Brain-Derived Neurotrophic Factor Acutely Inhibits AMPA-Mediated Currents in Developing Sensory Relay Neurons

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The Journal of Neuroscience, March 1, 2000, 20(5):1904-1911

Brain-Derived Neurotrophic Factor Acutely Inhibits AMPA-Mediated Currents in Developing Sensory Relay Neurons
Agnieszka Balkowiec, Diana L. Kunze, 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) is expressed by many primary sensory neurons that no longer require neurotrophinsfor survival, indicating that BDNF may be used as a signalingmolecule by the afferents themselves. Because many primary afferentsalso express glutamate, we investigated the possibility that BDNFmodulates glutamatergic AMPA responses of newborn second-ordersensory relay neurons. Perforated-patch, voltage-clamp recordingswere made from dissociated neurons of the brainstem nucleus tractussolitarius (nTS), a region that receives massive primary afferentinput from BDNF-containing neurons in the nodose and petrosalcranial sensory ganglia. Electrophysiological analysis was combinedin some experiments with anterograde labeling of primary afferentterminals to specifically analyze responses of identified second-orderneurons. Our data demonstrate that BDNF strongly inhibits AMPA-mediatedcurrents in a large subset of nTS cells. Specifically, AMPA responseswere either completely abolished or markedly inhibited by BDNFin 73% of postnatal day (P0) cells and in 82% of identified P5second-order sensory relay neurons. This effect of BDNF is mimickedby NT-4, but not NGF, and blocked by the Trk tyrosine kinase inhibitorK252a, consistent with a requirement for TrkB receptor activation.Moreover, analysis of TrkB expression in culture revealed a closecorrelation between the percentage of nTS neurons in which BDNFinhibits AMPA currents and the percentage of neurons that exhibitTrkB immunoreactivity. These data document a previously undefinedmechanism of acute modulation of AMPA responses by BDNF and indicatethat BDNF may regulate glutamatergic transmission at primary afferentsynapses.

Key words: AMPA; BDNF; glutamate; nucleus tractus solitarius; sensory neurons; synaptic plasticity; synaptic transmission

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Brain-derived neurotrophic factor (BDNF) acts as a target-derived survival factor for subsets of developing primary sensoryneurons (Hallbook and Fritzsch, 1997; Brady et al., 1999; Fritzschet al., 1999). In addition, however, many primary sensory neuronsthemselves express and can release BDNF, even when they are nolonger dependent on BDNF for survival (Schecterson and Bothwell,1992; Wetmore and Olson, 1995; Apfel et al., 1996; Zhou et al.,1998; Brady et al., 1999). This finding raises the possibilitythat BDNF plays additional roles in sensory pathway developmentor function, including a role in afferent synaptic transmission.In support of this possibility, a subset of dorsal root ganglion(DRG) sensory neurons transports BDNF in their projections tothe spinal cord (Zhou and Rush, 1996; Tonra, 1999), and BDNF islocalized to dense-core vesicles within DRG central axon terminals(Michael et al., 1997). In addition, Kerr et al. (1999) demonstratedthat BDNF can potentiate nociceptive spinal reflexes, most likelyby enhancing NMDA receptor-mediated responses. Moreover, studiesin other neural systems have shown that BDNF can acutely regulatesynaptic transmission and neuronal activity. For example, BDNFapplication increases the frequency of EPSCs at the neuromuscularjunction (Lohof et al., 1993) and in cultured hippocampal neurons(Lessmann et al., 1994; Levine et al., 1995, 1996) as well asexcitability of cortical (Rutherford et al., 1997), hippocampal-entorhinal(Scharfman, 1997), and spinal motoneurons (Gonzalez and Collins,1997). In addition, BDNF induces a long-lasting increase in synaptictransmission in hippocampal slices from adult rat (Kang and Schuman,1995a) and facilitates induction of hippocampal long-term potentiation(LTP; Figurov et al., 1996). BDNF knock-out mice have a deficitin basal synaptic transmission, as well as LTP (Korte et al.,1995), both of which can be reversed by exogenous BDNF (Pattersonet al., 1996). These data, coupled with findings that BDNF synthesisand release are activity-dependent (Castrén et al., 1992; Bozziet al., 1995; Thoenen, 1995; McAllister et al., 1997), supportthe view that BDNF can act acutely as a synapticneuromodulator.

BDNF-containing primary sensory neurons are most abundant in cranial sensory ganglia, including the nodose-petrosal ganglion(NPG) of the vagal and glossopharyngeal nerves (Brady et al.,1999). These neurons convey visceral sensory information and projectcentrally to the brainstem nucleus tractus solitarius (nTS), whichexpresses high levels of the BDNF receptor TrkB (Yan et al., 1997).The major transmitter of NPG sensory neurons is L-glutamate (Andresenand Yang, 1990; Ambalavanar et al., 1998; Smith et al., 1998;Zhang and Mifflin, 1998; Botsford et al., 1999), raising the possibilitythat BDNF modulates glutamatergic transmission between primaryafferents and second-order neurons in nTS. The present study wasdesigned to test this possibility using voltage-clamp recordingfrom identified second-order nTS neurons. We focused in particularon interactions between BDNF and the AMPA subtype of glutamatereceptors, which mediates fast excitatory neurotransmission (Ozawaet al., 1998). Our data demonstrate that BDNF, acting throughthe TrkB receptor, strongly inhibits AMPA responses in second-ordersensory relayneurons.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell preparation. Newborn rats (Sprague Dawley strain; Zivic-Miller, Zelienople, PA) were killed by exposure to carbon dioxideand decapitated. Blocks of tissue were isolated from the nucleustractus solitarius (nTS) at the level of the obex of the fourthventricle. The tissue was subdivided into several smaller piecesand dissociated by gentle trituration through glass Pasteur pipettesof successively smaller tip diameters. The cells were plated onpoly-D-lysine-treated coverslips and grown for 24 hr in DMEM-F12medium (Life Technologies, Gaithersburg, MD) with 10% fetal bovineserum (HyClone, Logan, UT). The analyzed cells were selected basedon morphological criteria characteristic of second-order relayneurons, i.e., round or oval bipolar cells, 10-20 µm in diameter,with thin processes (Fig. 4B, large arrow; see also Mendelowitzet al., 1992).

Dye labeling. We used a modification of the technique previously described by Mendelowitz and colleagues (1992) to label presynapticboutons on second-order nTS neurons. Briefly, newborn [postnatalday 0 (P0)] rats were anesthetized by hypothermia combined withlocal application of Lidocaine HCl (Abbott Laboratories). Bothvagal nerves were exposed in the neck by a ventral midline excisionand isolated from surrounding tissues with Parafilm "M" (FisherScientific, Houston, TX). Small crystals of the anterograde tracer4-(4-(didecylamino)styryl)-N-methyl-pyridinium iodide (DiA) (4-Di-10-ASP;Molecular Probes, Eugene, OR) were placed on the isolated intactnerves at the level of the carotid bifurcation and caudal to thenodose ganglion. To prevent dye leakage to surrounding tissues,the region was isolated with a fast hardening silicone elastomer(Kwik-Sil; World Precision Instruments). The animals were thensutured and allowed to recover for 5-9 d. All experiments wereperformed in compliance with the guidelines of the Case WesternReserve University Institutional Animal Care and Use Committee.nTS neurons were prepared essentially as described above for P0animals, except that the cells were dissociated and plated inthe presence of reduced calcium (0.2 mM; Mendelowitz et al., 1992).Recordings from labeled P5/P9 neurons began 6-8 hr after dissociation,and the second-order sensory neurons were identified by the presenceof fluorescing boutons attached to the soma. Only brief exposureto UV light, not exceeding 10-20 sec, was used to identify labeledneurons.

Electrophysiology. The neurons were studied using the amphotericin perforated-patch recording technique in voltage-clamp mode(Hamill et al., 1981; Rae et al., 1991). The extracellular solutioncontained (in mM): NaCl 137, KCl 5.4, MgCl₂ 1, CaCl₂ 2, glucose10, and HEPES 10. In experiments in which voltage-activated calciumchannels were blocked, the CaCl₂ concentration was decreased to0.02 mM, and 0.5 mM cadmium succinate was added. The pipette solutioncontained (in mM): NaCl 10, KCl 50, K₂SO₄ 50, MgCl₂ 5, and HEPES10. Recordings were performed in room temperature with patch pipettespulled from 7052 glass and fire-polished to a final resistanceof 3-5 M $Omega$ , using an Axopatch-200A (Axon Instruments, Foster City,CA) patch-clamp amplifier. The membrane potential was held at $-$ 60 mV. Signals were filtered at 2 kHz, digitized on-line at asampling rate of 10 kHz, and stored for later computer analysisusing pClamp version 5.7 software (Axon Instruments).

BDNF and NT-4 were generously provided by Regeneron Pharmaceuticals (Tarrytown, NY), and NGF was provided by Dr. Kenneth Neet(Chicago Medical School). All other reagents were purchased: AMPA(Sigma, St. Louis, MO), K252a and K252b (Calbiochem, La Jolla,CA). All drugs were diluted in the extracellular solution andapplied to the cell using a multibarrel pipette and a rapid, gravity-drivenperfusion system (a modification of the U-tube design; Muraseet al., 1989). K252a and K252b were initially dissolved in DMSOat 2 mM; the final concentration of DMSO in the working solutions,0.01%, has no effect on neuronal function (Kang and Schuman, 1995b).

TrkB immunocytochemistry. Cultures grown as described above for 24 or 72 hr, and tissue sections, were stained as previouslydescribed (Brady et al., 1999) using chicken polyclonal anti-TrkB(Promega, Madison, WI) and donkey anti-chicken biotinylated IgG(Accurate Chemicals, Westbury, NY). Control slides, in which primaryantibody was omitted, were completely devoid of staining. Becausethe percentage of TrkB-positive neurons was not different in 24and 72 hr nTS cultures, the data werepooled.

Confocal microscopy. Images of labeled second-order nTS neurons were taken with a Zeiss LSM 410 confocal laser microscope(Zeiss, Göttingen, Germany), using an argon-krypton laser (excitationline 488) and a 100× Plan-Neofluar, numerical aperture 1.3, oilobjective.

Statistical analysis. Data were analyzed by integrating, for each neuron, the AMPA-evoked current under control conditionsand during drug application, using Clampfit version 6.0 software(Axon Instruments). Data are presented as mean ± SEM and wereanalyzed by ANOVA for repeated measures followed by Duncan's multiplecomparison procedure. p < 0.05 was consideredsignificant.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

To assess the effects of BDNF on postsynaptic AMPA responses in dissociated nTS neurons, we recorded currents evoked by a2 sec pulse application of AMPA (150 µM), a selective agonistof the AMPA subtype of glutamatergic receptors, in the absenceand presence of 50 ng/ml BDNF, using the perforated-patch technique(Materials and Methods). Studies were performed on 113 P0 neurons,selected on the basis of morphological criteria characteristicof second-order relay cells (Materials and Methods), and on 11P5/P9 nTS neurons specifically identified as second-order relayneurons by dye labeling of presynaptic boutons (Materials andMethods). In both unlabeled and labeled cells, application ofAMPA alone activated a rapidly decaying inward current followedby a prolonged component of lower amplitude (Fig. 1A). AMPA-evokedcurrents were completely blocked by CNQX (20 µM, n = 12), a competitiveantagonist of non-NMDA receptors.

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Figure 1. Effects of BDNF on AMPA currents in P0 nTS neurons. A, Sample recording of BDNF effect on AMPA currents in a P0 nTS neuron. The neuron was first superfused with control bath solution followed by a 2 sec pulse of 150 µM AMPA alone (horizontal bar; AMPA). The solution was then switched to one containing BDNF (50 ng/ml), and, 1 min later, 150 µM AMPA plus 50 ng/ml BDNF was simultaneously applied for 2 sec (AMPA + BDNF). After 1 min rinse with control bath solution, the application of AMPA alone was repeated (AMPA recovery). Calibration: 4 sec, 50 pA. B, The distribution of AMPA currents in the presence (top panel) and absence (bottom panel) of BDNF in the entire population of P0 nTS neurons tested. AMPA currents in the presence of BDNF are expressed as a percentage of control AMPA currents evoked by the application of AMPA alone before BDNF treatment. AMPA currents in the absence of BDNF represent currents evoked by a second control application of AMPA expressed as a percentage of the first control application. The distribution of control AMPA currents shows a variability of 25% in the control responses. Therefore, the effect of BDNF was considered significant when the AMPA current in the presence of BDNF was <75% of the control AMPA current.

The effects of BDNF were analyzed using an experimental paradigm in which, after two or three control applications of AMPA,50 ng/ml BDNF was applied to the extracellular solution for 1min, followed by BDNF plus AMPA for 2 sec. The simultaneous applicationof AMPA and BDNF was repeated twice in 1 min intervals duringwhich 50 ng/ml BDNF was continuously present in the extracellularsolution. Following the test applications of AMPA and BDNF, theextracellular solution containing BDNF was replaced with controlsolution, and 1 min later, AMPA was applied alone (recovery; Fig.1A). The BDNF concentration of 50 ng/ml was chosen based on previousstudies of acute BDNF effects on neuronal function in culture(Lessmann et al., 1994; Levine et al., 1995; Song et al., 1998).

In unlabeled, P0 nTS neurons, AMPA responses were either completely abolished (27 cells, 24%) or inhibited (55 cells, 49%)by BDNF. An AMPA response was considered inhibited by BDNF if,in the presence of BDNF, it fell below the distribution of controlAMPA responses, i.e., it was <75% of control current (see Fig.1B for details). The distribution analysis of BDNF effects onAMPA responses in the entire population of 113 P0 nTS neuronstested, expressed as a percent of control, revealed three subpopulations:(1) 0-5%, corresponding to complete blockade of AMPA currents,(2) 5-75%, corresponding to partial inhibition of AMPA responses,and (3) 75-125%, representing a neuronal population not affectedby BDNF and matching the distribution of control AMPA responses(Fig. 1B). This result suggests that there are three distinctsubpopulations of nTS neurons with respect to the effects of BDNFon AMPA responses. However, because we were not able to identifyany additional independent feature distinguishing the two subpopulationsof cells in which AMPA responses were affected by BDNF, such ascell size or the magnitude of the control AMPA responses, thesetwo groups were combined for furtheranalysis.

In the subpopulation of P0 nTS neurons affected by BDNF, AMPA responses were inhibited on average by 67.9 ± 5.5% (n = 82,p < 0.001) during the first BDNF application. Two subsequent applicationsof AMPA in the presence of BDNF showed a similar degree of inhibition(68.3 ± 5.6% and 67.8 ± 5.5%, respectively; Fig. 2). This demonstratesthat the maximum BDNF effect is already reached during the firstminute of application and persists in the continued presence ofBDNF.

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Figure 2. Comparison of the effects of three subsequent applications of AMPA + BDNF (closed circles) after control application of AMPA alone (open circle, time 0). Recovery from the BDNF effect was reached 1 min after BDNF was removed from the bath (open circle). n = 82; ** p < 0.01; *** p < 0.001.

To rule out the possibility that BDNF acts presynaptically, e.g., by stimulating release of an inhibitory transmitter fromadherent synaptic boutons (Drewe et al., 1988), we tested theeffect of blocking voltage-activated calcium channels (0.5 mMCd²⁺, 0.02 mM Ca²⁺) on BDNF inhibition of AMPA currents. In 7 of the 11 P0 nTS neuronstested, AMPA responses were either completely abolished (n = 3)or markedly inhibited (49.9 ± 13.16% of control, n = 4, p = 0.019)by BDNF, paralleling results obtained in normal calcium-containingmedium. The persistence of BDNF inhibition of AMPA responses inthe absence of calcium influx indicates a direct effect, not requiringcalcium-mediated transmitter release from either presynaptic terminalsor the nTS neurons themselves. In addition, application of BDNFalone was not accompanied by any significant or consistent changein the input resistance (mean percentage of baseline: 95.62 ±7.96, n = 10, p > 0.05), indicating that the intrinsic membraneproperties of the cells were not affected byBDNF.

To specifically identify second-order sensory relay neurons (defined as nTS cells that receive primary afferent input), primaryafferents were prelabeled in newborn animals with the anterogradetracer DiA (Materials and Methods). Five to nine days later thenTS region was dissociated, and second-order sensory neurons wereidentified by the presence of fluorescent presynaptic boutons(Fig. 3A). In 9 of the 11 identified neurons tested, AMPA responseswere either completely abolished (two neurons) or markedly inhibited(seven neurons) by BDNF. On average, there was 76.4 ± 5.2% inhibitionof AMPA currents by BDNF (n = 9, p < 0.01; Fig. 3B). The resultsobtained from identified second-order nTS neurons were virtuallyidentical to those obtained in unlabeled P0 nTS cells (Fig. 3C),indicating that the population of P0 neurons tested was representativeof the population of relay neurons. Therefore, unlabeled P0 cellswere used for further analysis.

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Figure 3. Effects of BDNF on AMPA currents in P5/P9 identified second-order sensory neurons. A, Confocal image (a single optical section of 719 nm) of a P9 nTS neuron showing an attached, DiA-filled, synaptic bouton (arrow), taken 6 hr after dissociation. Scale bar, 5 µm. B, C, Mean integrated currents evoked by a control 2 sec application of AMPA alone (AMPA control), simultaneous application of AMPA and BDNF after 1 min BDNF pretreatment (AMPA + BDNF), and after return to superfusion with control bath solution (AMPA recovery), recorded in P5/P9 labeled nTS neurons (B; n = 9), and compared to P0 neurons (C; n = 82). * p < 0.05; **p < 0.01; *** p < 0.001.

Immunocytochemical staining demonstrated that a subset of nTS neurons expresses the BDNF receptor TrkB in vivo (Fig. 4A) andin dissociate culture (Fig. 4B). To determine whether the percentageof TrkB-positive nTS neurons correlated with the percentage ofneurons in which BDNF inhibited AMPA currents, detailed analysisof TrkB staining was performed on a population of cultured nTSneurons selected according to the same morphological criteriaused in our electrophysiological studies. This analysis revealedthat 83% (76 of 92) of P0 cells and 78% (57 of 73) of P5 cellswere TrkB-positive, findings that closely match the percentageof cells in which BDNF inhibited AMPA responses at both ages (74%,P0; 82%, P5). Therefore, to directly examine the role of TrkBactivation in BDNF inhibition of AMPA currents, we analyzed theeffect of the Trk tyrosine kinase inhibitor K252a. Eight P0 nTSneurons in which AMPA responses were either abolished (n = 3)or partially blocked (n = 5) by BDNF were tested for the effectsof K252a. Following control applications of AMPA and AMPA plusBDNF (as described above; Fig. 4C, control), the cells were superfusedwith 200 nM K252a for 12-15 min, after which application of AMPAand AMPA plus BDNF was repeated as before (Fig. 4C, K252a). FollowingK252a treatment, BDNF had no effect on AMPA responses (Fig. 4D),consistent with the hypothesis that BDNF inhibition of AMPA currentsrequires Trk receptor tyrosine kinase activity. Because K252ainhibits Trk receptor tyrosine kinases preferentially, but notwith absolute specificity, we also tested the effect of K252b,a structural analog of K252a that is characterized by a markedlylower potency for Trk receptor tyrosine kinase inhibition (Kangand Schuman, 1995b). We tested four cells in which BDNF completelyabolished AMPA responses under control conditions. Using the sameexperimental protocol that was used for K252a, 200 nM K252b wasineffective at inhibiting the effect of BDNF on AMPA responses(Fig. 4E). To further define the specificity of BDNF action onAMPA responses, we also examined the effect of NT-4, the otherknown TrkB receptor ligand (Ip et al., 1992; Klein et al., 1992),as well as NGF, which acts through the TrkA receptor. In 22 nTSneurons in which BDNF inhibited AMPA responses, NT-4 (50 ng/ml)completely mimicked the effect of BDNF (Fig. 5A). In contrast,NGF (50 ng/ml) had no detectable effect on AMPA responses in 12neurons in which BDNF either partially or completely inhibitedAMPA currents (Fig. 5B). Together, these results strongly indicatethat BDNF inhibition of AMPA responses is mediated through TrkBreceptor activation.

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Figure 4. The effects of BDNF on AMPA currents are TrkB-mediated. A, TrkB immunoreactivity in the commissural subnucleus of the nucleus tractus solitarius in a P0 rat (transverse section). Scale bar, 100 µm. In control sections in which the primary antibody was omitted during the staining procedure, no staining was detected above background (data not shown). B, TrkB-positive (large arrow) and TrkB-negative (small arrow) cell in a P0 nTS culture, 24 hr after plating. Scale bar, 20 µm. C, Sample recording of the AMPA currents measured in a P0 nTS neuron during control AMPA application (AMPA) and during the coapplication of AMPA and BDNF after 1 min BDNF pretreatment (AMPA + BDNF), before (Control) and after K252a treatment. The cell was superfused with 200 nM K252a for 12 min. Calibration: 4 sec, 50 pA. D, Mean integrated currents in P0 nTS neurons evoked by control 2 sec application of AMPA alone (AMPA control), AMPA, and BDNF after 1 min BDNF pretreatment (AMPA + BDNF), and after return to superfusion with control bath solution (AMPA recovery) in the absence or presence of 200 nM K252a; n = 8. E, Mean integrated currents in four P0 nTS neurons in which the effects of 200 nM K252b on BDNF inhibition of AMPA currents were tested. AMPA responses were abolished by BDNF in all neurons tested before and after K252b treatment.

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Figure 5. The effects of BDNF, NT-4, and NGF on AMPA currents measured in P0 nTS neurons. A, B, The response to AMPA + BDNF was determined first, as described in Figure 1. After recovery of control AMPA responses, the response to AMPA + 50 ng/ml NT-4 (A) or 50 ng/ml NGF (B) was determined using the same protocol. A, n = 22; *p < 0.05; **p < 0.01; B, n = 12; *p < 0.05; n.s., not significant.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study demonstrates that BDNF markedly inhibits AMPA receptor-mediated currents in a large subset of newborn nTSneurons, including identified second-order sensory relay cells.This effect of BDNF was mimicked by NT-4, but not NGF, and blockedby the Trk tyrosine kinase inhibitor K252a, consistent with arequirement for TrkB receptoractivation.

Most studies on the acute neuromodulatory effects of neurotrophins at central synapses have focused on NMDA responses anddemonstrated enhanced glutamatergic transmission in the presenceof BDNF (Lessmann et al., 1994; Kang and Schuman, 1995a; Lessmannand Heumann, 1998; Levine et al., 1998). In contrast, our dataindicate that AMPA responses are strongly inhibited by BDNF. Previousstudies have hinted at an inhibitory action of BDNF on centralneurons. Lessmann et al. (1994) reported a reversible inhibitionof evoked synaptic currents in 15% of hippocampal cells afterapplication of BDNF or NT-4. Similarly, BDNF and NT-4 depressedglutamatergic synaptic transmission in 10% of cultured hippocampalneurons (Lessmann and Heumann, 1998). Exogenous BDNF has alsobeen shown to acutely suppress spontaneous synaptic activity inhippocampal cultures via non-NMDA receptors and to increase activitythrough NMDA receptors (Song et al., 1998). Thus, we considerit likely that BDNF inhibition of AMPA responses is a generalphenomenon and not restricted to sensory relay cells innTS.

Several lines of evidence indicate that BDNF inhibition of AMPA responses is mediated by activation of TrkB receptors. First,BDNF action was mimicked, in the same cells, by NT-4, also a TrkBligand, but not by NGF, which acts through TrkA (Chao, 1992; Barbacid,1994). Second, the effect of BDNF was blocked by K252a, a Trkreceptor tyrosine kinase inhibitor (Berg et al., 1992; Nye etal., 1992), but not by the relatively inactive isoform K252b (Kangand Schuman, 1995b; Ross et al., 1995). These findings argue stronglyagainst other potential mechanisms, such as competitive inhibitionbetween BDNF and AMPA at the AMPA-binding site. Moreover, we observeda close correlation between the percentage of nTS neurons in whichBDNF inhibited AMPA currents and the percentage of neurons exhibitingTrkB immunoreactivity inculture.

Kafitz and colleagues (1999) recently described a rapid activation of sodium currents by BDNF that is also TrkB-mediated andblocked by K252a. These authors postulate that the rapidity ofthis response and its sensitivity to tyrosine kinase inhibitionmay reflect a direct interaction between sodium channels and apool of already phosphorylated TrkB receptors, a pool that wouldturn over during the period of pretreatment with K252a. We speculatethat a similar mechanism, in which phosphorylated TrkB receptorsinteract directly with AMPA receptors, may underlie the rapidinhibition of AMPA currents by BDNF describedhere.

Neuronal activity can regulate the accumulation of AMPA receptors at synapses by rapid membrane trafficking (Lissin et al.,1999) and by regulating the turnover of postsynaptic AMPA receptors(O'Brien et al., 1998), leading to changes in EPSC amplitude.Lissin et al. (1999) demonstrated that the number of AMPA receptorGluR1 subunits can be regulated very rapidly by membrane traffickingand, within minutes, lead to pronounced changes in synaptic efficacy.Therefore, one possible mechanism underlying acute inhibitionof AMPA currents by BDNF is a rapid change in the number of availableAMPA receptors. Alternatively, TrkB activation could lead to achange in AMPA receptor function without altering receptor availability.BDNF has been shown to rapidly increase phosphorylation of thepostsynaptic NMDA receptor subunits 1 and 2B in hippocampal andcortical neurons (Suen et al., 1997; Lin et al., 1998). In fact,activity of AMPA receptors has also been shown to be modulatedby phosphorylation (Barria et al., 1997; Hayashi et al., 1997;Mammen et al., 1997; Carroll et al., 1998; Carvalho et al., 1999),however, a role for BDNF in this process has not yet beendemonstrated.

Our current findings may be of a particular significance in view of recent studies on activity-dependent homeostatic regulationof AMPA receptor-mediated synaptic currents. Turrigiano et al.(1998) have demonstrated a form of synaptic plasticity, termed"synaptic scaling", that changes, in an activity-dependent manner,the strength of synaptic inputs in cortical neuron cultures. Specifically,chronic activity blockade increased, whereas blockade of inhibitorytransmission decreased, the amplitude of miniature EPSCs (Turrigianoet al., 1998). In cortical neurons, synaptic scaling is mediatedthrough the activity-dependent release of BDNF (Rutherford etal., 1998), and BDNF has been shown to have opposite effects onthe amplitude of AMPA currents in two classes of cortical synapses.Specifically, although chronic exposure to BDNF decreases AMPAcurrents in pyramidal cells, it increases them in interneurons(Rutherford et al., 1998). Recently, Liao et al. (1999) demonstratedthat AMPA receptor blockade also increases the number and sizeof AMPA receptor clusters in cultured hippocampal neurons andrapidly induces the appearance of AMPA receptors at "silent" synapses.This result suggests that BDNF inhibition of AMPA responses innewborn nTS neurons could ultimately lead to an increase in functionalexpression of AMPA receptors and an increase in postsynaptic AMPAresponses. Indeed, nTS neurons are functionally immature at birthand undergo marked changes in synaptic contacts (Miller et al.,1983), dendritic growth, and electrophysiological properties (Kaliaet al., 1993; Denavit-Saubié et al., 1994) during the early postnatalperiod. Thus, BDNF may play a developmental role in regulatingexcitability of second-order sensory relay cells in nTS. Thiscould explain why genetic loss of BDNF results in a depressionof motor output from the brainstem respiratory rhythm generator(Balkowiec and Katz, 1998), a network that is driven in part byexcitatory inputs from nTS interneurons (Bianchi et al., 1995).It is also possible that BDNF plays an acute role in synapticsignaling by restricting the total EPSC. In fact, low-frequencystimulation of primary afferent inputs to nTS has been shown toinactivate AMPA receptors on second-order relay neurons and depresssynaptic strength by a highly robust, Ca²⁺-independent mechanism (Zhou et al., 1997). Based on our findings,we think it plausible that BDNF, released from primary afferentterminals, could mediate this kind of synaptic modulation. Restrictionof total excitatory current might also protect nTS neurons againstmassive activation of glutamate receptors at high rates of stimulationand potential excitotoxicity (Choi, 1992). BDNF has, for example,been shown to protect cerebellar granule (Lindholm et al., 1993)and cortical (Shimohama et al., 1993) neurons against glutamate-inducedneurotoxicity. In distinguishing among these possibilities, itwill be important to determine the conditions under which BDNFis released from primary afferent terminals in nTS and whetherprimary afferents are the only source of BDNF inputs to second-orderrelaycells.

In summary, our findings demonstrate a novel function for BDNF in acute modulation of AMPA responses in developing sensoryrelay neurons. These data, combined with the fact that many primaryafferents express BDNF, indicate that BDNF could play an importantrole in regulating excitatory transmission at primary afferentsynapses.

  FOOTNOTES

Received Oct. 14, 1999; revised Dec. 6, 1999; accepted Dec. 17, 1999.

This work was supported by Public Health Service grants (National Heart, Lung, and Blood Institute) to D.M.K. and D.L.K. Wegratefully acknowledge the helpful comments of Drs. Stephen Jonesand BenStrowbridge.
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.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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