Brain-Derived Neurotrophic Factor Is Released in the Dorsal Horn by Distinctive Patterns of Afferent Fiber Stimulation

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The Journal of Neuroscience, June 15, 2001, 21(12):4469-4477

Brain-Derived Neurotrophic Factor Is Released in the Dorsal Horn by Distinctive Patterns of Afferent Fiber Stimulation
Isobel J. Lever¹, Elizabeth J. Bradbury¹, Joanna R. Cunningham², David W. Adelson³, Martyn G. Jones¹, Stephen B. McMahon¹, Juan Carlos G. Marvizón³, and Marzia Malcangio¹
¹ Neuroscience Research Center and ² Department of Pharmacology, Guy's, King's, and St. Thomas' School of Biomedical Sciences, King's College London, London SE1 1UL, United Kingdom, and ³ CURE: Digestive Diseases Research Center, Neuroenteric Disease Program, Department of Medicine, University of California, Los Angeles, California 90073

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Brain-derived neurotrophic factor (BDNF) is synthesized by small neuron cell bodies in the dorsal root ganglia (DRG) and isanterogradely transported to primary afferent terminals in thedorsal horn where it is involved in the modulation of painfulstimuli. Here we show that BDNF is released in the rat isolateddorsal horn after chemical stimulation by capsaicin or electricalstimulation of dorsal roots. Capsaicin superfusion (1-100 µM)induced a dose-dependent release of BDNF, measured using ELISA.The highest dose of capsaicin also induced a depletion of BDNFprotein in the dorsal horn. BDNF release was also seen after electricalstimulation of the dorsal roots at C-fiber strength. This releasewas encoded by specific patterns of afferent fiber stimulation.Neither continuous low-frequency (480 pulses, 1 Hz) nor tetanichigh-frequency (300 pulses in 3 trains, 100 Hz) stimulation evokedrelease of BDNF, although substance P (SP) release was observedunder both of these conditions. However, BDNF was released aftershort bursts of high-frequency stimulation (300 pulses in 75 trains,100 Hz) along with SP and glutamate. The NMDA antagonist D-AP-5inhibited electrically evoked BDNF release. BDNF release was alsomeasured after systemic or intrathecal NGF treatment. This upregulatedBDNF content in the DRG and increased the capsaicin-evoked releaseof BDNF. Similarly, the amount of BDNF released by burst stimulationwas increased after NGF treatment. This activity-dependent releasecontinued to be encoded solely by this stimulation pattern. Theseexperiments demonstrate that BDNF release in the dorsal horn isencoded by specific patterns of afferent fiber stimulation andis mediated by NMDA receptoractivation.

Key words: neurotrophin release; sensory neurons; capsaicin; burst stimulation; NMDA receptor; nociception

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

There is now good evidence that neuronally derived brain-derived neurotrophic factor (BDNF) contributes to the process ofhippocampal synaptic plasticity via its activity-dependent release(Canossa et al., 1997; Schuman, 1999). It has also been proposedrecently that this neurotrophin might regulate synaptic efficacyin the dorsal horn of the spinal cord (Snider and McMahon, 1998;Woolf and Salter, 2000). BDNF is synthesized by a subpopulationof unmyelinated primary afferents (primarily nociceptors) thatcontain substance P (SP) and glutamate (De Biasi and Rustioni,1988; Apfel et al., 1996; Zhou and Rush, 1996; Conner et al.,1997; Michael et al., 1997). These neurons use glutamate (storedin clear vesicles) as a fast neurotransmitter, but some of themalso release SP from dense-core vesicles when they fire repetitively(Duggan et al., 1995; Marvizón et al., 1997). Like SP, BDNF ispackaged in large dense-core vesicles in dorsal root ganglion(DRG) cells, and it is anterogradely transported to axon terminalsin the dorsal horn (Zhou and Rush, 1996; Conner et al., 1997;Michael et al., 1997). BDNF is found in laminas I and II, theknown termination area for SP-containing C fibers that expressreceptors for capsaicin (VR1) and nerve growth factor (NGF) (TrkA)(Averill et al., 1995; Tominaga et al., 1998). Small fibers arethought to be the major source for BDNF in the superficial laminasof the dorsal horn because after axotomy both small DRG cellsand axon terminals in the superficial laminas downregulate BDNFexpression (Cho et al., 1998; Michael et al., 1999; Zhou et al.,1999). However, BDNF immunoreactive cells are found in the ventralspinal cord white matter (Dreyfus et al., 1999), and descendingnoradrenergic fiber terminals might contribute to BDNF spinalcord pools as reported for some brain areas (Fawcett et al., 1998).The receptor for BDNF, TrkB, is found throughout the dorsal hornwith particularly high density in the superficial laminas (Zhouet al., 1993) where it is associated with dorsal horn cells butnot with afferent terminals (Bradbury et al., 1998). BDNF presentin C-fiber terminals may exert positive modulation of spinal glutamatergicNMDA-mediated nociceptive signaling, sharing this role with SP(Kerr et al., 1999; Woolf and Salter, 2000). Differently, in thebrainstem, BDNF can negatively modulate glutamatergic AMPA-mediatedcurrents in second-order sensory neurons (Balkowiec et al., 2000).Because BDNF is released with activity and in a frequency-dependentmanner in cranial ganglion cells in culture (Balkowiec and Katz,2000), this neurotrophin may play a role in the modulation ofvisceral sensory information in thebrainstem.

Until now, signaling through the TrkB receptor in the dorsal horn was accepted as evidence of BDNF release. We have used anin vitro preparation consisting of dorsal horn slices with attacheddorsal roots (Malcangio and Bowery, 1993; Malcangio et al., 1997)to make direct measurement of BDNF release evoked by electricalstimulation of the roots, as well as chemical stimulation. Concomitantrelease of glutamate and SP has also beenevaluated.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

NGF administration. Adult male Wistar rats (250 gm body weight) were used and killed by decapitation. All procedures werein accordance with United Kingdom Home Office regulations. Humanrecombinant NGF (Genentech, South San Francisco, CA) was administeredto adult rats either systemically (1 mg/kg, s.c., three timesper week for 1-2 weeks) (Malcangio et al., 1997) or intrathecally(Michael et al., 1997) for 14 d (12 µg/d) or 10 d (24 µg/d). Controlanimals received vehicle (saline containing 0.1% rat serum albumin;Sigma, Poole,UK).

Release of BDNF, SP, and glutamate from dorsal horn slices. Horizontal dorsal horn slices (400 µm thick) with dorsal rootsattached were obtained from the lumbar spinal cord of adult ratsas described previously (Malcangio and Bowery, 1993; Malcangioet al., 1997). Only one slice was obtained from each rat, mountedin the central compartment of a three-compartment chamber, andcontinuously superfused (1 ml/min) with oxygenated (95% O₂ and5% CO₂) Krebs' solution containing 0.05-0.1% bovine serum albumin(BSA), 1 µg/ml aprotinin, 0.03 µg/ml cystatin, 0.2 µg/ml bestatin,0.1 mM benzethonium chloride, 1 mM benzamidine, 10 µg/ml leupeptin,1 µM phosphoramidon, 100 µM captopril, 20 µg/ml bacitracin, and6 µM dithiothreitol (Sigma). Experiments were performed at roomtemperature because peptide release was shown previously to bemeasurable but submaximal under these conditions and thus susceptibleto pharmacological manipulation (Malcangio et al., 1997).

BSA and protease inhibitors were added to minimize loss of detectable BDNF-like immunoreactivity (LI) and SP-LI through surfaceadhesion and to prevent degradation. The dorsal roots were placedin the lateral compartments on bipolar platinum electrodes andcovered in mineral oil to avoid dehydration. Before, during, andafter dorsal root stimulation, fractions of 3 or 8 ml of the superfusateswere collected in ice-cooled siliconized tubes (Sigmacote; Sigma)to minimize BDNF-LI loss or in acetic acid (0.1N) to stabilizeSP. Three different stimulation protocols were used: (1) continuousstimulation (CS) for 8 min at 1 Hz (480 pulses) or 1 min at 30Hz (1800 pulses); (2) tetanic stimulation (TS), which was threeor six trains of 100 pulses at 100 Hz separated by 10 sec intervals;and (3) burst stimulation (BS), which was 75 trains of four pulsesat 100 Hz separated by 0.2 sec intervals. Square pulses of 0.5msec duration and 20 V [corresponding to 10-14 mA of current inour conditions (Malcangio and Bowery, 1993)] or 10 mA were usedto recruit C fibers. To selectively stimulate A fibers, pulsesof 0.1 msec duration and 0.1-2 mA were used (Malcangio et al.,2000). In another set of experiments, BDNF release was inducedby superfusing the slices with capsaicin (1-100 µM) at 1 ml/minfor 3 min (Malcangio et al., 1998). Capsaicin was dissolved inethanol (1 mM) and then diluted with modified Krebs' solution.Capsaicin was also superfused at the end of some experiments afterelectrical stimulation had been applied to check the viabilityof thepreparations.

Processing of collected samples. To quantify BDNF-LI and glutamate contents in the same superfusates, samples were desaltedand concentrated by Ultrafree-15 centrifugal device 10K (WatersAssociates, Watford, UK). Retentates were freeze-dried and reconstitutedin 300 µl of block and sample buffer (Promega, Southampton, UK)and 100 µl assayed for BDNF-LI content by ELISA (see below). Filtrateswere used for determining glutamate concentration by HPLC coupledwith o-phthalaldehyde precolumns derivatization and fluorometricdetection (Neal et al., 1994). SP-LI content could not be measuredin the filtrates because the recovery of the peptide through theUltrafree-15 dialysis membrane was <30%. Separate experimentswere performed, and superfusates were used for measuring SP andglutamate contents. Samples were desalted and partially purifiedby using Sep-Pak C₁₈ reverse-phase silica gel cartridges (WatersAssociates) (Malcangio et al., 1997). The cartridges were conditionedwith acetonitrile (100%; HPLC grade; BDH Chemicals, Poole, UK)and trifluoroacetic acid (TFA) (0.1%; HPLC grade; BDH Chemicals).Samples were then loaded into the columns, and the peptide waseluted using acetonitrile/TFA (80:20) solution. The eluates weredried by evaporation under nitrogen (recovery not <85%). Driedsamples were reconstituted in 300 µl of phosphate buffer and 100µl assayed by radioimmunoassay in duplicate (1.3 pg/100 µl assaysensitivity) using scintillation proximity assay (Amersham PharmaciaBiotech, Buckinghamshire, UK) as described previously (Malcangioand Bowery 1993; Malcangio et al., 1997). The remaining 100 µlof reconstituted samples were used for glutamate content determinationby HPLC (seeabove).

BDNF tissue extraction. DRG were harvested from both naïve and NGF-treated rats and processed to extract detectable levelsof BDNF-LI using ELISA (see below). Several methods were usedto maximize BDNF recovery from the tissue. A cocktail of proteaseinhibitors was added to the homogenization buffer to reduce enzymaticbreakdown of BDNF [137 mM NaCl, 20 mM Tris-HCl, 1% NP-40, 10%glycerol, 0.1% BSA, 1 mM $alpha$ -toluenesulfonil fluoride, 10 µg/mlaprotinin, 0.5 mM sodium vanadate (Sigma)]. Samples were keptat 4°C to slow down proteolytic activity. Non-ionic detergents(NP-40) were added to the buffer, to both aid tissue dissociationand prevent nonspecific adsorption of BDNF. BSA (1 mg/ml) wasadded in the homogenization buffer to provide soluble bindingsites for BDNF. Tissue samples were acidified for 15 min becausethis has been reported to aid dissociation of bound trophic factorsfrom their receptors (Okragly and Hakk-Frendscho, 1997). In ourconditions, BDNF-LI content in DRG (four per rat) increased from20.9 ± 5.6 to 55.0 ± 5.6 pg/mg protein (n = 4 rats per group)after acidification. Samples were neutralized and centrifugedto remove particulates and then diluted 1:10 with assay bufferto prevent interference with the ELISA (see below). Protein contentwas determined by the Bradfordassay.

BDNF ELISA. Nunc (Roskilde, Denmark) MaxiSorp 96-well plates were used. BDNF standards (100 µl of 4-500 pg/ml solutions) and100 µl of unknown samples were run in duplicate and triplicate,respectively, following a protocol slightly modified from theinstructions of the manufacturer (Emax ImmunoAssay kit; Promega)(Son et al., 1999; Cejas et al., 2000). The plates were incubatedfor 48 hr with the monoclonal primary antibody. A standard curvewas run for each plate, and this was linear at all levels of detection(r² = 0.994 ± 0.002; n = 10). In each plate, some wells were spikedand DRG extracts were also run because they would contain moreBDNF and prove that the assay was adequate to distinguish amongdifferent BDNF levels: from zero, to modest (>4 pg/ml), moderatelyhigh (20 pg/ml), and high (DRG extracts, 100 pg/ml). Samples wereconsidered BDNF positive when their signal was higher than thebackground signal (modified Krebs' solution) and within the rangeof the standardcurve.

The assay showed <3% cross-reactivity with human recombinant NGF. Human recombinant BDNF standard was used to assess BDNFrecovery. This was determined by adding 5-20 pg/3 ml BDNF to modifiedKrebs' solution (see above) that had not been superfused throughdorsal horn tissue and then processing under the same conditionsas experimental samples. Recovery was 60% for 10 pg/3 mlBDNF.

Data calculation and statistical analysis of release data. The data are presented as mean ± SEM. ANOVA, followed by Tukey'sor Dunnett's tests, and Student's t test were used whenappropriate.

Neurokinin-1₁ receptor internalization. Neurokinin-1 (NK₁) receptor internalization in lumbar spinal cord slices obtainedfrom 14- to 30-d-old rats was assessed in transverse slices (400µm) with one dorsal root attached (Marvizón et al., 1997, 1999).After electrical stimulation at the root (300 pulses, BS; seeabove), slices were fixed and cryoprotected. Sections (25 µm)were immunostained for NK₁ receptor (Marvizón et al., 1997, 1999).Internalization was quantified as the percentage of NK₁ receptor-IRneuronal somas showing internalization (Marvizón et al., 1997,1999). All NK₁ receptor-IR somas in at least three sections perslice were counted by a person blinded to the treatment. Confocalimages were acquired with a Leica (Nussloch, Germany) TCS-SP confocalmicroscope.

BDNF immunostaining in the dorsal horn. After the release experiments, tissue was post-fixed in 4% paraformaldehyde (2 hrat 4°C), cryopreserved in 20% sucrose (overnight at 4°C), andblocked in OCT embedding compound (BDH Chemicals), and transversesections (20 µm) were cryostat cut. Sections were immunostainedfor BDNF using indirect tyramide signal amplification (DuPontNEN, Boston, MA) (Michael et al., 1997). Sections were incubatedwith the following (all reagents were diluted in PBS containing0.2% Triton X-100): normal goat serum (10%, 1 hr), rabbit polyclonalanti-BDNF (0.4 µg/ml, 12 hr; a gift from Amgen, Thousand Oaks,CA), biotin-conjugated goat anti-rabbit antibody (1:400, 2 hr;Vector Laboratories, Burlingame, CA), avidin-biotin complex (1:5with no Triton X-100, 30 min; Vector Laboratories), biotinyl tyramide(1:75, 10 min; DuPont NEN), and FITC-conjugated extra-avidin (1:500,2 hr; Sigma, St Louis, MO). Slides were coverslipped in Vectashieldmounting medium (Vector Laboratories) and visualized under a Leitz(Wetzlar, Germany) fluorescent microscope. For quantification,images of BDNF staining in the dorsal horn of naïve and capsaicin-treatedrats (n = 4 per group) were captured using a Hamamatsu (Bridgewater,NJ) digital camera. The intensity of BDNF immunostaining in thesuperficial laminas from four sections per animal was quantifiedusing SigmaScan image analysis software (SPSS, Chicago,IL).

Electrophysiology. The tibial nerve of anesthetized adult male Sprague Dawley rats (280 gm body weight) was exposed, and theuncut nerve was placed on a bipolar tungsten stimulating electrodeimmediately proximal to the ankle in a pool of warm mineral oil.A bipolar platinum wire (diameter of 30 µm) recording electrodewas positioned above the nerve 5-7 mm proximal to the stimulatingelectrode. A noxious heat stimulus was used to locate nociceptivefibers having receptive fields in the footpad. Successive finenerve filaments (10-15 µm diameter) were dissected from the nerveuntil one was obtained containing a unit responsive to heatingof the footpad to 47-48°C using a Peltier-effect thermal stimulator(1 cm square element; courtesy of Dr. Bruce Naliboff, Universityof California, Los Angeles, CA). The response to noxious heatingwas tested, and the plantar surface was explored for mechanosensitivereceptive fields using a blunt probe and calibrated von Frey typestimulators (Stoelting Inc., Kiel, WI). At least 10 min afterthe final stimulus, capsaicin (100 mg/100 ml) was injected subdermallyinto the footpad, and the response was recorded. At the end ofexperiments, the tibial nerve was cut proximal to the recordingelectrode, and the nerve was stimulated to determine conductionvelocities for the units recorded. Single-unit records were obtainedvia sorting of multiunit activity (one to six units typically)using Spike2 software (Cambridge Electronic Design, Cambridge,UK). For one fiber, a reliable conduction velocity could not bedetermined and its identity as a C fiber was inferred from itsspikewaveform.

Receptor antagonists. D( $-$ )2-Amino-5-phosphonopentanoate (D-AP-5) and 6-cyano-7-nitro-quinoxaline-2,3-dione (CNQX) were fromResearch Biochemicals (Natick, MA). Naloxone was from Sigma. ( $-$ )Bicucullinemethobromide was from Tocris Cookson (Bristol,UK).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrically evoked release of BDNF in the dorsal horn

Because BDNF and nociceptive peptides are colocalized in some C fibers (Michael et al., 1997), BDNF-LI release in dorsal hornwas first examined using a pattern of sensory neuron electricalstimulation known to induce SP-LI release, an indication of highthreshold fiber recruitment (Malcangio et al., 2000). Glutamaterelease was also evaluated in the same samples, although bothA and C fibers contribute to its release (Kangrga and Randiç,1991; Teoh et al., 1996).

As shown previously (Malcangio and Bowery, 1993; Malcangio et al., 1997), CS of the dorsal roots at C-fiber strength and lowfrequency (1 Hz, 480 pulses in 8 min) was effective at releasingSP-LI but did not lead to detectable release of BDNF-LI or glutamate(Fig. 1A). The lack of glutamate detection in this set of experimentsmay be explained by fast uptake of the amino acid by both neuronsand glia. The absence of BDNF-LI release could have been the consequenceof poor tissue penetrability and/or loss of detectable BDNF-LIthrough surface adhesion (Leibrock et al., 1989; Anderson et al.,1995). However, in this study, BSA addition in the superfusionbuffer and sample collection in siliconized tubes resulted inBDNF-LI basal outflow values that were in the range of those foundin hippocampal slice perfusates (Canossa et al., 1997).

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Figure 1. BDNF-LI, SP-LI, and glutamate (GLU) were released in the dorsal horn by different patterns of afferent fiber stimulation. Basal (B), high-threshold fiber strength-stimulated (S) and recovery (R₁ and R₂) fractions were collected at a rate of 1 ml/min for 8 (A) or 3 (B, C) min. Basal values (B) represent the mean of BDNF content in three fractions collected before the stimulated fraction (S). R₂ values represent content in two fractions collected after the first recovery fraction (R₁). Dorsal root stimulation was at high-threshold fiber strength (20 V or 5 mA, 0.5 msec) and was started at the beginning of the collection of the S fraction. A, CS of the dorsal roots at low frequency (1 Hz, 480 pulses, 8 min) induced SP-LI (n = 4 slices), but not BDNF-LI (n = 4 slices) or glutamate, release (n = 4 slices). B, TS (300 pulses in 3 trains, 100 Hz) evoked the release of SP-LI (n = 6 slices) and glutamate (n = 4 slices) but not of BDNF-LI (n = 7 slices). C, BS (300 pulses in 75 trains, 100 Hz) induced release of BDNF-LI (n = 6 slices), SP-LI (n = 7 slices), and glutamate (n = 4 slices). Values (means ± SE) express concentrations in reconstituted samples. *p < 0.05 versus both B and R₂ fraction values (ANOVA, followed by Tukey's test).

High-frequency stimulation (100 Hz, three trains of 100 pulses) of primary afferent fibers evokes long-term potentiation (LTP)of their synapses with dorsal horn neurons (Randiç et al., 1993;Liu and Sandkühler, 1998). The same pattern of stimulation wasvery effective in evoking SP-LI release in the dorsal horn (Marvizónet al., 1997), which may participate in this form of LTP (Liuand Sandkühler, 1997). We applied the same stimulation pattern(TS, 300 pulses at 100 Hz in three trains separated 10 sec) tothe dorsal roots to test whether it was able to evoke BDNF release.Significant release of SP-LI and glutamate was detected (Fig.1B). BDNF-LI release was not detected even after 600 pulses weredelivered at 100 Hz in six trains (basal outflow was 8.0 ± 0.8pg/ml; release was 8.3 ± 0.2 pg/ml; n = 3; p > 0.05). Likewise,1800 pulses delivered at 30 Hz as a single 1 min train did notproduce any significant BDNF-LI release (11.2 ± 0.5 pg/ml) overbasal (10.7 ± 0.01 pg/ml; n = 3; p > 0.05). In vivo, C fiberstend to fire in short bursts of high frequency in response toseveral forms of noxious stimulation (see below) (Puig and Sorkin,1995; Adelson et al., 1996, 1997). Therefore, we stimulated thedorsal roots with the same number (300) of high-intensity pulsesused for TS but delivered in 75 trains (bursts) of four pulsesat 100 Hz, separated by a 0.2 sec interburst interval (BS). Asshown in Figure 1C, BS induced significant release of BDNF-LI,SP-LI, and glutamate. Interestingly, whereas the release of glutamatepeaked during the BS period, SP-LI release persisted after stimulation(first recovery, R₁) and BDNF release was significant in the firstrecovery fraction (Fig. 1C) and then returned to basal values.BDNF-LI release evoked by BS was intensity dependent (Fig. 2A)and occurred only above the intensity threshold to recruit C fibers(5-10 mA), remaining constant at higher stimulation strengths.Electrically evoked BDNF-LI release (basal outflow increased to240 ± 37.9% at 10 mA intensity) was comparable with glutamate-inducedBDNF-LI release in hippocampal slices (Canossa et al., 1997).However, activity-induced BDNF-LI release in the hippocampus wasnot dependent on extracellular Ca²⁺ (Canossa et al., 1997), whereas BDNF-LI release in the dorsalhorn was abolished in Ca²⁺-free medium (Fig. 2B). To further ascertain that BDNF releasewas attributable to nerve impulse conduction, experiments wereperformed in the presence of tetrodotoxin (TTX), which abolishedelectrically evoked BDNF-LI release but did not modify basal outflow(Fig. 2C).

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Figure 2. Intensity dependence of BS-induced BDNF release (A). BS was applied at intensities and durations ranging from A-fiber (0.1-1 mA, 0.1 msec) to C-fiber (5-10 mA, 0.5 msec) strength. Numbers inside columns indicate the number of slices. *p < 0.05 versus basal values (B) (ANOVA, followed by Dunnett's test). B, Calcium dependence of BS-induced BDNF release. BS induced the release of BDNF-LI in the presence of Ca²⁺ ions ( $black-triangle$ ) but not when slices were superfused with Ca²⁺-free Krebs' solution containing 10 mM EDTA ( $black-square$ ). BS (300 stimuli; 10 mA, 0.5 msec, 100 Hz) was applied (arrow) after collection of two basal outflow fractions. Points represent means ± SE of four slices. *p < 0.05 versus analog fractions collected in the presence of Ca²⁺ (ANOVA, followed by Tukey's test). C, TTX superfusion blocked BS-induced BDNF release without changing basal outflow. TTX (2 µM) was superfused during the last 2 min of the third fraction (basal) and the first minute of the fourth fraction (stimulated) (; n = 4 slices). Four slices were run in the absence of TTX as controls ( $black-triangle$ ). BS (300 stimuli; 10 mA, 0.5 msec, 100 Hz) was applied (arrow) after collection of three basal outflow fractions. Points represent means ± SEM. *p < 0.05 versus analog fractions collected in the presence of TTX (ANOVA, followed by Tukey's test).

To confirm that BS of the dorsal roots recruited some C fibers, SP release was indirectly assessed via NK₁ receptor activationin spinal cord transverse slices (Marvizón et al., 1997). BSof the dorsal root produced NK₁ receptor internalization in themajority (Fig. 3B,C) of the NK₁ receptor-immunoreactive neuronsin laminas I and II_o of the stimulated side of the slices butnot in the contralateral side or in deeper laminas (Fig. 3A,C).

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Figure 3. BS produces NK₁ receptor internalization in the dorsal horn. Confocal images of the contralateral (A; 10 optical sections) and the stimulated (B; 3 optical sections) side of a representative slice. Insets, Higher magnification of the neurons in the rectangles (8 optical sections in A; 5 optical sections in B). Scale bar: 50 and 16 µm for low- and high-magnification, respectively. I, II, and III indicate the location of Rexed's laminas. C, Percentage of NK₁ receptor-immunoreactive (NK₁R-ir) neuronal somata in laminas I-II_o with internalization after BS; mean ± SEM of four slices obtained from two rats. ***p < 0.0001 (t test).

Electrically evoked release of BDNF in the dorsal horn after NGF treatment

Primary afferent fibers expressing TrkA receptor can retrogradely transport NGF produced by their target cells to the DRGcells in which NGF can stimulate the expression of BDNF (Apfelet al., 1996; Michael et al., 1997). Thus, we investigated whetherNGF induced alterations in BDNF content, and these were reflectedin altered release in the dorsalhorn.

Figure 4A shows that both systemic and intrathecal NGF treatments increased BDNF-LI content in the DRG of approximately threefold.In addition, when cords from NGF-treated rats that upregulatedBDNF were used, enhanced amount of BDNF-LI was released in thedorsal horn after BS (Fig. 4B). BDNF-LI basal outflow was unchanged,and TS was still ineffective in eliciting BDNF-LI release in bothNGF-treated and nontreated rats (Fig. 4B). Thus, TS effectivenessin evoking BDNF release was not increased by increasing the amountof BDNF available.

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Figure 4. A, NGF treatment upregulated BDNF-LI content in DRG. NGF and control vehicle (Con) (saline plus 0.1% rat serum albumin) were administered either systemically (NGF-s; 1 mg/kg 3 times per week for 1 or 2 weeks) or intrathecally (NGF-it; 12 µg/d for 14 d or 24 µg/d for 10 d), and BDNF content in the DRG was measured by ELISA (see Materials and Methods). B, NGF treatment increased the amount of BDNF-LI released over basal outflow (white columns) evoked by BS of the dorsal roots (striped columns). TS was still ineffective after NGF treatment (white and black columns indicate basal and stimulated fractions, respectively). Both BS and TS consisted of 300 pulses of 10 mA or 20 V, 0.5 msec, given at 100 Hz in 75 (BS) or three (TS) trains. *p < 0.05 versus basal values; #p < 0.05 versus BS-evoked release in controls (ANOVA, followed by Tukey's test). Numbers inside columns indicate number of animals per slice.

Capsaicin-induced release of BDNF in the dorsal horn in naïve and NGF-treated rats

Peripheral noxious stimuli can cause bursting activity in fine afferent fibers (Puig and Sorkin, 1995; Adelson et al., 1996,1997). Thus, we evaluated whether the chemical irritant capsaicininjected into the paw would induce a similar pattern of activityin C fibers. Using a thermal moderately noxious heat search stimulus(ramp to 47-48°C via a Peltier-effect thermal stimulator, 1 cmsquare element) we surveyed dissected thin filaments (10-15 µmdiameter) of the tibial nerve until we isolated one containinga heat-sensitive C unit having a receptive field in the footpad.We tested the responses to the heating ramp several times (Fig.5B) and explored the mechanosensitivity of the units. Capsaicin(20-25 µl, 100 mg/ml) injected into the footpad adjacent to theheat-sensitive receptive field produced bursting activity (Fig.5A,C,D) in three of three experiments. Capsaicin can stimulatepolymodal nociceptors to release their contents and, when superfusedthrough the dorsal horn preparation, can dose dependently releaseSP-LI (EC₅₀ of 100 nM) (Malcangio et al., 1993, 1998). Thus, inthis study, the ability of capsaicin to release BDNF-LI from thedorsal horn was evaluated. Figure 6A shows that capsaicin dosedependently released BDNF-LI but at higher doses than those effectivein releasing SP. The highest dose (100 µM) induced a significantrelease of BDNF-LI during superfusion (fourth fraction) comparedwith basal outflow (first three fractions) (Fig. 6B). The releasepersisted in the following (fifth) fraction, and then BDNF-LIvalues recovered to basal (Fig. 6B). Capsaicin-induced BDNF-LIrelease was abolished by cosuperfusion of capsazepine (100 µM)(Fig. 6B). The doses of capsaicin necessary to release BDNF wereunexpectedly high, so we tested whether capsaicin would be moreeffective if BDNF contents were increased by NGF treatment, whichwould have also increased nociceptor sensitivity to capsaicin(Winter et al., 1988). Figure 6C shows that capsaicin (1 µM) significantlyreleased BDNF in spinal cords of rats treated with NGF but wasineffective in controls. We then examined slices after high-dosecapsaicin superfusion to determine whether this noxious stimulusled to BDNF depletion. Superfusion of capsaicin (300 µM) produceda significant loss of BDNF immunoreactivity throughout the dorsalhorn (Fig. 7B) compared with control slices that displayed theexpected dense BDNF immunostaining in laminas I and II (Fig. 7A).Simultaneous staining of control and experimental slices revealeda 40% reduction in BDNF labeling after capsaicin treatment (Fig.7C). To check that this decrease in BDNF immunoreactivity wasnot attributable to nonspecific terminal damage caused by capsaicinsuperfusion, we stained adjacent sections for a primary afferentmarker. Staining of the isolectin B4 revealed no difference betweencapsaicin and control sections, indicating that binding siteswere still present in the tissue (data not shown).

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Figure 5. Intraplantar injection of capsaicin induces bursting discharge in nociceptors. A, Instantaneous frequency plot of burst discharge of a heat-sensitive C nociceptor in response to subdermal injection of 100 µg/100 µl capsaicin (CAPS; rectangle indicates the duration of the injection). B, Response of the same unit as in A to repeated heating to 47.6°C (bottom trace indicates the temperature ramp). C, A different type of bursting discharge in another heat-sensitive C nociceptor evoked by subdermal injection of 100 µg/100 µl capsaicin (first rectangle indicates the duration of the injection). D, Detail of period of discharge indicated by second (bold) rectangle in C.

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Figure 6. Superfusion of dorsal horn slices with capsaicin induced BDNF release. A, Capsaicin (Caps; superfused for 3 min) dose dependently released BDNF. Values are obtained from at least four slices for each dose. *p < 0.05 versus basal outflow (B) (ANOVA, followed by Dunnett's test). B, Superfusion of dorsal horn slices with capsaicin (Caps; 100 µM, black horizontal bar) during collection of the fourth fraction (3 min) caused significant release of BDNF-LI in the fourth and fifth fractions (n = 6 slices). BDNF release returned to basal afterward. Superfusion of capsazepine (Cpz; 100 µM; white horizontal bar; n = 4 slices) one fraction before and during capaicin superfusion blocked BDNF release. C, Capsaicin (Caps; 1 µM)-induced release of BDNF-LI over basal outflow (B) was increased after NGF pretreatment (n = 10 slices). *p < 0.05 (Student's t test versus basal values); #p < 0.05 versus capsaicin in controls (n = 6 slices).

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Figure 7. Capsaicin superfusion induced depletion of BDNF immunostaining in the dorsal horn. BDNF-IR in the dorsal horn of a naïve dorsal horn slice (A) and a slice superfused with 300 µM capsaicin for 3 min (B). In control slices (A), BDNF is present in fibers (probably primary afferent terminals) in laminas I and II, being particularly abundant in the medial portion. After capsaicin treatment (B), there is a marked reduction in BDNF immunoreactivity in the superficial dorsal horn (arrows in B). C, Quantitative analysis (see Materials and Methods) confirms a significant reduction in BDNF immunoreactivity after capsaicin treatment. *p < 0.05 (Student's t test; n = 4 dorsal horn slices in each group).

Modulation of electrically evoked release of BDNF in the dorsal horn

It has been shown previously that SP and glutamate release from primary afferent terminals in the dorsal horn are modulatedby glutamate acting on NMDA receptors located presynaptically(Liu et al., 1997; Marvizón et al., 1997; Malcangio et al., 1998).The possibility that glutamate released after BS of the dorsalroots controlled the release of BDNF was tested by assessing theeffect of antagonists for NMDA and non-NMDA receptors on evokedBDNF release. Figure 8A shows that, in control dorsal horn slices,BS of primary afferent fibers induced a significant and reversiblerelease of BDNF-LI (9-12 min time interval) over basal outflow(3-9 min time interval). However, superfusion of the NMDA receptorantagonist D-AP-5 significantly inhibited BS-induced release ofBDNF-LI (Fig. 8A). In contrast, the presence of the non-NMDA antagonistCNQX did not inhibit BS-induced release of BDNF-LI (Fig. 8A).These data indicate that BDNF release, like SP release, is likelyto be modulated by glutamate activating NMDA receptors, whereasnon-NMDA receptors are not involved.

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Figure 8. Pharmacological modulation of BS-induced release of BDNF-LI. Burst stimulation (300 stimuli; 10 mA, 0.5 msec, 100 Hz) was applied (arrow) during collection of the fourth fraction. In control slices ( $black-triangle$ ; n = 9), BS induced significant and reversible release of BDNF over basal outflow (first 3 fractions) (A, B). Superfusion of D-AP-5 (50 µM; n = 5) in the fractions before, during, and after stimulation (horizontal white bar) inhibited evoked release of BDNF-LI (A). Superfusion of CNQX (A; 5 µM; n = 4), naloxone (B, NAL; 1 µM; n = 7), or ( $-$ ) bicuculline methobromide (B, BIC; 100 µM; n = 5) did not modify BDNF-LI release. *p < 0.05, stimulated (fourth fraction) versus correspondent basal outflow fractions (first plus second or third fractions); ANOVA, followed by Tukey's test.

Importantly, SP release from primary afferent terminals in the dorsal horn is also under the inhibitory control of endogenousopioid and GABAergic systems that counteract NMDA-evoked facilitation(Jessell and Iversen, 1977; Malcangio et al., 1993; Teoh et al.,1996). Thus, we tested the effect of naloxone and bicuculline(antagonists for µ and GABA_A receptors, respectively) on BS-inducedBDNF release and found that neither antagonist could modify theevoked release (Fig. 8B). These findings fail to support the possibilitythat BS of primary afferent fibers activates endogenous dorsalhorn inhibitory systems sufficiently to affect BDNFrelease.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

BDNF may act as a modulator of synaptic transmission in the spinal dorsal horn (Snider and McMahon, 1998; Woolf and Salter,2000), as found previously in the hippocampus (Canossa et al.,1997; Schuman, 1999). To understand the action of BDNF in thecord, it is important to establish what type of stimuli are effectiveat releasing BDNF. Here we report that BDNF-LI release from thedorsal horn is evoked by capsaicin and electrical stimulationof the dorsal roots. We have used several protocols of electricalstimulation, and we found that BDNF release was dependent on thepattern of stimulation of primary afferents. Thus, dorsal rootstimulation with short bursts of high-frequency pulses (BS) evokedBDNF release, whereas sustained stimulation at low frequency (1Hz, CS) or high frequency (100 Hz, TS) failed to produce any measurablerelease. Remarkably, CS or TS were unable to evoke any BDNF release,even when the number of pulses was increased well above thoseused for BS. Moreover, TS was ineffective even when the BDNF contentwas increased by NGF treatment, indicating that the pattern ofstimulation of primary afferent fibers is the main determinantof BDNF release. BS-induced BDNF release was greatly increasedafter NGF treatment, probably because of an increased BDNF contentin C fibers expressing the TrkA receptor. However, it cannot beexcluded that prolonged treatment with NGF might have enhancedafferent fiber excitability, for example by sodium channel induction(Toledo-Aral et al., 1995).

The physiological relevance of these findings is underscored by the transition of C fibers to a bursting firing pattern whenthe intensity of nociceptive stimuli increases over a certainthreshold (Puig and Sorkin, 1995; Adelson et al., 1996, 1997).We show that C fibers in the tibial nerve develop bursting activityafter an injection of capsaicin into the footpad. Other studieshave shown C-fiber bursting activity in visceral nerves in responseto hydrogen peroxide (Adelson et al., 1996) or bradykinin (Adelsonet al., 1997). Therefore, certain noxious stimuli may producebursting activity in C fibers, which in turn elicits BDNF releasein the dorsalhorn.

BS of the dorsal roots was also able to evoke the release of SP in the dorsal horn preparation. Previous studies (Go and Yaksh,1987; Duggan et al., 1995; Marvizón et al., 1997) have shownthat SP release is facilitated at high frequencies of stimulation,although it also occurs if enough pulses are given at low frequency(Malcangio and Bowery, 1993; Allen et al., 1999). Interestingly,unlike BDNF, approximately the same amount of SP-LI release waselicited by TS and BS. Confirming this, BS (Fig. 3) and TS (Marvizónet al., 1997) produced similar amounts of NK₁ internalizationin the superficial dorsal horn, an indicator of NK₁ receptor activationby released tachykinins. CS also produced a substantial amountof SP release. Hence, SP appears to be released by a wider rangeof firing patterns than BDNF. This observation is somewhat surprisinggiven the fact that SP and BDNF are likely to be present in thesame population of primary afferent fibers (Michael et al., 1997)and may be both packaged in large, dense-core synaptic vesicles.Alternatively, BDNF may be stored in a different population ofdense-core vesicles that undergo exocytosis after BS, which mightlead to a substantial buildup of calcium concentrations in presynapticterminals. (Muschol and Salzberg, 2000) Indeed, BS-evoked releaseof BDNF was Ca²⁺ dependent and returned to basal levels after stimulation, suggestingthat it was produced by a synaptic mechanism and was not attributableto electropermeabilization of neuronal membranes. Moreover, electricallyevoked release of BDNF was inhibited by TTX perfusion, indicatingthat the release was a consequence of neuronal activity involvingvoltage-dependent Na⁺ channels. In contrast, BDNF basal outflow was neither calciumdependent nor modified by TTX superfusion and was likely to beunrelated to neuronal firing. The observation that NGF treatmentdid not increase BDNF basal outflow further supports thisidea.

Importantly, BDNF release evoked by BS of the dorsal roots was associated with glutamate release, inhibited by the NMDA receptorantagonist D-AP-5 but not by the non-NMDA antagonist CNQX, indicatingthat glutamate stimulates BDNF release by activating NMDA receptorsin the dorsal horn. However, TS did not produce significant BDNFrelease but increased extracellular glutamate content, suggestingthat glutamate alone is not sufficient to induce BDNF release.Glutamate also stimulates SP release from primary afferent terminalsby putatively activating presynaptically located NMDA receptors(Liu et al., 1997; Marvizón et al., 1997; Malcangio et al., 1998).Thus, one explanation for our findings would be that BDNF releaseis modulated by presynaptic NMDA receptors, which have been foundin the central terminals of primary afferents (Liu et al., 1994).Alternatively, postsynaptic NMDA receptors may stimulate BDNFrelease by triggering the release of diffusible retrograde messengers(such as nitric oxide) from dorsal horn cells. Synaptic transmissionbetween primary afferents and dorsal horn neurons is primarilydriven by AMPA receptors (Gerber and Randiç, 1989; Yoshimuraand Jessell, 1990; Randiç et al., 1993; Yoshimura and Nishi,1993), with NMDA receptors contributing only a small componentof the EPSP. Therefore, our observation that the AMPA receptorantagonist CNQX did not inhibit BS-evoked BDNF release suggeststhat BDNF is likely to be mainly released from primary afferentterminals, although we cannot rule out entirely that BDNF wasreleased from dorsal horn neurons. Although GABA_A and opioid receptorsplay an important role in modulating nociceptive signals in thedorsal horn (Millan, 1999), these inhibitory mechanisms do notappear to modulate BDNF release, because it was not altered bythe GABA_A antagonist bicuculline or the opioid antagonistnaloxone.

Our findings suggest that different patterns of stimulation of primary afferents may encode the release of different transmitters.Notably, neuropeptide release is likely to depend on stimulationfrequency (Bartfai et al., 1986), whereas neurotrophin releaseappears to depend on the pattern of stimulation, which may becritical for the activation of specific transmission pathwaysto evoke BDNF release. One consequence may be that different transmitters-modulatorsare released in different pain states, which would have importantimplications for analgesictherapy.

Our data are consistent with a recent report (Balkowiec and Katz, 2000) showing that BDNF is released from cultured neonatalnodose and petrosal ganglia (NPG) neurons by high-frequency burstfield stimulation but not short-term KCl depolarization. Theseauthors suggested that the magnitude of BDNF release in NPG neuronsdepended on the pattern and frequency of stimulation. Likewise,we show that stimulus pattern-dependent release of BDNF occursin the dorsal horn of the spinal cord, under conditions that resemblenociceptive sensory neuronactivation.

BDNF release was also evoked by capsaicin, and BDNF immunoreactivity measured in situ in the dorsal horn was substantiallyreduced after capsaicin application, indicating that primary afferentBDNF pools can be readily depleted. Concentrations of capsaicinnecessary to stimulate BDNF release (1-100 µM) were higher thanthose that release SP under the same experimental conditions (EC₅₀of 100 nM) (Malcangio et al., 1997), which raised the issue ofspecificity of the action of capsaicin (Bevan and Szolcsanyi,1990). Although VR1 and SP have been shown to colocalize (Tominagaet al., 1998), no such data exist for BDNF, and the effect ofcapsaicin might be indirect, for example, mediated by glutamaterelease and nitric oxide production. Capsazepine prevented BDNFrelease, however, suggesting that the effect of capsaicin wasattributable to VR1 activation. Moreover, after NGF treatment,capsaicin significantly released BDNF at a dose (1 µM) that isclose to its affinity for VR1 receptors (Caterina et al., 1997).

The release of BDNF in the dorsal horn may have important physiological consequences. Existing evidence suggests that BDNFparticipates in central sensitization and inflammatory pain states(Kerr et al., 1999; Mannion et al., 1999). Moreover, BDNF increasesthe excitability of nociceptive spinal reflexes and potentiatesNMDA receptor-mediated responses in the dorsal horn (Kerr et al.,1999). However, there is evidence suggesting that chronic spinaldelivery of BDNF alleviates allodynia and hyperalgesia in neuropathicrats (Cejas et al., 2000). Furthermore, BDNF is antinociceptivein normal and inflamed rats when injected into the brainstem (Siuciaket al., 1994, 1995) where this neurotrophin can strongly inhibitAMPA-mediated currents via TrkB receptor activation (Balkowiecet al., 2000). Thus, the action of BDNF is likely to be complexand dependent on the specific site within nociceptivepathways.

In summary, this study shows that BDNF is released by specific patterns of stimulation of afferent fibers and is mediatedby NMDA receptor activation. These data support the idea thatendogenous BDNF plays a role in the modulation of nociceptivestimuli in the dorsalhorn.

  FOOTNOTES

Received Jan. 19, 2001; revised March 13, 2001; accepted March 26, 2001.

This work was supported by a Wellcome Trust Career Development Fellowship (to M.M.). S.B.M. and E.J.B. thank the WellcomeTrust for support. We thank Drs. Reg Docherty, Tim Boucher, andGreg Michael for helpful discussion, Drs. Emeran A. Mayer andYvette Taché for their support, and Viv Cheah for technicalassistance.
Correspondence should be addressed to Marzia Malcangio, Sensory Function, Center for Neuroscience, Hodgkin Building, King'sCollege London, Guy's Campus, London Bridge, London SE1 1UL, UK.E-mail: marzia.malcangio{at}kcl.ac.uk.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Adelson DW, Wei JY, Kruger L (1996) H₂O₂ sensitivity of afferent splanchnic C fiber units in vitro. J Neurophysiol 76:371-380[Abstract/Free Full Text].
Adelson DW, Wei JY, Kruger L (1997) Warm-sensitive afferent splanchnic C-fiber units in vitro. J Neurophysiol 77:2989-3002[Abstract/Free Full Text].
Allen BJ, Li J, Menning PM, Rogers SD, Ghilardi J, Mantyh PW, Simone DA (1999) Primary afferent fibers that contribute to increased substance P receptor internalization in the spinal cord after injury. J Neurophysiol 81:1379-1390[Abstract/Free Full Text].
Anderson KD, Alderson RF, Altar CA, DiStefano PS, Corcoran TL, Lindsay RM, Wiengand SJ (1995) Differential distribution of exogenous BDNF, NGF and NT-3 in the brain corresponds to the relative abundance and distribution of the high affinity and low affinity neurotrophin receptors. J Comp Neurol 357:296-317[ISI][Medline].
Apfel SC, Wright DE, Wiideman AM, Dormia C, Snider WD, Kessler JA (1996) Nerve growth factor regulates the expression of brain-derived neurotrophic factor mRNA in the peripheral nervous system. Mol Cell Neurosci 7:134-142[ISI][Medline].
Averill S, McMahon SB, Clary SB, Reichart LF, Priestley JV (1995) Immunocytochemical localisation of trkA receptors in chemically identified subgroups of adult rat sensory neurons. Eur J Neurosci 7:1484-1494[ISI][Medline].
Balkowiec A, Katz DM (2000) Activity-dependent release of endogenous brain-derived neurotrophic factor from primary sensory neurons detected by ELISA in situ. J Neurosci 20:7417-7423[Abstract/Free Full Text].
Balkowiec A, Kunze DL, Katz DM (2000) Brain-derived neurotrophic factor acutely inhibits AMPA-mediated currents in developing sensory relay neurons. J Neurosci 20:1904-1911[Abstract/Free Full Text].
Bartfai T, Iverfeldt K, Brodin E, Ögren S-O (1986) Functional consequences of coexistence of classical and peptide neurotransmitters. Prog Brain Res 68:321-330[ISI][Medline].
Bevan S, Szolcsanyi J (1990) Sensory neuron-specific actions of capsaicin: mechanisms and application. Trends Pharmacol Sci 11:330-333[Medline].
Bradbury EJ, King V, Simmons LJ, Priestley JV, McMahon SB (1998) NT-3 but not BDNF prevents atrophy and death of axotomised spinal cord projection neurons. Eur J Neurosci 10:3058-3068[ISI][Medline].
Canossa M, Griesbeck O, Berninger B, Campana G, Kolbeck R, Thönen H (1997) Neurotrophin release of neurotrophins: implications for activity-dependent neuronal plasticity. Proc Natl Acad Sci USA 94:13279-13286[Abstract/Free Full Text].
Caterina MJ, Scumacher MA, Tominaga M, Rosen TA, Levine JD, Julius D (1997) The capsaicin receptor: a heat-activated ion channel in the pain pathway. Nature 389:816-824[Medline].
Cejas PJ, Martinez M, Karmally S, McKillop M, McKillop J, Plunkett JA, Oudega M, Eaton MJ (2000) Lumbar transplant of neurons genetically modified to secrete brain-derived neurotrophic factor attenuates allodynia and hyperalgesia after sciatic nerve constriction. Pain 86:195-210[Medline].
Cho H-J, Kim J-K, Park H-C, Kim J-K, Kim D-S, HA S-O, Hong H-S (1998) Changes in brain-derived neurotrophic factor immunoreactivity in rat dorsal root ganglia, spinal cord, and gracile nuclei following cut or crush injuries. Exp Neurol 154:224-230[ISI][Medline].
Conner JM, Lauterborn JC, Yan Q, Gall CM, Varon S (1997) Distribution of brain-derived neurotrophic factor (BDNF) protein and mRNA in the normal adult rat CNS: evidence for anterograde axonal transport. J Neurosci 17:2295-2313[Abstract/Free Full Text].
De Biasi S, Rustioni A (1988) Glutamate and substance P coexist in primary afferent terminals in the superficial laminae of spinal cord. Proc Natl Acad Sci USA 85:7820-7824[Abstract/Free Full Text].
Dreyfus CF, Dai X, Lercher LD, Racey BR, Friedman WJ, Black IB (1999) Expression of neurotrophins in the adult spinal cord in vivo. J Neurosci Res 56:1-7[ISI][Medline].
Duggan AW, Riley RC, Mark MA, Macmillan SJA, Schaible H-G (1995) Afferent volley patterns and the spinal release of immunoreactive substance P in the dorsal horn of the anaesthetized spinal cat. Neuroscience 65:849-858[ISI][Medline].
Fawcett JP, Bamji SX, Causing CG, Aloyz R, Ase AR, Reader TA, McLean JH, Miller FD (1998) Functional evidence that BDNF is an anterograde neuronal trophic factor in the CNS. J Neurosci 18:2802-2821.
Gerber G, Randiç M (1989) Excitatory amino acid-mediated components of synaptically evoked input from dorsal roots to deep dorsal horn neurons in the rat spinal cord slice. Neurosci Lett 106:211-219[ISI][Medline].
Go VLW, Yaksh TL (1987) Release of substance P from the cat spinal cord. J Physiol (Lond) 391:141-167[Abstract/Free Full Text].
Jessell TM, Iversen LL (1977) Opiate analgesics inhibit substance P release from rat trigeminal nucleus. Nature 268:549-551[Medline].
Kangrga I, Randiç M (1991) Outflow of endogenous amino acids from the rat spinal dorsal horn in vitro by activation of low- and high-threshold primary afferent fibers-modulation by µ opioids. Brain Res 553:342-352[Medline].
Kerr BJ, Bradbury EJ, Bennett DLH, Trivedi PM, Dassan P, French J, Shelton DB, McMahon SB, Thompson SWN (1999) Brain-derived neurotrophic factor modulates nociceptive sensory inputs and NMDA-evoked responses in the rat spinal cord. J Neurosci 19:5138-5148[Abstract/Free Full Text].
Leibrock J, Lottspeich F, Hohn A, Hofer M, Hengerer B, Masiakowski P, Thonen H, Barde Y-A (1989) Molecular cloning and expression of brain-derived neurotrophic factor. Nature 341:149-152[Medline].
Liu H, Wang H, Sheng M, Jan LY, Jan YN, Basbaum AI (1994) Evidence for presynaptic N-methyl-D-aspartate autoreceptors in the spinal cord dorsal horn. Proc Natl Acad Sci USA 91:8383-8387[Abstract/Free Full Text].
Liu H, Mantyh PW, Basbaum AI (1997) NMDA-receptor regulation of substance P release from primary afferent nociceptors. Nature 386:721-724[Medline].
Liu X-G, Sandkühler J (1997) Characterization of long-term potentiation of C-fiber-evoked potentials in spinal dorsal horn of adult rat: essential role of NK₁ and NK₂ receptors. J Neurophysiol 78:1973-1982[Abstract/Free Full Text].
Liu X-G, Sandkühler J (1998) Activation of spinal N-methyl-D-aspartate or neurokinin receptors induces long-term potentiation of spinal C-fiber-evoked potentials. Neuroscience 86:1209-1216[ISI][Medline].
Malcangio M, Bowery NG (1993) Gamma-aminobutyric acid_B, but not $gamma$ -aminobutyric acid_A receptor activation, inhibits electrically evoked substance P-like immunoreactivity release from the rat spinal cord in vitro. J Pharmacol Exp Ther 266:1490-1496[Abstract/Free Full Text].
Malcangio M, Garrett NE, Cruwys S, Tomlinson DR (1997) Nerve growth factor- and neurotrophin-3-induced changes in nociceptive threshold and the release of substance P from the rat isolated spinal cord. J Neurosci 17:8459-8467[Abstract/Free Full Text].
Malcangio M, Fernandes K, Tomlinson DR (1998) NMDA receptor activation modulates evoked release of substance P from rat spinal cord. Br J Pharmacol 125:1625-1626[ISI][Medline].
Malcangio M, Ramer MS, Jones MG, McMahon SB (2000) Abnormal substance P release from the spinal cord following injury to primary sensory neurons. Eur J Neurosci 12:397-399[ISI][Medline].
Mannion RJ, Costigan M, Decosterd I, Amaya F, Ma Q-P, Holstege JC, Ji R-R, Acheson A, Lindsay RM, Wilkinson GA, Woolf CJ (1999) Neurotrophins: peripherally and centrally acting modulators of tactile stimulus-induced inflammatory pain hypersensitivity. Proc Natl Acad Sci USA 96:9385-9390[Abstract/Free Full Text].
Marvizón JCG, Martínez V, Grady EF, Bunnett NW, Mayer EA (1997) Neurokinin receptor internalization in spinal cord slices induced by dorsal root stimulation is mediated by NMDA receptors. J Neurosci 17:8129-8136[Abstract/Free Full Text].
Marvizón JCG, Grady EF, Stefani E, Bunnett NW, Mayer EA (1999) Substance P release in the dorsal horn assessed by receptor internalization: NMDA receptors counteract a tonic inhibition by GABA_B receptors. Eur J Neurosci 11:417-426[ISI][Medline].
Michael GJ, Averill S, Nitkunan A, Rattray M, Bennett DHL, Yan Q, Priestley JV (1997) Nerve growth factor treatment increases brain-derived neurotrophic factor selectively in tyrosine-kinase-A expressing dorsal root ganglion cells and their central terminations within the spinal cord. J Neurosci 17:8476-8490[Abstract/Free Full Text].
Michael GJ, Averill S, Shortland PJ, Yan Q, Priestley JV (1999) Axotomy results in major changes in BDNF expression by dorsal root ganglion cells: BDNF expression in large trkB and trkC cells, in pericellular baskets, and in projections to deep dorsal horn and dorsal column nuclei. Eur J Neurosci 11:3539-3551[ISI][Medline].
Millan MJ (1999) The induction of pain: an integrative review. Prog Neurobiol 57:1-164[ISI][Medline].
Muschol M, Salzberg BM (2000) Dependence of transient and residual calcium dynamics on action-potential patterning during neuropeptide secretion. J Neurosci 20:6773-6780[Abstract/Free Full Text].
Neal MJ, Cunningham JR, Hutson PH, Hogg J (1994) Effects of ischaemia on neurotransmitter release from the isolated retina. J Neurochem 62:1025-1033[ISI][Medline].
Okragly AJ, Hakk-Frendscho M (1997) An acid-treatment method for the enhanced detection of GDNF in biological samples. Exp Neurol 145:592-596[ISI][Medline].
Puig S, Sorkin LS (1995) Formalin-evoked activity in identified primary afferent fibers: systemic lidocaine suppresses phase-2 activity. Pain 64:345-355.
Randiç M, Jiang MC, Cerne R (1993) Long-term potentiation and long-term depression of primary afferent neurotransmission in the rat spinal cord. J Neurosci 13:5228-5241[Abstract].
Schuman EM (1999) Neurotrophin regulation of synaptic transmission. Curr Opin Neurobiol 9:105-109[ISI][Medline].
Siuciak JA, Altar CA, Wiengand SJ, Lindsay RM (1994) Antinociceptive effect of brain-derived neurotrophic factor and neurotrophin-3. Brain Res 633:326-330[ISI][Medline].
Siuciak JA, Wong V, Pearsall D, Wiegand SJ, Lindsay RM (1995) BDNF produces analgesia in the formalin test and modifies neuropeptide levels in rat brain and spinal cord areas associated with nociception. Eur J Neurosci 7:663-670[Medline].
Snider WD, McMahon SB (1998) Tackling pain at the source: new ideas about nociceptors. Neuron 20:629-632[ISI][Medline].
Son JH, Chun HS, Joh TH, Cho S, Conti B, Lee JW (1999) Neuroprotection and neuronal differentiation studies using substantia nigra dopaminergic cells derived from transgenic mouse embryos. J Neurosci 19:10-20[Abstract/Free Full Text].
Teoh H, Malcangio M, Bowery NG (1996) GABA, glutamate and substance-P like immunoreactivity release: effects of novel GABA_B antagonists. Br J Pharmacol 118:1153-1160[ISI][Medline].
Toledo-Aral JJ, Brehm P, Halegoua A, Mandel G (1995) A single pulse of nerve growth factor triggers long term neuronal excitability through sodium channels induction. Neuron 14:607-611[ISI][Medline].
Tominaga M, Caterina MJ, Malmberg AB, Rosen TA, Gilbert H, Skinner K, Raumann BE, Basbaum AI, Julius D (1998) The cloned capsaicin receptor integrates multiple pain-producing stimuli. Neuron 21:531-543[ISI][Medline].
Winter J, Forbes CA, Sternberg J, Lindsay RM (1988) Nerve growth factor (NGF) regulates adult rat cultured dorsal root ganglion neuron responses to the excitotoxin capsaicin. Neuron 1:973-981[Medline].
Woolf CJ, Salter MW (2000) Neuronal plasticity: increasing the gain in pain. Science 288:1765-1768[Abstract/Free