Long-Term Enhancement of Central Synaptic Transmission by Chronic Brain-Derived Neurotrophic Factor Treatment

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The Journal of Neuroscience, August 15, 1999, 19(16):7025-7036

Long-Term Enhancement of Central Synaptic Transmission by Chronic Brain-Derived Neurotrophic Factor Treatment
Nina Tang Sherwood and Donald C. Lo
Department of Neurobiology, Duke University Medical Center, Durham, North Carolina 27710

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Acute effects of neurotrophins on synaptic plasticity have recently received much attention, but the roles of these factorsin regulating long-lasting changes in synaptic function remainunclear. To address this issue we studied the long-term (daysto weeks) and short-term (minutes to hours) effects of brain-derivedneurotrophic factor (BDNF) on excitatory synaptic transmissionin autaptic cultures of hippocampal CA1 neurons. We found thatBDNF induced long-term enhancement of the strength of non-NMDAreceptor-mediated glutamatergic transmission. This upregulationof EPSC amplitude occurred via an increase in the size of unitarysynaptic currents, with no significant contribution from otheraspects of neuronal electrical and synaptic function includingcell size, voltage-gated sodium and potassium current levels,the number and size of synaptic contacts, and the frequency ofspontaneous neurotransmitter release. Chronic BDNF treatment alsodecreased the degree of synaptic depression measured in responseto paired stimuli. Thus, BDNF induced long-term synaptic enhancementof both basal and use-dependent synaptic transmission via specificchanges to the synapse rather than through generalized potentiationof neuronal growth and differentiation. Finally, we showed thatthe long-term effects of BDNF are functionally and mechanisticallydistinct from its acute effects on synaptic transmission, suggestingthat, in vivo, BDNF activation of Trk receptors can have differentfunctional effects depending on the time course of itsaction.

Key words: neurotrophins; BDNF; Trk receptors; TrkB; hippocampal neurons; synaptic plasticity; excitatory synaptic transmission; autapses; microcultures

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In contrast to the many known extracellular signaling molecules that are involved in short-term neuromodulation on the timescale of seconds to hours [e.g., purines and neuropeptides (forreview, see Kaczmarek and Levitan, 1987; Nicoll et al., 1990)],little is known about signaling molecules that modulate longer-lastingforms of plasticity that, once induced, persist for days, weeks,or more. In recent years the neurotrophins have been associatedwith the regulation of neuronal activity on an acute time scalein vitro (Kim et al., 1994; Lessmann et al., 1994; Kang and Schuman,1995; Levine et al., 1995; Figurov et al., 1996; Patterson etal., 1996; Gottschalk et al., 1998; Lessmann and Heumann, 1998;Li et al., 1998). However, increasing evidence indicates thatneurotrophins also regulate synaptic plasticity in the long term,particularly in areas of the nervous system such as hippocampusand neocortex that exhibit robust activity-dependent neuronalplasticity (for review, see McAllister et al., 1998).

Compelling in vivo evidence of a long-term role for neurotrophins in modulating synaptic plasticity is suggested by experimentsdemonstrating involvement of TrkB ligands in establishing properconnectivity between neurons of the lateral geniculate nucleiand layer IV of the visual cortex (Cabelli et al., 1995, 1997).This activity-dependent refinement of connections occurs overa developmental period of days to weeks. Consistent with thistime frame, in vivo and in vitro experiments indicate that activitycan regulate neurotrophin expression with relatively slow kinetics.In response to physiological levels of stimuli such as LTP induction(Patterson et al., 1992; Castren et al., 1993; Bramham et al.,1996), brain-derived neurotrophic factor (BDNF) mRNA levels donot increase for at least 2 h, but then can remain enhanced for24 hr or more. Even in cases of extreme activity such as limbicseizures, BDNF mRNA levels do not peak until 6-12 hr after seizurein the hippocampus and neocortex (Isackson et al., 1991). Changesat the protein level are slower still; hippocampal BDNF proteinlevels peak at 16 hr after seizure activity and are maintainedfor several days (Nawa et al., 1995).

Neurotrophin action in target neurons, mediated in part through the Trk family of tyrosine kinase receptors, also occurs ona relatively slow time scale. Although Trk activation can inducerapid post-translational modification of neuronal proteins (Jovanovicet al., 1996; Suen et al., 1997), additional signal transductionpathways lead to the regulation of gene expression over a periodof hours to days (Halegoua et al., 1991; Lewin and Barde, 1996;Segal and Greenberg, 1996). The slow time course of these latteractions suggests that long-term effects of neurotrophins on synaptictransmission, even if initiated rapidly, may require prolongedinduction periods for their full manifestation. Regulation atthe level of gene expression also suggests that many effects ofneurotrophins will persist beyond the initial period of Trk receptoractivation. Thus, it is probable that neurotrophin regulationof neuronal function, like its promotion of neuronal survivaland differentiation (Davies, 1994), includes important componentsthat occur over the time scale of days ormore.

Studies in several systems have suggested that long-term treatment with neurotrophins can alter synaptic transmission indirectly,by regulating neuronal morphology or excitability (Dichter etal., 1977; Mandel et al., 1988; Purves et al., 1988; McAllisteret al., 1995; Causing et al., 1997; Gonzalez and Collins, 1997;Lesser et al., 1997), or directly, by modulating unitary synapticproperties (Wang et al., 1995; Liou et al., 1997; Wang and Poo,1997; Rutherford et al., 1998). Here, we have addressed the long-termversus short-term neurotrophin effects on synaptic transmissionin excitatory central neurons from the hippocampal CA1 regionand compared the cellular mechanisms underlying these effects.Using isolated autaptic neurons, we examined glutamatergic synaptictransmission after chronic (>1 week) or acute (<2.5 hr) treatmentwith BDNF, focusing in particular on non-NMDA-type glutamate receptorcurrents, which initiate postsynaptic depolarization in theseneurons. We found that chronic BDNF treatment increased basalevoked current amplitudes by 70%. This regulation occurred viaspecific and selective enhancement of unitary synaptic strength,rather than as a consequence of generalized cell growth, synaptogenesis,or changes in neuronal excitability. Neurons treated chronicallywith BDNF also showed reduced synaptic depression during repetitivefiring. In comparison, the rapid effects of BDNF were very different,both mechanistically and functionally, from its long-term effectson synaptictransmission.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiology. Neurons growing in isolation formed electrophysiologically detectable "autaptic" synaptic connections ontothemselves by 7 d after plating and were used in whole-cell patch-clampexperiments up to 16 d after plating. Cultures of matched ageswere used for short-term and long-term experiments, averaging9-10 d in vitro at the time of recording. Short-term experimentswere performed by two independent methods: either by using singleexcitatory neurons sequentially recorded in the untreated and+BDNF conditions or by comparing the synaptic properties of controlpopulations with those treated briefly with BDNF (10-150 min).Recordings for long-term experiments were performed on parallelpopulations of untreated neurons and neurons treated with BDNFor TrkB-IgG for >6 d. Extracellular solutions contained (in mM):137 NaCl, 5 KCl, 1 MgCl₂, 3 CaCl₂, 10 glucose, 5 HEPES, adjustedto ~350 mOsm, pH 7.3. To ensure that EPSCs consisted only of non-NMDA-typeglutamate receptor currents, APV (100 µM) was added to the extracellularsolution just before recording. Potassium currents were isolatedand recorded using an extracellular solution of 145 mM n-methyl-glucamine,2.8 mM KCl, 2 mM MgCl₂, 10 mM HEPES. Intracellular solutions contained(in mM): either 150 potassium gluconate, 10 NaCl, 10 HEPES, 10EGTA, 3 Mg-ATP, adjusted to pH 7.2 with KOH, or 100 gluconic acid,0.6 EGTA, 5 MgCl₂, 2 Na₂-ATP, 0.3 Na-GTP, 40 HEPES, adjusted topH 7.2 with CsOH. Voltage-clamp recordings were obtained withan Axopatch-1D patch clamp (Axon Instruments, Foster City, CA)and acquired using WinClamp3.7, a Visual Basic program writtenin-house. Borosilicate patch pipettes (VWR, West Chester, PA;Sutter Instrument Co., Novato, CA) were pulled to resistancesof 3-5 M $Omega$ . Leak currents were generally 20-50 pA; recordings withleak currents $>=$ 100 pA or series resistances exceeding 20 M $Omega$ werediscarded. Cell capacitance measurements were made by integrationof capacitive transients. Data were sampled at 100 µsec intervalsfor sodium currents, 200 µsec intervals for synaptic currents,and 500 µsec intervals for potassium currents; recordings werefiltered at 1-5 kHz. Neurons were confirmed to be excitatory bythe reversal of evoked synaptic currents near 0 mV. Cells werevoltage-clamped such that spontaneous action potentials were rarelyobserved when the cell was held at its resting potential (V_hold= $-$ 70 mV); when they did occur, action potential-driven spontaneousevents were preceded by a rapid, high-amplitude spike and wereeasily distinguished from miniature EPSCs (mEPSCs). In all cases,no differences in spontaneous event frequencies were observedafter the addition of TTX (1 µM); thus, the measured spontaneousevents reflected true action potential-independent mEPSCs. mEPSCamplitudes and kinetics were measured via an automatic detectionsoftware program (MiniMAD) written in-house. Detection criteriawere set such that recognized spontaneous events had peak amplitudesat least twofold greater than baseline noise; such events wereconfirmed by the user to have rise times under 5 msec and decaykinetics that were well fitted by single exponential functions.Spontaneous and evoked synaptic current rise times were measuredfrom the start to the peak of the currents; decay time constantswere determined by fitting single exponential functions to thefalling phase of the currents. Quantal content, the number ofunitary release events occurring in response to an action potential(and thus a measure of the number of synapses contributing toan EPSC), was calculated for individual cells as (peak EPSC amplitude)/(meanmEPSC amplitude), where the mean mEPSC amplitude was taken torepresent the average amplitude of a unitary event. Mean valuesare shown ± SE; statistical significance was tested byANOVA.

Cell culture. All long-term experiments were performed in CF-1 murine cultures. Short-term experiments used both Sprague Dawleyrats (single-cell experiments) and mice (single-cell and populationexperiments); no differences in the rapid effects of BDNF wereobserved between the two species. Autaptic cultures (Bekkers andStevens, 1991; Pan et al., 1993) were made using hippocampal neuronsdissected from postnatal day 0 rat pups or embryonic day 17 mice.We used only CA1 neurons to reduce the likelihood of intrinsicdifferences in the responsiveness of different cell types sincelevels of BDNF and TrkB expression (as well as the other neurotrophinsand Trks) are differentially regulated among hippocampal regions(Maisonpierre et al., 1990; Ernfors et al., 1991). Briefly, glasscoverslips or plastic tissue culture dishes (VWR; Corning, CorningNY) were coated with 0.15% agarose, then sprayed with an atomizercontaining poly-D-lysine and collagen (Collaborative Research,Bedford, MA) to yield "microdots" of growth substrate. Cells wereplated at low density to yield single neurons growing on islandsof glia, confined by the agarose to the microdots. Media containedMEM (Life Technologies, Gaithersburg, MD) with 5% non-heat-inactivatedFBS (Hyclone, Logan, UT), 20 mM glucose, 1% Mito-Serum Extender(Collaborative Research), and 1% sodium pyruvate (Life Technologies).For chronic treatment experiments, BDNF or TrkB-IgG (generousgifts of Regeneron Pharmaceuticals, Tarrytown, NY) was added tocultures the day after plating at 100 ng/ml or 10 µg/ml, respectively.Cultures were maintained in 5% CO₂ and fed BDNF or TrkB-IgG every3-4 d. Proliferation of non-neuronal cells was controlled by theaddition of mitotic inhibitors (5-fluoro-2-deoxyuridine and uridine)to themedia.

Immunocytochemistry and quantification of fluorescent staining. Autaptic cultures were fixed at 7-9 d in vitro in 4% paraformaldehydeand 5% sucrose for 10 min, then incubated at 4°C overnight witha polyclonal antibody directed against synapsin Ia,b (1:500; generousgift of P. De Camilli, Yale University, New Haven, CT) and a monoclonalantibody directed against glutamic acid decarboxylase (GAD) (1:750;Boehringer Mannheim, Indianapolis, IN). Primary antibodies werevisualized using Texas Red-conjugated goat anti-rabbit IgG (Vector,Burlingame, CA; Molecular Probes, Eugene, OR) and fluorescein-or Oregon Green-conjugated goat anti-mouse IgG (Molecular Probes),each incubated at 1:750 for 1 hr. Immunostained neurons were imagedfor uniform exposure times using a 25×, 0.8 NA oil immersion objectivewith a 12-bit cooled CCD camera (Princeton Instruments, Trenton,NJ) and were analyzed with IPLabs software (Signal Analytics,Vienna, VA; courtesy of D. Chikaraishi, Duke University). Analysisof anti-synapsin staining was performed by imaging GAD-negativeautaptic neurons on islands not significantly larger than thevisual field, manually tracing individual fluorescently stainedanti-synapsin punctae that occurred along neuronal processes foreach imaged neuron, and then quantifying number and area of punctaeusing IPLabs software. The resolution of the imaging system wassuch that one image pixel represented 0.06 µm².

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Because of the complexity of neural circuits even in conventional dissociated cultures, we studied BDNF regulation of synaptictransmission in microdot cultures of rodent CA1 hippocampal neurons(Furshpan et al., 1976; Segal and Furshpan, 1990; Bekkers andStevens, 1991; Pan et al., 1993). Neurons in this system are confinedto grow in isolation and form synapses only on themselves (autapses).Autaptic synaptic transmission is functionally indistinguishablefrom that found in conventional dissociated culture (Bekkers andStevens, 1991), and the simplicity of these cultures has beencritical for the investigation of several fundamental propertiesof synaptic transmission (Landis, 1976; Furshpan et al., 1986;Pan et al., 1993; Mennerick and Zorumski, 1995a, 1996; Mennericket al., 1995; Stevens and Tsujimoto, 1995; Tong et al., 1996;Kimura et al., 1997). We identified excitatory autaptic neuronsby the reversal of their postsynaptic currents at ~0 mV in electrophysiologyexperiments or by the absence of GAD immunoreactivity in morphologicalexperiments. In combination with whole-cell patch-clamping, immunocytochemistry,and image analysis, this system enabled clear determination ofBDNF-induced changes in excitability, morphology, synaptic transmission,and short-term synaptic plasticity at the level of individualexcitatory neurons andsynapses.

Chronic enhancement of basal synaptic transmission by BDNF

We studied the long-term actions of BDNF by measuring non-NMDA receptor-mediated EPSCs (Fig. 1A) elicited in autaptic neuronsgrown under each of three experimental conditions for 6-15 d:untreated, +TrkB-IgG to block potential activity of endogenousBDNF (10 µg/ml) (Shelton et al., 1995; Binder et al., 1999), or+BDNF (100 ng/ml). Consistent with other neurotrophin studiesin hippocampal systems, neither addition of BDNF nor of TrkB-IgGaffected neuronal survival (Ip et al., 1993; Ohsawa et al., 1993;M. Bolton and D. Lo, unpublished observations). The number ofsurviving neurons after 1 week of BDNF or TrkB-IgG treatment,normalized to survival in untreated plates, was 1.06 ± 0.07 and1.25 ± 0.28, respectively (mean ± SE; p > 0.38 and 0.42 by ANOVA;n = 3 separate experiments). Because TrkB-IgG-treated neuronsdid not differ from untreated neurons in any parameter measured,these treatment groups were combined ("control") (Table 1).

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Figure 1. Chronic BDNF treatment increased the amplitude of evoked non-NMDA-type postsynaptic currents. A, Top, EPSCs were elicited by depolarizing CA1 autaptic neurons from a prepulse potential of $-$ 120 mV to +10 mV for 1.6 msec and returning to $-$ 70 mV, causing a rapid inward sodium spike (arrow) and subsequent EPSC (arrowhead). Recorded EPSCs could be completely blocked by NBQX, leaving only a residual Na⁺ current (center). The NBQX-sensitive component of such traces (bottom; difference of top and center traces) defined non-NMDA-type glutamate receptor-mediated synaptic currents that reversed at or near 0 mV. B, C, Chronic BDNF treatment (100 ng/ml; n = 61) increased average EPSC peak amplitude by 1.7 ± 0.1-fold (mean ± SE) compared with those recorded from controls (i.e., untreated or 10 µg/ml TrkB-IgG-treated neurons; n = 109; p < 8.8 × 10⁸ by ANOVA; statistically significant difference denoted by the asterisk). Representative EPSCs are shown in B. Mean EPSC amplitudes (C) ranged from ~1 to 4 nA and were normalized to controls within each experiment to compare results from different platings.


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Table 1. TrkB-IgG had no effect on CA1 excitatory neurons

In contrast, neurons grown in the continuous presence of BDNF showed basal excitatory postsynaptic responses that were onaverage 1.7-fold greater than controls (Fig. 1B,C) (p < 8.8 ×10⁸; combination of five separate experiments). These potentiatingeffects of BDNF were maintained for at least several hours inthe absence of added BDNF or TrkB-IgG in the recording salines.The possible cellular mechanisms underlying this potentiationfall into one or more of the following categories: (1) changesin neuronal excitability; (2) an increase in synaptogenesis; and(3) changes in the function of individual synapses. We thus experimentallyexamined each of these areas inturn.

Intrinsic excitability
Several observations suggested that changes in passive membrane properties and action potential propagation were not significantfactors in the synaptic potentiation induced by BDNF. First, therise times for both evoked and spontaneous synaptic currents wereunchanged by BDNF treatment, indicating an absence of significantchanges in passive membrane properties (Table 2). Second, cellmembrane area, as measured by electrical capacitance, was notaffected by BDNF (Fig. 2A) (p > 0.15).


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Table 2. BDNF had no effect on the rise or decay times of synaptic currents

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Figure 2. BDNF did not appreciably affect neuronal size or membrane excitability. A, BDNF did not affect cell size. Cell capacitance was used to measure total membrane area, which did not differ between neurons grown in the presence or absence of added BDNF (p > 0.15). Average capacitances ranged from 40 to 60 pF (Control, n = 85; +BDNF, n = 41). B, BDNF did not affect potassium currents. Voltage-gated potassium currents were elicited by depolarizing neurons from a 20 msec prepulse of $-$ 120 mV to between $-$ 40 and +40 mV in 20 mV increments for 200 msec; representative traces are shown for control and BDNF-treated cells. Currents at +40 mV were measured at peak and at steady state to reflect the contributions of transient and sustained potassium current components. No differences were observed between untreated controls and neurons grown in BDNF for either of these measurements. Average potassium currents were ~2 nA. Control, n = 10; +BDNF, n = 9. p > 0.35 for both peak and steady-state current comparisons. C, BDNF did not alter sodium currents. Whole-cell sodium currents were recorded by depolarizing neurons to $-$ 10 mV from a brief hyperpolarizing pulse of $-$ 120 mV; representative traces are shown. Sodium currents activated and inactivated within 5 msec after the start of the depolarizing pulse. Average peak sodium currents were equivalent in BDNF-treated neurons and controls (n = 41 and 60, respectively; p > 0.09) and ranged from 4 to 8 nA.

We also measured functional levels of whole-cell voltage-gated potassium and sodium currents. Neither peak nor steady-statepotassium current component amplitudes were affected by BDNF (Fig.2B) (p > 0.35). Similarly, BDNF treatment did not alter the amplitudesor kinetics of voltage-gated sodium currents measured concurrentlywith evoked synaptic currents (Fig. 2C) (p > 0.09). Thus, neitherchanges in the passive nor the active electrical characteristicsof neuronal membranes appeared to be the mechanisms by which EPSCamplitudes wereincreased.

Synaptogenesis
We next examined whether BDNF could, on this time scale, be acting simply as a "growth factor" for synaptogenesis. We addressedthis directly by quantifying the number and size of synapses inBDNF-treated and control cultures. Synapses were visualized byimmunostaining cultures with a polyclonal antibody directed againstsynapsin Ia and Ib (gift of Dr. P. De Camilli) (Fig. 3A). Localizedin mature presynaptic terminals, these proteins are importantin synaptogenesis and the regulation of neurotransmitter release(Greengard et al., 1993). Quantitation of anti-synapsin immunostainingin isolated glutamatergic neurons showed that BDNF affected neitherthe number of synapses per neuron (Fig. 3B) (p > 0.16) nor theiraverage size (Fig. 3C) (p > 0.56). This provided direct evidencethat BDNF did not alter the rate of synaptogenesis in these culturesand thus that the increase in evoked current amplitude was notcaused by differences in synapse number or size.

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Figure 3. Synaptogenesis was not affected by chronic BDNF treatment. A, Fluorescence image of an autaptic neuron labeled with an antibody directed against synapsin Ia,b and visualized using a Texas Red-conjugated secondary antibody. Each bright puncta represents a presynaptic specialization. Scale bar, 20 µm. B, The number of synapses per neuron did not differ between treatment groups. Average numbers of synapses per cell were (mean ± SE) 506 ± 58 in controls and 594 ± 74 in BDNF-treated neurons (n = 13 and 7, respectively; p > 0.37). C, The average size of synapses was unaffected by BDNF. Mean synapse size, with each synapse defined as the pixel area of an isolated puncta, was 0.35 ± 0.01 and 0.37 ± 0.04 µm² per synapse for control (n = 13) and +BDNF (n = 7) cells, respectively; p > 0.56.

Synaptic function
Because the preceding experiments suggested that the principal regulatory effects of BDNF were not on neuronal excitability,cell growth, or synaptogenesis, we examined the remaining possibilitythat BDNF modified the unitary properties of synaptic transmission.Because mEPSCs occur independently of action potentials, we coulddirectly examine changes localized at synapses by measuring theamplitudes and kinetics of these spontaneousevents.
Autaptic neurons are unique in that mEPSCs and EPSCs arise from the same neuron and thus the same set of synapses. Becauseonly one set of synapses is involved, direct correspondences canbe drawn between the properties of evoked versus miniature synapticcurrents. To address most rigorously the possibility that changesin unitary synaptic properties underlie the BDNF-induced increasein EPSC amplitude, we first focused on the set of experimentsthat had the greatest number of mEPSC and EPSC recordings fromthe same cells. In these experiments, evoked postsynaptic currentamplitudes increased on average by 1.8-fold in BDNF-treated culturesrelative to controls (Fig. 4A,B) (p < 0.02). Strikingly, the amplitudeof spontaneous events in BDNF-treated neurons increased proportionallywith the increase in evoked current amplitudes, by 1.8-fold relativeto control neurons (Fig. 4A,B) (p < 0.03). No differences in riseor decay kinetics were observed for EPSCs or mEPSCs recorded fromcontrol versus BDNF-treated neurons (Fig. 4A, Table 2), nor didBDNF affect the frequency of mEPSCs (Fig. 4C) (p > 0.25).

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Figure 4. BDNF increased EPSC and mEPSC amplitudes proportionally but did not affect mEPSC frequency. A, EPSC (left) and mEPSC (right) traces were averaged for control (dashed traces) and +BDNF-treated (solid traces) cells and superimposed. BDNF increased EPSCs and mEPSCs to similar extents. Scaling the averaged control traces to their respective +BDNF traces (dotted lines) showed that the kinetics of activation and decay were indistinguishable between treatment groups for both evoked and spontaneous responses. B, EPSC amplitudes (shaded bars) were 1.8 ± 0.03-fold greater in BDNF-treated cells compared with controls (p < 0.02; +BDNF, n = 13; Control, n = 16). BDNF increased the amplitudes of mEPSCs to the same extent (1.8 ± 0.02-fold; p < 0.03; +BDNF, n = 10; Control, n = 12). Mean EPSC amplitudes were 3.6 and 2.0 nA for +BDNF and control cells, respectively, whereas mEPSC amplitudes averaged 34.2 and 18.6 pA. Values normalized to control cells are shown; asterisks denote statistical significance. C, In contrast, BDNF did not affect the average frequency of mEPSCs (+BDNF, n = 10; Control, n = 12; p > 0.25). mEPSCs were measured from 51.2 sec of continuous recording while cells were held at $-$ 70 mV.

These data suggested that at the level of individual neurons, increases in evoked EPSC amplitude induced by BDNF were quantitativelyaccounted for by a parallel increase in mEPSC size. We furthertested this idea by comparing EPSC amplitudes versus mEPSC amplitudesfor a larger population of neurons, combining multiple experimentaltrials. Even across different experiments, EPSC and mEPSC amplitudeswere strongly correlated and covaried (Fig. 5) (r = 0.57, p <0.0001). In contrast, a plot of EPSC amplitudes versus mEPSC frequenciesfor individual cells showed no correlation (Fig. 5) (r = 0.01,p > 0.9).

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Figure 5. mEPSC amplitude, but not frequency, covaried with EPSC amplitude in populations of BDNF-treated and control neurons. Top, Amplitudes of spontaneous and evoked postsynaptic currents covaried with a correlation coefficient of r = 0.57 (p < 1 × 10⁴); best linear least-squares fit is shown (solid line). Each point represents recordings from a single neuron; mEPSC amplitudes are the mean ± SE of all events occurring within the 51.2 sec recording period. Two sources of variation in these data points were evident. (1) Limitations in the signal-to-noise of some recordings reduced the detectability of mEPSCs smaller than ~3 pA, leading to an overestimation of average mEPSC amplitudes in these neurons. Hence, there is more scatter above the linear fit than below it. (2) Although BDNF never altered the quantal content of neurons within a given cell culture plating, there was some variation in overall quantal content from plating to plating (122-225). Thus, the slope of the linear fit here reflects the weighted average of the quantal contents of all neurons in all platings (178). It is noteworthy that the strong correlation between mEPSCs and EPSC amplitudes remained clear despite these significant sources of experimental variation. Bottom, In contrast, a plot of mEPSC frequency versus EPSC amplitude for individual cells revealed no correlation: r = 0.01, p > 0.9. n = 36 and 30 for control ( $open circle$ ) and BDNF-treated () cells, respectively.

The above findings thus indicated that the BDNF-induced increase in EPSC amplitudes arose from a proportional increase inaverage mEPSC amplitude. Furthermore, if a change in mEPSC amplitudecompletely accounted for the change in EPSC amplitude, these resultspredicted that quantal content, the average number of quanta contributingto an EPSC [= (EPSC amplitude)/(mEPSC amplitude); see Materialsand Methods], should be unaffected by BDNF treatment. In factthis was observed: 211 ± 36 and 225 ± 43 quanta were releasedper EPSC (control vs BDNF-treated neurons, n = 12 and 9, respectively;p > 0.8). Thus, chronic BDNF treatment increased basal evokedsynaptic current amplitudes via regulation of the amplitudes ofunitary synaptic currents and not by increasing the probabilityof neurotransmitterrelease.

Chronic BDNF enhances use-dependent synaptic transmission

In the above experiments, synaptic currents were elicited at very low frequencies ( $<=$ 0.05 Hz). However, neurons in vivo normallyrespond to repetitive stimuli at substantially higher frequencies.To determine whether BDNF also regulated the efficacy of synaptictransmission in response to higher frequency stimuli, we examineda simple form of use-dependent synaptic plasticity in these cells,synaptic depression, using a paired-pulse depression (PPD) paradigm(Zucker, 1989).

Pairs of evoked currents were elicited 1 sec apart, and the resultant degree of synaptic depression was determined by measuringthe amplitude of the second EPSC relative to the first. Autapticneurons treated chronically (>1 week) with BDNF were much lessdepressed by successive firing than were controls. While EPSCselicited by the second stimulus were 36% smaller than the initialEPSC in control cells (i.e., 36% PPD), BDNF-treated neurons showedonly 8% PPD (p < 0.005) (Fig. 6A,B). Chronic treatment with BDNFthus significantly enhanced synaptic efficacy in response to repetitivestimuli as evidenced by a four- to fivefold reduction in PPD ata 1 sec interpulse interval.

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Figure 6. Chronic BDNF treatment attenuated paired-pulse depression. A, Sample traces of EPSCs recorded using a paired-pulse depression (PPD) paradigm for cells grown in the presence or absence of exogenous BDNF. The dotted traces (arrowhead) show the first evoked postsynaptic current. Solid traces show the second EPSC (arrow) evoked 1 sec later. In the BDNF-treated neuron the two traces are nearly overlapping, indicating that little PPD occurred. In contrast, in the control neuron the second EPSC was substantially depressed relative to the first. B, On average, control neurons showed 36 ± 5% PPD at an interpulse interval of 1 sec (n = 13). In contrast, BDNF-treated cells showed only 8 ± 8% PPD (n = 12; p < 0.005; statistical significance denoted by asterisk). C, The rate of recovery from PPD was not affected by BDNF. PPD was measured for a range of interpulse intervals ranging from 1 to 12.5 sec. The plot of PPD versus interpulse interval shows that control neurons were more depressed than BDNF-treated neurons at all intervals. The time courses of recovery from PPD, however, were fitted well by single exponential functions with similar time constants (Control, 6.3 ± 1.1 sec, n = 12; +BDNF, 5.8 ± 1.1 sec, n = 8; fits constrained to be asymptotic to zero).

In several systems, including hippocampal autapses, PPD has been attributed to the depletion of the readily releasable poolof synaptic vesicles (Mennerick and Zorumski, 1995a; Dobrunz andStevens, 1997). Thus, one simple mechanism by which the observeddecrease in PPD could have occurred is via an increase in therate at which this pool is replenished. We examined the possibilitythat BDNF increased the refilling rate of the readily releasablepool in the range of stimulation frequencies that cause PPD (1-12.5sec) (Fig. 6C). We found that recovery rates from PPD did notdiffer between BDNF-treated and BDNF-deprived neurons at any ofthese stimulus intervals ( $tau$ _BDNF = 5.8 ± 1.1 sec; $tau$ _control = 6.3± 1.1 sec). This suggested that although BDNF attenuated synapticdepression by several-fold, this effect did not occur via alterationsin the rate at which synapses recover fromPPD.

Acute effects of BDNF on synaptic transmission

Recent work from several laboratories has provided evidence for rapid effects of BDNF on non-NMDA receptor-mediated glutamatergictransmission in hippocampal neurons (Kim et al., 1994; Lessmannet al., 1994; Kang and Schuman, 1995, 1996; Levine et al., 1995;Figurov et al., 1996; Patterson et al., 1996; Tanaka et al., 1997;Gottschalk et al., 1998; Lessmann and Heumann, 1998; Li et al.,1998). We were interested in whether the chronic effects on synaptictransmission described above $---$ -increased amplitudes of both evokedand spontaneous EPSCs $---$ -were related to potential effects of briefBDNF exposure on synaptic transmission, or whether BDNF regulatessynaptic function in distinct ways over acute versus prolongedtimescales.

We examined the acute effects of BDNF on basal synaptic transmission using two independent methods. First, non-NMDA receptor-mediatedEPSC and mEPSC amplitudes were measured in continuous recordingsfrom single neurons before and after bath application of BDNF.In contrast to the effects of chronic BDNF treatment describedabove, no appreciable change in the amplitude of EPSCs was detectedfor the duration of these recordings, which lasted from 40 minto >2 hr (Figs. 7, 8A, bottom). This is consistent with resultsobserved in hippocampal slices (Figurov et al., 1996; Korte etal., 1996; Patterson et al., 1996; Tanaka et al., 1997; Frerkinget al., 1998; Gottschalk et al., 1998; but see also Kang and Schuman,1995, 1996). The amplitudes of mEPSCs were also unaffected byBDNF addition for at least 1.5 hr after BDNF addition (Figs. 7,8A, center). However, the frequency of spontaneous events increasedsignificantly within 10 min after the addition of BDNF, by 2.5-foldon average (Figs. 7, 8A, top), similar to other findings in conventionaldissociated hippocampal cultures (Lessmann et al., 1994; Lessmannand Heumann, 1998; Li et al., 1998). These events were insensitiveto TTX, indicating that BDNF increased the frequency of true "minis"(Fig. 7).

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Figure 7. Acute application of BDNF increased only the frequency of mEPSCs. In this example, synaptic currents from a single autaptic neuron were first recorded in the absence of BDNF to establish baseline synaptic transmission properties (mEPSC frequency, mEPSC amplitude, and EPSC amplitude). Each mEPSC point represents 25.6 sec of recording. BDNF was then added to the bath (100 ng/ml at t = 57 min), and these synaptic properties were monitored for 35 min. Finally, TTX was added at t = 92 min to confirm that the mEPSCs measured were true action potential-independent minis. Top, The frequency of mEPSCs increased 5.2-fold (p < 2 × 10⁹) in response to BDNF addition. This effect was seen within minutes and was not affected by the subsequent addition of TTX (p > 0.1, comparing average post-BDNF frequencies measured before and after TTX). Center, No differences were observed in average mEPSC amplitudes (±SE) throughout the recording; p > 0.9 for mEPSC amplitudes measured before and after BDNF addition. Blank periods in this and the graph above are due to EPSCs being recorded during these intervals. Bottom, Similarly, EPSCs were unaffected by the addition of BDNF (p > 0.8, comparing pre-BDNF and post-BDNF measurements). Note that the last two EPSC amplitudes are zero, confirming that sodium channels were blocked by TTX, eliminating all action potentials and EPSCs.

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Figure 8. Acute application of BDNF increased mEPSC frequency but not mEPSC or EPSC amplitudes. A, Summary of single-cell neuron recordings. Each symbol represents an individual neuron recorded continuously, first in control salines and then for up to 80 min after the addition of BDNF. Values are normalized to the control (pre-BDNF) measurement for each neuron. Top, mEPSC frequency increased significantly by 10 min after the addition of BDNF, by an average of 2.5-fold (n = 6; p < 0.006). This increase was insensitive to TTX, indicating that BDNF increased the frequency of true minis (Fig. 7 and data not shown). Center, mEPSC amplitudes were unchanged by BDNF addition (n = 6). Bottom, EPSC amplitudes were also unaffected by short-term BDNF treatment (n = 7). B, Summary of data taken from populations of neurons untreated or treated with BDNF for <2.5 hr. Top, As in the single cell experiments, BDNF increased mEPSC frequency by 2.5-fold (Control, 0.88 ± 0.14 sec¹, n = 24; +BDNF, 2.23 ± 0.39 sec¹, n = 18; p < 0.001; significance denoted by asterisk). Center, mEPSC amplitudes were indistinguishable between control and BDNF-treated cells (Control, n = 26; +BDNF, n = 19; p > 0.1). Bottom, Similarly, evoked postsynaptic currents did not differ significantly in amplitude between control and BDNF-treated neurons (Control, n = 27; +BDNF, n = 22; p > 0.17).

Because of the difficulty in recording stable currents from autaptic neurons for prolonged periods of time, we confirmed theseresults in a larger number of neurons by recording from neuronalpopulations that were either untreated or treated briefly withBDNF (<2.5 hr, with BDNF present throughout the recording period).The results of these experiments were identical to those observedin the continuous recordings: neither EPSC nor mEPSC amplitudeswere affected by brief BDNF treatment (Fig. 8B, bottom and center)(EPSC, p > 0.17; mEPSC, p > 0.10), but the average frequency ofmEPSCs increased by 2.5-fold (Fig. 8B, top) (p < 0.001).

Finally, we asked whether BDNF had rapid effects on short-term synaptic depression by measuring PPD. We found that untreatedneurons and neurons treated briefly (<1 hr) with BDNF were equivalentlydepressed at a 1 sec interpulse interval, by 28 ± 2% and 32 ±5% (control and BDNF-treated, respectively; p > 0.37). Thus, ona rapid time scale, BDNF had no effect on the use dependence ofevoked synaptic transmission as assessed by PPD. Rather, the predominanteffect of BDNF treatment on the time scale of minutes to hourswas an increase in the frequency of mEPSCs. All of the effectsof brief BDNF treatment were thus distinct from its long-termactions: the selective increase in the size but not the frequencyof mEPSCs and the enhancement of both basal and use-dependentevoked synaptictransmission.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although much evidence has accumulated in recent years of a role for neurotrophins in the rapid modulation of neuronal activity,the slow time courses of neurotrophin regulation and action, aswell as the known long-term effects of neurotrophins on neuronalmorphology and excitability, suggest that these growth factorsalso regulate neuronal activity on longer time scales. We addressedthis issue directly by using isolated excitatory hippocampal neuronsto investigate the long- versus short-term effects of BDNF oncentral excitatory synaptictransmission.

We found that chronic treatment (1-2 weeks) of autaptic CA1 neurons with BDNF led to a 70% enhancement of action potential-evokedsynaptic currents mediated through non-NMDA-type glutamate receptors.This effect was unlikely to be caused by selection for a populationof neurons with larger EPSCs, because no effects of BDNF or TrkB-IgGwere observed on neuronal survival. Long-term treatment of autapticneurons with BDNF also regulated a form of use-dependent, transientsynaptic plasticity, paired-pulse depression. BDNF-treated neuronsshowed substantially less PPD than controls in that successivefiring only marginally depressed EPSC amplitudes in these neurons.Notably, these long-term effects of BDNF were directly on synapticfunction, rather than occurring as a secondary consequence ofenhanced synaptogenesis or neuronal excitability. Our resultsare particularly interesting in light of observations in hippocampalneurons of mice chronically deficient in BDNF [BDNF heterozygousand homozygous knockouts (Patterson et al., 1996)]. These animalsshow a gene dosage-dependent reduction in levels of basal synaptictransmission, which can be partially rescued only after at least12 hr of BDNFincubation.

In contrast to the long-term effects of BDNF, brief BDNF application (<2.5 hr) affected neither the amplitude nor the extentof paired-pulse depression of evoked EPSCs. Rather, BDNF acutelyregulated the frequency of mEPSCs, a target that was not affectedin long-term studies. Thus, although BDNF directly regulated synapticfunction in both the short term and long term, it did so on thesetwo time scales in distinct ways, via distinct cellular mechanisms.The clear differences between these rapid versus long-term effectsof BDNF suggest that, in vivo, BDNF can have very different consequenceson synaptic transmission and plasticity depending on the timecourse of BDNF availability andaction.

Cellular mechanisms of chronic BDNF regulation

Of the three cellular mechanisms by which BDNF could have increased EPSC amplitudes $---$ regulation of membrane excitability, synapsenumber, or synapse strength $---$ only one mechanism was observed inCA1 neurons: an increase in synaptic strength. BDNF's long-termeffects on basal evoked synaptic transmission were caused by theupregulation of quantal size, as evidenced by the proportionalincrease in mEPSC amplitudes that quantitatively accounted forthe change in EPSCamplitude.

Because mEPSCs increased in amplitude but not frequency, our evidence was most consistent with a postsynaptic locus of regulationby BDNF. Changes in mEPSC amplitude typically arise from postsynapticmodifications (Korn and Faber, 1991; Bekkers and Stevens, 1995);for example, changes in the number, localization, or phosphorylationstate of AMPA-type glutamate receptors could increase quantalamplitudes without affecting kinetics (Craig et al., 1993; Smart,1997). Changes indicative of a presynaptic site of modulationwere notably absent; namely, BDNF did not increase the probabilityof neurotransmitter release because no differences were observedeither in the frequency of mEPSCs or in quantal content. However,it is also possible that the amount of neurotransmitter packagedper quantum was the target of BDNF regulation, as has been observedfor the regulation of midbrain dopamine neurons by GDNF (Pothoset al., 1998). Such a scenario would require that postsynapticglutamate receptors are not saturated by basal levels of neurotransmitterrelease per quantum (Bekkers and Stevens, 1990; Liu and Tsien,1995) (but see Clements et al., 1992; Tong and Jahr, 1994; Fortiet al., 1997).

Interestingly, Rutherford et al. (1998) have reported very different effects of BDNF on quantal size at excitatory synapsesin mixed cultures of visual cortical neurons. In their studies,long-term treatment with BDNF decreased, rather than increased,the amplitude of mEPSCs onto excitatory neurons. Several experimentaldifferences could account for this discrepancy in BDNF's long-termeffects, including brain region and cell type. Indeed, these differencesunderscore the diversity of actions that, depending on the specificcell context of a particular target neuron, may result from activationof a given receptor (Sherwood et al., 1997).

Our observation of a BDNF-mediated reduction in PPD in the absence of a concomitant change in the probability of release (P_r)may seem initially surprising, because it is well known that changingoverall P_r (for instance, by changing the extracellular Ca²⁺ concentration) results directly in a change in PPD. However,the converse of this relationship may not be obligatory. BecausePPD is a function not only of initial P_r (P_r1), but also of P_rduring the second stimulus (P_r2), our observation that PPD wasmodified in the absence of a change in P_r1 suggests that BDNFinduced a change in P_r2 only. The cellular mechanism by whichPPD occurs in most systems, including hippocampal autaptic cultures,is thought to be via depletion of neurotransmitter vesicles availablefor release at individual presynaptic terminals [the readily releasablepool (Zucker, 1989; Mennerick and Zorumski, 1995a; Dobrunz andStevens, 1997)]. Because our experiments ruled out an increasedrefilling rate of this pool, a potential mechanism for the decreasein PPD caused by chronic BDNF treatment is a change in the abilityof vesicles to be released in response to the second stimulus.Such selective changes in "fusion efficiency" (Stevens and Wesseling,1999) could occur, for example, if vesicular release in responseto the second pulse occurs at sites distinct from initial release(Jiang and Abrams, 1998).

Rapid effects of BDNF

The above mechanisms of chronic regulation by BDNF were distinct from its rapid effects: a selective increase in the frequencyof spontaneous events with no change in evoked EPSCs, mEPSC size,or paired-pulse depression. The dissociation between mEPSC frequencyand EPSC amplitude in the rapid action of BDNF is notable becausethese two properties of synaptic transmission are usually linked.However, because "true" mEPSCs are independent of action potentials,it is possible to regulate mEPSC frequency and EPSC amplitudeindependently. In cortical autapses, for example, Kimura et al.(1997) have found that not all synapses that are capable of spontaneousrelease also release neurotransmitter in response to depolarization.Cash et al. (1996) have observed that heterosynaptic depressionof EPSC amplitude in neuromuscular cultures occurs without a correspondingchange in the frequency of spontaneous events. Similarly, Deitcheret al. (1998) and Yoshihara et al. (1999) have reported dissociationof these properties at the Drosophila neuromuscular junction.In their neuronal synaptobrevin (n-syb) mutants, evoked synapticcurrents are eliminated but spontaneous release still occurs ina Ca²⁺-dependent manner, demonstrating that synaptobrevin mechanisticallydistinguishes evoked from spontaneous vesicularrelease.

In contrast to our findings, several recent studies have reported rapid enhancement of EPSC amplitude by BDNF in dissociatedhippocampal neurons (Levine et al., 1995; Lessman and Heumann,1998; Li et al., 1998). Such discrepancies may have arisen, atleast in part, from differences in analysis and in the preparationof hippocampal cultures. For example, the acute effects of BDNFin mixed cultures of whole hippocampi reported in these studiesmay have arisen from subpopulations of neurons not representedin our CA1 autaptic cultures. Furthermore, Lessmann and Heumann(1998) have suggested the intriguing possibility that the responsivenessof neurons to BDNF is dependent on previous levels of activity,a parameter that may have varied considerably among these differentculturesystems.

Rapid versus chronic effects of BDNF

The relationship between the rapid and chronic effects of BDNF that we observed is of interest. One possibility is that thedifferences between acute versus chronic BDNF treatment representfunctionally independent effects, elicited by the same initialsignaling event but manifested along different time courses. Wangand Poo (1997) have suggested, for example, that NT-4/5 has immediatepostsynaptic regulatory actions on Xenopus neuromuscular acetylcholinereceptors but that it also elicits presynaptic effects on neurotransmittersecretion that are longer lasting ( $>=$ 1 hr) and do not requirethe constant presence of the neurotrophin. Similarly, the short-and long-term effects of BDNF may be mechanistically and functionallydistinct in the mammalian central excitatory neurons studiedhere.

Alternatively, the differences we observed between rapid and chronic BDNF treatment may reflect different time points in alinear series of cellular changes initiated by TrkB activation.In developing neurons in culture, spontaneous events can be detectedwell before evoked currents (Basarsky et al., 1994; Gottmann etal., 1994), suggesting that the increases in mEPSC frequency thatwe observed may represent an early, obligatory phase of the later,chronic regulatory effects of BDNF on synaptic transmission. Suchincreases in mEPSC frequency are also characteristic of developingneuromuscular junctions (Hume et al., 1983; Young and Poo, 1983)and, indeed, have been observed shortly after neurotrophin applicationto embryonic neuromuscular cultures (Lohof et al., 1993; Wanget al., 1995; Wang and Poo, 1997). In either case, our resultsindicate that the action of a single signaling molecule such asBDNF can elicit multiple types of synaptic regulation dependingon (1) the temporal characteristics of its availability and (2)the time window in which its synaptic effects areobserved.

Classical studies of long-term nerve growth factor effects in the peripheral nervous system have established the requirementfor this prototypic neurotrophin in promoting the survival andmorphology of specific neuronal cell types (for review, see Purveset al., 1988). More recent studies in visual cortex have providedstrong evidence that neurotrophins play an essential role in theactivity-dependent establishment of synaptic connectivity betweenthe LGN and visual cortex during development (Bonhoeffer, 1996;Cellerino and Maffei, 1996; Riddle et al., 1996). Intriguingly,BDNF has most recently been implicated in the establishment ofL-LTP (Korte et al., 1998), a transcription-dependent form ofsynaptic potentiation that can last for days (Bailey et al., 1996).Our results indicate that neurotrophins such as BDNF can playimportant roles in regulating synaptic function on such prolongedtime scales through the direct modulation of synaptic strengthand reliability. Because the production, release of, and responseto BDNF are intimately tied to levels of neuronal activity (Thoenen,1995; McAllister et al., 1996), findings such as these furtherstrengthen the idea that neurotrophins are key regulators of synapticplasticity in the CNS in the long term as well as the shortterm.

  FOOTNOTES

Received Feb. 26, 1999; revised May 19, 1999; accepted May 24, 1999.

This work was supported by the Bryan Scholars Fund and National Research Service Award Grant 5F31MH11058 (N.T.S.), and theAlfred P. Sloan Foundation, the McKnight Endowment for the Neurosciences,and National Institutes of Health Grant NS32742 (D.C.L.). We alsothank Regeneron Pharmaceuticals for BDNF and TrkB-IgG; P. De Camilliand O. Mundigl for anti-synapsin I; C. Jahr, C. Stevens, J. Wesseling,and C. Boyer for autapse and other advice; D. Chikaraishi forimaging equipment; and T. Blanpied, M. Bolton, T. Yacoubian, andD. Sherwood for stimulatingdiscussions.
Correspondence should be addressed to Dr. Donald C. Lo, Department of Neurobiology, Box 3209, Duke University Medical Center,Durham, NC27710.

Dr. Sherwood's present address: Division of Biology, California Institute of Technology, Pasadena, CA,91125.

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