssaySystem; Promega, Madison, WI) (Balkowiec and Katz, 2000), after30 min preplating in uncoated 35 mm Petri dishes. Hippocampalcultures were grown for 3 d in Neurobasal-A medium supplementedwith B-27 serum-free supplement, 0.5 mM L-glutamine, 1% penicillin-streptomycin-neomycinantibiotic mixture and 5 ng/ml human recombinant basic fibroblastgrowth factor (Invitrogen, Gaithersburg,MD).

BDNF immunoassay. BDNF protein was measured with a modified sandwich ELISA, termed ELISA in situ, as described previously(Balkowiec and Katz, 2000). Briefly, 96-well ELISA plates were(1) UV-sterilized for 15 min, (2) treated with poly-D-lysine (0.1mg/ml; Sigma) for 30 min at room temperature, (3) rinsed witha sterile double-distilled water, and (4) coated with anti-BDNFmonoclonal antibody (BDNF E_max ImmunoAssay System; Promega) at4°C for 16.5 hr. Next, plates were washed and blocked, followedby two 1 hr incubations with culture medium to remove any residueof the ELISA washing solution. Then, the hippocampal neurons wereprepared as described above, plated in anti-BDNF-coated wells,and grown for 3 d (see Results). The BDNF E_max ImmunoAssay System(Promega) was used according to the protocol of the manufacturer,except that the concentration of the anti-BDNF monoclonal andanti-human BDNF polyclonal antibody was 5 and 2 µg/ml, respectively,and the dilution of the anti-IgY-HRP antibody was 1:100. All reagentsused before cell plating were sterilized with 0.2 µm Acrodiscsyringe filters (Pall, Ann Arbor, MI). BDNF samples used to generatethe standard curves were incubated in the same plate as the cells.At the end of the culture period, plates were extensively washedto remove all cells and cell debris, and the anti-human BDNF polyclonalantibody was applied, followed by subsequent steps according tothe protocol of the manufacturer. Absorbance values were readat 450 nm in a plate reader (V_max; Molecular Devices, Sunnyvale,CA). For control wells in which anti-BDNF monoclonal antibodywas omitted, absorbance values were not significantly differentfrom the absorbance of blankwells.

Electrical field stimulation of hippocampal neurons. After an initial 3 d incubation, two adjacent culture wells were connectedto each other through a thin strip of 1% agarose gel permeatedwith culture medium and to the stimulator (MultiStim System; Digitimer,Hertfordshire, UK) through Ag/AgCl stimulating electrodes (Balkowiecand Katz, 2000) (modified from Brevet et al., 1976; McDonoughet al., 1994). Two additional wells were also connected to eachother by agarose bridges but were not connected to the stimulatorand served as controls. The plate was put back to the incubator,and the neurons were stimulated for 30 min with biphasic rectangularpulses delivered at various patterns (see Results). In experimentscomparing the effects of patterned electrical stimulation withpotassium-induced continuous depolarization, KCl was added tothree additional wells, to a final concentration of 50 mM, asdescribed previously (Ghosh et al., 1994; Androutsellis-Theotokiset al., 1996; Goodman et al., 1996; Heymach et al., 1996; Griesbecket al., 1999; Balkowiec and Katz, 2000).

Drugs used. Tetrodotoxin (TTX) (Sigma), D,L-2-amino-5-phosphonovaleric acid (APV) (Sigma), 1-aminoindan-1,5-dicarboxylic acid(AIDA) (Sigma), trans-(1S,3R)-1-amino-1,3-cyclopentane-dicarboxylicacid (trans-[1S,3R]-ACPD) (Sigma), $omega$ -Conotoxin GVIA (Sigma), andcaffeine (Sigma) were dissolved in PBS and used at final concentrationsof 1.5, 100, 500, 100, 1, and 30 µM, respectively. 6-Cyano-7-nitroquinoxaline-2,3-(1H,4H)-dione(CNQX) (Sigma) was dissolved in 0.1 M NaOH and used at a finalconcentration of 20 µM. LY341495 (Tocris Cookson, Ellisville,MO) was dissolved in 15 mM NaOH and used at a final concentrationof 100 µM. Nimodipine (Sigma) and ionomycin (Calbiochem, La Jolla,CA) were dissolved in methyl alcohol and used at final concentrationsof 2 and 1 µM, respectively. Bay K-8644 (Calbiochem), dantrolene(Sigma), and thapsigargin (Sigma), dissolved in DMSO, were usedat final concentrations of 5, 50, and 10 µM, respectively, andthe final concentration of DMSO was 0.02%.

Immunocytochemistry. Cultures for immunocytochemical staining were fixed with 4% paraformaldehyde in 0.1 M sodium phosphatebuffer, pH 7.4, for 30 min at room temperature. Neuron-specificenolase (NSE) immunostaining was performed as described previouslyfor protein gene product 9.5 (Brady et al., 1999), using rabbitpolyclonal anti-NSE (1:2000 dilution; Polysciences, Warrington,PA). The number of neurons in each culture was evaluated by countingall NSE-immunoreactive cells per well. Experiments were repeatedtwice with four cultures per experimental group. Values were comparedusing ANOVA, followed by Duncan's multiple comparison procedure,and p < 0.05 was considered significant. Phosphorylated cAMP responseelement-binding protein (P-CREB) immunostaining was performedas described previously (Balkowiec and Katz, 2000). Control cultures,in which primary antibody was omitted, were completely devoidofstaining.

Calculations and statistical analysis. BDNF levels were calculated from the standard curve prepared for each plate, usingSOFTmax PRO version 3.0 software (Molecular Devices, Sunnyvale,CA). The standard curves were linear within the range used (0-500pg/ml), and the quantities of BDNF in experimental samples werealways within the linear range of the standard curve. Data areexpressed as mean ± SE. Samples were compared using ANOVA, followedby Duncan's multiple comparison procedure, and p < 0.05 was consideredsignificant.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The goal of the present study was to define the role of action potentials and voltage-activated calcium channels in activity-dependentBDNF release from hippocampal neurons. In view of the fact thatBDNF can be released from hippocampal neurons by activation ofglutamate receptors (GluR) (Ghosh et al., 1994; Griesbeck et al.,1999; Hartmann et al., 2001), we sought to examine release inthe absence of potentially confounding trans-synaptic interactions.We therefore used 3-d-old cultures of newborn hippocampal neurons,taking advantage of the fact that synaptic connections betweenhippocampal neurons in culture do not form until >4 d in vitro(Bito et al., 1996), and functional synapses do not appear until6-8 d in vitro (Deisseroth et al., 1996). Consistent with theseobservations, blockade of glutamatergic transmission did not affectelectrical stimulation-evoked BDNF release in this study (fordetails, seebelow).

Short-term patterned electrical stimulation, but not short-term continuous KCl depolarization, significantly increases native BDNF release from hippocampal neurons

Initial studies sought to determine whether release of native BDNF from hippocampal neurons is regulated by patterned neuronalactivity, as in sensory neurons (Balkowiec and Katz, 2000). Wecompared the effects of theta-burst electrical field stimulation,which mimics the typical firing mode of hippocampal pyramidalcells during learning (O'Keefe and Recce, 1993), and continuousdepolarization by 50 mM KCl (Ghosh et al., 1994; Goodman et al.,1996; Griesbeck et al., 1999; Hoener, 2000) on BDNF release fromnewborn hippocampal neurons. BDNF levels, measured by ELISA insitu, were compared after 30 min of control conditions, theta-burststimulation (TBS) (trains of 25 bursts, each burst of four pulsesat 100 Hz, delivered with an interburst interval of 200 msec andan intertrain interval of 20 sec) (see Fig. 2A, TBS), or KCl-inducedcontinuous depolarization. After theta-burst stimulation, therewas a highly significant increase in BDNF release from hippocampalneurons (44.32 ± 3.08 pg/ml, n = 30 vs 3.18 ± 1.29 pg/ml in control,n = 48; p < 0.0001) (Fig. 1). In contrast, 50 mM KCl-induced continuousdepolarization over the same time period did not result in a detectableincrease in BDNF release (5.44 ± 1.87 pg/ml; n = 39; p = 0.3154)(Fig. 1). To determine whether, under our experimental conditions,continuous membrane depolarization activated hippocampal neurons,we performed immunostaining with an antibody against P-CREB, amarker of neuronal depolarization (Ghosh et al., 1994; Moore etal., 1996). After 30 min treatment with 50 mM KCl, there was amarked increase in P-CREB staining in the vast majority of cells(data not shown), indicating that this treatment was effectiveat activating neurons in our cultures. Together, these data indicatethat patterned neuronal activity is significantly more effectivethan continuous depolarization at releasing native BDNF from hippocampalneurons.

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Figure 1. Short-term patterned electrical stimulation, but not short-term continuous KCl depolarization, significantly increases release of native BDNF from hippocampal neurons. Mean levels of BDNF measured in sister cultures of newborn hippocampal neurons after 3 d in vitro plus 30 min of the following: (1) control conditions (no stimulation; n = 48), (2) TBS (25 bursts of 4 pulses at 100 Hz, delivered at 5 Hz, every 20 sec; n = 30), or (3) continuous depolarization with 50 mM KCl (n = 39). ***p < 0.001; n.s., not significant.

High-frequency patterns of electrical stimulation that are known to induce hippocampal LTP are significantly more effective at releasing native BDNF from hippocampal neurons than low-frequency stimulation

The magnitude of native BDNF release from primary sensory neurons is regulated by the frequency and pattern of stimulation(Balkowiec and Katz, 2000; Lever et al., 2001). To determine whethersimilar mechanisms regulate activity-dependent secretion of BDNFfrom hippocampal neurons, we next examined the relationship betweenthe pattern of stimulation and the magnitude of native BDNF releasein hippocampal cultures. Because the magnitude of release of otherpeptides depends on the total number of pulses delivered (Whimand Lloyd, 1994), we designed five stimulation protocols in whichthe overall number of pulses, and consequently, average frequency,as well as the number of pulses in individual bursts, remainedconstant, whereas intraburst frequency and interburst intervalwere varied (Fig. 2A): (1) continuous stimulation at 5Hz, a frequency that corresponds to physiological levels of restingactivity at hippocampal synapses (Bito et al., 1996); (2)bursts of 100 pulses at 10 Hz, delivered once every 20 sec, afrequency that does not produce significant changes of synapticstrength in hippocampal cultures (Deisseroth et al., 1996) andslices (Dudek and Bear, 1992); (3) bursts of 100 pulsesat 25 Hz, delivered once every 20 sec, a "weak" LTP-inducing stimulus(Huber et al., 1998); (4) bursts of 100 pulses at 100 Hz,delivered once every 20 sec, a protocol that is commonly usedto induce hippocampal LTP (Patterson et al., 1992; Dragunow etal., 1993; Korte et al., 1995, 1996; Figurov et al., 1996; Pattersonet al., 1996; Kang et al., 1997); and (5) trains of 25bursts, each burst of four pulses at 100 Hz, delivered with aninterburst interval of 200 msec (at 5 Hz) and an intertrain intervalof 20 sec, i.e., TBS, which mimics the typical firing patternof hippocampal neurons during learning (O'Keefe and Recce, 1993)and is optimal for the induction of hippocampal LTP (Larson etal., 1986; Staubli and Lynch, 1987; Larson and Lynch, 1988; Staubliet al., 1999). The magnitude of BDNF release was compared amongthese stimulation protocols applied to newborn hippocampal neuronsover a 30 min period.

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Figure 2. High-frequency patterns of electrical stimulation that are known to induce LTP are significantly more effective at releasing native BDNF from hippocampal neurons than low-frequency stimulation. A, Schematic representation of the stimulation pattern applied to each group of cultures. B, Mean levels of BDNF released in sister cultures of newborn hippocampal neurons during 30 min of electrical field stimulation with 100 biphasic rectangular pulses of 4 msec, delivered at 5 Hz (n = 16), 10 Hz (n = 14), 25 Hz (n = 40), 100 Hz (n = 42), or TBS (n = 30), with interburst intervals, respectively, of 0, 10, 16, 19, and 15 sec, as shown in A. *p < 0.05; **p < 0.01; ***p < 0.001; n.s., not significant.

Each stimulation protocol evoked detectable release of BDNF. However, 100 Hz tetanic stimulation and TBS resulted in significantlyhigher BDNF release compared with the other stimulation protocols(TBS, 44.32 ± 3.08 pg/ml, n = 30; 100 Hz, 39.27 ± 2.06 pg/ml,n = 42; 25 Hz, 25.13 ± 1.83 pg/ml, n = 40; 10 Hz, 11.76 ± 1.89pg/ml, n = 14; 5 Hz, 2.36 ± 2.01 pg/ml, n = 16) (Fig. 2B). Interestingly,tetanic stimulation at 25 Hz, a protocol that has been shown toinduce a lower magnitude of LTP compared with 100 Hz tetanic stimulation(Huber et al., 1998), resulted in an intermediate level of BDNFrelease that was significantly lower compared with BDNF releaseevoked by 100 Hz tetanus or TBS (Fig. 2B). These data indicatethat there is a strong relationship between the pattern of stimulationand the magnitude of BDNF release from hippocampal neurons, suchthat stimulus protocols that are known to be most effective atinducing LTP are also most effective at evoking BDNFrelease.

To rule out the possibility that the increase in BDNF release detected in stimulated cultures was attributable to damage ofcells by electrical activation, we compared cell survival betweencontrol and stimulated cultures, using the same stimulus protocolsthat were used for the analysis of BDNF release. Twenty-four hoursafter stimulation, there were no significant differences in thenumber of cells between control and stimulated cultures for anystimulation protocol tested (per well: 5 Hz, control, 8649 ± 483.98,stimulated, 10,287 ± 1163.21, n = 8, p = 0.2146; 25 Hz, control,8343 ± 918.90, stimulated, 9432 ± 558.87, n = 8, p = 0.3285; 100Hz, control, 11,241 ± 1101.61, stimulated, 10,026 ± 715.26, n= 8, p = 0.3706; TBS, control, 11,808 ± 904.36, stimulated, 11,700± 1043.91, n = 8, p = 0.9388).

Electrical stimulation-evoked release of native BDNF requires activation of TTX-sensitive sodium channels and can occur in the absence of glutamate receptor activation

We next examined whether native BDNF release from hippocampal neurons evoked by patterned electrical stimulation requiresactivation of voltage-gated sodium channels and, consequently,generation of action potentials. Regardless of the stimulationprotocol used, evoked release of BDNF was abolished by treatmentof cultures with 1.5 µM TTX, an inhibitor of voltage-dependentsodium channels, before stimulation (Fig. 3), indicating thataction potentials are required for this release.

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Figure 3. Activity-dependent release of native BDNF depends on action potentials. Mean levels of BDNF released in sister cultures of newborn hippocampal neurons during 30 min of electrical field stimulation [100 biphasic rectangular pulses of 4 msec, delivered at 25 Hz (n = 12), 100 Hz (n = 10), and TBS (n = 4), once every 20 sec] in the absence (black bars) or presence (gray bars) of 1.5 µM TTX, an inhibitor of voltage-dependent sodium channels. **p < 0.01; ***p < 0.001.

Previous studies showed that BDNF release from hippocampal neurons can be evoked by stimulation with glutamate receptor agonists(Ghosh et al., 1994; Griesbeck et al., 1999) and by high-frequencyactivation of glutamatergic synapses (Hartmann et al., 2001).Because glutamate is the major excitatory neurotransmitter synthesizedby hippocampal neurons and can be released in response to electricalstimulation, we tested whether activation of hippocampal neuronsby glutamate played a role in BDNF release evoked by patternedelectrical stimulation in our experiments. Pretreatment of hippocampalcultures with 20 µM CNQX, a non-NMDA receptor antagonist, and100 µM APV, an NMDA receptor antagonist, had no significant effecton the magnitude of BDNF release evoked by 25 Hz, 100 Hz, or TBSpatterns (Fig. 4A).

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Figure 4. Release of native BDNF evoked by patterned electrical stimulation does not require glutamatergic synaptic activity. A, Mean levels of BDNF released in sister cultures of newborn hippocampal neurons during 30 min of electrical field stimulation [100 biphasic rectangular pulses of 4 msec, delivered at 25 Hz (n = 8), 100 Hz (n = 8), and TBS (n = 10), once every 20 sec] in the absence (black bars) or presence of CNQX (20 µM) and APV (100 µM), antagonists of, respectively, non-NMDA and NMDA glutamate receptors (CNQX-APV; gray bars). B, Mean levels of BDNF released in sister cultures during 30 min of either exposure to 100 µM trans-[1S,3R]-ACPD, an agonist of mGluR I and II (t-ACPD; n = 12), or electrical field stimulation at the theta-burst pattern (TBS; n = 12) in the absence (black bars) or presence of metabotropic glutamate receptor antagonists AIDA (500 µM; gray bars) and LY341495 (100 µM; white bars); ***p < 0.001; n.s., not significant.

Canossa et al. (2001) demonstrated that activation of metabotropic glutamate receptors (mGluR) leads to secretion of nativeBDNF from adult hippocampal slices. Therefore, we next examinedthe role of mGluR in BDNF release. Thirty minute exposure to 100µM trans-[1S,3R]-ACPD, an agonist of mGluR I and II, evoked asignificant increase in native BDNF release that was blocked by100 µM LY341495, used as a general mGluR antagonist (Leslie etal., 2001), and by 500 µM AIDA, a specific mGluR I inhibitor (Canossaet al., 2001) (Fig. 4B). However, the magnitude of TBS-evokedBDNF release was not affected by pretreatment with these samemGluR antagonists (Fig. 4B). Together, these data indicate thatglutamatergic receptor activation did not contribute to BDNF releaseevoked by patterned electrical stimulation in ourstudy.

Release of native BDNF evoked by patterned electrical stimulation requires calcium influx through N-type voltage-activated calcium channels

To begin characterizing cellular mechanisms underlying activity-dependent release of native BDNF from hippocampal neurons,we next examined the role of extracellular calcium and specificvoltage-activated calcium channels. Our initial experiments showedthat removal of calcium from the extracellular solution completelyabolishes release of native BDNF from hippocampal neurons evokedby 25 Hz, 100 Hz, and TBS stimulation (Fig. 5A), indicating thatextracellular calcium is required for this release.

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Figure 5. Release of native BDNF evoked by patterned electrical stimulation requires calcium influx through N-type voltage-activated calcium channels. Mean levels of BDNF released in sister cultures of newborn hippocampal neurons during 30 min of electrical field stimulation (100 biphasic rectangular pulses of 4 msec, delivered at 25 Hz, 100 Hz, and TBS, once every 20 sec): A, in the presence (Control; black bars) or absence (Ca-free; gray bars) of extracellular calcium (25 Hz, n = 6; 100 Hz, n = 4; TBS, n = 4); B, in the absence (Control; black bars) or presence of 1 µM $omega$ -Conotoxin GVIA, an N-type channel antagonist ( $omega$ -Conotoxin; gray bars) (25 Hz, n = 4; 100 Hz, n = 10; TBS, n = 4); C, in the absence (Control; black bars) or presence of 2 µM nimodipine, an L-type channel antagonist (Nimodipine; gray bars) (25 Hz, n = 4; 100 Hz, n = 4; TBS, n = 6). **p < 0.01; ***p < 0.001; n.s., not significant.

Previous studies have shown that multiple calcium channels coexist in nerve terminals and control release of neurotransmittersand peptide neuromodulators from central neurons (Dunlap et al.,1995). Moreover, different voltage-gated calcium channels canbe coupled to transmitter release during low- versus high-frequencyelectrical stimulation (Wright and Angus, 1996). Therefore, wenext sought to determine the requirement for specific voltage-activatedcalcium channels in BDNF release evoked by different patternsof stimulation. Pretreatment of hippocampal cultures with 1 µM $omega$ -Conotoxin GVIA, an N-type calcium channel antagonist, completelyabolished BDNF release evoked by 25 Hz, 100 Hz, and TBS stimulation(Fig. 5B). On the other hand, treatment with an L-type channelantagonist, nimodipine (2 µM), had no significant effect on BDNFrelease evoked by any of the stimulation protocols tested (Fig.5C). These data indicate that native BDNF release from hippocampalneurons evoked by patterned electrical stimulation requires calciumentry specifically through N-type voltage-activated calciumchannels.

Calcium entry through L-type channels has been shown to play an important role in activity-dependent BDNF expression in hippocampalneurons (Zafra et al., 1990, 1991; Ghosh et al., 1994; Tabuchiet al., 2000). Therefore, to determine whether calcium entry throughL-type channels is capable of regulating release of native BDNFfrom hippocampal neurons, we exposed hippocampal cultures to 5µM Bay K-8644, a selective agonist of L-type channels (Nowyckyet al., 1985; Brosenitsch et al., 1998), in the presence of 15mM KCl, a protocol that optimizes the efficacy of Bay K-8644 byslightly depolarizing the cells (Brosenitsch et al., 1998). Thirtyminute exposure to Bay K-8644 and 15 mM KCl did not evoke detectableBDNF release (control, 2.48 ± 1.26 pg/ml; Bay K-8644, 2.50 ± 0.96pg/ml; n = 8; p = 0.9896), whereas 3 d exposure led to a highlysignificant increase in extracellular BDNF concentration (control,6.27 ± 1.66 pg/ml; Bay K-8644, 44.89 ± 10.76 pg/ml; n = 8; p =0.0239). Exposure to 15 mM KCl alone, either for 30 min or 3 d,did not significantly affect BDNF release (data not shown). Consideringthe role of L-type channels in regulation of BDNF expression,this result indicates that calcium entry through L-type channelsdoes not influence native BDNF release from hippocampal neuronsin response to short-term stimulation but may increase the sizeof the releasable BDNF pool by increasing expression during prolongedchronic depolarization. In addition, exposure of hippocampal culturesto 1 µM ionomycin, a calcium ionophore, for 30 min had no significanteffect on BDNF release (control, 4.34 ± 2.79 pg/ml; ionomycin,5.96 ± 3.32 pg/ml; n = 6; p = 0.7219), further demonstrating thatincreasing calcium influx per se is not sufficient to increasenative BDNF release in response to short-termstimulation.

Electrical stimulation-evoked release of native BDNF from hippocampal neurons involves calcium mobilization from intracellular stores by a CICR mechanism

Previous studies have indicated that regulated secretion of neurotrophins requires calcium release from intracellular calciumstores, including caffeine-ryanodine-sensitive stores (Blöchland Thoenen, 1995; Griesbeck et al., 1999; Canossa et al., 2001).To establish whether calcium release from caffeine-ryanodine-sensitivestores is capable of inducing release of native BDNF from hippocampalneurons, we initially examined the effects of caffeine alone.Thirty minute treatment of hippocampal cultures with 30 µM caffeine,an agonist of ryanodine receptors, resulted in a significant increasein BDNF release that was blocked by 10 min pretreatment with 50µM dantrolene, a ryanodine receptor antagonist (Blöchl and Thoenen,1995) and 10 µM thapsigargin (Fig. 6A). These data show that activationof ryanodine-sensitive calcium stores is sufficient to evoke nativeBDNF release from hippocampal neurons. Because the caffeine-ryanodine-sensitivestore is involved in CICR (Kuba, 1994), we next sought to examinethe possibility that native BDNF release evoked by patterned electricalstimulation involves CICR. One of several criteria to establishthe involvement of CICR is the presence of a caffeine-sensitiveintracellular calcium store that is modulated by inhibitors ofsarcoplasmic-endoplasmic reticulum Ca²⁺-ATPase, such as thapsigargin (Treiman et al., 1998). Therefore,we next examined the effect of blocking CICR with thapsigarginand dantrolene on release of native BDNF from hippocampal neuronsin response to patterned electrical stimulation. Pretreatmentwith 10 µM thapsigargin, which by itself resulted in a significantrelease of BDNF (10.52 ± 2.45 pg/ml; n = 8), and 50 µM dantrolenesignificantly inhibited BDNF release evoked by TBS (Fig. 6B).These data demonstrate that release of native BDNF from hippocampalneurons in response to electrical stimulation requires intactintracellular calcium stores, as well as calcium influx throughN-type channels.

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Figure 6. Release of native BDNF in response to patterned electrical stimulation requires calcium mobilization from ryanodine-sensitive stores. Mean levels of BDNF released in sister cultures of newborn hippocampal neurons during 30 min exposure to either 30 µM caffeine or electrical field stimulation at the theta-burst pattern (TBS) in the absence (black bars) or presence of dantrolene (50 µM), a selective antagonist of ryanodine receptor channels. Cultures were pretreated with thapsigargin (10 µM), which selectively inhibits the endoplasmic reticulum Ca²⁺-ATPase (gray bars); n = 8. ***p < 0.001.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study demonstrates for the first time the properties and cellular mechanisms of native BDNF release from hippocampalneurons in response to physiologically relevant patterns of electricalstimulation, including those known to induce LTP in the intacthippocampus. Our study shows that frequency-dependent releaseof native BDNF can be triggered directly by activation of voltage-gatedsodium channels, in the absence of glutamate receptor activation.Moreover, this release requires both calcium influx through N-typechannels and calcium mobilization from intracellularstores.

The most extensive studies on the role of BDNF in synaptic plasticity have focused on hippocampal LTP. Induction of LTP isa cooperative process that requires simultaneous activity of alarge number of axons and a threshold of stimulus frequency andintensity (Bennett, 2000). Several studies indicate that, in fact,a critical level of BDNF is needed for LTP induction. For example,the postnatal increase in the ability of developing hippocampalsynapses to undergo LTP (Jackson et al., 1993) is paralleled byan increase in the expression of BDNF and its receptor TrkB inthe hippocampus (Maisonpierre et al., 1990). In addition, BDNF^/ and BDNF^+/ animals show the same degree of impairment in LTP (Korte et al.,1995; Patterson et al., 1996). The present study demonstratesthat TBS, which mimics the typical firing pattern of hippocampalneurons during learning, is highly effective at releasing BDNFfrom hippocampal neurons, whereas 5 Hz stimulation, which correspondsto resting activity at hippocampal synapses, is not. Our data,therefore, raise the possibility that the pattern dependence ofhippocampal LTP is related to the fact that the magnitude of BDNFrelease from hippocampal neurons depends on the pattern and frequencyofstimulation.

Several studies have indicated that, although 100 Hz tetanus and TBS are both effective at inducing hippocampal LTP, onlyTBS-induced LTP requires BDNF (Kang et al., 1997; Chen et al.,1999; Patterson et al., 2001) (but see Korte et al., 1995; Figurovet al., 1996). It has been suggested that this difference couldbe attributable to differential release of BDNF by TBS versus100 Hz tetanus (Kang et al., 1997; Chen et al., 1999). Our datado not support this possibility, because 100 Hz tetanus and TBSwere equally effective at releasing native BDNF in our model.Thus, although the frequency dependence of BDNF release couldcontribute to the relative effectiveness of TBS versus low-frequencystimulation at inducing LTP, other factors likely influence therelative importance of BDNF signaling in TBS-induced versus 100Hz tetanus-inducedLTP.

The role of calcium influx in activity-dependent release of neurotrophins has been a subject of considerable controversy.Most previous studies, in which chronic depolarizing agents wereused to induce BDNF release, suggested a mechanism independentof extracellular calcium (Griesbeck et al., 1999) (but see Goodmanet al., 1996). However, it has been demonstrated recently thatextracellular calcium is required for BDNF-GFP release evokedby both KCl depolarization and high-frequency electrical stimulationof hippocampal neurons (Hartmann et al., 2001). Our results demonstratethat activity-dependent BDNF secretion requires both calcium influx,specifically through N-type channels, and calcium mobilizationfrom intracellular stores. This dual requirement for extracellularand intracellular calcium strongly implicates a role for calcium-inducedcalcium release in activity-dependent secretion ofBDNF.

It has been demonstrated previously that depolarization-induced calcium entry in hippocampal neurons can activate calciumrelease from intracellular stores (Sandler and Barbara, 1999).This observation is consistent with recent evidence that activity-dependentregulation of intracellular calcium levels is tightly controlledby interactions between calcium influx and activation of intracellularcalcium stores. For example, decreasing extracellular calciumlevels can prime activity-dependent calcium release from intracellularstores (Nohmi et al., 2000). Therefore, because high levels ofneuronal activity can decrease the extracellular calcium concentration(Heinemann and Pumain, 1980; Borst and Sakmann, 1999; Stanley,2000), it seems plausible that BDNF release from hippocampal neuronsis potentiated during high-frequency firing, as occurs duringhippocampal learning (O'Keefe and Recce, 1993), by increasingcalcium mobilization from intracellularstores.

Our studies were conducted with 3-d-old cultures of newborn hippocampal neurons that lack excitatory glutamatergic synapses(Bito et al., 1996), as confirmed by our experiments with glutamatereceptor antagonists. This model, therefore, allowed us to characterizein detail the requirement for calcium influx in BDNF release byusing selective calcium channel antagonists without potentiallyconfounding effects on glutamate release. Our results demonstratethat activity-dependent release of native BDNF from newborn hippocampalneurons requires calcium influx specifically through N-type channels,regardless of the pattern of stimulation. A similar requirementfor N-type channels in release of neurotrophin-3 from retinotectalaxon terminals has been reported recently (Wang et al., 2002).Our findings are supported by observations that blockade of N-type,but not L-type, channels also leads to a significant reductionof synaptic vesicle recycling in newborn hippocampal neurons (Pravettoniet al., 2000). Moreover, the fact that N-type calcium channelsare located almost exclusively on axons of newborn hippocampalneurons grown for 3 d in culture (Pravettoni et al., 2000) suggeststhat our data primarily reflect BDNF release from axonal sites.Although it is a subject of debate whether BDNF is released presynapticallyor postsynaptically or both (Hartmann et al., 2001; Kohara etal., 2001), findings from several laboratories indicate that BDNFcan be released from axons (Altar et al., 1997; Conner et al.,1997; Fawcett et al., 1998; Fawcett et al., 2000; Kohara et al.,2001; Kojima et al., 2001). Our data are consistent with thesefindings but do not rule out the possibility that, in more matureneurons, release can occur from other sites aswell.

Although there are limitations in extrapolating data from dissociate cultures to more intact systems, we believe that ourresults may help shed light on the role of BDNF in activity-dependentsynaptic plasticity. For example, previous studies have indicatedthat BDNF, by promoting synaptic vesicle docking, enhances transmitterrelease in response to tetanic stimulation (Gottschalk et al.,1998; Pozzo-Miller et al., 1999). Moreover, highly active synapsesare more susceptible to the potentiating effects of BDNF on presynaptictransmitter release (Gottschalk et al., 1998). Thus, based onthe present findings, we propose that highly active synapses,in contrast to inactive or weakly active synapses, are more likelyto meet the threshold conditions both for BDNF concentration andthe potentiating effects of activity on BDNF-induced transmitterrelease and, therefore, induce LTP. This is essentially the modelproposed by Gottschalk et al. (1998) based on their analysis ofBDNF-stimulated glutamate release in hippocampal neurons. A similarmechanism could underlie the role of BDNF in activity-dependentsynaptic plasticity leading to morphological changes in neuronalcircuits, such as refinement of neuronal connections in developingvisual cortex (Goodman and Shatz, 1993; Katz and Shatz, 1996;Schinder and Poo, 2000). Several studies indicate that BDNF canalso act postsynaptically in hippocampal neurons by rapidly enhancingbasal excitatory synaptic responses, including increases in postsynapticNMDA receptor activity (Lessmann et al., 1994; Levine et al.,1995). Thus, one implication of our findings is that the increasein BDNF release with increasing frequency of presynaptic neuronalactivity could partially compensate for the effects of synapticfatigue by enhancing postsynaptic NMDAresponses.

The duration of patterned electrical stimulation used in our study was significantly longer than standard LTP-inducing protocolsbecause of the fact that the levels of native BDNF released duringshorter stimulation periods were below the detectability limitsof the ELISA assay (data not shown). This observation suggeststhat, in our model, release of native BDNF from hippocampal neuronsoccurs over a prolonged period of stimulation. Very recently,Gärtner and Staiger (2002) demonstrated that release of AdVBDNFfrom hippocampal neurons peaks within the first minute of stimulationand decays rapidly thereafter. On the other hand, Hartmann etal. (2001) demonstrated that tetanic stimulation-evoked releaseof BDNF-GFP from hippocampal neurons is characterized by a slowonset, in the range of minutes. These apparent discrepancies inthe time course of BDNF secretion could reflect differences inthe sorting and release of native BDNF, AdVBDNF, and BDNF-GFP(cf. Fawcett et al., 1997; Mowla et al., 1999) or other differencesamong the models used in these threestudies.

Similar to primary sensory neurons, patterned electrical stimulation of hippocampal neurons is strikingly more effective thanKCl depolarization at releasing native BDNF (present findings;Balkowiec and Katz, 2000). This result is in agreement with Griesbecket al. (1999) who were unable to detect native BDNF release fromprimary cultures of hippocampal neurons briefly exposed to elevatedKCl. The same treatment, however, led to a significant increasein release of AdVBDNF (Griesbeck et al., 1999). This result, togetherwith our current findings, raises the possibility that, afteradenovirus-mediated overexpression, at least some BDNF is shuntedto a pool that is sensitive to KCl depolarization, whereas nativeBDNF isnot.

In conclusion, the present study shows that activity-dependent secretion of native BDNF from hippocampal neurons is highlyfrequency dependent, indicating that BDNF release can encode temporalfeatures of neuronal activity. Moreover, our data provide supportfor a novel mechanism of activity-dependent BDNF release involvingcalcium influx specifically through N-type channels, as well ascalcium-induced calcium release from intracellularstores.

  FOOTNOTES

Received May 31, 2002; revised Aug. 15, 2002; accepted Sept. 25, 2002.

This work was supported by United States Public Health Service grants (National Heart, Lung, and Blood Institute) (D.M.K.).

Correspondence should be addressed to Dr. David M. Katz, Department of Neurosciences, Case Western Reserve University Schoolof Medicine, 10900 Euclid Avenue, Cleveland, OH 44106. E-mail:dmk4{at}po.cwru.edu.

A. Balkowiec's present address: Department of Biological Structure and Function, Oregon Health and Science University, 611Southwest Campus Drive, Portland, OR97239.

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