Abstract
Brain-derived neurotrophic factor (BDNF) has been postulated to be a key signaling molecule in regulating synaptic strength and overall circuit activity. In this context, we have found that BDNF dramatically increases the frequency of spontaneously initiated action potentials in hippocampal neurons in dissociated culture. Using analysis of unitary synaptic transmission and immunocytochemical methods, we determined that chronic treatment with BDNF potentiates both excitatory and inhibitory transmission, but that it does so via different mechanisms. BDNF strengthens excitation primarily by augmenting the amplitude of AMPA receptor-mediated miniature EPSCs (mEPSCs) but enhances inhibition by increasing the frequency of mIPSC and increasing the size of GABAergic synaptic terminals. In contrast to observations in other systems, BDNF-mediated increases in AMPA-receptor mediated mEPSC amplitudes did not require activity, because blocking action potentials with tetrodotoxin for the entire duration of BDNF treatment had no effect on the magnitude of this enhancement. These forms of synaptic regulations appear to be a selective action of BDNF because intrinsic excitability, synapse number, and neuronal survival are not affected in these cultures. Thus, although BDNF induces a net increase in overall circuit activity, this results from potentiation of both excitatory and inhibitory synaptic drive through distinct and selective physiological mechanisms.
- neurotrophins
- BDNF
- hippocampal neurons
- synaptic plasticity
- excitatory synaptic transmission
- inhibitory synaptic transmission
- AMPA receptors
- NMDA receptors
Members of the neurotrophin family of peptide growth factors, particularly brain-derived neurotrophic factor (BDNF), are emerging as important mediators of activity-dependent modifications in synaptic strength. Their biological roles in such processes, however, remain uncertain. Whereas in some situations BDNF has been found to increase synaptic strength, such as at developing neuromuscular synapses and at excitatory synapses onto CA1 hippocampal neurons (Lohof et al., 1993; Vicario-Abejon et al., 1998; Sherwood and Lo, 1999), in cortical cultures, BDNF has been proposed to regulate the strength of all synapses onto a given neuron to maintain homeostasis (Rutherford et al., 1998). Consistent with both of these potential biological roles, the production and release of BDNF is activity-dependent in a variety of neuronal systems (McAllister et al., 1999).
Evidence supporting a role for BDNF in activity-dependent strengthening of specific synapses falls into two categories: acute experiments in which the effects of BDNF manifest within minutes, and chronic experiments in which effects take days to develop. Suppression of BDNF expression by gene deletion or introduction of antisense oligonucleotides results in deficiencies in hippocampal long-term potentiation (LTP), which can be rescued by acute provision of exogenous BDNF (Korte et al., 1995, 1996a,b; Patterson et al., 1996). BDNF has also been reported to enhance basal synaptic transmission at Schaffer collateral–CA1 synapses (Kang and Schuman, 1995a,b) (but see Figurov et al., 1996; Patterson et al., 1996;Frerking et al., 1998; Gottschalk et al., 1998) and to interact with tetanus-induced LTP in this region (Figurov et al., 1996;Gottschalk et al., 1998; Korte et al., 1998). Similar acute potentiative effects have been found in the hippocampal CA3 region and dentate gyrus (Scharfman, 1997, 1999). In neocortex, there is evidence that BDNF potentiates basal synaptic transmission (Akaneya et al., 1996, 1997; Carmignoto et al., 1997) (but see Huber et al., 1998;Kinoshita et al., 1999) and that BDNF increases the probability of inducing LTP rather than long-term depression for a range of stimulus paradigms (Akaneya et al., 1996, 1997; Huber et al., 1998; Kinoshita et al., 1999; Sermasi et al., 1999). Finally, rapid enhancement of excitatory transmission has also been demonstrated in dissociated hippocampal cultures (Lessmann et al., 1994; Levine et al., 1995, 1996,1998; Lessmann and Heumann, 1998; Li et al., 1998; Song et al., 1998) and at developing neuromuscular synapses in culture (Lohof et al., 1993; Wang et al., 1995; Stoop and Poo, 1996; Boulanger and Poo, 1999a,b).
More recently, long-term synaptic strengthening by BDNF has been observed in cultured hippocampal neurons. In autaptic cultures of glutamatergic CA1 neurons, chronic BDNF treatment increases quantal amplitude and the amplitude of evoked synaptic transmission in parallel (Sherwood and Lo, 1999). In dissociated cultures of early embryonic hippocampal neurons, BDNF increases the number of functional synaptic connections (Vicario-Abejon et al., 1998). In contrast, studies of long-term effects of BDNF in dissociated cortical cultures have suggested that BDNF decreases neuronal firing rate by reducing the strength of all excitatory inputs onto a given neuron (Rutherford et al., 1998; Turrigiano and Nelson, 1998; Turrigiano et al., 1998;Turrigiano, 1999).
To begin to understand this apparent pleiotropy of BDNF action, we examined the regulation of synaptic activity by BDNF in hippocampal cultures in which effects on overall action potential activity, excitation, and inhibition can be analyzed separately. In these cultures, we observed that, rather than maintaining action potential firing rates at a constant level, BDNF increased overall spontaneous firing rate by approximately threefold. We found that actions of BDNF underlying this increase in activity involved enhancement of both excitatory and inhibitory synaptic transmission in parallel but via distinct cellular mechanisms. BDNF selectively increased the quantal amplitude of AMPA receptor-mediated excitatory transmission, an increase that did not require ongoing action potential activity. In contrast, BDNF did not affect the quantal amplitude of GABAergic transmission but rather increased the frequency of spontaneous quantal inhibitory transmission. Thus, although these effects contained a homeostatic component, the overall action of BDNF was strongly stimulatory and supports a role for BDNF as a mediator of activity-dependent plasticity in vivo.
MATERIALS AND METHODS
Cell culture. Standard dissociated hippocampal cultures were prepared from postnatal day 0 rat pups using the technique of Pan et al. (1993). Briefly, rat pups were anesthetized using isofluorane, and hippocampi were dissected into HBSS (Life Technologies, Gaithersburg, MD) with 10 mmHEPES. Each hippocampus was diced and incubated at 37°C for 45 min in HBSS containing 20 U/ml papain (Worthington, Freehold, NJ), 0.5 mm EDTA, 1.5 mmCaCl2, and 10 mm HEPES (Sigma, St. Louis, MO). The papain solution was removed, and residual papain was inactivated by the addition of serum-containing medium. The cells were then triturated by passage through fire-polished Pasteur pipettes with sequentially smaller diameter openings. Cells were plated at a density of 200,000 cells per dish in 35 mm dishes that had been coated with poly-d-lysine and merosin (Life Technologies). After 1 d in culture, 25% of the medium was exchanged, and the mitotic inhibitor 5-fluoro-2-deoxyuridine was added to minimize glial proliferation.
Neurotrophin treatment. Hippocampal cultures were allowed to establish for 3 d, after which either 100 ng/ml BDNF or 5 μg/ml TrkB-IgG (both generous gifts from Regeneron Pharmaceuticals, Tarrytown, NY) was added; we have shown previously that these concentrations of BDNF and TrkB-IgG are effective over the time course of several days and are low enough to avoid cross activation of other neurotrophin receptors (Lesser and Lo, 1995; Lesser et al., 1997;Riddle et al., 1997; Sherwood et al., 1997; Sherwood and Lo, 1999). Electrophysiological recordings were made after 4–7 d of treatment.
Electrophysiology. Electrophysiological recordings were made with an Axopatch 1D patch-clamp amplifier (Axon Instruments, Foster City, CA), and data were acquired using an INDEC Systems analog-to-digital converter and custom software written in-house in Visual Basic (Microsoft, Seattle, WA). Whole-cell patch-clamp recording was done using standard methods (Hamill et al., 1981). Borosilicate patch pipettes were pulled to resistances of 3–4 MΩ. For synaptic currents, data were acquired continuously at 2.5 kHz sampling frequency and filtered at 1 kHz using a four-pole Bessel filter. Recordings with leak currents >100 pA or series resistances >20 MΩ were discarded.
For recording AMPA receptor-mediated synaptic currents, the extracellular solution contained (in mm): 137 NaCl, 5 KCl, 3 CaCl2,1 MgCl2, 10 glucose, and 5 HEPES, adjusted to 310 mOsm and pH 7.25. To block GABAA receptor-mediated and action potential-driven synaptic transmission, 25 μm bicuculline and 1 μm tetrodotoxin (TTX) were included in the extracellular solution. The intracellular solution contained (in mm): 100 gluconic acid, 0.6 EGTA, 5 MgCl2, 2 Na2-ATP, 0.3 Na2-GTP, and 40 HEPES, adjusted to 310 mOsm and pH 7.25. For recording NMDA receptor-mediated synaptic currents, identical solutions were used, except that the extracellular solution was nominally Mg2+-free and contained 3 μm2,3-dihydroxy-6-nitro-7-sulphamoylbenzo(f)-quinoxalinedione (NBQX) and 10 μm glycine. For recording GABAA receptor-mediated synaptic currents, the intracellular solution contained (in mm): 110 KCl, 10 EGTA, 5 MgCl2, 2 Na2-ATP, 0.3 Na2-GTP, and 30 HEPES, adjusted to 310 mOsm and pH 7.25. The extracellular solution was the same as described for AMPA receptor-mediated currents but containing 3 μm NBQX instead of bicuculline.
Intrinsic excitability was measured in current-clamp mode. The intracellular solution contained (in mm): 144 K-gluconate, 0.5 EGTA, 1 MgCl2, 2 Na2ATP, 0.3 Na2GTP, and 0.5 HEPES, adjusted to 310 mOsm and pH 7.25. Membrane voltages were sampled at 10 kHz and filtered at 2 kHz. To elicit action potential activity, a series of depolarizing pulses of 160 msec duration were delivered to the cells. Input–output relationships were determined by plotting the current injected versus action potential firing frequency. Action potential height, half-width, and spike threshold were measured off-line. Membrane capacitance, series resistance, and input resistance were measured under voltage clamp.
On-cell patch-clamp recording was used for noninvasive measurement of the frequency of action potential activity. Data were acquired at 5 kHz in voltage-follower recording mode and filtered at 2 kHz. The extracellular and pipette solutions were the same, containing (in mm): 137 NaCl, 5 KCl, 3 CaCl2, 1 MgCl2, 10 glucose, 0.01 glycine, and 5 HEPES, adjusted to 310 mOsm and pH 7.25.
Immunocytochemistry. To measure neuronal survival and the percentage of inhibitory neurons, parallel cultures were double-labeled using a mouse monoclonal antibody directed against the GABAergic neuronal marker glutamic acid decarboxylase (GAD) (1:500; Chemicon, Temecula, CA) and a rabbit polyclonal antibody against neuron-specific enolase (NSE) (1:500; Chemicon). GAD immunostaining was visualized with an Oregon Green 488-conjugated goat anti-mouse secondary antibody (1:400; Molecular Probes, Eugene, OR); NSE immunostaining was visualized with a Cy3-conjugated goat anti-rabbit secondary antibody (1:400; Chemicon). On the fifth day of neurotrophin treatment, cultures were fixed in 4% paraformaldehyde and 5% sucrose in PBS and then washed with PBS. Nonspecific binding was blocked with 10% goat serum in PBS, and cells were permeabilized with 0.1% Triton X-100. Cultures were then incubated overnight with primary antibody at 4°C, followed by incubation in secondary antibody for 1 hr at room temperature. Finally, cultures were rinsed with PBS, mounted in Molwiol, and coverslipped.
Cell counts were done with the experimenter blinded on an invertedZeiss (Oberkochen, Germany) microscope (Axiovert) with a 10× objective. Mean numbers of GAD- or NSE-positive neurons per field were calculated by counting the number of GAD-positive cells in a field using fluorescein filters and then switching to rhodamine filters and recounting the same field for NSE-positive cells. Fields were analyzed by randomly placing the objective and then sequentially moving the dish through a vertical strip of 10 fields.
To quantify total numbers of synapses per field and numbers of inhibitory synapses per field, cultures were double-labeled using a mouse anti-synapsin monoclonal antibody (1:500; Chemicon) and a rabbit anti-GAD polyclonal antibody (1:1000; Chemicon). GAD immunostaining was visualized with an Oregon Green 488-conjugated goat anti-rabbit secondary antibody (1:500; Molecular Probes); synapsin immunostaining was visualized with a Cy3-conjugated goat anti-mouse secondary antibody (1:500; Chemicon). The immunostaining procedure was the same as described above.
As for cell counts, synapse quantification was done with the experimenter blinded. Images were acquired and digitized using a Hamamatsu (Shizouka, Japan) chilled CCD camera on a Zeiss Axioscope using a 40× oil-immersion objective; exposure times were held constant for each fluorochrome. Images were taken by randomly placing the objective and then sequentially moving the dish through a vertical strip of 10 fields. Images were analyzed using Scion Image software (Scion Corp., Frederick, MD); briefly, a mask containing the location and area of each synapsin or GAD puncta was made using a combination of thresholding and manual highlighting. Numbers, areas, and intensities of these punctae were then determined using built-in Scion Image functions.
RESULTS
BDNF increases spontaneous activity in dissociated cultures of hippocampal neurons
To investigate the role of BDNF in regulating the overall excitability of dissociated cultures of hippocampal neurons, cultures were treated for 4–7 d with 100 ng/ml BDNF and compared with untreated controls and cultures in which endogenous BDNF was neutralized with 5 μg/ml TrkB-IgG (Shelton et al., 1995; McAllister et al., 1996, 1997). Spontaneous action potentials in neurons with pyramidal morphology were then recorded using cell-attached patch-clamp recording as a rapid and relatively noninvasive measurement of circuit activity. BDNF treatment increased the average spontaneous action potential firing rates of neurons by approximately threefold compared with untreated controls (n = 33, 27, and 36 for BDNF, control, and TrkB-IgG cultures, respectively; BDNF vs control, p < 0.009 by ANOVA) (Fig. 1). Interestingly, there was no significant difference between untreated controls and TrkB-IgG-treated neurons with respect to firing rate (p > 0.60) or for any other electrophysiological parameter measured in this study, suggesting that levels of endogenous BDNF are below the physiological threshold required to modulate activity in these low-density cultures. This is consistent with the finding that endogenous BDNF levels are negligible in autaptic hippocampal cultures (Sherwood and Lo, 1999).
This striking increase in spontaneous firing rate could have arisen from an increase in the strength of excitation, a decrease in the strength of inhibition, or both. To evaluate the effect of BDNF on excitation directly, the contribution of inhibition to circuit activity was eliminated during the period of electrophysiological recording by pharmacologically blocking GABAA receptors acutely with bicuculline and measuring action potential firing rates in these disinhibited circuits. Under these conditions, BDNF still elevated spontaneous action potential firing rate by approximately twofold, indicating that the action of BDNF must include, at least in part, a direct potentiation of excitatory synaptic transmission (n = 43, 36, and 12 for BDNF, control, and TrkB-IgG cultures, respectively; BDNF vs control, p < 3 × 10−5 by ANOVA) (Fig. 1).
BDNF does not influence neuronal survival
We next asked whether the action of BDNF contained a component that influenced the balance of excitation and inhibition in these cultures via differential regulation of survival of excitatory versus inhibitory neurons. We found that, by quantifying neuronal density in BDNF-treated, control, and TrkB-IgG-treated cultures, BDNF had no measurable effect on total neuronal survival (n = 161 fields counted for each condition; p > 0.35 by ANOVA for any pairwise comparison) (Fig.2A). Although there was no change in overall neuronal density, BDNF increased the percentage of neurons expressing the inhibitory neuronal marker GAD (n = 180 fields counted for each condition; BDNF vs control, p < 0.008 by ANOVA) (Fig.2B).
There are two possible interpretations of this result. First, BDNF may have caused a decrease in the survival of non-GABAergic neurons that was exactly balanced by an increase in survival of GABAergic neurons. Second, BDNF may have promoted the neurochemical maturation of inhibitory neurons such that the level of GAD expression was increased to detectable levels in a greater percentage of inhibitory neurons, with no effect on neuronal survival per se. The latter interpretation is consistent with previous work suggesting that BDNF potentiates phenotypic differentiation of GABAergic neurons (Ip et al., 1993; Nawa et al., 1993; Mizuno et al., 1994; Ventimiglia et al., 1995;Marty et al., 1996a,b; Rutherford et al., 1997; Vicario-Abejon et al., 1998). Furthermore, other studies have shown that BDNF-mediated increases in GABA and neuropeptide expression levels are reversible, thus arguing against differential survival as a mechanism for BDNF action (Marty and Onteniente, 1997; Rutherford et al., 1997).
Because BDNF did not affect overall neuronal density and its enhancement of inhibitory neuronal differentiation would be predicted to decrease circuit activity, these factors were not likely to contribute positively to the observed increase of circuit activity induced by BDNF. Thus, these findings suggested that BDNF must increase circuit activity by other mechanisms, such as enhanced synaptic drive or by increased intrinsic membrane excitability.
BDNF does not regulate intrinsic excitability
Because the action potential firing properties of a network depend on the intrinsic excitability of its neuronal elements as well as the synaptic connectivity of the ensemble, we next investigated whether BDNF regulated intrinsic membrane excitability in these cultures. Accordingly, we measured several parameters of action potential activity that was generated by injecting a series of current pulses of increasing amplitude into current-clamped neurons; voltage responses to these current pulses were measured while all synaptic transmission was blocked pharmacologically. Most importantly, we found that BDNF did not change the firing rate of neurons at any of the current injection amplitudes examined (Fig. 3). Additionally, we found that BDNF affected neither action potential shape, as measured by action potential height and half-width (Table1), nor the voltage threshold at which the regenerative action potentials were first observed.
Similarly, there were no differences between BDNF-treated and control or TrkB-IgG-treated neurons in resting membrane potential (Table 1), but BDNF did cause a small increase in capacitance and a decrease in input resistance (Table 1). These minor differences in particular membrane properties suggested that BDNF may have had small effects on the morphology of these neurons, but it is unlikely that these differences contributed significantly to increasing spontaneous circuit activity for two reasons: first, neither the shape, frequency, or voltage-threshold of action potentials, nor any other aspect of intrinsic excitability measured, was changed by BDNF; second, the rise and decay kinetics of AMPA receptor-mediated synaptic currents were not affected by BDNF (see following sections).
BDNF selectively increases the amplitude of AMPA receptor-mediated miniature EPSCs
Because the firing rate of neurons is determined, in part, by the number, strength and temporal characteristics of its individual excitatory and inhibitory synaptic inputs, we next examined the effects of BDNF on unitary synaptic transmission. We first measured the behavior of miniature EPSCs (mEPSCs) by blocking sodium channel-mediated action potential activity with TTX and recording spontaneous mEPSCs under whole-cell voltage clamp (Fig.4). We found that BDNF significantly increased the amplitude of AMPA receptor-mediated mEPSCs by ∼30% (n = 82, 44, and 69 for BDNF, control, and TrkB-IgG cultures, respectively; BDNF vs control, p < 0.007 by ANOVA) (Fig. 5A). BDNF shifted the cumulative probability distribution of AMPA receptor-mediated mEPSC amplitudes uniformly toward larger amplitudes (Fig. 5C), suggesting that the action of BDNF was not limited to a subset of synapses of a particular quantal size and that there was no saturation of mEPSC sizes at higher amplitudes. This increase in the amplitude of unitary synaptic transmission by BDNF was accompanied by a significant increase in mEPSC frequency in BDNF-treated compared with TrkB-IgG-treated cells, but not compared with control cells (n = 83, 45, and 73 for BDNF, control, and TrkB-IgG cultures, respectively; BDNF vs TrkB-IgG, p < 0.04 by ANOVA; BDNF vs control, p > 0.7 by ANOVA) (Fig.5B). BDNF had no effect on the decay rates of either AMPA or NMDA receptor-mediated synaptic currents (Table2). Together, these findings suggested that BDNF increased excitation in these cultures predominantly by selectively increasing the amplitude of AMPA receptor-mediated synaptic currents without substantially affecting other aspects of excitatory synaptic transmission.
BDNF induction of AMPA receptor-mediated mEPSC amplitude does not require activity
Several previous studies have reported that the actions of neurotrophins are activity-dependent or that activity and neurotrophins interact in their regulation of the physiological properties of neurons and neuronal circuits (Marty et al., 1996a; McAllister et al., 1996; Rutherford et al., 1997). We therefore asked whether the potentiative effect of BDNF on excitation observed here was dependent on ongoing electrical activity by blocking action potential activity with 5 μm TTX for the entire duration of BDNF or TrkB-IgG treatment. We found, surprisingly, that TTX had no effect on the enhancement of mEPSC amplitude by BDNF (n = 38, 30, 39, and 29 for BDNF, TrkB-IgG, BDNF plus TTX, and TrkB-IgG plus TTX cultures, respectively; BDNF vs TrkB-IgG, p < 0.01 by ANOVA; BDNF plus TTX vs TrkB-IgG plus TTX, p < 10−4 by ANOVA) (Fig.6A). In fact, TTX appeared to increase slightly the magnitude of enhancement by BDNF, from 31 to 53% in the presence of TTX. We verified that the TTX used remained active for the duration of the experiment by applying media containing the TTX to naı̈ve cells and observing complete sodium channel blockade (data not shown). Thus, the regulation of AMPA receptor-mediated mEPSC amplitude by BDNF did not require concurrent action potential activity and thus may differ from other reported actions of BDNF.
BDNF selectively increases the frequency of GABAA-mediated mIPSCs
To determine whether BDNF also regulated the unitary properties of inhibitory synaptic transmission, we next recorded mIPSCs arising from GABAergic inputs onto neurons with pyramidal morphology. During the recording period, TTX and NBQX were added to the extracellular solution to block action potentials and glutamatergic inputs, respectively. We found that BDNF treatment increased the frequency of mIPSCs by almost twofold (n = 35, 31, and 35 for BDNF, control, and TrkB-IgG cultures, respectively; BDNF vs control, p < 0.028 by ANOVA) (Fig. 7D). In contrast to the increase in AMPA receptor-mediated mEPSC amplitude described above, GABAA receptor-mediated mIPSC amplitudes were not affected by BDNF (n = 35, 31, and 35 for BDNF, control, and TrkB-IgG cultures, respectively; BDNF vs control, p > 0.6 by ANOVA) (Fig. 7C). As with AMPA- and NMDA-mediated synaptic currents, BDNF did not alter the kinetics of synaptic currents mediated by GABAAreceptors (Table 2). These findings indicated that, although BDNF potentiated both excitatory and inhibitory synaptic transmission in these cultures, it did so through distinct physiological mechanisms.
BDNF does not change synapse number but enhances differentiation of GABAergic terminals
Finally, we asked whether BDNF regulated inhibition by regulating numbers of GABAergic inputs because we observed that BDNF increased the frequency of mIPSCs. First, we quantified total numbers of presumptive synapses by immunostaining with antibodies against the synaptic vesicle protein synapsin I (Fig.8A). Because synapsin I is present in the terminals of both excitatory and inhibitory neurons, these initial measurements reflected the combined number of glutamatergic and GABAergic synapses. BDNF did not increase numbers of synapses per field, terminal size, or intensity of synapsin labeling; in fact, there was a slight increase in numbers of synapses in cultures in which endogenous BDNF had been antagonized with TrkB-IgG (Fig.9, left).
We next examined GABAergic terminals specifically with an antibody directed against GAD (Fig. 8B). BDNF did not increase the number of GAD-positive synapses; as found for synapsin staining, however, there was a slight increase in the number of GAD punctae with TrkB-IgG treatment (Fig. 9A, right). Strikingly, BDNF increased average GABA terminal size by 50% and concomitantly increased the fluorescence intensity of these punctae, presumably reflecting an increase in the level of GAD expression (Fig.9B, right). Together with the increased mIPSC frequency described above, these observations suggest that BDNF increased inhibition by increasing the efficacy and/or probability of transmission at GABAergic synapses.
DISCUSSION
We have found that BDNF strongly regulates both excitation and inhibition in dissociated cultures of hippocampal neurons. Although the increase in excitation was dominant in that overall levels of spontaneous activity in these cultures were increased after BDNF treatment, this parallel enhancement of excitation and inhibition also resulted in partial homeostasis in terms of circuit activity. The increase in circuit activity produced by BDNF arose principally from changes in excitatory and inhibitory synaptic drive, both relative and absolute, but via distinct physiological mechanisms, with no significant changes in intrinsic neuronal excitability or neuronal survival.
BDNF regulation of excitation
We found that long-term treatment of hippocampal cultures with BDNF led to a selective increase in the quantal size of AMPA receptor-mediated mEPSCs. Such a change is consistent with a postsynaptic mechanism. Moreover, the absence of kinetic changes in AMPA receptor-mediated synaptic currents limits possible cellular and molecular mechanisms to those that do not alter the kinetic profile of postsynaptic currents. For example, an increase in numbers of functional AMPA receptors at synaptic sites would be expected to increase mEPSC amplitude without affecting kinetics; in fact, changes in the half-life of AMPA receptors can result in changes in receptor density that have been shown to correlate with quantal size (O'Brien et al., 1998). Recently, rapid insertion and removal of AMPA receptors from potentiated and depressed synapses has been proposed to underlie changes in synaptic efficacy (Carroll et al., 1999; Lissin et al., 1999; Shi et al., 1999), suggesting that longer term action of BDNF such as those reported here may similarly involve increases in the density of AMPA receptors at synapses. BDNF has, for example, recently been demonstrated to increase the expression of AMPA receptor subunit 1 and 2/3 protein in neocortical neurons (Narisawa-Saito et al., 1999a,b). Alternatively, BDNF may induce the accumulation of AMPA receptors at synapses previously devoid of these receptors as has been proposed for “silent” synapses in neonatal hippocampus (Isaac et al., 1995; Liao et al., 1995; Durand et al., 1996; Wu et al., 1996).
Changes in the composition or functional states of AMPA receptors are also possible that have minimal effects on the overall time course of mEPSCs. For example, induction of LTP in CA1 hippocampus and Ca2+/calmodulin kinase II phosphorylation of the glutamate receptor subunit GluR1 have been shown to produce increases in AMPA receptor single-channel conductance (Tan et al., 1994; Barria et al., 1997a,b; Mammen et al., 1997; Benke et al., 1998; Derkach et al., 1999). Our results are also consistent, however, with an increase in the amount of glutamate packaged per vesicle (for review, see Reimer et al., 1998) as has been reported recently for catecholamines (Pothos et al., 1998). In this context, it is interesting that there was increased mEPSC frequency in BDNF-treated neurons because changes in the frequency of mEPSCs is often associated with presynaptic alterations, such as in probability of release.
Interestingly, BDNF did not affect the kinetics of the synaptic currents measured in this study (neither AMPA, NMDA, nor GABAA receptor-mediated), a finding that has several implications. First, any effects BDNF may have had on neuronal morphology, spatial distribution of synaptic inputs, or input resistance did not alter the passive membrane properties of the neuron sufficiently to affect the time course of such fast synaptic currents (Mennerick et al., 1995; Bekkers and Stevens, 1996). Second, in the case of AMPA receptor-mediated mEPSCs, the potential cellular mechanisms responsible for the quantal amplitude increase induced by BDNF are limited to those that do not affect the rate of decay of synaptic currents, as discussed above; however, our experiments do not specifically address mechanisms such as regulation of glutamate transporter function, whose contribution to synaptic current kinetics remains uncertain (for review, see Clements, 1996; Diamond and Jahr, 1997; Mennerick et al., 1999). Finally, that BDNF did not regulate the decay time course of NMDA receptor-mediated synaptic currents suggests that BDNF does not alter the subunit composition of the NMDA receptors under these conditions because changes in the relative expression of NR2A–NR2D subunits have been shown, for example, to alter NMDA receptor decay times significantly (Carmignoto and Vicini, 1992;Hestrin, 1992).
A previous study using hippocampal cultures from embryonic day 16 rats found similar BDNF-mediated increases in the amplitude of sucrose-evoked mEPSCs, but at this early developmental stage, the dominant effect was an increase in the number of functional synapses (Vicario-Abejon et al., 1998). Our results are more consistent with studies in CA1 hippocampal autapses in which BDNF induces a 1.7-fold increase in quantal amplitude of AMPA receptor-mediated mEPSCs and a parallel increase in the amplitude of evoked synaptic currents (Sherwood and Lo, 1999). Interestingly, the effects of BDNF described here and by Vicario-Abejon et al. (1998) and Sherwood and Lo (1999) are quite different from those reported recently in dissociated cultures of visual cortical neurons (Rutherford et al., 1998; Turrigiano et al., 1998). In these studies, the quantal amplitude of AMPA-mediated synaptic currents was scaled by activity; Rutherford et al. (1998)reported that BDNF prevents this increase in AMPA receptor-mediated quantal amplitude in response to activity blockade, the opposite of the action of BDNF found here. Interestingly, however, bipolar interneurons as described by Rutherford et al. (1998) responded to BDNF similarly to the hippocampal pyramidal neurons in the present study.
Such differences in BDNF regulation of synaptic transmission presumably arise from the pleiotropy and cell context-dependence of BDNF action and emphasize the diversity of roles BDNF may transpire to play in synaptic development and plasticity. In this context, it is notable that there are developmental differences in the relative abundance of GluR1–GluR4 subunits and the alternative splicing variants, GluR Flip and GluR Flop, between pyramidal cells of the hippocampus and cortex (Boulter et al., 1990; Keinanen et al., 1990;Sommer et al., 1990; Monyer et al., 1991; Pellegrini-Giampietro et al., 1991; Petralia and Wenthold, 1992; Craig et al., 1993; Eshhar et al., 1993; Conti et al., 1994). Such differences in subunit expression may contribute to the apparent regional difference in regulation of quantal amplitude by BDNF in hippocampus versus cortex.
BDNF regulation of inhibition
We found that inhibitory synaptic transmission was also enhanced by chronic BDNF treatment but that the physiological mechanisms underlying this potentiation were different from those that enhanced excitatory synaptic drive. In this case, BDNF selectively increased the frequency of mIPSCs with no effects on their quantal amplitude or kinetic properties. Such frequency changes could have arisen from changes in probability of transmitter release, numbers of inhibitory synaptic contacts, or both. Our finding that the number of GABAergic terminals was not affected by BDNF but that the size of inhibitory terminals and intensity of GAD immunostaining was increased suggests that BDNF is likely to have enhanced the probability of transmitter release presynaptically.
The 40% increase in the ratio of neurons that showed detectable anti-GAD staining we observed after BDNF treatment was similar to previous reports of increases in GABAergic phenotypic differentiation, but not inhibitory neuronal numbers, after treatment with BDNF in vitro and in vivo (Ip et al., 1993; Nawa et al., 1993,1994; Croll et al., 1994; Marty et al., 1996a,b). Interestingly, BDNF is not synthesized by GABAergic interneurons (Cellerino et al., 1996; Rocamora et al., 1996; Schmidt-Kastner et al., 1996), but rather their source of BDNF is thought to be neighboring glutamatergic neurons (Nawa et al., 1995; Marty et al., 1996a). Such observations continue to support a general role for BDNF in regulating inhibitory synaptic transmission and are consistent with BDNF acting as an activity-dependent, target-derived differentiation factor for GABAergic interneurons. In turn, such regulation of GABAergic transmission by BDNF and activity would be expected to have major ramifications for neural development and function (Hendry and Jones, 1988).
In summary, our experiments have shown that BDNF can have profound effects on the function of neural circuits and that it can do so via regulation of selective aspects of excitatory and inhibitory synaptic function. In combination with activity-dependent production and localized release of neurotrophins (Wetmore et al., 1994; Blochl and Thoenen, 1995, 1996; Goodman et al., 1996; Fawcett et al., 1997, 1998;Smith et al., 1997; Wang and Poo, 1997; Moller et al., 1998), such effects of BDNF provide powerful mechanisms of action in their increasingly apparent roles in regulating synaptic development and plasticity.
Footnotes
This work was supported by National Institutes of Health Grants NS32742 (to D.L.) and MH11519 (to M.B.) and The McKnight Endowment Fund for Neuroscience (D.L.). We thank D. Fitzpatrick, S. Lesser, N. Tang Sherwood, and T. Yacoubian for their helpful comments on this manuscript and valuable discussions on experimental design. We also thank Regeneron Pharmaceuticals for their generous provision of recombinant BDNF and TrkB-IgG.
Correspondence should be addressed to Donald C. Lo, Department of Neurobiology Box 3209, Duke University Medical Center, Durham, NC 27710. E-mail: lo{at}neuro.duke.edu.