Activity- and Ca2+-Dependent Modulation of Surface Expression of Brain-Derived Neurotrophic Factor Receptors in Hippocampal Neurons

doi:10.1083/jcb.150.6.1423

Published online 18 September 2000. doi:10.1083/jcb.150.6.1423

This Article

	Abstract
	Full Text (PDF, 536K)
	PPT slides of all figures
	Alert me when this article is cited
	Citation Map

Services

	Email this article
	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new content in the JCB
	Download to citation manager

Citing Articles

	Citing Articles via CrossRef
	Citing Articles via Google Scholar

Google Scholar

	Articles by Du, J.
	Articles by Lu, B.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Du, J.
	Articles by Lu, B.


Social Bookmarking

	What's this?

© The Rockefeller University Press, 0021-9525/2000//1423 $5.00
The Journal of Cell Biology, Volume 150, Number 6, , 2000 1423-1434

Original Article

Activity- and Ca²⁺-Dependent Modulation of Surface Expression of Brain-Derived Neurotrophic Factor Receptors in Hippocampal Neurons

Jing Du^a, Linyin Feng^b, Feng Yang^a, and Bai Lu^a

^a Unit on Synapse Development and Plasticity, Laboratory of Developmental Neurobiology, National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, Maryland 20892-4480
^b Institutes of Neuroscience, Shanghai, China 200031
Unit on Synapse Development and Plasticity, NICHD, NIH, Bldg. 49, Rm. 5A38, 49 Convent Dr., Bethesda, MD 20892-4480.(301) 496-9939(301) 435-2970

Brain-derived neurotrophic factor (BDNF) has been shown to regulateneuronal survival and synaptic plasticity in the central nervoussystem (CNS) in an activity-dependent manner, but the underlyingmechanisms remain unclear. Here we report that the number ofBDNF receptor TrkB on the surface of hippocampal neurons canbe enhanced by high frequency neuronal activity and synaptictransmission, and this effect is mediated by Ca²⁺ influx. Usingmembrane protein biotinylation as well as receptor binding assays,we show that field electric stimulation increased the numberof TrkB on the surface of cultured hippocampal neurons. Immunofluorescencestaining suggests that the electric stimulation facilitatedthe movement of TrkB from intracellular pool to the cell surface,particularly on neuronal processes. The number of surface TrkBwas regulated only by high frequency tetanic stimulation, butnot by low frequency stimulation. The activity dependent modulationappears to require Ca²⁺ influx, since treatment of the neuronswith blockers of voltage-gated Ca²⁺ channels or NMDA receptors,or removal of extracellular Ca²⁺, severely attenuated the effectof electric stimulation. Moreover, inhibition of Ca²⁺/calmodulin-dependentkinase II (CaMKII) significantly reduced the effectiveness ofthe tetanic stimulation. These findings may help us to understandthe role of neuronal activity in neurotrophin function and themechanism for receptor tyrosine kinase signaling.

Key Words: TrkB receptors • tetanic stimulation • calcium influx • Ca²⁺/calmodulin-dependent kinase II • synaptic transmission

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Brain-derived neurotrophic factor (BDNF), a member of the neurotrophinfamily, is a potent neurotrophic protein that regulates neuronalsurvival and differentiation (Lewin and Barde 1996). Signaltransduction and neurotrophic functions of BDNF are mediatedprimarily by TrkB, a high affinity receptor tyrosine kinase(Kaplan and Stephens 1994). BDNF is also capable of bindingto the low affinity receptor p75 (p75NR) and eliciting apoptoticfunction in certain populations of neurons (Casaccia-Bonnefil et al. 1996,Casaccia-Bonnefil et al. 1998; Frade et al. 1996). Evidenceaccumulated in the last few years suggests that BDNF is involvedin synapse development and plasticity, in addition to its traditionalrole in neuronal survival and differentiation (Thoenen 1995;Bonhoeffer 1996; Berninger and Poo 1996; Lu and Chow 1999; McAllister et al. 1999).BDNF has been shown to exert complex modulation of dendriticand axonal growth in the brain, particularly in the visual system(Cohen-Cory and Fraser 1996; Cohen-Cory and Lom 1999; McAllister et al. 1995,McAllister et al. 1996, McAllister et al. 1997). BDNF is alsoinvolved in activity-dependent synaptic competition and formationof ocular dominance columns in the visual cortex (Maffei et al. 1992;Gu et al. 1994; Cabelli et al. 1995; Riddle et al. 1995; Galuske et al. 1996;Huang et al. 1999). BDNF is capable of rapidly regulating synaptictransmission at the neuromuscular junction and central nervoussystem (CNS) synapses (Lohof et al. 1993; Knipper et al. 1994;Lessmann et al. 1994; Levine et al. 1995; Takei et al. 1997).In the hippocampus, BDNF promotes tetanus-induced long-termpotentiation (LTP; Korte et al. 1995, Korte et al. 1996; Figurov et al. 1996;Patterson et al. 1996; Kang et al. 1997). Moreover, BDNF selectivelyenhances high frequency but not low frequency synaptic transmission(Tanaka et al. 1997; Frerking et al. 1998; Gottschalk et al. 1998).Recent experiments using BDNF knockout mice demonstrate thatBDNF enhances high frequency synaptic transmission by facilitatingsynaptic vesicle docking in the hippocampus, possibly by increasingthe levels of the vesicle protein synaptobrevin in the presynapticterminals of CA1 synapses (Pozzo-Miller et al. 1999).

Based on the above discoveries, BDNF has been proposed to participatein several forms of activity-dependent plasticity in the CNS(Thoenen 1995; Bonhoeffer 1996; Lu and Chow 1999). A criticalelement of such proposition is that BDNF acts preferentiallyon active neurons. Indeed, blockade of neuronal activity andsynaptic transmission prevents the increase of dendritic arborizationinduced by BDNF (McAllister et al. 1996). BDNF cannot enhancethe survival of retinal ganglion neurons unless they are depolarizedby high K⁺ or glutamate agonists, or their intracellular cAMPis increased (Meyer-Franke et al. 1995). Presynaptic depolarizationgreatly facilitates the BDNF modulation of synaptic transmissionat the neuromuscular junction (Boulanger and Poo 1999). In thehippocampus, the effect of BDNF on CA1 synapses is observedonly when presynaptic neurons are stimulated at high frequency(Gottschalk et al. 1998). These results support the notion thatcertain levels of neuronal activity are required for neuronalresponsiveness to BDNF.

As a diffusible molecule, how does BDNF distinguish active andinactive neurons or synapses, and restrict its action preferentiallyon active neurons/synapses? One possible mechanism is that cellularresponsiveness of neurons to BDNF is enhanced by neuronal activity.Thus, whether or how well a neuron can respond to BDNF may dependon its activity levels. It is unclear, however, how activity-dependentregulation of BDNF responsiveness is achieved. Neuronal activitycould increase the number of BDNF receptors on the cell surface,facilitate the internalization of BDNF–receptor complex,or facilitate the signaling mechanisms for BDNF. Depolarizationor cAMP elevation has been shown to increase the levels of theBDNF receptor TrkB on the cell surface of retinal ganglion cellsand spinal neurons (Meyer-Franke et al. 1998). Here we investigatewhether physiologically relevant stimuli such as electric stimulationcan modulate the BDNF receptors on the cell surface of neuronsin the hippocampus, where activity-dependent plasticity is mostcommonly observed. Using three independent approaches (biotinylation,receptor binding, and immunocytochemistry), we show that highfrequency tetanic stimulation, but not low frequency stimulationor simple depolarization, can rapidly enhance the insertionof TrkB into the cell surface. We also demonstrate that theactivity-dependent modulation requires Ca²⁺ influx through NMDAand Ca²⁺ channels, and involves Ca²⁺/calmodulin-dependent kinaseII (CaMKII). Not only may these findings provide insights intothe mechanistic link between activity-dependent and neurotrophicmodulation of CNS neurons and synapses, but they may also havegeneral implications in the cell biology of growth factor signaling.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Culture Preparations
Cultures of hippocampal neurons were prepared according to thepublished procedure (Feng et al. 1999) with minor modifications.In brief, hippocampus was dissected from embryonic day 18 rats,dissociated in Ca²⁺- and Mg²⁺-free HBSS containing 0.125% tyrosinefor 15 min, triturated in DMEM/10% FBS, and plated at 2 x 10⁵cells per well in 12-well plates. Cells were grown at 37°C,5% CO₂ and 95% humidity, first in 10% FBS/DMEM, and 1 d laterswitched to serum-free medium Neurobasal plus B27 (Life Technologies).Cultures were grown in serum-free medium for 11–14 d beforebeing used for experiments, and the medium was changed every3 d. Fresh medium was applied 24 h before each experiment. Thesecultures yielded virtually pure neurons (data not shown). Drugswere applied immediately before electric stimulation. In somecases, serum-free medium was replaced with Ca²⁺-free medium(Ca²⁺-free DMEM; Life Technologies) for 30 min before electricstimulation.

Electric Stimulation of Neuronal Cultures
Hippocampal neurons were stimulated using a method similar toone that has been described previously (Bito et al. 1996; Deisseroth et al. 1996;Fields et al. 1997). Field electric stimulation was appliedacross a 12-well dish through a homemade lid, which containedplatinum wires contacting the medium in each well. Each stimulationpulse (1 msec, 2–8 V) was sufficient to elicit actionpotentials in these cultured neurons (see Fig. 1 A). The entireelectric stimulation was performed in a 37°C, 5% CO₂ incubator.The following stimulation paradigms were used. (i) TBS: eachepisode consisted of four bursts, each with five biphasic pulsesat 100 Hz (10-msec interval), separated by an interburst intervalof 200 msec. One episode was given every 5 s throughout thewhole incubation period. (ii) Tetanic stimulation: 1 s, 100Hz, given every 10 min for for 30 min. (iii) Low frequency stimulation:0.16 Hz during the entire incubation period. (iv) Long-termdepression (LTD)-inducing stimulation: 4 min, 5 Hz. Whole-cellrecording was performed under the current-clamped or voltageclamped conditions as previously described (Kim et al. 1994).Data were collected by an Axopatch 200B amplifier, filteredat 5 kHz, digitized at 10 kHz, and analyzed by P-clamp software(Axon Instruments).

View larger version (45K):
[in this window]
[in a new window]
[Download PPT slide]

Figure 1 Effects of TBS on BDNF receptors on neurons. Hippocampal neurons were grown in serum free medium for 11–14 d. Two platinum electrodes were positioned on opposite sides of the culture well, and the hippocampal neurons were stimulated with TBS for 60 min in a 37°C incubator in the presence or absence of various inhibitors. After electric stimulation, proteins on the surface of hippocampal neurons were biotinylated, and then examined by Western blot using antibodies against the high affinity receptor TrkB or the low affinity receptor p75. (A) Electrophysiological recording of firing patterns in cultured hippocampal neurons elicited by field electric stimulation. Top traces show that a supra-threshold field stimulation induced a single action potential. Arrow indicates application of a single field electric pulse. Scale: 20 mV and 100 ms. Bottom trace shows an example of action potentials elicited by TBS. 2 out of the 10 bursts are shown. (B) Western blot analysis of cell surface TrkB receptors. Cultures were stimulated with TBS in the presence of indicated agents as follows: TTX (1 µM); kyn (1 mM); Q/M (0.1 mM CNQX plus 80 µM MK801); anisomycin (10 µg/ml); cycloheximide (10 µg/ml); Na⁺ (50 mM) and K⁺ (50 mM). (B1) High frequency electric stimulation increases surface expression of TrkB. Both full length (145 kD) and truncated (95 kD) TrkB receptors in stimulated (stim) or unstimulated (unstim) cultures are shown. (B2) Blockade of excitatory synaptic transmission prevents the TBS-induced increase in surface TrkB. The surface TrkB was measured in cultures in the presence or absence of blockers for excitatory transmission, kyn or Q/M. (B3) The total levels of TrkB are not changed by electric stimulation. Hippocampal neurons were stimulated with TBS in the presence or absence of TTX or kyn, harvested by RIPA buffer. Total amount of TrkB were measured directly by Western blot. (B4) TBS-induced increase in surface TrkB does not require protein synthesis. Cultures were stimulated by TBS in the presence or absence of the protein synthesis inhibitor anisomycin or cycloheximide. The surface TrkB were determined by biotinylation. (B5) Simple depolarization induced by high K⁺ does not change the levels of surface TrkB. Biotinylation was used to determine the levels of surface TrkB in cultures that were treated with 50 mM of either control agent Na⁺ or the depolarizing agent K⁺. (C) Summary of the biotinylation experiments for surface TrkB (full length, p145). (Left) The levels of surface TrkB in TBS-stimulated cultures (set as 100%) are compared with unstimulated cultures (unst) and cultures stimulated with TBS in the presence of TTX, kyn, or Q/M; n = 7. (Right) Simple depolarization by high K⁺ has no effect; n = 4. The surface TrkB levels were determined in cultures that were treated with Na⁺ (50 mM, set as 100%) and K⁺ (50 mM). Asterisk indicates statistically different results (P < 0.05, ANOVA followed by post hoc tests). (D) Summary of the biotinylation experiments for surface p75NR. TTX and kyn have no effect on surface p75NR; n = 3. In this and all other bar graph figures, data from a specific experimental condition (e.g., TBS plus TTX) were normalized to the mean in control (TBS stimulation alone) groups. The results in several independent experiments (n) were pooled and averaged, and presented as mean ± SE.

Surface Biotinylation and Western Blot Analysis of TrkB
Surface TrkB receptors was measured by biotinylation followedby Western blot using either a TrkB antibody or a p75NR antibody,as described elsewhere (Meyer-Franke et al. 1998). In brief,various blockers were added to the hippocampal cultures, andelectric stimulation was applied immediately in a 37°C incubator.At the end of electric stimulation (60 min), ice-cold PBS, pH7.4, with Ca²⁺ and Mg²⁺, pH 7.4; Life Technologies) was addedto the cultures to prevent receptor internalization. After threewashes with ice-cold PBS, cells were incubated in Sulfo-NHS-LC-biotin(0.25 mg/ml in cold PBS; Pierce) for 30 min. The surface biotinylationwas stopped by removing the above solution and incubating thecells in 10 mM ice-cold glycine in PBS for 20 min. Cells werethen washed three times with cold PBS and lysed by RIPA buffer,which contains 20 mM Hepes, pH 7.4, 100 mM NaCl, 1 mM EGTA,1 mM Na₃VO₄, 50 mM NaF, 1% NP-40, 1% deoxycholate, 0.1% SDS,1 mM [4-(2-aminoethyl)-benzenesulfluoride hydrochloride], 10µg/ml leupeptin, and 1 µg/ml aprotinin. Biotinylatedproteins (160 µg) were precipitated with 100 µlof ImmunoPure Immobilized Streptavidin (Pierce). Western blotswere performed by separating the biotinylated protein precipitateson SDS-PAGE gel and transferring the proteins to Immobilon Pmembrane. The membranes were probed with a monoclonal anti-TrkBantibody (1:250; Transduction Laboratories), or an anti-p75NRantibody (1:250; Upstate Biotechnology), followed by peroxidase-conjugatedgoat anti–rabbit IgG (1:10,000; Vector Laboratories).Immunoreactive bands were visualized by enhanced chemiluminescence(ECL; Amersham Pharmacia Biotech). The ECL signal intensitieswere quantified by NIH Image program. To measure the total amountof TrkB, cultured hippocampal neurons were simply harvestedby RIPA buffer and processed for Western blot. Quantitationfor each experimental condition was based on three to six independentexperiments (samples), each was repeated at least two to threetimes. The results were pooled and averaged, and presented asmean ± SE.

BDNF Receptor Binding
Binding assays were performed in hippocampal cultures in a 37°C,5% CO₂ incubator in quadruplicates. In brief, cells were washedthree times with warm DMEM, and then incubated in binding buffer(DMEM plus 0.5 mg/ml protamine sulfate and 10 mM Hepes, pH 7.4)containing I¹²⁵-BDNF (2,200 Ci/mmol, 5 x 10^–11 M; NENLife Science Products) with or without excess cold BDNF (5 x10^–8 M; provided by Regeneron Pharmaceuticals, Inc.) for30 min. During the entire period of incubation, the hippocampalneurons were electrically stimulated in the incubator in thepresence or absence of various blockers. After incubation, the12-well dishes were placed on ice to prevent receptor internalization.Nonspecifically bound BDNF was removed by washing three timeswith 1 ml of ice-cold PBS. The I¹²⁵-BDNF bound to cell surfacewas obtained by a 10-min acid wash on ice (0.2 M acetic acid,pH 2.2, 0.5 M NaCl, 0.5 ml), and the counts were used as themeasure for BDNF surface binding. An LKB ${gamma}$ counter was used tocount the radioactivity. Raw data (quadruplicates) from a specificexperimental condition were normalized to the mean in controlcondition. The results in several experiments were pooled andaveraged, and presented as mean ± SE.

Immunofluorescence Staining of TrkB Receptors
To visualize surface TrkB, cultured hippocampal neurons werefixed with 2% paraformaldehyde, 120 mM sucrose in PBS at roomtemperature for 3 min. After paraformaldehyde was quenched with0.1 M glycine in PBS, the nonspecific binding was blocked with50% goat serum, 1% BSA, and 100 mM lysine in PBS for 40 min.The cells were then incubated with a chicken antibody againstextracellular domain of TrkB (a gift from Dr. Louis Reichardt,University of California, San Francisco, CA) in blocking solutionovernight at 4°C, or in room temperature for 40 min. Thesecondary antibody was Cy3-conjugated goat anti–chickenY antibody (1:100; Jackson ImmunoResearch Laboratories). Afterseveral washes, cells were mounted with mounting medium Vectashield(Vector Laboratories). To visualize both surface and intracellularTrkB, the cells were fixed with 4% paraformaldehyde, 120 mMsucrose in PBS for 20 min at room temperature, followed by quenchingwith 0.1 M glycine in PBS. The cells were permeabilized andnonspecific binding was blocked with 10% goat serum, 0.4% TritonX-100 in PBS for 40 min at room temperature. The cells werestained with rabbit anti-TrkB (1:50; Chemicon) overnight at4°C. After several washes the cells were incubated withCy3-conjugated anti–rabbit antibody (1:200; Jackson ImmunoResearchLaboratories) in 5% goat serum in PBS for 1 h at room temperature.The cells were washed three times and then mounted with Vectashield.Fluorescence images were acquired by a MicroMax 1300 cool CCDcamera mounted on a Nikon Eclipse E800 microscope, and assignedto a pseudo color (green or red). In some cases, immunostainedcells were examined using a confocal microscope (MRC1024; Bio-Rad).The images were processed by IPLab software. Each experimentalcondition was repeated at least three times.

Antennapedia Fusion Peptide Experiments
The autocamtide-2–related inhibitory peptide (AIP) wasas a specific inhibitor for CaMKII (Ishida et al. 1995). Tofacilitate the translocation of AIP across the cell membrane,we fused AIP to a 16-residue antennapedia homeopeptide (antp-AIP;Prochiantz 1996; Passafaro et al. 1999). A control peptide wasmade using antp and scrambled AIP sequences (antp-AIPscm). Thisscrambled sequence was analyzed by Program Blastp, and no significantsimilarity was found in the current database. The sequencesof the peptides are listed below:

[H]-RQIKIWFQNRRMKWKKALRRRAVEDAL—Antp-AIP

[H]-RQIKIWFQNRRMKWKKRLAAADLVERR—Antp-AIPscm

The peptides were synthesized and HPLC-purified by PrincetonBiomolecules. To allow sufficient penetration of the peptidesinto the cytoplasm of hippocampal neurons, the cells were pretreatedwith Antp-AIP or Antp-AIPscm (20 µM) 3 h before the biotinylationor binding assay was performed.

Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

BDNF receptors on the surface of cultured hippocampal neuronswere determined by a biotinylation assay. All membrane proteinswere biotinylated, followed by precipitation with ImmunoPureImmobilized Streptavidin and Western blot analysis using antibodiesagainst the high affinity TrkB receptors or the p75NRs. Fieldelectric stimulation was applied to the culture dishes in a37°C incubator to induce neuronal firings (Bito et al. 1996;Deisseroth et al. 1996; Fields et al. 1997). Whole-cell currentclamp recording indicated that field stimulation reliably elicitedaction potentials (Fig. 1 A). The firing patterns of the neuronsfollowed well with either TBS (Fig. 1 A) or 100 Hz tetanus (datanot shown). When equal amounts of biotinylated proteins wereloaded into the SDS gel, significant differences in the amountof both full-length (145 kD, or p145) and truncated (95 kD,or p95) forms of TrkB receptors on the cell surface were observedbetween active and inactive hippocampal neurons (Fig. 1B andFig. C). Neurons stimulated with TBS exhibited significantlymore surface TrkB as compared with those in unstimulated cultures(Fig. 1, B1 and C). To control for any nonspecific effects ofelectric stimulation on surface expression of TrkB, we performedmost of our experiments in cultures stimulated with TBS eitheralone (active) or in the presence of activity blockers (inactive).The stimulation alone group is referred to as control (Ctr).Tetrodotoxin (TTX; 1 µM), which blocks Na⁺ channels andtherefore all neuronal action potentials, significantly reducedthe amount of surface TrkB (Fig. 1 C). TBS had no effect onsurface expression of p75NRs (Fig. 1 D), suggesting that theeffect of TBS is specific for TrkB receptors. In these cultures,neurons were well connected, and electric stimulation oftenelicited excitatory synaptic transmission (data not shown).Inhibition of excitatory transmission, either by the generalglutamate receptor antagonist kynurenic acid (kyn; 1 mM) ora combination of the non-NMDA receptor antagonist 6-cyano-7-nitroquinozaline-2,3-dione(CNQX; 100 µM) and the NMDA receptor antagonist MK801(80 µM), significantly attenuated the TBS-induced increasein surface TrkB (Fig. 1, B1 and C). Blockade of high frequencytransmission by kyn had no effect on surface p75NR (Fig. 1 D).Thus, high frequency neuronal activity modulates TrkB, but notp75NR, on the surface of hippocampal neurons, and this effectappears to require action potentials coupled to excitatory synaptictransmission.

The increase of surface TrkB could be due to an increase inTrkB insertion into the cell surface, a decrease in TrkB internalization,or an increase in TrkB synthesis. Several pieces of evidenceargue against a general increase in TrkB synthesis. First, therewas no difference in the total amount of TrkB between active(TBS) and inactive (TBS plus TTX or Kyn) hippocampal neurons(Fig. 1 B2). Second, inhibition of protein synthesis by anisomycin(10 µg/ml) or cycloheximide (10 µg/ml) did not decreasethe levels of surface TrkB in neurons stimulated with TBS (Fig. 1B3). Thus, the synthesis of TrkB receptors is not enhanced byhigh frequency neuronal activity. Finally, electric stimulationof hippocampal neurons resulted in an increase, rather thana decrease in TrkB internalization (data not shown). These results,together with the immunocytochemistry experiments (see below),suggest that TBS facilitates the insertion of TrkB onto thesurface membrane, rather than its production, in hippocampalneurons.

A previous study showed that depolarization induced by highconcentration of K⁺ (50 mM) resulted in a significant increasein the surface TrkB in retinal ganglion cells (Meyer-Franke et al. 1998).In our study, we found that simple depolarization by high K⁺did not affect the amount of surface TrkB in hippocampal neurons.The levels of surface TrkB were the same in neurons treatedwith 50 mM of K⁺, 50 mM of Na⁺, or nothing at all (Fig. 1 B4and data not shown). In retinal ganglion cells, the full-length(p145) but not the truncated (p95) form of TrkB was detected(Meyer-Franke et al. 1998). Both the full-length and truncatedTrkB receptors were found on the cell surface of hippocampalneurons and both were increased by TBS (Fig. 1 B1). Moreover,very low levels of p75NR were detected in the hippocampal neurons(data not shown), whereas those in the retinal cells are knownto be high (Frade et al. 1996; von Bartheld et al. 1996). Thus,modulation of surface TrkB receptors in hippocampal neuronsmay be different from that in retinal ganglion neurons.

Application of BDNF significantly reduced the amount of surfaceTrkB, presumably due to ligand-induced receptor internalization(data not shown). It was difficult to determine by the biotinylationassay whether electric activity could still modulate TrkB inthe presence of BDNF, a situation more likely to occur in thephysiological conditions in vivo. We thus turned to a more sensitiveassay using radiolabeled BDNF (I¹²⁵-BDNF). The neuronal cultureswere incubated at 37°C with I¹²⁵-BDNF (5 x 10^–11 M)with or without cold BDNF (5 x 10^–8 M) for 30 min. SurfaceBDNF receptors were determined by the amount of I¹²⁵-BDNF thatcan be washed off from the cell surface by mild acid (0.2 Macetic acid, 0.5 M NaCl, pH 2.2). Surface binding of I¹²⁵-BDNFwas reduced by 80–90% when an excess amount of cold BDNFwas added to the cultures (data not shown). Thus, the bindingwas specifically mediated by BDNF receptors. Stimulation ofthe hippocampal neurons with TBS reliably elicited an increasein surface binding of I¹²⁵-BDNF (Fig. 2). Compared with neuronsstimulated with TBS alone, I¹²⁵-BDNF surface binding was significantlyreduced in neurons stimulated with TBS plus TTX, which completelyblocked action potentials in these neurons (Fig. 2 A). The glutamatereceptor antagonists kyn or CNQX/MK801 also blocked the effectof TBS (Fig. 2 A), suggesting that the excitatory synaptic transmissionis required for TBS-induced increase in surface TrkB.

View larger version (28K):
[in this window]
[in a new window]
[Download PPT slide]

Figure 2 Activity-dependent modulation of the surface binding of BDNF receptors. Cultured hippocampal neurons were incubated with I¹²⁵-labeled BDNF (5 x 10^–11 M) with or without cold BDNF (5 x 10^–8 M) for 30 min while stimulated with TBS. Surface binding is defined as acid washable radioactivity at the end of I¹²⁵-BDNF incubation. The numbers associated with each column represent the total number of experiments. (A) Blockade of neuronal activity or excitatory synaptic transmission prevents the TBS-induced increase in BDNF surface binding. Hippocampal cultures were stimulated with TBS in the presence or absence of TTX, CNQX plus MK801, or kyn. All drug-treated groups were significantly lower than their paired stimulation alone (control) groups, which were set as 0% (P < 0.01, Student's t test). (B) Modulation of BDNF receptor binding by patterned electric stimulation. Percentage of changes is presented. The data in control (no stimulation at all) are set as 0%. TBS and tetanic stimulation (three times, 100 Hz, 1 s every 10 min), but not continuous low frequency stimulation (0.16 Hz) or high K⁺ (50 mM) stimulation, elicited much higher BDNF receptor binding as compared with control. LTD-inducing stimulus (5 Hz, 4 min) also had no effect. Asterisk indicates statistically different results (P < 0.05, ANOVA followed by post hoc tests).

As with the biotinylation experiments, the enhancement of BDNFreceptor binding was dependent on high frequency tetanic stimulation.TBS reliably elicited an increase in I¹²⁵-BDNF surface bindingas compared with nonstimulated controls (Fig. 2 B). Anothertetanic stimulation (three times, 100 Hz, 1 s every 10 min),which elicited a train of high frequency action potentials,resulted in an increase in BDNF binding similar to the resultfrom TBS (Fig. 2 B). In contrast, low frequency stimulation,such as the LTD-inducing stimuli (5 Hz, 4 min) or a constantlow frequency train (0.16 Hz), had no effect on I¹²⁵-BDNF surfacebinding (Fig. 2 B). It is worth pointing out that the same numberof pulses was delivered during 30 min of stimulation in boththe 100 Hz tetanic stimulation and the 0.16 Hz stimulation.Thus, the modulation of surface BDNF receptors appears to dependon the stimulation frequency, rather than the number of pulses.Again, simple depolarization induced by high K⁺ had little effecton surface binding (Fig. 2 B).

An immediate consequence of tetanus-induced neuronal activityis Ca²⁺ influx through voltage-gated Ca²⁺ channels or NMDA receptors.To determine the mechanisms underlying TBS-induced increasein the surface expression of TrkB, we studied effects of a numberof manipulations known to interfere with Ca²⁺ influx. Usingthe biotinylation assay, we found that blockade of Ca²⁺ influxby the NMDA receptor blocker MK801 (80 µM) markedly reducedthe amount of both full-length and truncated TrkB receptorson the surface of hippocampal neurons stimulated with TBS (Fig. 3A). Inhibition of Ca²⁺ influx by the general Ca²⁺ channel blockersCd²⁺ (0.2 mM) had similar effects (Fig. 3 A). These resultswere further confirmed by the I¹²⁵-BDNF surface binding assays.The surface binding was reduced when TBS was applied togetherwith the general Ca²⁺ channel blockers Cd²⁺ (Fig. 3 B) or Co²⁺(3 mM, not shown), or NMDA antagonists MK801 (80 µM; Fig. 3B) or 2-amino-5-phosphonovalerate (50 µM; data not shown).Moreover, surface BDNF receptors were significantly reducedin neurons stimulated by TBS in Ca²⁺-free medium, as comparedwith that in regular medium (Fig. 3 B). Thus, the TBS modulationof surface expression of BDNF receptors appears to depend onCa²⁺ influx through voltage-gated Ca²⁺ channels and/or NMDAreceptors.

View larger version (34K):
[in this window]
[in a new window]
[Download PPT slide]

Figure 3 Role of Ca²⁺ influx in activity-dependent modulation of cell surface TrkB receptors. Western blot analysis of cell surface TrkB receptors (A) and surface binding of I¹²⁵-BDNF (B) were performed under conditions that affect Ca²⁺ influx. TBS was applied in all conditions. Asterisk indicates statistically different results (P < 0.05, ANOVA followed by post hoc tests). (A) Summary of the effect of Ca²⁺ influx on surface TrkB. Inset shows an example of biotinylation analysis of surface TrkB receptors showing that MK801 and Cd²⁺ reduce both p145 and p95 TrkB proteins in TBS-stimulated cultures. The amount of full length TrkB (p145) in control conditions (TBS in regular medium) was set as 100%. Ca²⁺ channels blocked by Cd²⁺ (0.2 mM) and NMDA receptors blocked by MK801 (80 µM) all inhibited BDNF receptor on the cell surface; n = 7. (B) Summary of the effect of Ca²⁺ influx on BDNF surface binding. Controls (TBS in regular medium) were set as 0%. In Ca²⁺-free condition, culture medium was replace and pretreated for 30 min with Ca²⁺-free DMEM before experiments were performed. The numbers associated with each column represent the total number of experiments.

To determine the changes in the distribution of TrkB receptorson the cell surface, we performed immunocytochemistry undernonpermeable (no detergent) conditions. Cultured hippocampalneurons were fixed in 2% paraformaldehyde for 3 min, and TrkBantibodies were incubated with the fixed cells in buffers containingno detergent. Under these conditions, an antibody against intracellulardomains of the TrkB did not stain hippocampal neurons, suggestingthat antibodies or proteins can not penetrate the cells (Fig. 4Aand Fig. B). The same antibody was able to detect a substantialamount of TrkB if the staining was performed in the presenceof detergent (Fig. 4 C). Under the nonpermeable (no detergent)conditions, surface TrkB were detected using an antibody againstextracellular domains of the TrkB. In cultures stimulated withTBS, many TrkB receptors were found on the surface of the cellbody. More importantly, a large number of TrkB receptors weredistributed along the neuronal processes (Fig. 4 D). In contrast,TrkB receptors were mainly clustered on the cell body and therewere very few receptors on the neuronal processes in culturesstimulated with TBS in the presence of kyn and Cd²⁺ (Fig. 4E). The reduction in surface TrkB in the cultures treated withkyn and Cd²⁺ was not due to a decrease in the number of neuronalprocesses, which were obviously observed under phase contrastmicroscopy (data not shown). To better visualize the surfaceTrkB, we used confocal microscopy. Thin section (2 µm)confocal images revealed a substantial increase in the amountof surface TrkB receptors in active (TBS alone) neurons as comparedwith the inactive (TBS plus kyn and Cd²⁺) neurons (Fig. 4F andFig. G). These experiments were repeated many times and strikingdifferences in surface TrkB were always observed between activeand inactive neurons. Unstimulated neurons also exhibited lesssurface TrkB receptors than stimulated neurons (data not shown).

View larger version (71K):
[in this window]
[in a new window]
[Download PPT slide]

Figure 4 Immunocytochemistry of TrkB on the surface of hippocampal neurons. (A and B) Phase and fluorescence images of neurons stained with an antibody against intracellular domain of TrkB under nonpermeabilizing conditions. (C) Immunofluorescence images of neurons stained with the same antibody permeabilizing conditions. There is no staining in B but good staining in C, indicating that the antibody cannot penetrate inside cells under nonpermeabilizing conditions. (D–G) Immunocytochemistry staining using an antibody against the extracellular domain of TrkB under non-permeabilizing conditions. Hippocampal neurons were stimulated with TBS in the presence (E and G) or absence (D and F) of Cd²⁺ (0.2 mM) and kyn (1 mM) for 30 min. Cells were fixed with 2% paraformaldehyde, 120 mM sucrose in PBS at room temperature for 3 min, followed by conventional immunofluorescence procedure without any detergent. D and E are conventional immunofluorescence images, and F and G are confocal immunofluorescence images. Arrows indicate surface TrkB stainings on neuronal processes and arrowheads indicate those on cell body. Note that far more surface TrkB receptors are seen in cultures stimulated with TBS alone, especially in neuronal processes. Bar, 5 µm.

To further investigate the changes in the TrkB receptors insidethe cells, we stained the hippocampal neurons under permeable(with detergent) conditions using the antibody against the intracellulardomain of TrkB. Both surface and intracellular TrkB were detected.In the stimulated cultures, it appeared that majority of TrkBreceptors were on the cell membrane (arrows) and only smallamounts of the receptors were inside the cells (Fig. 5 A). Significantlyfewer TrkB receptors were found on the cell surface but a lotmore receptors were detected inside cells (arrowheads) in culturesstimulated with TBS in the presence of kyn and Cd²⁺ (Fig. 5B). Confocal microscopy was again used to better separate surfaceand cytoplasmic TrkB. Indeed, active neurons exhibited a "ring"pattern of staining in sections across the middle of the cellbody region, with a lot of TrkB receptors on the cell surfacebut very little in the cytoplasm (Fig. 5 C). In contrast, agreat deal of cytoplasmic TrkB was observed in inactive neuronsin similar sections (Fig. 5 D). These results further supportthe notion that high frequency neuronal activity facilitatesthe insertion of TrkB receptor into the cell surface.

View larger version (61K):
[in this window]
[in a new window]
[Download PPT slide]

Figure 5 Immunocytochemistry of hippocampal neurons stained by an antibody against the intracellular domain of TrkB under permeabilizing conditions. TBS was applied to the hippocampal neurons in the presence (B and D) or absence (A and C) of Cd²⁺ and kyn for 30 min. The cultures were then fixed with 4% paraformaldehyde for 30 min, permeabilized with 0.4% Triton X-100 for 60 min, and processed for immunofluorescence staining of TrkB. A and B are conventional immunofluorescence images, and C and D are confocal immunofluorescence images. Arrows indicate cell surface and arrowheads indicate cytoplasmic stainings, respectively. Note that active cells (stimulated by TBS) exhibit TrkB receptors mostly on the cell surface, whereas inactive cells (TBS plus Cd²⁺ and kyn) show more cytoplasmic staining of TrkB.

Ca²⁺ influx is known to activate CaMKII, which has been implicatedin the activity-dependent insertion of AMPA-type glutamate receptorsinto the postsynaptic membrane during LTP (Hayashi et al. 2000).To determine whether CaMKII is also involved in the insertionof the tyrosine kinase receptor TrkB, we measured the amountof surface TrkB in cultures stimulated with TBS in the presenceor absence of CaMKII inhibitors. Biotinylation experiments demonstratedthat inhibition of CaMKII by either KN62 or KN93 significantlyreduced the amount of TrkB receptors in cultures stimulatedwith TBS, whereas inactive compound KN92 had no effect (Fig. 6Aand Fig. B). KN62 and KN93 also significantly inhibited BDNFsurface binding on hippocampal neurons (Fig. 6 C). Since KN62and KN93 have been shown to inhibit other CaM kinases and maycause some nonspecific effects in certain conditions, we usedAIP, a peptide known to selectively inhibit CaMKII (Ishida et al. 1995).The NH₂ terminus of AIP or a control peptide with scrambledsequence (AIPscm) was fused to the antennapedia homeopeptide(antp, 16 residues) derived from antennapedia gene to facilitatethe translocation of the peptide across the cell membrane ofhippocampal neurons (Prochiantz 1996; Passafaro et al. 1999).To determine whether the peptides can penetrate into the hippocampalneurons, we labeled the peptides with biotin, and treated thecells with the biotinylated peptides for a few hours. Cy3-conjugatedstreptavidin detected the biotinylated peptides inside the hippocampalneurons 3 h after peptide incubation (data not shown). In culturesstimulated with TBS in the presence of antp-AIP, significantlylower levels of surface TrkB were detected as compared withthose in cultures stimulated with TBS alone (Fig. 6A and Fig. B).The control peptide antp-AIPscm had no effect (Fig. 6A and Fig. B).Similar results were obtained using the I¹²⁵-BDNF surface bindingassay (Fig. 6 C). These results strongly suggest the involvementof CaMKII in the activity-modulation of surface TrkB.

View larger version (32K):
[in this window]
[in a new window]
[Download PPT slide]

Figure 6 Role of CaMKII in activity-dependent modulation of cell surface TrkB receptors. Hippocampal neurons were stimulated with TBS in the presence or absence of KN compounds, or pre-treated with peptides for 3 h before TBS stimulation. Cells were processed either for biotinylation assay for cell surface TrkB receptors (A and B) or for surface binding of I¹²⁵-BDNF (C). The numbers associated with each column represent the number of experiments. Asterisk indicates statistically different results (P < 0.05, ANOVA followed by post hoc tests). (A) Examples of biotinylation experiments showing that KN62 (10 µM), KN93 (20 µM), and antp-AIP (20 µM), but not KN92 (20 µM) and antp-AIPscm (20 µM), reduce both p145 and p95 TrkB proteins in TBS-stimulated cultures. (B) Summary of the effects of CaMKII inhibitors on surface TrkB (p145). Controls (TBS in regular medium) were set as 100%. (C) Summary of the effect of CaMKII inhibitors on BDNF surface binding. In both B and C, KN62, KN93, and antp-AIP were all effective, whereas KN92 and antp-AIPscm were not.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

A critical but unresolved question in the neurotrophin researchis how a diffusible molecule such as BDNF achieves preferentialregulation of active neurons or synapses. In our study, we haveinvestigated whether neuronal responsiveness to BDNF is dependenton, or modified by, neuronal activity. Using three independentapproaches, we demonstrate that several forms of tetanic stimulation,but not low frequency stimulation or simple depolarization,promotes the insertion of the BDNF receptor TrkB into the cellsurface of hippocampal neurons. We also show that excitatorysynaptic transmission, Ca²⁺ influx, and activation of CaMKIIare important for the cell membrane insertion of TrkB. Thus,activity-dependent increase in the number of surface TrkB receptorsmay explain why BDNF acts preferentially on active neurons.This study reveals a novel mechanism by which neurotrophin signalingand function may be regulated, and provides a potential linkbetween activity-dependent and BDNF-induced modulation of neuronaland synaptic function in the hippocampus.

In this study, hippocampal neurons were grown for 11–14d. Electrophysiological recording indicated that these neuronswere well connected synaptically (data not shown). We show thatexcitatory synaptic activity plays an important role in regulatingsurface expression of the TrkB receptor tyrosine kinase. Electricstimulation is a more physiological form of stimulation thathas been successfully used to study activity-dependent regulationof signal transduction and gene transcription in cultured hippocampalneurons (Bito et al. 1996; Deisseroth et al. 1996; Fields et al. 1997).LTP-inducing tetanic stimuli enhanced surface expression ofTrkB, whereas blockade of excitatory synaptic transmission inhibitedthe tetanus-induced insertion. Immunocytochemical studies demonstratethat the increase in surface TrkB induced by TBS occurred mostlyon neuronal processes rather than cell bodies. Remarkably, lowfrequency stimulation such as those used to induce LTD, or continuous0.16 Hz (which delivers the same number of pulses as the 100Hz tetanus), had no effect. These results suggest that temporalpattern of neuronal activity and the kinetics of changes inintracellular Ca²⁺ concentrations, rather than the number ofaction potentials or the total amount of Ca²⁺ influx, are thecritical factors for the activity-dependent insertion of TrkBreceptors. Consistent with this idea, simple depolarizationby high K⁺ (Fig. 1 and Fig. 2) or veratridine (data not shown)had no effect on the number of surface TrkB. Using freshly dissociatedretinal ganglion cells as a model, Barres and colleagues demonstratedthat depolarization by high K⁺ or glutamate agonists increasesthe number of cells expressing surface TrkB (Meyer-Franke et al. 1998).The mechanisms underlying the apparent discrepancy remain unclear.A simple explanation is that different types of neurons mayuse different mechanisms to regulate surface expression of TrkB.In the retinal ganglion cells, simple depolarization by highK⁺ may increase intracellular cAMP concentrations, which inturn facilitate the incorporation of TrkB into the surface througha number of unknown steps (Meyer-Franke et al. 1998). In thehippocampal neurons, high frequency stimulation may induce Ca²⁺influx that is qualitatively different from that induced byhigh K⁺, leading to the activation of CaMKII. Alternatively,freshly dissociated retinal ganglion neurons and synapticallyconnected hippocampal neurons (grown for 11–14 d) mayrespond differently to high K⁺. In retinal ganglion cells, highK⁺ may be sufficient to generate the intracellular signals neededto facilitate surface expression of TrkB (Meyer-Franke et al. 1998).In the hippocampal neurons, however, high K⁺ could not producethe specific temporal pattern of neuronal activity and Ca²⁺influx and subsequent CaMKII activation required for the modulation.

Our results suggest that the modulation of TrkB receptors bytetanic stimulation is mediated, at least in part, by high frequencyexcitatory synaptic transmission. We have also demonstratedthat the activity-dependent modulation of TrkB requires Ca²⁺influx. Since Ca²⁺-free medium and Cd²⁺ not only prevent Ca²⁺influx into the postsynaptic neurons through Ca²⁺ channels butalso inhibit transmitter release from presynaptic terminals,it is unclear whether blockade of Ca²⁺ influx directly affectsthe insertion of TrkB receptor into the cell surface, or indirectlyby blocking excitatory synaptic transmission. However, blockadeof NMDA receptors, which are primarily localized in the postsynapticcells rather than presynaptic nerve terminals, also attenuatessurface expression of TrkB (Fig. 3). Moreover, CaMKII appearsto be involved in the activity-dependent insertion of TrkB (Fig. 6).Given that CaMKII has been shown to be important for the insertionof AMPA-type receptors postsynaptically during hippocampal LTP(Hayashi et al. 2000), it is conceivable that similar postsynapticmechanisms may be used for the insertion of the tyrosine kinasereceptor TrkB. It is important to point out, however, that tetanicstimulation does not increase all surface molecules. The surfacep75NR is not increased in neurons stimulated with TBS (Fig. 1D).

One of the remarkable features of the nervous system is thatneuronal activity can modulate synaptic efficacy and connectivityin a local and synapse-specific manner (Stent 1973; Goodman and Shatz 1993;Katz and Shatz 1996; Constantine-Paton et al. 1990). Recentstudies strongly implicate a role of BDNF in activity-dependentsynaptic modulation, such as the formation of ocular dominancecolumns in the visual cortex and hippocampal LTP (Thoenen 1995;Lu and Chow 1999; McAllister et al. 1999). It is important tounderstand how diffusible factors such as BDNF achieve localand synapse-specific modulation, and how BDNF strengthens activesynapses without affecting their neighbors. One such mechanismwould be a localized secretion of BDNF at the site of activesynapses. Although there is some evidence for an activity-dependentsecretion of BDNF (Wang and Poo 1997; Goodman et al. 1996; Heymach et al. 1996),so far local or synapse-specific secretion of any neurotrophinshas not been demonstrated. It is difficult to imagine that locallysecreted factors would not spread to their neighboring, lessactive synapses. Our results demonstrate an alternative andmore practical strategy. Active neurons may respond better toBDNF, and this is achieved by an activity-dependent controlof the number of TrkB receptors on the cell surface. These resultsprovide a molecular basis for the facilitation of BDNF-inducedsynaptic potentiation when coupled to presynaptic depolarizationat the neuromuscular junction (Boulanger and Poo 1999), andthe restricted action of BDNF on highly active synapses in thehippocampus (Gottschalk et al. 1998). In this context, it isimportant to note that the tetanic stimuli such as TBS or tetanicstimulation were capable of modulating TrkB receptors, whereaslow frequency stimulation was not. Since all of our experimentswere done using cultured neurons, their relevance to the BDNFmodulation of hippocampal synaptic plasticity in vivo has yetto be established. Nevertheless, activity-dependent enhancementof the number of surface TrkB receptor may define an importantmechanism by which the specificity of BDNF modulation is achieved.

The results in our study may have general implications in thecell biology of tyrosine kinase receptors. First, we have demonstratedan activity-dependent increase in the number of surface TrkBreceptors in the hippocampal neurons. This is due to an increasein the insertion of TrkB receptors into the neuronal cell surface,rather than an increase in TrkB synthesis or decrease of TrkBinternalization. The mechanisms underlying membrane insertionof TrkB receptors, and tyrosine kinase receptors in general,are largely unexplored. This study may trigger further interestsin investigating the mechanisms for membrane insertion of tyrosinekinase receptors. It will be interesting to examine whethermolecules important for vesicle fusion, such as NSF and SNAP,are involved in the delivery of tyrosine kinases onto cell membrane.Second, we show that the membrane insertion of the TrkB receptorsis enhanced by Ca²⁺ influx. To our knowledge, this is the firstreport for Ca²⁺-dependent modulation of the number of surfacetyrosine kinase receptors. Thus, our results suggest a novelmechanism for cross-talk between Ca²⁺ and tyrosine kinase signalingpathways. Whether the tyrosine kinase activity of the TrkB receptorscan be regulated by intracellular Ca²⁺ is an interesting topicfor future study. Finally, CaMKII has recently been implicatedin the insertion of AMPA-type glutamate receptors onto the postsynapticmembrane of hippocampal neurons (Hayashi et al. 2000). Our studydemonstrates that similar mechanisms are used for the tetanus-inducedincrease in the tyrosine kinase receptor TrkB on the surfaceof hippocampal neurons. It remains to be established whetherCaMKII also regulates the membrane insertion of other tyrosinekinases in neurons and in other cell types.

Acknowledgments

We thank Dr. Phillip Nelson for his valuable advice throughoutthis work, Drs. Doug Fields, Serena Dudek, Lin Mei, and Hao-ChiaChen, as well as the members of the Lu laboratory for criticalcomments on the manuscript. We also thank Regeneron Pharmaceuticalsfor providing recombinant BDNF.

This work is supported in part by a grant from Shanghai Scienceand Technology Commission and National Natural Science Foundationof China.

Submitted: 5 May 2000

Revised: 22 June 2000

Accepted: 17 July 2000

Abbreviations used in this paper: AIP, autocamtide-2-relatedinhibitory peptide; BDNF, brain-derived neurotrophic factor;CaMKII, Ca²⁺/calmodulin-dependent kinase II; CNS, central nervoussystem; CNQX, 6-cyano-7-nitroquinozaline-2,3-dione; kyn, kynurenicacid; LTD, long-term depression; LTP, long-term potentiation;p75NR, low affinity receptor p75; TBS, theta burst stimulation;TTX, tetrodotoxin.

References

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Berninger B. Poo M.-m. Fast actions of neurotrophic factors, Curr. Opin. Neurobiol., 6, 1996, 324–330.[Medline]

Bito H. Deisseroth K. Tsien R.W.. CREB phosphorylation and dephosphorylationa Ca²⁺- and stimulus duration-dependent switch for hippocampal gene expression, Cell, 87, 1996, 1203–1214.[Medline]

Bonhoeffer T.. Neurotrophins and activity-dependent development of the neocortex, Curr. Opin. Neurobiol., 6, 1996, 119–126.[Medline]

Boulanger L. Poo M.m.. Presynaptic depolarization facilitates neurotrophin-induced synaptic potentiation, Nat. Neurosci., 2, 1999, 346–351.[Medline]

Cabelli R.J. Horn A. Shatz C.J.. Inhibition of ocular dominance column formation by infusion of NT-4/5 or BDNF, Science, 267, 1995, 1662–1666.[Abstract/Free Full Text]

Casaccia-Bonnefil P. Carter B.D. Dobrowsky R.T. Chao M.V.. Death of oligodendrocytes mediated by the interaction of nerve growth factor with its receptor p75, Nature, 383, 1996, 716–719.[Medline]

Casaccia-Bonnefil P. Kong H. Chao M.V.. Neurotrophinsthe biological paradox of survival factors eliciting apoptosis, Cell Death Differ, 5, 1998, 357–364.[Medline]

Cohen-Cory S. Fraser S.E.. Effects of brain-derived neurotrophic factor on optic axon branching and remodelling in vivo, Nature, 378, 1996, 192–196.[Medline]

Cohen-Cory S. Lom B.. BDNF modulates, but does not mediate, activity-dependent branching and remodeling of optic axon arbors in vivo, J. Neurosci., 19, 1999, 9996–10003.[Abstract/Free Full Text]

Constantine-Paton M. Cline H.T. Debski E.. Patterned activity, synaptic convergence, and the NMDA receptor in developing visual pathways, Annu. Rev. Neurosci., 13, 1990, 129–154.[Medline]

Deisseroth K. Bito H. Tsien R.W.. Signaling from synapse to nucleuspostsynaptic CREB phosphorylation during multiple forms of hippocampal synaptic plasticity, Neuron, 16, 1996, 89–101.[Medline]

Feng L. Wang C.Y. Jiang H. Oho C. Mizuno K. Dugich-Djordjevic M. Lu B.. Differential effects of GDNF and BDNF on cultured ventral mesencephalic neurons, Mol. Brain Res, 66, 1999, 62–70.[Medline]

Fields R.D. Eshete F. Stevens B. Itoh K.. Action potential-dependent regulation of gene expressiontemporal specificity in ca²⁺, cAMP-responsive element binding proteins, and mitogen-activated protein kinase signaling, J. Neurosci., 17, 1997, 7252–7266.[Abstract/Free Full Text]

Figurov A. Pozzo-Miller L. Olafsson P. Wang T. Lu B.. Regulation of synaptic responses to high-frequency stimulation and LTP by neurotrophins in the hippocampus, Nature, 381, 1996, 706–709.[Medline]

Frade J.M. Rodriguez-Tebar A. Barde Y.A.. Induction of cell death by endogenous nerve growth factor through its p75 receptor, Nature, 383, 1996, 166–168.[Medline]

Frerking M. Malenka R.C. Nicoll R.A.. Brain-derived neurotrophic factor (BDNF) modulates inhibitory, but not excitatory, transmission in the CA1 region of the hippocampus, J. Neurophysiol., 80, 1998, 3383–3386.[Abstract/Free Full Text]

Galuske R.A. Kim D.S. Castren E. Thoenen H. Singer W.. Brain-derived neurotrophic factor reversed experience-dependent synaptic modifications in kitten visual cortex, Eur. J. Neurosci., 8, 1996, 1554–1559.[Medline]

Goodman C.S. Shatz C.J.. Developmental mechanisms that generate precise patterns of neuronal connectivity, Neuron., 10, 1993, 77–98.

Goodman L.J. Valverde J. Lim F. Geschwind M.D. Federoff H.J. Geller A.I. Hefti F.. Regulated release and polarized localization of brain-derived neurotrophic factor in hippocampal neurons, Mol. Cell. Neurosci., 7, 1996, 223–228.

Gottschalk W. Pozzo-Miller L.D. Figurov A. Lu B.. Presynaptic modulation of synaptic transmission and plasticity by brain-derived neurotrophic factor in the developing hippocampus, J. Neurosci., 18, 1998, 6830–6839.[Abstract/Free Full Text]

Gu Q. Liu Y. Cynader M.S.. Nerve growth factor-induced ocular dominance plasticity in adult cat visual cortex, Proc. Natl. Acad. Sci. USA, 91, 1994, 8408–8412.[Abstract/Free Full Text]

Hayashi Y. Shi S.H. Esteban J.A. Piccini A. Poncer J.C. Malinow R.. Driving AMPA receptors into synapses by LTP and CaMKIIrequirement for GluR1 and PDZ domain interaction, Science, 287, 2000, 2262–2267.[Abstract/Free Full Text]

Heymach J.V. Jr. Kruttgen A. Suter U. Shooter E.M.. The regulated secretion and vectorial targeting of neurotrophins in neuroendocrine and epithelial cells, J. Biol. Chem., 271, 1996, 25430–25437.[Abstract/Free Full Text]

Huang Z.J. Kirkwood A. Pizzorusso T. Porciatti V. Morales B. Bear M.F. Maffei L. Tonegawa S.. BDNF regulates the maturation of inhibition and the critical period of plasticity in mouse visual cortex, Cell, 98, 1999, 739–755.[Medline]

Ishida A. Kameshita I. Okuno S. Kitani T. Fujisawa H.. A novel highly specific and potent inhibitor of calmodulin-dependent protein kinase II, Biochem. Biophys. Res. Commun, 212, 1995, 806–812.[Medline]

Kang H. Welcher A.A. Shelton D. Schuman E.M.. Neurotrophins and timedifferent roles for TrkB signaling in hippocampal long-term potentiation, Neuron, 19, 1997, 653–664.[Medline]

Kaplan D.R. Stephens R.M.. Neurotrophin signal transduction by the Trk receptor, J. Neurobiol., 25, 1994, 1404–1417.[Medline]

Katz L.C. Shatz C.J.. Synaptic activity and the construction of cortical circuits, Science, 274, 1996, 1133–1138.[Abstract/Free Full Text]

Kim H.G. Wang T. Olafsson P. Lu B.. Neurotrophin 3 potentiates neuronal activity and inhibits g-aminobutyrateric synaptic transmission in cortical neurons, Proc. Natl. Acad. Sci. USA., 91, 1994, 12341–12345.[Abstract/Free Full Text]

Knipper M. da Penha Berzaghi M. Blochl A. Breer H. Thoenen H. Lindholm D.. Positive feedback between acetylcholine and the neurotrophins nerve growth factor and brain-derived neurotrophic factor in the rat hippocampus, Eur. J. Neurosci., 6, 1994, 668–671.[Medline]

Korte M. Carroll P. Wolf E. Brem G. Thoenen H. Bonhoeffer T.. Hippocampal long-term potentiation is impaired in mice lacking brain-derived neurotrophic factor, Proc. Natl. Acad. Sci. USA, 92, 1995, 8856–8860.[Abstract/Free Full Text]

Korte M. Griesbeck O. Gravel C. Carroll P. Staiger V. Thoenen H. Bonhoeffer T.. Virus-mediated gene transfer into hippocampal CA1 region restores long-term potentiation in brain-derived neurotrophic factor mutant mice, Proc. Natl. Acad. Sci. USA, 93, 1996, 12547–12552.[Abstract/Free Full Text]

Lessmann V. Gottmann K. Heumann R.. BDNF and NT-4/5 enhance glutamatergic synaptic transmission in cultured hippocampal neurons, Neuroreport, 6, 1994, 21–25.[Medline]

Levine E.S. Dreyfus C.F. Black I.B. Plummer M.R.. Brain-derived neurotrophic factor rapidly enhances synaptic transmission in hippocampal neurons via postsynaptic tyrosine kinase receptors, Proc. Natl. Acad. Sci. USA, 92, 1995, 8074–8077.[Abstract/Free Full Text]

Lewin G.R. Barde Y.-A.. Physiology of the neurotrophins, Annu. Rev. Neurosci., 19, 1996, 289–317.[Medline]

Lohof A.M. Ip N.Y. Poo M.M.. Potentiation of developing neuromuscular synapses by the neurotrophins NT-3 and BDNF, Nature, 363, 1993, 350–353.[Medline]

Lu B. Chow A.. Neurotrophins and hippocampal synaptic plasticity, J. Neurosci. Res., 58, 1999, 76–87.[Medline]

Maffei L. Berardi N. Domenici L. Parisi V. Pizzorusso T.. Nerve growth factor (NGF) prevents the shift in ocular dominance distribution of visual cortical neurons in monocularly deprived rats, J. Neurosci., 12, 1992, 4651–4662.[Abstract]

McAllister A.K. Lo D.C. Katz L.C.. Neurotrophins regulate dendritic growth in developing visual cortex, Neuron, 15, 1995, 791–803.[Medline]

McAllister A.K. Katz L.C. Lo D.C.. Neurotrophin regulation of cortical dendritic growth requires activity, Neuron, 17, 1996, 1057–1064.[Medline]

McAllister A.K. Katz L.C. Lo D.C.. Opposing roles for endogenous BDNF and NT-3 in regulating cortical dendritic growth, Neuron, 18, 1997, 767–778.[Medline]

McAllister A.M. Katz L.C. Lo D.C.. Neurotrophins and synaptic plasticity, Annu. Rev. Neurosci., 22, 1999, 295–318.[Medline]

Meyer-Franke A. Kaplan M.R. Pfrieger F.W. Barres B.A.. Characterization of the signaling interactions that promote the survival and growth of developing retinal ganglion cells in culture, Neuron, 15, 1995, 805–819.[Medline]

Meyer-Franke A. Wilkinson G.A. Kruttgen A. Hu M. Munro E. Hanson M.G. Jr. Reichardt L.F. Barres B.A.. Depolarization and cAMP elevation rapidly recruit TrkB to the plasma membrane of CNS neurons, Neuron, 21, 1998, 681–693.[Medline]

Passafaro M. Sala C. Niethammer M. Sheng M.. Microtubule binding by CRIPT and its potential role in the synaptic clustering of PSD-95, Nat. Neurosci., 2, 1999, 1063–1069.[Medline]

Patterson S.L. Abel T. Deuel T.A. Martin K.C. Rose J.C. Kandel E.R.. Recombinant BDNF rescues deficits in basal synaptic transmission and hippocampal LTP in BDNF knockout mice, Neuron, 16, 1996, 1137–1145.[Medline]

Pozzo-Miller L. Gottschalk W.A. Zhang L. McDermott K. Du J. Gopalakrishnan R. Oho C. Shen Z. Lu B.. Impairments in high frequency transmission, synaptic vesicle docking and synaptic protein distribution in the hippocampus of BDNF knockout mice, J. Neurosci., 19, 1999, 4972–4983.[Abstract/Free Full Text]

Prochiantz A.. Getting hydrophilic compounds into cellslessons from homeopeptides, Curr. Opin. Neurobiol., 6, 1996, 629–634.[Medline]

Riddle D.R. Lo D.C. Katz L.C.. NT-4-mediated rescue of lateral geniculate neurons from effects of monocular deprivation, Nature, 378, 1995, 189–191.[Medline]

Stent G.. A physiological mechanism for Hebb's postulate of learning, Proc. Natl. Acad. Sci. USA., 70, 1973, 997–1001.[Abstract/Free Full Text]

Takei N. Sasaoka K. Inoue K. Takahashi M. Endo Y. Hatanaka H.. Brain-derived neurotrophic factor increases the stimulation-evoked release of glutamate and the levels of exocytosis-associated proteins in cultured cortical neurons from embryonic rats, J. Neurochem., 68, 1997, 370–375.[Medline]

Tanaka T. Saito H. Matsuki N.. Inhibition of GABAa synaptic responses by brain-derived neurotrophic factor (BDNF) in rat hippocampus, J. Neurosci., 17, 1997, 2959–2966.[Abstract/Free Full Text]

Thoenen H.. Neurotrophins and neuronal plasticity, Science, 270, 1995, 593–596.[Abstract/Free Full Text]

von Bartheld C.S. Williams R. Lefcort F. Clary D.O. Reichardt L.F. Bothwell M.. Retrograde transport of neurotrophins from the eye to the brain in chick embryosroles of the p75NTR and trkB receptors, J. Neurosci., 16, 1996, 2995–3008.[Abstract/Free Full Text]

Wang X.H. Poo M.M.. Potentiation of developing synapses by postsynaptic release of neurotrophin-4, Neuron, 19, 1997, 825–835.[Medline]

CiteULike

Complore

Connotea

Del.icio.us Add to Digg

Digg

Facebook

Technorati

Twitter What's this?

This Article

	Abstract
	Full Text (PDF, 536K)
	PPT slides of all figures
	Alert me when this article is cited
	Citation Map

Services

	Email this article
	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new content in the JCB
	Download to citation manager

Citing Articles

	Citing Articles via CrossRef
	Citing Articles via Google Scholar

Google Scholar

	Articles by Du, J.
	Articles by Lu, B.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Du, J.
	Articles by Lu, B.


Social Bookmarking

	What's this?