Functionally Antagonistic Interactions between the TrkA and p75 Neurotrophin Receptors Regulate Sympathetic Neuron Growth and Target Innervation

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The Journal of Neuroscience, July 1, 1999, 19(13):5393-5408

Functionally Antagonistic Interactions between the TrkA and p75 Neurotrophin Receptors Regulate Sympathetic Neuron Growth and Target Innervation
Judi Kohn¹, Raquel S. Aloyz¹, Jean G. Toma¹, Mary Haak-Frendscho², and Freda D. Miller¹
¹ Centre for Neuronal Survival, Montréal Neurological Institute, McGill University, Montréal, Québec, Canada, H3A 2B4, and ² Department of Immunology, Promega Corporation, Madison, Wisconsin 53711

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this report, we provide evidence that NGF and BDNF have functionally antagonistic actions on sympathetic neuron growthand target innervation, with NGF acting via TrkA to promote growthand BDNF via p75NTR to inhibit growth. Specifically, in culturedsympathetic neurons that themselves synthesize BDNF, exogenousBDNF inhibits and function-blocking BDNF antibodies enhance processoutgrowth. Both exogenous and autocrine BDNF mediate this effectvia p75NTR because (1) BDNF does not inhibit growth of neuronslacking p75NTR, (2) function-blocking p75NTR antibodies enhanceNGF-mediated growth, and (3) p75NTR^/ sympathetic neurons grow more robustly in response to NGF thando their wild-type counterparts. To determine the physiologicalrelevance of this functional antagonism, we examined the pinealgland, a well defined sympathetic target organ. BDNF is presentin the pineal gland during target innervation, and incoming sympatheticaxons are p75NTR positive. Moreover, the pineal glands of BDNF^+/ and BDNF^/ mice are hyperinnervated with sympathetic fibers, and tyrosinehydroxylase (TH) levels are elevated. Increased tyrosine hydroxylaseis also observed in the BDNF^+/ carotid artery, another sympathetic neuron target. Thus, BDNF,made by sympathetic neurons and/or their target organs, acts viap75NTR to antagonize NGF-mediated growth and target innervation,suggesting that sympathetic target innervation is determined bythe balance of positively and negatively acting neurotrophinspresent in developing and potentially maturetargets.

Key words: nerve growth factor; brain-derived neurotrophic factor; sympathetic neurons; target innervation; neurotrophin receptor; TrkA; p75NTR; pineal gland

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The neurotrophic factor hypothesis states that neuronal growth and survival are regulated by target-derived neurotrophic factors,such as nerve growth factor (NGF) (for review, see Thoenen andBarde, 1980; Levi-Montalcini, 1987), so that competition for limitingamounts of trophic factors match the number of innervating neuronsto target cells (Oppenheim, 1991). This hypothesis is based largelyon peripheral sympathetic neurons, which are absolutely dependenton NGF during the period of target competition (Levi-Montalcini,1987). During this developmental window, target-derived NGF isthought to regulate the density of target innervation by stimulatingterminal growth (Miller et al., 1994) and by serving as a discriminatorthat allows elimination of neurons that fail to sequester adequatetargetterritory.

Target-derived NGF binds to two different cell surface receptors on sympathetic neurons to elicit these responses: the tyrosinekinase receptor TrkA (Cordon-Cardo et al., 1991; Kaplan et al.,1991a,b; Klein et al., 1991) and the p75 neurotrophin receptor(p75NTR) (Johnson et al., 1986; Radeke et al., 1987). In additionto these two receptors, postmitotic sympathetic neurons expresslow levels of another Trk family member, TrkC (Belliveau et al.,1997). Two lines of evidence indicate that NGF binding to TrkAalone is sufficient to mediate sympathetic neuron survival andgrowth. First, ligand-mediated activation of TrkA, but not p75NTR,supports sympathetic neuron growth and survival (Weskamp and Reichardt,1991; Ibáñez et al., 1992; Clary et al., 1994; Belliveau etal., 1997; Bamji et al., 1998). Second, all sympathetic neuronsare lost in TrkA^/ mice (Smeyne et al., 1994) as they are in NGF^/ mice (Crowley et al., 1994).

Implicit to the neurotrophic factor hypothesis is the assumption that positive signals, such as those elicited by target-derivedNGF binding to TrkA, are sufficient to determine both the lifeand death of a developing neuron and the appropriate level oftarget innervation. However, we have demonstrated recently thatsympathetic neuron survival is not only determined by TrkA, butit is also regulated by negatively acting neurotrophins such asBDNF, which signal though p75NTR to mediate neuronal apoptosis(Aloyz et al., 1998; Bamji et al., 1998). Specifically, when survivalsignals are suboptimal, BDNF-mediated activation of p75NTR causessympathetic neuron apoptosis. Moreover, in BDNF^/ mice, sympathetic neuron number is increased, and in p75NTR^/ mice, the normal period of sympathetic neuron death is greatlydelayed. This latter deficit in apoptosis is intrinsic to sympatheticneurons, because cultured p75NTR^/ neurons die much more slowly than their wild-type counterpartsin the absence of NGF. Thus, naturally occurring sympathetic neurondeath is regulated by positively and negatively acting neurotrophinsthat signal through TrkA versusp75NTR.

Because the apoptotic effect of p75NTR signaling occurs only under suboptimal survival conditions, we hypothesized that p75NTRmight also inhibit other TrkA-mediated responses when survivalconditions are optimal. In this report, we test this hypothesisand demonstrate that BDNF acts via p75NTR to inhibit NGF-mediatedgrowth and target innervation. Thus, the balance of signalingmediated by the TrkA versus p75 neurotrophin receptors ultimatelydetermines both the survival and growth of developing sympatheticneurons.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mass cultures of sympathetic neurons. Mass cultures of pure sympathetic neurons from the superior cervical ganglion (SCG)of postnatal day (P) 1 Sprague Dawley rats (Charles River BreedingLaboratories, St. Constant, Quebec, Canada) were prepared as describedpreviously (Ma et al., 1992). Neurons were plated at low density(approximately one ganglion/well) in Nunclon four-well culturedishes (Life Technologies, Burlington, Ontario, Canada) coatedwith either rat tail collagen or poly-D-lysine and laminin (bothfrom Collaborative Biomedical Products, Bedford, MA). Culturemedium was UltraCulture (BioWhittaker, Walkersville, MD), supplementedwith 3% rat serum (Harlan Bioproducts, Madison, WI), 2 mM glutamine,100 U/ml penicillin, 100 µg/ml streptomycin (all from BioWhittaker),and for days 2 and 3, 7 µM cytosine arabinoside (Sigma-AldrichCanada Ltd., Oakville, Ontario,Canada).

CD-1 mouse sympathetic neurons were cultured by a modification of the method used to prepare rat neurons. Mouse cultures wereessentially prepared the same way, but were dissociated in UltraCulturemedium rather than in HBSS. Instead of rat serum, 3% fetal bovineserum (Life Technologies) was used, and 3.5 µM cytosine arabinosidewas added to the culture medium on day 1 afterplating.

NGF used in these experiments was purified from mouse salivary glands and supplied by Cedarlane Laboratories (Hornby, Ontario,Canada). The sources of recombinant human BDNF were PeproTech(Rocky Hill, NJ), for the neuritogenesis assays, and Promega Corporation(Madison, WI), for the recombinant human (rh) BDNF neutralizationexperiments. The p75NTR function-blocking antibody REX (Weskampand Reichardt, 1991) was the kind gift of Dr. L. Reichardt (Universityof California, San Francisco, CA). REX is directed against theextracellular domain of p75NTR and was used as an antiserum ata dilution of 1:100 (Weskamp and Reichardt, 1991). Rabbit serum(Life Technologies) of the same concentration was used as thenegative control for REX. Anti-human BDNF (Promega) was used at10 µg/ml. As a negative control for anti-BDNF, nonimmune chickenIgY (Promega) was used at up to 40 µg/ml in BDNF neutralizationexperiments and at 10 µg/ml in neuritogenesisexperiments.

BDNF neutralization. To test the capacity of anti-BDNF to neutralize BDNF, TrkB-expressing NIH-3T3 cells (the kind gift ofDr. D. Kaplan, McGill University) were cultured in DMEM. Briefly,cells were washed twice and incubated for 1 hr at 37°C in buffer,followed by a 30 min wash at 37°C in a phosphate-free buffer.Treatment consisted of incubating cells for 5 min with either50 ng/ml BDNF (Promega) or BDNF preadsorbed for 4 hr at 4°C withincreasing concentrations of the BDNF antibody (5-40 µg/ml). Inaddition, TrkB-3T3 cells were treated with medium only or mediumplus 40 µg/ml nonimmune chicken IgY. After these treatments, cellswere lysed and immunoprecipitated with anti-pan Trk (Hempsteadet al., 1992), and the immunoprecipitates were analyzed for TrkBactivation by Western blot analysis with phosphotyrosine antibody4G10 (Upstate Biotechnology, Lake Placid, NY), as we have describedpreviously (Belliveau et al., 1997; Bamji et al., 1998).

Survival assays. NGF-dependent neurons were selected by culturing sympathetic neurons for 5 d in the presence of 50 ng/mlNGF, as described previously (Ma et al., 1992; Belliveau et al.,1997; Bamji et al., 1998). Neurons were washed three times for1 hr each in neurotrophin-free media and then fed with media containing10 ng/ml NGF with or without 100 ng/ml BDNF, 10 µg/ml $alpha$ BDNF, ora 1:100 dilution of antiserum containing the p75NTR antibody REX(Weskamp and Reichardt, 1991). Each condition was repeated intriplicate, and analysis of survival was performed 48 hr laterby using nonradioactive MTT survival assays that measure mitochondrialfunction (Celltitre 96, Promega, Madison, WI) (Belliveau et al.,1997). Specifically, 50 µl of the MTT reagent was added to 500µl of media in each well and incubated for 2 hr at 37°C. Afteraspiration of the MTT-containing media, 100 µl of a 0.065N HCL/isopropanolmixture was added to each well to lyse the cells, and colorimetricanalysis was performed using an ELISA reader. For rat sympatheticneurons, 10 ng/ml NGF represents 100% survival (Bamji et al.,1998); therefore all other values were considered to be relativeto 10 ng/ml NGF. For mouse neurons, 7.5 ng/ml NGF represents 100%survival and was thus considered to be the 100% survival thresholdfor neuritogenesisexperiments.

Analysis of transgenic animals. Mice heterozygous for a targeted mutation in the BDNF gene (Ernfors et al., 1994) or homozygousfor a targeted mutation in the p75NTR gene (Lee et al., 1992)were obtained from Jackson Labs (Bar Harbor, ME). The BDNF^+/ mice were maintained in a C129/BALB/c background. The p75NTR^/ mice were originally generated in a C129 background (Lee et al.,1992) and were crossed back into a C129 background before purchasefrom Jackson Labs and then maintained as homozygotes. Progenyfrom BDNF heterozygote crosses were screened for the mutant allele(s)using PCR, as we have described previously (Bamji et al., 1998).

Analysis and quantification of process outgrowth. p75NTR/BDNF regulation of neuronal growth was analyzed using two differenttypes of neuritogenesis assays. Similar results were obtainedwith both approaches. The first assay, which measures the numberof process intersections/neuron, is described in detail in Belliveauet al. (1997) and Yang et al. (1998). Briefly, P1 rat sympatheticneurons were cultured in 50 ng/ml NGF for 2-3 d to upregulatep75NTR, whose increased expression in response to NGF occurs independentlyof neuronal survival (Miller et al., 1991; Ma et al., 1992). Aftera 1 hr washout in neurotrophin-free medium, cultures were maintainedfor an additional 2 d in 10 ng/ml NGF plus or minus 100 ng/mlBDNF. Fields in low-density sister cultures were randomly selectedand photographed; six to eight sampling windows were used perculture. We then determined, in each field, (1) the number ofvisible neurite intersections and (2) the number of neuronal cellbodies. We expressed these data as the number of intersections/numberof cell bodies to give us a measure of intersections/neuron. Wethen determined the mean number of intersections/neuron for allof the photographed fields in a given culture and used the Student'st test to determine the statistical significance of density differencesbetween experimental groups. Results were expressed as the meanprocess network density per neuron ±SEM.

The second approach allowed us to quantitate, in any given field, (1) number of neuronal cell bodies and (2) apoptotic cells,and (3) amount of area covered by neuritic processes. Specificallysympathetic neurons were labeled with terminal deoxynucleotidyltransferase-mediated biotinylated UTP nick end labeling (TUNEL)to visualize apoptotic cells, followed by immunolabeling withanti- $alpha$ -tubulin to visualize neurites, and then staining with Hoechst33250 to visualize nuclei. To perform these experiments, P1 SCGneurons were plated onto eight-well Nunc-Nalgene plastic Lab Tekchamber slides (Life Technologies) that were coated twice, firstwith a polylysine-collagen mixture followed by a second collagencoating. After the experimental treatments, cultures were washedtwice with PEM (PIPES-EGTA-MgCl₂) buffer and fixed for 15 minin 4% paraformaldehyde in PEM buffer containing 0.25% glutaraldehydeand 0.2% Triton X-100. After three 10 min washes in PBS, TUNELwas performed as described previously (Slack et al., 1996) (reagentsfrom Promega) with a Streptavidin-CY3 conjugate (1:2000 in PBS;Jackson ImmunoResearch Laboratories, West Grove, PA). Cultureswere then washed three times for 10 min each in PBS and incubatedfor 2 hr with anti- $alpha$ -tubulin (1:500 in PBS, Clone DM1A; Sigma-AldrichCanada). The tubulin immunolabel was visualized using FITC-conjugatedgoat anti-mouse IgG (1:800 in PBS; Jackson ImmunoResearch). Finally,cultures were incubated with Hoechst 33250 (2 µg/ml in PBS; ICNBiomedicals, Costa Mesa, CA) for 1 min to label cell nuclei andwashed an additional three times for 10 min each in PBS. Slideswere then coverslipped using Sigma Mounting Medium (Sigma Diagnostics,St. Louis, MO) and viewed by epifluorescencemicroscopy.

To analyze these cultures, images were captured using a Sony XC-75CE CCD video camera module attached to an Axioskop microscope(Carl Zeiss Canada) and a 16× plan-neofluar lens. The NorthernEclipse image analysis system (Empix Imaging, Mississauga, Ontario,Canada) was used to analyze these images as follows. Images oflow-density neuronal fields were captured, and the area labeledwith tubulin was measured and expressed as a percentage of thetotal field area. The numbers of Hoechst-positive and TUNEL-positivecell bodies were quantitated by viewing the same field with theappropriate filters and analyzed using the same software package.For each culture, seven to eight independent, randomly chosenfields were analyzed. These data were expressed as average percentagetubulin immunoreactive area per live cell, and Student's t testwas used to determine the statistical significance of differencesbetween experimentalgroups.

Immunocytochemistry and analysis of sympathetic innervation density. For quantitative analysis of sympathetic innervationdensity, P13-P15 BDNF^+/+, ^+/, and ^/ mice were deeply anesthetized with isoflurane and decapitated.Pineal glands were removed immediately, immersion-fixed in 4%paraformaldehyde in phosphate buffer, pH 7.4, overnight, and subsequentlycryoprotected in graded sucrose solutions. Pineal glands takenfrom mice of each genotype were cut on a cryostat (12 µm sections),and the entire pineal gland was serially thaw-mounted onto threeSuperfrost slides (Fisher Scientific, Houston, TX). Thus, eachpineal gland was completely represented on each of three slides,and an entire pineal gland of each genotype could be analyzed,after immunostaining, to obtain a quantitative measure of innervationdensity. These sections were then post-fixed in 4% paraformaldehydefor 10 min at room temperature and washed for 10 min in PBS, pH7.4. After nonspecific blocking with 4% goat serum and 4% ratserum (both from Jackson ImmunoResearch) plus 0.2% Triton X-100in PBS, pH 7.4, the sections were incubated overnight at 4°C witha commercially available polyclonal antibody directed againsttyrosine hydroxylase (TH) (1:400; Chemicon International, Temecula,CA) in blocking solution. Slides were then washed three timesfor 10 min each in PBS, and incubated for 2 hr in blocking solutioncontaining a CY3-conjugated secondary antibody (goat anti-rabbitIgG, 1:2000, Jackson ImmunoResearch). After three 10 min washesin PBS, slides were coverslipped using Sigma Mounting Medium andviewed by epifluorescencemicroscopy.

To quantitatively analyze sympathetic innervation density, images were captured and analyzed using the Northern Eclipse ImagingSystem. For a given slide, the percentage area covered by TH immunolabelingwas measured for every section on that slide, and the mean percentagearea covered by TH immunolabeling was determined from all of thesesections, thereby avoiding errors attributable to potential differencesin distribution of sympathetic fibers in pineal glands of differentgenotypes. Comparisons were only made between slides that wereprocessedtogether.

To directly compare the pattern of p75NTR immunoreactivity with that of TH immunoreactivity, two slides containing serialsections obtained from the same P13 BDNF^+/ pineal gland were immunostained as described above with eitheranti-TH (Chemicon) or anti-human p75NTR (Promega, 1:500) antibodies.The secondary antibody used was a CY3-conjugated goat anti-rabbitIgG (1:2000 in blocking solution; JacksonImmunoResearch).

Western blot analysis. For biochemistry, groups of P13-P15 pineal glands from ^+/+, ^+/, or ^/ BDNF mice, or portions of ^+/+ or ^+/ common carotid artery (dissected at the point of bifurcationinto the internal and external branches), or adult rat pinealglands or cortex were homogenized in Tris buffered saline (TBS)containing 137 mM NaCl, 20 mM Tris, pH 8.0, 1% v/v NP-40, 0.1%SDS, 10% glycerol, and the protease inhibitors phenylmethyl sulfonylfluoride (1 mM), aprotinin (10 µg/ml), leupeptin (0.2 µg/ml),and sodium vanadate (1.5 mM). The tissue was rocked for 10 minat 4°C, and after a 10 min centrifugation at 4°C, the supernatantwas collected and lysates were normalized for protein concentrationusing a BCA Protein Assay kit (Pierce Chemical Co., Rockford,IL). For Western blot analysis, equal amounts of pineal, carotid,or cortical protein were boiled in sample buffer for 5 min andseparated by 7.5 or 15% SDS-PAGE (7.5% gel for TH, p75NTR, $alpha$ -tubulin,and ERK1; 15% gel for BDNF). rhBDNF (20 ng) (Amgen, Thousand Oaks,CA) was also run on a 15% SDS-PAGE gel. After electrophoresis,proteins were transferred to 0.2 µm nitrocellulose membranes for1.5 hr at 0.6 amps, and washed three times for 10 min each witheither PBS (for BDNF) or TBS (for all other proteins). After a1.5 hr block in blotto (3% nonfat milk in PBST for BDNF, or TBSTfor all other proteins) at room temperature, membranes were incubatedovernight at 4°C in blocking solution containing either anti-BDNF(1:3000; Santa Cruz Biotechnology, Santa Cruz, CA), anti-recombinanthuman p75NTR (1:10,000; Promega), anti-TH (1:5000; Chemicon),anti- $alpha$ -tubulin (1:5000; Calbiochem/Oncogene Research Products,Cambridge, MA), or anti-ERK1 (1:10,000; Santa Cruz Biotechnology).The membranes were washed four times for 10 min each with eitherPBST (for BDNF) or TBST (for all other proteins) and then incubatedwith secondary antibody [1:10,000 goat anti-rabbit HRP (BoehringerMannheim, Laval, Quebec, Canada) for anti-BDNF, anti-p75NTR, anti-ERK1,and anti-TH, or 1:10,000 goat anti-mouse HRP (also from Boehringer)for anti- $alpha$ -tubulin] for 1.5 hr at room temperature. After three10 min washes in PBST (for BDNF protein) or TBST (for all otherproteins), detection was performed using enhanced chemiluminescence(ECL Western blotting detection reagent; Amersham Canada Ltd.,Oakville, Ontario, Canada) and XAR x-ray film (Eastman Kodak Co.,Rochester,NY).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

BDNF-mediated activation of p75NTR inhibits NGF-induced growth of cultured sympathetic neurons.

BDNF-mediated activation of p75NTR antagonizes TrkA-mediated sympathetic neuron survival when NGF levels are suboptimal, buthas no effect on survival at higher levels of NGF (Aloyz et al.,1998; Bamji et al., 1998). To determine whether p75NTR activationalso antagonized other TrkA-mediated biological responses, wefocused on sympathetic neuron growth. Specifically, we culturedsympathetic neurons in NGF to maintain their survival and thenactivated p75NTR using BDNF. For rat sympathetic neurons, 10 ng/mlNGF mediates 100% sympathetic neuron survival but elicits limitedmorphological growth and TrkA activation relative to higher concentrationsof NGF (Ma et al., 1992; Belliveau et al., 1997), whereas 100ng/ml BDNF is sufficient to activate p75NTR in apoptosis experiments(Bamji et al., 1998) but does not bind to the two Trk receptors,TrkA and TrkC, that are present on sympathetic neurons (Belliveauet al., 1997).

Initially, we confirmed, as we have reported previously (Bamji et al., 1998), that the addition of 100 ng/ml BDNF in the presenceof 10 ng/ml NGF had no negative effects on sympathetic neuronsurvival (Fig. 1A). Sympathetic neurons were cultured for 5 din 50 ng/ml NGF, washed free of neurotrophin, and then switchedinto 10 ng/ml NGF plus or minus 100 ng/ml BDNF. Two days later,neuronal survival was measured using MTT assays, which measuremitochondrial function (Belliveau et al., 1997; Bamji et al.,1998). As shown previously (Bamji et al., 1998), the additionof 100 ng/ml BDNF had no effect on sympathetic neuron survivalin 10 ng/ml NGF (Fig. 1A).

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Figure 1. BDNF decreases the growth of sympathetic neurons in vitro without affecting their survival. A, Results of colorimetric MTT assays to measure mitochondrial function and cell survival. Neonatal sympathetic neurons were cultured in 50 ng/ml NGF for 5 d, washed free of neurotrophin-containing medium, and then switched for 2 d to NGF or NGF plus BDNF. The data derive from a representative survival assay that was performed in triplicate. In these assays, absolute values are normalized so that the value obtained with 0 neurotrophin is 0% survival, whereas that obtained with 10 ng/ml NGF is considered 100% survival. Error bars represent SEM. The values obtained for NGF versus NGF plus BDNF were not significantly different (p > 0.05). B-D, Quantitative analysis of neurite process density in sympathetic neuron cultures grown in the presence of NGF or NGF plus BDNF. B, Six separate experiments were performed to determine the effect of BDNF on NGF-mediated process density in sympathetic neurons. Sympathetic neurons were plated at low density on collagen or poly-D-lysine and laminin in 50 ng/ml NGF for 2-3 d and were then switched to 10 ng/ml NGF plus or minus 100 ng/ml BDNF for 2 d. In all six experiments, significantly fewer neurite intersections were observed after exposure to NGF + BDNF versus NGF alone (*p < 0.05). C, The experiments shown in B were normalized so that the neurite density at 10 ng/ml NGF is 100, and then averaged to provide an index of the relative neurite density. D, Dose-response curve to determine the effect of different concentrations of BDNF on NGF-mediated process density. Experiments were performed as in B. No significant different in process density was observed when 50 ng/ml BDNF was added, but statistically significant differences were seen with both 100 and 200 ng/ml BDNF (*p < 0.05). The data derive from one neurite outgrowth assay, where each condition was sampled four to five times. E, Results of TUNEL to measure apoptotic neurons. Neurons were treated as in A, but were TUNEL-labeled to measure apoptotic cells and then stained with Hoechst 33250 to quantitate total neuronal nuclei. Seven to eight fields of cells were analyzed per treatment in each experiment, and results are expressed as the percentage of TUNEL-labeled nuclei/total neuronal nuclei. Results represent the mean ± SEM. Note that BDNF had no effect on the number of TUNEL-labeled neurons in these experiments. F, G, Quantitative analysis of the area covered by tubulin immunoreactive neurites in sympathetic neuron cultures grown in 10 ng/ml NGF with or without BDNF. The same fields of cells shown in E were analyzed for the percentage of area within a given field that was covered by tubulin-immunoreactive processes. These data were normalized for the total number of neuronal cell bodies in the same field (as indicated by Hoechst staining) and then used to determine the relative tubulin-immunolabeled area per neuron. Results represent the mean ± SEM; in both experiments, BDNF caused a statistically significant decrease in tubulin-immunoreactive processes (*p < 0.05), with no effect on neuronal apoptosis (E). G, The experiments shown in F were normalized so that the tubulin immunolabeled area at 10 ng/ml NGF was 100 and then averaged to provide an index of the mean relative tubulin immunolabel.

We next determined whether p75NTR activation by BDNF affected neuronal growth by measuring the level of neurite extensionthat occurs in response to 10 ng/ml NGF with or without BDNF.For these experiments, neurons were cultured for 2-3 d in 50 ng/mlNGF and switched to 10 ng/ml NGF plus or minus 100 ng/ml BDNF,and the density of neuritic processes was determined 2 d laterby quantitating the number of neurite intersections per neuron(Figs. 1B,C, 2A,B). Results from six separate experiments indicatedthat BDNF reduced the process network density from 22 to 52%,for an average decrease of 40% (Figs. 1B,C, 2A,B). Having determinedthat BDNF reduced neurite density, we then performed a dose-responsecurve with 50, 100, and 200 ng/ml BDNF, using the same experimentalapproach. This analysis revealed that 50 ng/ml BDNF produced asmall decrease in process density that was not statistically significant,whereas both 100 and 200 ng/ml BDNF produced similar, significantdecreases (Fig. 1D). This dose-response is similar to that observedfor the apoptotic effects of BDNF on the same neurons (Bamji etal., 1998).

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Figure 2. Exogenous BDNF inhibits and anti-BDNF and anti-p75NTR enhance NGF-promoted growth of sympathetic neurons in vitro. Phase-contrast micrographs of cultured neonatal rat sympathetic neurons maintained in 50 ng/ml NGF for 2-3 d, and then switched to (A) 10 ng/ml NGF, (B) 10 ng/ml NGF plus 100 ng/ml BDNF, (C) 10 ng/ml NGF plus 10 µg/ml anti-BDNF, or (D) 10 ng/ml NGF plus anti-p75NTR (REX). Exogenous BDNF inhibited and BDNF or p75NTR antibodies enhanced process outgrowth. Scale bar, 65 µM.

To confirm that the observed decrease in neurite intersections per neuron reflected a decrease in the total amount of growthin these cultures, we used a second approach. As in the previousexperiments, neurons were first grown for 2-3 d in 50 ng/ml NGFand then switched to 10 ng/ml NGF plus or minus 100 ng/ml BDNFfor 2 additional days. As a control, neurons were withdrawn fromNGF for these final 2 d. We triple-labeled these neurons (Fig.3) by (1) using TUNEL to assess the number of apoptotic neurons(pink/red nuclei in Fig. 3), (2) using anti-tubulin to visualizethe neuritic network (green in Fig. 3), and (3) using Hoechst33250 to visualize neuronal nuclei (blue in Fig. 3). We then selectedrandom fields in each sister culture and used image analysis toquantitate the amount of area covered by tubulin-immunoreactiveprocesses per Hoechst-labeled neuron and to determine the numberof apoptotic neurons per field. This analysis confirmed that,as indicated by the MTT assay, the number of dying cells was similarin cultures maintained in 10 ng/ml NGF alone versus those in 10ng/ml NGF plus 100 ng/ml BDNF (Fig. 1E). Moreover, the relativeamount of tubulin-immunoreactive processes per neuron was decreased~40% in the neurons treated with BDNF (Fig. 1F,G), a decreasesimilar to that seen when the number of neuritic intersectionsper neuron was determined (Fig. 1B,C). Thus, these two approachesindicate that under these conditions, BDNF was able to antagonizeNGF-promoted sympathetic neuron growth with no perturbation ofneuronal survival.

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Figure 3. BDNF decreases neurite outgrowth in cultured neonatal rat sympathetic neurons without decreasing their survival. Digitized micrographs are of postnatal day 1 sympathetic neuron cultures triple-labeled to visualize neurite outgrowth ( $alpha$ -tubulin, green), apoptotic cells (TUNEL-labeled, red/pink), and total number of cells in the culture (Hoechst nuclear stain, blue). Cultures were grown in 50 ng/ml NGF for 2 d and then switched to either (A) 10 ng/ml NGF or (B) 10 ng/ml NGF plus 100 ng/ml BDNF, or (C) withdrawn from NGF. After 2 additional days, the cultures were labeled as indicated above. Arrows point to nuclei of apoptotic cells. Note that the addition of BDNF to the cultures did not increase the degree of TUNEL over that observed in cultures treated with NGF alone, whereas cultures in which NGF was withdrawn exhibit a high number of TUNEL-labeled neurons and a complete disintegration of neurites. Magnification, 160×.

Autocrine BDNF, acting through p75^NTR, decreases the growth of cultured sympathetic neurons

These data suggested that exogenous BDNF is able to activate p75NTR and negatively influence TrkA-mediated neuritogenesis.However, because sympathetic neurons themselves synthesize BDNF(Causing et al., 1997), which can be detected in conditioned mediumobtained from cultured SCG neurons (C. G. Causing, R. Aloyz, andF. D. Miller, unpublished observations), we hypothesized thatautocrine BDNF might play a role in negatively regulating levelsof sympathetic neuron growth through a BDNF/p75NTR autocrine loop.To test this hypothesis, we used a function-blocking BDNFantibody.

Initially, to ensure that this anti-BDNF was capable of neutralizing BDNF, we incubated TrkB-expressing NIH-3T3 cells for5 min with 50 ng/ml BDNF plus or minus 5-40 µg/ml of anti-BDNF.TrkB protein was then immunoprecipitated using anti-panTrk, andthe immunoprecipitates were analyzed by Western blot analysiswith anti-phosphotyrosine. As controls, cells were incubated eitherwith culture medium or medium with BDNF plus 40 µg/ml nonimmuneIgY. This analysis revealed that BDNF caused a robust increasein tyrosine phosphorylation of TrkB and that anti-BDNF inhibitedBDNF-stimulated TrkB phosphorylation at concentrations of 10 µg/mlor higher (data not shown). In contrast, the control IgY had noeffect on BDNF-mediated TrkB activation (data notshown).

We then used this function blocking anti-BDNF to test the role of autocrine BDNF in sympathetic neuron growth. Initially,we determined whether anti-BDNF had any effect on sympatheticneuron survival under the conditions of our growth experiments;neurons were cultured for 5 d in 50 ng/ml NGF and then were switchedto 10 ng/ml NGF with or without 10 µg/ml anti-BDNF. Measurementof neuronal survival using MTT assays 2 d later revealed thatanti-BDNF had no effect on sympathetic neuron survival (Fig. 4A).We then determined whether anti-BDNF affected neuronal growthunder these same conditions; neurons were grown in 50 ng/ml NGFfor 2-3 d and then switched into 10 ng/ml NGF plus or minus 10µg/ml anti-BDNF. Measurement of neurite process density revealedthat in three separate experiments, cultures exposed to anti-BDNFexhibited an average increase in neuritogenesis of 80% relativeto 10 ng/ml NGF alone (Figs. 2A,C, 4B,C). Nonimmune IgY had noeffect on NGF-mediated growth (Fig. 4B), demonstrating the specificityof the effect. Thus, autocrine BDNF inhibits TrkA-mediated neuritogenesis,at least in vitro.

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Figure 4. Function-blocking antibodies directed against BDNF or p75NTR enhance growth of sympathetic neurons without affecting their survival. A, Results of colorimetric MTT assays to measure mitochondrial function and cell survival. Neonatal sympathetic neurons were cultured in 50 ng/ml NGF for 5 d, washed free of neurotrophin-containing medium, and then switched for 2 d to 10 ng/ml NGF or 10 ng/ml NGF plus 10 µg/ml anti-BDNF ( $alpha$ -BDNF). These data represent the values obtained in a representative survival assay that was performed in triplicate. In these assays, absolute values are normalized so that the value obtained with 0 neurotrophin is 0% survival, whereas that obtained with 10 ng/ml NGF is considered 100% survival. Error bars represent SEM. These two values were not significantly different (p = 0.3710). B-H, Quantitative analysis of neuritic process density in sympathetic neuron cultures grown in the presence of NGF, NGF plus anti-BDNF (B, C), NGF plus REX (D, E), increased NGF (F), or (G, H) NGF and REX plus or minus BDNF. B, Three separate experiments were performed to determine the effect of anti-BDNF on NGF-promoted neurite process growth in sympathetic neurons. Sympathetic neurons were plated at low density in 50 ng/ml NGF on collagen, or poly-D-lysine and laminin for 2-3 d, and then switched for an additional 2 d to 10 ng/ml NGF plus or minus 10 µg/ml anti-BDNF ( $alpha$ -BDNF) or, as a control, 10 µg/ml nonimmune IgY. In all three experiments, significantly more neurite intersections were observed after exposure to anti-BDNF relative to NGF alone (*p < 0.05). C, The experiments shown in B were normalized so that the neuritic density at 10 ng/ml NGF is 100 and then averaged to provide an index of the relative neurite density. D, Three separate experiments were performed to determine the effect of anti-p75NTR on NGF-promoted neurite process growth in sympathetic neurons. Sympathetic neurons were treated as in B, except that they were treated with a 1:100 dilution of p75NTR antiserum (REX) or, as a control, with the same dilution of nonimmune rabbit serum. In all three experiments, significantly more neurite intersections were observed after exposure to anti-p75NTR than after NGF alone (*p < 0.05). Serum itself had no effect (p > 0.05). E, The experiments shown in D were normalized so that the neuritic density at 10 ng/ml NGF is 100 and then averaged to provide an index of the relative neurite density. F, The increase in relative neurite process density in 40 ng/ml NGF relative to 10 ng/ml NGF. These data represent the results from one experiment and are shown here for comparison only. We have previously documented the reproducibility and significance of this increase in Belliveau et al. (1997). G, Three separate experiments were performed to determine whether BDNF could antagonize the p75NTR-mediated increase in sympathetic neuron growth. Sympathetic neurons were treated as in B, except that they were treated with a 1:100 dilution of p75NTR antiserum (REX) plus or minus 100 ng/ml BDNF. In all three experiments, exogenous BDNF significantly inhibited the REX-induced increase in process density (*p < 0.05). H, The experiments shown in G were normalized so that the neuritic density at 10 ng/ml NGF is 100 and then averaged to provide an index of the relative neurite density.

If autocrine BDNF is mediating these effects via p75NTR, then we would predict a similar increase in TrkA-mediated neuritogenesisif we blocked p75NTR. To test this prediction, we performed neuritogenesisexperiments using the function-blocking p75NTR antibody REX. Asbefore, cultures were initially grown for 2 d in 50 ng/ml NGFand then incubated for 2 additional days with 10 ng/ml NGF withor without REX (Figs. 2A,D, 4D,E). As a control, sister cultureswere incubated with rabbit serum at the same volume as the REXantiserum. These experiments revealed that when p75NTR was blockedby REX, neuritogenesis was enhanced almost twofold relative toNGF alone (Figs. 2A,D, 4D,E), an effect that was not observedwith rabbit nonimmune serum (Fig. 4D) and was similar to the responseelicited by anti-BDNF (Fig. 4B,C). The increased neuritogenesisobserved with both REX and anti-BDNF is similar to the 2- to 2.5-foldincrease that occurs when NGF is increased from 10 to 40 ng/mlNGF (Fig. 4F) (Belliveau et al., 1997), a treatment that causesincreased TrkA activation (Belliveau et al., 1997), supportingthe idea that a BDNF/p75NTR autocrine loop antagonizes TrkA-mediatedsympathetic neurongrowth.

In a final experiment, we tested whether exogenous BDNF could reverse the effect of REX on neuritogenesis, as it should ifREX is acting by disrupting a BDNF/p75NTR loop. Neurons were culturedfor 2-3 d in 50 ng/ml NGF and then switched to 10 ng/ml NGF withREX plus or minus 100 ng/ml BDNF for an additional 2 d; in experimentswith REX and BDNF, cultures were preincubated with REX for 2 hrbefore the addition of BDNF. These experiments revealed that exogenousBDNF blocked the ability of REX to increase sympathetic neurongrowth (Fig. 4G,H). This antagonism between REX and exogenousBDNF is similar to results we have obtained previously when examiningBDNF-induced apoptosis of sympathetic neurons (Bamji et al., 1998)and supports the idea of an inhibitory BDNF/p75NTR growthloop.

p75NTR^/ sympathetic neurons show enhanced neuritogenesis in response to NGF and do not respond to exogenous BDNF

Although our data strongly suggest that BDNF acts through p75NTR to antagonize TrkA, they do not conclusively demonstratethe necessity of p75NTR for BDNF's effects. To examine this moredirectly, we cultured neurons from both p75NTR^/ and wild-type control mice and repeated the neuritogenesis assays.Because mouse sympathetic neurons have been reported to be moresensitive to NGF than rat sympathetic neurons, we initially performedsurvival assays to determine an appropriate NGF concentration.Neurons were maintained for 5 d in 50 ng/ml NGF and were switchedto concentrations of NGF ranging from 0.1 to 10 ng/ml NGF for3 d, and survival was then measured using MTT assays. These experimentsrevealed that 5, 7.5, and 10 ng/ml NGF were all able to mediatemaximal mouse sympathetic neuron survival (Fig. 5A). To ensurethat BDNF had no apoptotic effect under these survival conditions,we performed similar experiments with 7.5 or 10 ng/ml NGF plusor minus 100 ng/ml BDNF. MTT assays revealed that, as for ratneurons (Fig. 1A), BDNF did not affect mouse sympathetic neuronsurvival in the presence of optimal concentrations of NGF (Fig.5B). On the basis of these data, we selected 7.5 ng/ml NGF forour experiments, a concentration that was optimal for survivaland in which BDNF had no significant effect on survival.

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Figure 5. Analysis of neurite outgrowth in response to NGF or NGF plus BDNF in p75NTR^/ versus p75NTR^+/+ sympathetic neurons. A, B, Results of colorimetric MTT assays to measure mitochondrial function and survival of murine sympathetic neurons in response to NGF or NGF plus BDNF. A, Neonatal murine sympathetic neurons were cultured in 50 ng/ml NGF for 5 d, washed free of neurotrophin-containing medium, and switched for 2 d to various concentrations of NGF as indicated on the x-axis. Results from one representative experiment performed in triplicate are shown. In these assays, absolute values are normalized so that the value obtained with 0 neurotrophin is 0% survival, whereas that obtained with 10 ng/ml NGF is considered 100% survival. Error bars represent SEM. Note that 5 ng/ml NGF is capable of eliciting maximal survival of murine sympathetic neurons. B, Neonatal murine sympathetic neurons were cultured as in A and were then switched into various concentrations of NGF plus 100 ng/ml BDNF, as denoted on the x-axis. These data represent values from one representative experiment performed in triplicate. Values are normalized as in A; error bars represent SEM. As with rat sympathetic neurons, BDNF does not affect survival in optimal concentrations of NGF. C, D, Quantitative analysis of neuritic process density in p75NTR^/ versus wild-type murine sympathetic neurons in response to NGF or NGF plus BDNF. In the two separate experiments shown here, p75NTR^/ versus wild-type neonatal sympathetic neurons were cultured as sister cultures for 3 d in 50 ng/ml NGF and were then switched for an additional 2 d to 7.5 ng/ml NGF plus or minus 100 ng/ml BDNF. * denotes values that were significantly different in the comparison between NGF versus NGF plus BDNF (*p < 0.05); ** denotes those values that were significantly different in the comparison between p75NTR^/ versus wild-type (WT) neurons in response to 7.5 ng/ml NGF (**p < 0.05). Note that p75NTR^/ neurons grow more robustly than wild-type neurons in response to the same concentration of NGF. Note also that BDNF significantly reduces the NGF-mediated growth of wild-type (p < 0.05) but not p75NTR^/ (in both experiments, p > 0.38) neurons. D, The experiments shown in C were normalized so that the neuritic density of wild-type neurons at 10 ng/ml NGF was 100 and then averaged to provide an index of the relative neurite density.

We then examined sympathetic neurons from p75NTR^/ mice to determine first whether the lack of p75NTR imparted to p75NTR^/ neurons an intrinsic ability to extend more neuritic processes,and second, whether BDNF was acting through p75NTR to inhibitTrkA-mediated growth. To perform these experiments, sympatheticneurons were cultured from p75NTR^/ versus control mice on the same day, were maintained for 3 din 50 ng/ml NGF, and were subsequently switched to 7.5 ng/ml NGFplus or minus 100 ng/ml BDNF. Measurement of neuritic processdensity revealed that p75NTR^/ neurons exhibited an almost twofold increase in neurite outgrowthrelative to their wild-type counterparts (Figs. 5C,D, Fig. 6A,C),a result similar to that observed with the REX and anti-BDNF antibodiesin experiments using rat sympathetic neuron cultures (Fig. 4).Moreover, although BDNF decreased the degree of neuritogenesisin wild-type mouse cultures by an average of 35% (Figs. 5C,D,6A,B), a result similar to that observed with rat neurons (Fig.1B,C), exogenous BDNF had no effect on growth of p75NTR^/ neurons (Figs. 5C,D, 6C,D). Thus p75NTR is required for BDNFto inhibit NGF-mediated sympathetic neuron growth, and NGF ismore effective at eliciting growth in the absence of p75NTR.

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Figure 6. p75NTR^/ sympathetic neurons show enhanced neuritogenesis in response to NGF and do not respond to exogenous BDNF. Phase-contrast micrographs of cultured Coomassie blue-stained (A, B) wild-type and (C, D) p75NTR^/ murine sympathetic neurons maintained in 50 ng/ml NGF for 2 d and then switched to (A, C) 7.5 ng/ml NGF or (B, D) 7.5 ng/ml NGF plus 100 ng/ml BDNF. As observed in cultured rat sympathetic neurons (Fig. 2B), exogenous BDNF inhibited NGF-promoted process outgrowth in wild-type but not p75NTR^/ murine sympathetic neurons. Note that the degree of process outgrowth is greatly enhanced in p75NTR^/ neurons, relative to their wild-type counterparts. Scale bar, 65 µM.

BDNF is present in sympathetic target organs and p75NTR is present in sympathetic neuron axons during the period of target innervation

If these culture results are relevant to the process of target innervation in vivo, then we would predict that BDNF (derivedfrom incoming sympathetic fibers or target tissue or both) wouldbe present in sympathetic neuron targets during the developmentalperiod of target competition. To test this prediction, we focusedon the pineal gland, a sympathetic target organ that (1) is bilaterallyinnervated by neurons from the SCG (Kappers, 1960; Owman, 1964),(2) does not receive any other peripheral innervation from sensoryor motor neurons (Stanley et al., 1987), and (3) is innervatedpostnatally. Ingrowth of sympathetic fibers to the pineal glandbegins during the first week of postnatal life, reaching adultlevels after 3-4 weeks (Hakanson et al., 1967). To perform thisexperiment, lysates of pineal glands from adult rats were separatedby PAGE, transferred to nitrocellulose, and probed for the presenceof BDNF using a BDNF antibody that we have previously characterizedextensively for specificity (Causing et al., 1997; Fawcett etal., 1997, 1998). This analysis revealed a BDNF-immunoreactiveband in the pineal gland that is the same size as BDNF in therat cortex and human recombinant BDNF (Fig. 7A,B). To confirmthe identity of this band, we analyzed the pineal gland from micein which the BDNF gene was mutated by homologous recombination(Ernfors et al., 1994). Western blot analysis revealed that theBDNF-immunoreactive band was completely lost in the pineal glandsof BDNF^/ mice (Fig. 7C), as we have observed previously for this BDNFband in other BDNF^/ tissues (Causing et al., 1997; Fawcett et al., 1998).

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Figure 7. BDNF is present in the pineal gland during the period of sympathetic target innervation, as detected by Western blot analysis. A, Western blot analysis for BDNF in the adult rat pineal gland. Tissue lysates were separated on polyacrylamide gels, transferred to nitrocellulose, and probed with an antibody to BDNF that we have previously extensively characterized (Causing et al., 1997; Fawcett et al., 1997, 1998). B, Pineal gland BDNF is the same size as recombinant human BDNF. Western blot analysis of tissue lysates revealed that the band seen in the adult pineal gland (Pineal) is similar in size to recombinant human BDNF (rhBDNF) and to BDNF in the adult rat cortex (Cortex). Lysates from the brain and pineal contain equal amounts of protein. C, Western blot analysis of BDNF in the pineal gland of BDNF^/ and BDNF^+/+ littermates at P13-P15. Note that the BDNF-immunoreactive band is not present in the BDNF^/ pineal gland.

We next determined whether incoming sympathetic axons were positive for p75NTR over this same time frame. Immunocytochemicalanalysis of the rat pineal gland using the anti-p75NTR antibodyMC192 revealed the presence of numerous p75NTR-positive fibersthroughout the pineal gland at P6 (data not shown), in a patternsimilar to that observed previously for tyrosine hydroxylase-positivesympathetic fibers (Kuchel, 1993). To confirm that this immunostainingcorresponded to bona fide p75NTR, we also performed Western blotanalysis, which demonstrated that p75NTR was present in both therat (data not shown) and mouse (see Fig. 9) pineal gland duringthe first few postnatal weeks. Thus, both BDNF and p75NTR arepresent in the pineal gland at the time of sympathetic targetcompetition.

The pineal gland, a sympathetic neuron target organ, is hyperinnervated in BDNF^+/ and ^/ mice

Together, our in vivo and in vitro data predict that when BDNF levels are lowered, sympathetic neuron target innervation shouldincrease. To test this prediction, we examined the level of sympatheticinnervation to the pineal gland of BDNF^+/ and BDNF^/ mice at P13-P15. Initially, we analyzed the density of sympatheticfibers immunocytochemically, using an antibody against TH, a proteinthat is a marker for sympathetic axons. To perform this analysis,we serially sectioned the pineal gland from BDNF^+/+, ^+/, and ^/ littermates and performed TH immunostaining on every third serialsection from pineal glands of each genotype. We then used an imageanalysis system to quantitate the percentage area covered by TH-positivefibers on each of these sections and averaged the percentage areaobtained from sections throughout each pineal gland, thereby ensuringthat sampling errors were not incurred as a result of differencesin the pattern of sympathetic innervation to the pineal glandin animals of different genotypes. This analysis revealed thatthick, TH-positive fibers were interspersed throughout the entirepineal gland of BDNF^+/ and BDNF^/ mice, whereas fibers in the pineal gland of BDNF^+/+ littermates were less abundant and appeared qualitatively thinner(Fig. 8A-C). This qualitative difference was reflected in thenumbers obtained using image analysis; in each of four sets oflittermates, the TH-positive innervation density was increasedapproximately two- to threefold in the pineal glands of BDNF^+/ versus BDNF^+/+ animals, and the level of innervation was similar in the BDNF^+/ and BDNF^/ pineal glands (Fig. 8F).

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Figure 8. The pineal gland is hyperinnervated with sympathetic fibers in BDNF^+/ and BDNF^/ mice at P13. A-C, Immunocytochemical analysis of tyrosine hydroxylase, a specific marker for sympathetic axons, in sections of the pineal gland from (A) BDNF^+/+, (B) BDNF^+/, and (C) BDNF^/ littermates. Note that the density of TH-positive fibers is increased in both the BDNF^+/ and ^/ sections relative to the section from the control littermate. D, E, Immunocytochemical analysis of TH (D) and p75NTR (E) in sections from the same P13 BDNF^+/ pineal gland. Note that although the p75NTR-immunoreactivity is somewhat fainter, the pattern of immunoreactivity is similar to that seen with anti-TH . F, Quantitative analysis of the relative amount of pineal gland area covered by TH-immunoreactive fibers in BDNF^+/+, ^+/, and ^/ animals, obtained using sections similar to those shown in A-C. For details of the analysis, see Results and Materials and Methods. Each experiment represents the results obtained from the pineal glands of one set of littermates of different genotypes. Note that in all four experiments, the amount of TH-positive innervation in the BDNF^+/+ pineal gland was significantly lower than that seen in either the BDNF^+/ or BDNF^/ pineal glands (*p < 0.05). A-E, Magnification, 160×.

To confirm the sympathetic hyperinnervation in the BDNF^+/ and ^/ pineal glands, we also measured the level of TH biochemically.Western blot analysis of equal amounts of protein from P13-P15pineal glands revealed that TH levels were increased in BDNF^+/ and BDNF^/ tissue relative to controls (Fig. 9), consistent with the immunocytochemicalresults (Fig. 8). We also used the same approach to quantitatethe levels of p75NTR and $alpha$ -tubulin, the former of which is presentin incoming sympathetic afferents (Fig. 8D,E), and the latterof which is enriched but not specific to all axons. Western blotanalysis revealed that like TH, levels of both of these proteinswere increased in quantity in the pineal glands of BDNF^+/ and ^/ mice relative to their wild-type littermates (Fig. 9). In contrast,levels of ERK1, a signaling protein that is present in all cells,were similar in all of the samples (Fig. 9).

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Figure 9. Levels of sympathetic axon markers are increased in sympathetic targets in BDNF^+/ and BDNF^/ mice. Western blot analysis of tyrosine hydroxylase (TH), p75NTR (P75), $alpha$ -tubulin (Tubulin), and ERK1 (Erk1) in equal amounts of protein from the pineal glands and carotid arteries of BDNF^+/+, BDNF^+/, and BDNF^/ littermates at P13-P15. Note that the blots shown for ERK1 are reprobes of the same blots shown for p75NTR, in the case of the pineal gland, and for $alpha$ -tubulin, in the case of the carotid artery.

To determine whether this increase in sympathetic innervation was limited to the pineal gland or whether it generalized toother sympathetic targets such as blood vessels, we also analyzedthe common carotid artery of BDNF^+/ versus BDNF^+/+ littermates. Western blot analysis of equal amounts of proteinrevealed that, as observed for the pineal gland, levels of TH,p75NTR, and tubulin were all increased in the ^+/ carotid artery (Fig. 9). In contrast, levels of ERK1 were similar(Fig. 9). Thus, when BDNF levels are reduced as they are in theBDNF^+/ mice (Fawcett et al., 1998), sympathetic innervation to at leasttwo peripheral targets isincreased.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Data presented in this paper demonstrate that BDNF-mediated activation of p75NTR antagonizes NGF-mediated growth of sympatheticneurons, thereby playing an essential role in the establishmentof appropriate target innervation in vivo. Specifically, theseexperiments indicate that when sympathetic neurons are culturedunder optimal survival conditions, exogenous BDNF and autocrineBDNF made by sympathetic neurons themselves inhibit NGF-promotedneuronal growth. BDNF mediates this inhibition via p75NTR because(1) function-blocking p75NTR antibodies enhance NGF-promoted growth,(2) BDNF cannot inhibit the growth of p75NTR^/ neurons, and (3) p75NTR^/ neurons grow more robustly in response to NGF than do their wild-typecounterparts. The physiological relevance of these culture findingsis demonstrated by the pineal gland studies presented in thispaper. Specifically, BDNF is present in the pineal gland, andp75NTR is localized to sympathetic neuron fibers at the time ofdevelopmental target innervation. When BDNF is reduced or absent,as in BDNF^+/ or BDNF^/ mice, the pineal gland is hyperinnervated with sympathetic fibers,and tyrosine hydroxylase levels are increased in two sympathetictargets, the pineal gland and the carotid artery. Together, thesedata indicate that BDNF, made by sympathetic neurons and/or theirtarget organs, acts via p75NTR to antagonize NGF-mediated growthand target innervation, suggesting that sympathetic target innervationis determined by the balance of positively and negatively actingneurotrophins present in developing targetorgans.

What is the biological rationale for having two neurotrophin receptors, one of which, TrkA, mediates survival and growth,and one of which, p75NTR, acts antagonistically to cause apoptosisand inhibit growth? With regard to neuronal survival, we havepreviously proposed that p75NTR provides a molecular mechanismfor ensuring rapid and active apoptosis when a neuron is unsuccessfulin competing for adequate amounts of the appropriate neurotrophin(Aloyz et al., 1998; Bamji et al., 1998; Miller and Kaplan, 1998).We propose that the antagonistic effects of TrkA and p75NTR ongrowth, as described here, are part of the same biological mechanism,as exemplified in the following three situations. First, if asympathetic neuron is late-arriving and/or reaches an inappropriatetarget, then TrkA would be only weakly induced as a consequenceof the lack of NGF, and p75NTR would be robustly activated byneurotrophins such as BDNF, leading to the rapid apoptotic eliminationof that neuron. Second, if a sympathetic neuron extends only onemain axon collateral and that collateral reaches an appropriatetarget and sequesters NGF, then TrkA would be robustly activated,allowing for survival of that neuron. The third possibility wouldoccur when a sympathetic neuron extends several axon collateralsor terminal branches. If one of those collaterals reaches an appropriatetarget and sequesters NGF, then the subsequent TrkA activationwould retrogradely mediate survival of the neuron and locallypromote terminal growth of that axon. If the second collateralarrives at a target that is already innervated or is inappropriate,then the low level of available NGF would cause only weak TrkAactivation, and p75NTR would be robustly activated by neurotrophinssuch as BDNF. In this final case, p75NTR activation would notaffect neuronal survival, because survival would be maintainedby TrkA activation from the other collateral. Instead, the majoreffect would be on target innervation itself, with p75NTR actinglocally to attenuate the growth of that specific axon branch.The net result would be selection of one collateral over the other.In this way, p75NTR would act as a "fine-tuning" mechanism thatwould allow both the selection of those neurons that reach appropriatetargets at an appropriate time, and the selection and maintenanceof axon collaterals or terminal branches that meet the same criteria.Disruption of such a mechanism could well explain the perturbationsin sympathetic neuron number (Bamji et al., 1998) and sympatheticinnervation (Lee et al., 1994) observed previously in the p75NTR^/ mice. In the absence of p75NTR, sympathetic target organs thatare innervated late, such as the pineal gland, are never appropriatelyinnervated (Lee et al., 1994), suggesting that the disruptionof appropriate competition for innervation of early sympathetictargets completely disrupts the later period of sympathetic targetinnervation.

Data presented here also indicate that BDNF is one p75NTR ligand that is responsible for regulating sympathetic neuron growth.Specifically, we have demonstrated that when BDNF in the pinealgland is reduced or absent, both the density of sympathetic innervationand the levels of tyrosine hydroxylase are increased. We believethat this increased pineal innervation is directly attributableto the loss of BDNF for the following reasons. First, the pinealgland does not receive peripheral sensory or motor innervation,making it unlikely that the observed effects are caused by a BDNF-dependentloss of, for example, sensory innervation. Second, although sympatheticneuron number is increased ~30% in BDNF^/ mice (Bamji et al., 1998), the increases in innervation leveland tyrosine hydroxylase are two- to threefold in the pineal gland,indicating that the degree of hyperinnervation is greater thanthe increase in cell number. Third, and perhaps most importantly,increased innervation to the pineal gland is also seen in BDNF^+/ mice, which are not delayed developmentally and have normal sympatheticand sensory neuron numbers. There are several precedents for sucha BDNF gene dosage effect in which the absence of one BDNF alleleis sufficient to significantly perturb nervous system structureand/or function (Korte et al., 1995; Carroll et al., 1998; Fawcettet al., 1998), strongly suggesting that even minor alterationsin the ratios of the neurotrophins are of major physiologicalimportance. In this regard, we believe that the most likely explanationfor our findings is that the BDNF present in the pineal glandinhibits NGF-mediated target innervation and that this inhibitionis lost when BDNF is reduced orabsent.

What is the source of BDNF in vivo? Although the CNS is the most abundant postnatal source of BDNF (Ernfors et al., 1990;Hofer et al., 1990; Phillips et al., 1990), it is clear that manyperipheral targets, including dermal mesenchyme, mandible, andwhisker pad (Schecterson and Bothwell, 1992), as well as muscle,heart, and lung (Maisonpierre et al., 1990), synthesize BDNF.Moreover, these same targets synthesize NGF (Levi-Montalcini,1987; Schecterson and Bothwell, 1992), suggesting that targetsthemselves determine the precise neurotrophin cohort encounteredby arriving axons. However, sympathetic neurons also synthesizeBDNF (Schecterson and Bothwell, 1992; Causing et al., 1997), andcultured neonatal sympathetic neurons secrete processed BDNF intothe media (Causing, Aloyz, and Miller, unpublished observations).Moreover, our data indicate that this autocrine BDNF is sufficientto inhibit NGF-mediated growth, at least in culture. However,it is not possible, on the basis of the data presented here, toassess the relative contribution of target-derived versus sympatheticneuron-derived BDNF in vivo. Nonetheless, it is tempting to speculatethat if BDNF is anterogradely trafficked into sympathetic axonsas it is into sensory (Zhou and Rush, 1996) and central (von Bartheldet al., 1996; Altar et al., 1997; Conner et al., 1997; Fawcettet al., 1998) axons, then secretion from sympathetic terminalsmay well provide a cellular mechanism whereby "successful" terminalscould eliminate and/or make the environment unfavorable for later-arrivingaxon collaterals. A precedent for a related mechanism derivesfrom the neuromuscular junction, where active synaptic sites apparentlydestabilize inactive synapses in their vicinity (Colman et al.,1997).

How does p75NTR inhibit TrkA-mediated neuronal growth? One potential mechanism involves p75NTR-mediated generation of intracellularceramide (Dobrowsky et al., 1994, 1995). Recently, Posse de Chaveset al. (1997) demonstrated that elevation of intracellular ceramidein distal sympathetic neurites locally inhibited NGF-promotedsympathetic axon growth. Thus, as proposed by the authors, activationof p75NTR could well attenuate neurite growth via increased ceramide.A similar and potentially additive attenuation would occur ifactivated p75NTR directly downregulated TrkA-mediated growth signalsby serine-threonine phosphorylation of the TrkA receptor via ceramide-activatedkinases (MacPhee and Barker, 1997). The net outcome of these ceramide-drivenmechanisms would be inhibition of growth and potential axonalretraction. This receptor cross-talk is also likely to be bidirectional.Robust TrkA activation would likely silence a p75NTR-mediatedceramide flux, as previously demonstrated in PC12 cells (Dobrowskyet al., 1995), thereby further favoring axonal growth. Such negativefeedback between these two receptors provides a mechanism forbiasing the cell to one of two outcomes, growth or no growth,thereby ensuring that axon collaterals that are only minimallysuccessful in terms of sequestering target territory do not remainto compete during this critical developmentalperiod.

Does this functional antagonism between TrkA and p75NTR generalize to neurons other than sympathetic neurons? The most compellingcase that it does, to at least some degree, derives from studieson basal forebrain cholinergic neurons. In p75NTR^/ mice, the number of basal forebrain cholinergic neurons increases(Van der Zee et al., 1996) and the hippocampus is hyperinnervated(Yeo et al., 1997), two phenotypes reminiscent of sympatheticneurons in p75NTR^/ and BDNF^/ mice (Lee et al., 1994; Bamji et al., 1998; data presented here).Such functional antagonism may also occur, in at least some situations,for TrkA-positive sensory neurons. For example, the local NGF-promotedgrowth of adult sensory neurons is inhibited by BDNF (Kimpinskiet al., 1997), cultured dorsal root ganglia neurons showed a decreasein growth cone turning toward NGF-coated beads in the presenceof BDNF (Gallo et al., 1997), and functional ablation of p75NTRusing antisense oligonucleotides enhanced the survival of culturedpostnatal sensory neurons (Barrett and Bartlett, 1994). Moreover,one recent study indicates that this functional antagonism betweenp75NTR and TrkA may not only regulate the innervation of appropriatetargets, but may also allow axons to distinguish between permissiveand nonpermissive growth substrates. In particular, when NGF isoverexpressed in astrocytes of transgenic mice, absence of p75NTRleads to robust sympathetic axon growth on myelinated tracts inthe mature CNS, indicating that p75NTR plays a significant rolein making CNS myelin an inhibitory growth environment, at leastfor sympathetic axons (Walsh et al., 1999). However, it is alsoclear that, like other members of the p75NTR family, the outcomeof p75NTR-mediated signal transduction is a function of cellularcontext. For example, depending on the cellular environment, p75NTRregulates cell migration (Anton et al., 1994) and gene expression(Itoh et al., 1995) and can positively modulate TrkA signaling(Barker and Shooter, 1994; Verdi et al., 1994).

In summary, our studies provide evidence for a mechanism whereby two receptors that are coexpressed in sympathetic neurons,TrkA and p75NTR, can functionally interact to regulate processoutgrowth during the time of target innervation, thereby ensuringappropriate matching of neurons and their target territory. Thus,not only do neurotrophins regulate neuronal survival and growth,depending on the particular receptors that they activate, butthey may also provide a mechanism whereby neurons can recognizewhether they are exposed to the "right" versus the "wrong" targets.Such functional antagonism, mediated by TrkA and p75NTR, appearsto be essential for appropriate sympathetic neuron target innervation,and similar mechanisms may well play an essential role in thematching of neurons with their targets throughout the nervoussystem.

  FOOTNOTES

Received July 13, 1998; revised March 26, 1999; accepted April 14, 1999.

This study was supported by grants from the Canadian Medical Research Council and NeuroSciences Network (F.D.M.). F.D.M. isa Killam Scholar, and during the course of this work, R. Aloyzwas a NeuroSciences Network fellow. We thank Christine Pozniakand Marta Majdan (both of McGill University) for their help withthe BDNF^+/ and p75NTR^/ colonies, and other members of the Miller laboratory for theiradvice and input throughout the course of thiswork.
Correspondence should be addressed to Dr. Freda D. Miller, Centre for Neuronal Survival, Montréal Neurological Institute,3801 rue University, Montréal, Québec, Canada, H3A2B4.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aloyz RS, Bamji SX, Pozniak CD, Toma JG, Atwal J, Kaplan DR, Miller FD (1998) p53 is essential for developmental neuron death as regulated by the TrkA and p75 neurotrophin receptors. J Cell Biol 143:1691-1703[Abstract/Free Full Text].
Altar CA, Cai N, Bliven T, Juhasz M, Conner JM, Acheson AL, Lindsay R, Wiegand SJ (1997) Anterograde transport of brain-derived neurotrophic factor and its role in the brain. Nature 389:856-860[Medline].
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