Endogenous Brain-Derived Neurotrophic Factor and Neurotrophin-3 Antagonistically Regulate Survival of Axotomized Corticospinal Neurons In Vivo

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The Journal of Neuroscience, May 15, 2001, 21(10):3492-3502

Endogenous Brain-Derived Neurotrophic Factor and Neurotrophin-3 Antagonistically Regulate Survival of Axotomized Corticospinal Neurons In Vivo
Klaus M. Giehl¹, Stephan Röhrig¹, Henk Bonatz¹, Martin Gutjahr¹, Britta Leiner¹, Ilse Bartke², Qiao Yan³, Louis F. Reichardt⁴, Carey Backus⁴, Andrew A. Welcher³, Kathrin Dethleffsen⁵, Pedro Mestres¹, and Michael Meyer⁵
¹ University of Saarland, Department of Anatomy, 66421 Homburg/Saar, Germany, ² Pharma Research Penzberg, Roche Diagnostics GmbH, Department of Cell Biology, 82372 Penzberg, Germany, ³ Amgen, Thousand Oaks, California 91320-1799, ⁴ Department of Physiology and Howard Hughes Medical Institute, University of California, San Francisco, California 94143, and ⁵ Max-Planck-Institue of Neurobiology, 82152 Martinsried, Germany

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ABSTRACT
INTRODUCTION
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DISCUSSION
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Neuronal growth factors regulate the survival of neurons by their survival and death-promoting activity on distinct populationsof neurons. The neurotrophins nerve growth factor (NGF), brain-derivedneurotrophic factor (BDNF), and neurotrophin-3 (NT-3) promoteneuronal survival via tyrosine kinase (Trk) receptors, whereasNGF and BDNF can also induce apoptosis in developing neurons throughp75^NTR receptors in the absence of their respective Trk receptors. Usingmutant mice and inactivation of neurotrophins and their receptorswith antibodies in rats, we show that endogenous NT-3 inducesdeath of adult BDNF-dependent, axotomized corticospinal neurons(CSNs). When NT-3 is neutralized, the neurons survive even withoutBDNF, suggesting complete antagonism. Whereas virtually all unlesionedand axotomized CSNs express both trkB and trkC mRNA, p75 is barelydetectable in unlesioned CSNs but strongly upregulated in axotomizedCSNs by day 3 after lesion, the time point when cell death occurs.Blocking either cortical TrkC or p75^NTR receptors alone prevents death, indicating that the opposingactions of NT-3 and BDNF require their respective Trk receptors,but induction of death depends on p75^NTR cosignaling. The results show that neuronal survival can be regulatedantagonistically by neurotrophins and that neurotrophins can induceneuronal death in the adult mammalian CNS. We further presentevidence that signaling of tyrosine kinase receptors of the trkfamily can be crucially involved in the promotion of neuronaldeath in vivo.

Key words: neuronal death; neurotrophins; TrkC; p75; cortex; lesion

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ABSTRACT
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Neurotrophins comprise a family of closely related neurotrophic factors expressed in target tissues of neurons and in thecentral and peripheral nervous systems. Four neurotrophins havebeen identified in rodents: nerve growth factor (NGF), brain-derivedneurotrophic factor (BDNF), neurotrophin-3 (NT-3), and neurotrophin-4/5(NT-4/5) (Lewin and Barde, 1996). The biological effects of thesefactors are mediated by the common neurotrophin receptor p75^NTR and the tyrosine kinase (trk) family receptors with NGF bindingTrkA, BDNF and NT-4/5 binding TrkB, and NT-3 binding TrkC (Barbacid,1995). At high concentrations, NT-3 can also stimulate TrkA andTrkB as nonpreferred receptors (Davies et al., 1995; Ryden andIbanez, 1996). Promotion of neuronal survival is one of the mostprominent physiological functions of the neurotrophins (Barbacid,1995). It has been shown, though, that NGF and BDNF can also induceneuronal death via p75^NTR receptors in developing neurons (Dechant and Barde, 1997; Kaplanand Miller, 1997; Bamji et al., 1998).

Until recently it was thought that neuronal survival is regulated by the limited access to survival-promoting factors (Lewinand Barde, 1996). This hypothesis was modified by the findingsthat developmental death is induced via p75^NTR in retinal neurons by endogenous NGF (Frade et al., 1996, 1997;Frade and Barde, 1998) and in sympathetic neurons by BDNF (Bamjiet al., 1998). Thus, a neurotrophin can promote neuronal survivalor death, depending on which receptor it activates. In this concept,Trk receptors mediate survival signals, whereas p75^NTR mediates the death signal in the absence of the respective Trkreceptor (Dechant and Barde, 1997; Kaplan and Miller, 1997; Bamjiet al., 1998). However, it is not known whether survival of theneurons that die because of a neurotrophin is promoted by anotherendogenous neurotrophin and whether neurotrophins can induce deathof mature neurons at all. The present study approaches this questionin the corticospinalsystem.

The corticospinal system constitutes a major central motor projection to spinal cord motoneurons (Nudo and Masterton, 1990).Approximately half of adult rat corticospinal neurons of the sensorymotor cortex (CSNs) die after axotomy at internal capsule levels(Fig. 1) (Giehl and Tetzlaff, 1996; Bonatz et al., 2000). Virtuallyall CSNs express trkB and trkC and are rescued from axotomy-induceddeath by high-dose BDNF and NT-3 treatment (Giehl and Tetzlaff,1996), indicating that these factors play a role in their survivalregulation. Indeed, endogenous BDNF is a crucial survival factorfor most axotomized CSNs (Giehl et al., 1998). However, the doseof NT-3 that completely rescues CSNs if applied alone (Giehl andTetzlaff, 1996) results only in partial survival if endogenousBDNF is simultaneously neutralized (Giehl et al., 1998). In addition,NT-3 infusions increase BDNF mRNA expression in cortical layers2-4 (Schütte et al., 2000). These findings suggest that the effectsof high-dose NT-3 treatment (Giehl and Tetzlaff, 1996) are notattributable to the activation of TrkC alone but rather resultfrom stimulation of endogenous BDNF protection of lesioned CSNs.They may, therefore, not reflect the physiological function ofNT-3 for CSNs.

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Figure 1. Schematic illustrating the corticospinal lesion model. The cell death area (cda; outlined in black) is the area where death of CSNs is regularly observed after ICL. The quantitative survival data were obtained from the cda. Indicated are the localization of CSNs, their projection pathway, and the extent of the ICL. ic, Internal capsule; ac, anterior commissure. A, Frontal plane of the forebrain. Axotomy side is left, control side right. L-B is the lateral level from which the sagittal plane in B is taken. B, Sagittal plane of the brain on the axotomy side. L-A is the frontal level from which A is taken. CSNs (sensory motor cortex) are localized in the posterior three quarters of the mediodorsal areas of corticospinal neurons (Miller, 1987; Bonatz et al., 2000). The corticospinal neurons of the anterior quarter belong to the medial prefrontal and the supplementary motor cortex (Miller, 1987; Bonatz et al., 2000).

The present study shows that endogenous NT-3 promotes the death of all BDNF-dependent CSNs, indicating that endogenous neurotrophinscan antagonistically regulate neuronal survival in the adult mammalianCNS. Activation of both p75^NTR and TrkC receptors is required for this effect of NT-3, suggestingthat cosignaling by a tyrosine kinase receptor and a tumor necrosisfactor receptor family member is essential for the promotion ofCSNdeath.

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Operation procedure. Experimental procedures and maintenance of animals were approved by the local Animal Care Committee accordingto the German law regulating the experimental use of animals.Five- to 9-week-old mice of both sexes of a BDNF (Korte et al.,1995) and NT-3 (Airaksinen et al., 1996) mutant strain and maleSprague Dawley rats weighing 190-330 gm were used. The procedureand stereotaxic coordinates for the operations, internal capsulelesion (ICL), confirmation of the axotomy of CSNs after ICL, intracorticaldelivery of solutions (only for rats), and the determination ofthe lesion and cell death areas have been described elsewhere(Giehl and Tetzlaff, 1996; Bonatz et al., 2000). In brief, todistinguish CSNs from other cortical layer 5 neurons, they wereretrogradely labeled by fluorescence tracer injections to thecorticospinal tracts at cervical spinal cord levels C4/5 beforeaxotomy. Fast Blue (FB) (2% in 0.2% DMSO) and/or a rhodamine tracermixture (RDX) (15% rhodamine dextran 10,000, 10% rhodamine dextran3000, and 10% rhodamine-b-isothiocyanate in 0.2% DMSO) were usedas tracers. FB was used as the primary tracer in all groups thatreceived ICL. One to 2 weeks after FB injection, CSNs of one sideof the brain were axotomized by ICL. ICL creates a horizontal,circle-shaped cut through the entire internal capsule (Bonatzet al., 2000) through which CSNs send their axons to their spinalcord targets (Fig. 1) (Nudo and Masterton, 1990). As determinedby the injection of RDX at spinal cord level C3/4 immediatelyafter the lesion, ICL results in axotomy of all corticospinalneurons of the sensory motor cortex (CSNs) of the lesion sidein rats (Giehl and Tetzlaff, 1996; Bonatz et al., 2000) and inmice (Fig. 2). In the rat treatment groups, Alzet 2001 osmoticminipumps were implanted in the same operation session for intracorticaldelivery of solutions. For this delivery, a 30 gauge steel cannulaconnected to the minipump via a silicone tube was implanted intraparenchymallyinto the lesion area of the cortex on the lesion side.

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Figure 2. Death of axotomized CSNs is increased in BDNF mutant mice but almost completely prevented in NT-3 mutant mice. A, Top pairs of the photomicrographs show FB-labeled CSNs of representative animals of each experimental group, 1 week after axotomy. Axotomy induces death in both BDNF (+/+) and NT-3 (+/+) animals (wild-type control groups). This death is increased in BDNF (+/ $-$ ) animals and almost completely prevented in NT-3 (+/ $-$ ) animals. The bottom pair of photomicrographs in each experimental group shows the same sections under illumination for RDX (red label) which has been applied after ICL to confirm the axotomy. This results in RDX labeling of unlesioned CSNs but does not label axotomized CSNs. On the control side, virtually all CSNs are double-labeled with FB and RDX. On the axotomy side, FB-labeled CSNs are not labeled with RDX, indicating the completeness of axotomy. Scale bar, 0.5 mm. B, Quantification of the survival of axotomized mice CSNs (indicated is mean survival ± SEM). One-third of the CSNs die in the control groups of the BDNF (n = 9) and NT-3 (n = 12) knock-out strains. This death is increased in BDNF (+/ $-$ ) animals [n = 9; p < 0.01 vs control as determined by (adb) NKT] and almost completely prevented in NT-3 (+/ $-$ ) animals [n = 10; p < 0.01 vs control adb NKT].

Intracortically infused solutions. The osmotic minipumps delivered either NT-3-neutralizing mouse monoclonal NT-3 antibodyof the IgG1 subclass (anti-NT-3; 1 mg/ml in P1 buffer) (Barreset al., 1994), the BDNF-neutralizing rabbit affinity-purifiedBDNF antibody RAB (anti-BDNF; 1 mg/ml in PBS) (Yan et al., 1997b;Giehl et al., 1998), a combination of anti-NT-3 and anti-BDNF(1 mg/ml each in P1 buffer), p75^NTR-blocking monovalent Fab fragments of IgG of the rabbit REX antibodyagainst p75^NTR (REX-Fab; 150 µg/ml or 300 µg/ml in P2 buffer) (Weskamp and Reichardt,1991), protein A column-purified IgG of the rabbit anti-TrkC antibodyTC89 (TC89; 2, 4, 8, or 16 mg/ml in P2 buffer), human recombinantNT-3 (0.5 mg/ml in PBS), rabbit anti-turkey IgG (RIgG; Sigma,St. Louis, MO; 1 or 16 mg/ml in PBS; as control for anti-BDNFand TC89), mouse IgG1 (MIgG1; Sigma; 1 mg/ml in P1-buffer; ascontrol for anti-NT-3), monovalent Fab fragments of rabbit IgG(RFab; Jackson ImmunoReseach, West Grove, PA; 150 µg/ml or 1 mg/mlin P2 buffer; as control for REX-Fab), 20 mM PBS (as control forRIgG and NT-3), a 1:1 mixture of PBS and 10 mM potassium phosphate/150mM sodium chloride buffer (P1 buffer; as control for MIgG1), or2.5 mM potassium phosphate-20 mM disodium phosphate-120 mM sodiumchloride buffer (P2 buffer; as control for RFab and as buffercontrol for TC89). All solutions contained 50 U/ml penicillin-streptomycinand were infused at a rate of 1 µl/hr for 7 d. The respectiveneutralizing and blocking properties of anti-NT-3 (Barres et al.,1994), anti-BDNF (Yan et al., 1997b; Giehl et al., 1998), andREX-Fab (Weskamp and Reichardt, 1991) have been demonstrated elsewhere.For TC89, see "Characterization of TC89." The correct generationof the REX-Fab fragments has been confirmed in protein-gels (datanot shown). The intracortical diffusion area of the infused antibodieswas controlled by immunohistochemistry and was never <4 mm indiameter, i.e., the CSNs of the cell death area (see "Analysisof Axotomy and Survival") were located within the diffusionareas.

Characterization of TC89. The TC89 antiserum was generated in rabbit against a fusion protein of trpE (Rimm and Pollard, 1989)linked to amino acids 127-429 of the extracellular domain of ratTrkC, expressed in Escherichia coli. Western blot analyses ofvarious recombinant Trk proteins (Yan et al., 1997a) indicatedthat the TC89 antisera was specific for TrkC (see Fig. 5B). TC89results in TrkC-like immunoreactivity in rat brain sections (datanot shown). The effects of protein A-purified IgG of TC89 serumon TrkC phosphorylation have been tested in TrkC-transfected NIH3T3cells essentially as described (Tsoulfas et al., 1996). TrkC phosphorylationafter 5 min of 100 ng/ml NT-3 served as positive control. TrkCphosphorylation was completely abolished by TC89 treatment (16µg/ml added for 10 min starting 5 min before NT-3 addition) (seeFig. 5C). Treatment with TC89 IgG alone had no effect on TrkCphosphorylation.

TrkB phosphorylation. Tyrosine phosphorylation of TrkB was assessed in 2 × 2 × 1.5 mm blocks of cortex of rats that had beentreated with NT-3 (500 ng/µl in vehicle, 10 µl) or vehicle (20mM PBS, 10 µl) for 30, 60, 120 or 360 min. Tissue processing wasas described (Tsoulfas et al., 1996) with the following modifications.One milliliter of extract was incubated overnight with 2 µg ofthe tyrosine phosphate-specific antibody 4G10 (Upstate Biotechnology,Lake Placid, NY) at 4°C. Protein A Sepharose was added and boundfor 2-3 hr at 4°C. Western blots were detected using a previouslygenerated and characterized TrkB antiserum (trkBMBSKLH; Offenhäuseret al., 1995).

RT-PCR of trkC isoforms. Total RNA was extracted from cortical tissue blocks (2 × 2 × 1.5 mm) of rats that had received NT-3(500 ng/µl in vehicle at a rate of 1 µl/hr) or vehicle (20 mMPBS at a rate of 1 µl/hr) for 3 or 7 d before analysis. Reactionswere performed essentially as described before (Offenhäuser etal., 1995) using primers on both sides of the kinase insert. The3' primer was modified to CTCCACACATCACTCTCTGTG. To control forlinear amplification, reactions of 26 and 30 cycles wererun.

Tissue processing. Seven days after tracer application (unlesioned animals) or after ICL (lesioned animals), the animals werekilled by an overdose of sodium pentobarbital and transcardiallyperfused with PBS followed by 4% paraformaldehyde (PFA) solution.The brains were post-fixed in 4% PFA (1 hr), cryoprotected in20% sucrose in PBS (12 hr), frozen, and cut into 20 µm cryostatserial coronal sections. In mice, every second section was collectedfor cell counts. In mice that received an ICL, the remaining sectionswere collected separately for in situ hybridizations (ISHs) (confirmationof neurotrophin receptor expression, data not shown). In rats,every fifth section was collected for cell counts, and the remainingsections were collected separately for ISH and other procedures.For the semiquantitative ISH on rat brain sections, only sectionsfrom the center of the cell death area (see "Analysis of survival")wereused.

Rat and mouse corticospinal systems. The developmental principles for establishing the corticospinal projection do not differbetween rat and mice (O'Leary and Koester, 1993; Uematsu et al.,1996). Rats have more and larger corticospinal neurons than micebut of very similar localization (Nudo and Masterton, 1990; Nudoet al., 1995). Detailed mapping (Bonatz et al., 2000) revealedthat mutant and wild-type mice have the same area-specific localizationof corticospinal neurons as rats (Miller, 1987; Bonatz et al.,2000), displaying three major areas of localization: (1) the sensorymotor cortex, (2) the supplementary motor and medial prefrontalcortex, and (3) the somatosensory cortex. All corticospinal neuronsof the sensory motor cortex (CSNs) are axotomized by ICL (Fig.2). In contrast, ICL does not result in complete axotomy of corticospinalneurons of the other areas which have, therefore, not been consideredin this study. Analyses of trkB, trkC, and p75 mRNA expressionin wild-type and neurotrophin mutant mice (data not shown) revealedthat their unlesioned and axotomized CSNs show identical expressionpatterns as rats and that p75 is upregulated also in mice afterICL. Thus, the organization and neurotrophin dependencies of bothrat and mouse corticospinal systems seem to be verysimilar.

Analysis of survival. The number of CSNs was assessed by blinded cell counts of every second section collected for cell counts,i.e., every fourth section of the mice and every 10th sectionof the rat brains were quantified. The criterion for a CSN wasa Tracer-filled pyramidal-shaped profile >4 µm (rats) or >3 µm(mice) in diameter (Giehl and Tetzlaff, 1996; Bonatz et al., 2000).Both in mice and in rats, all CSNs of the lesion side are axotomizedby ICL (see operation procedure). The central 2.8 mm in rats andthe central 1.6 mm in mice of the CSN area were defined as "celldeath area" (Bonatz et al., 2000), the area where dying CSNs wereregularly observed in both lesion-only animals (rats and wild-typemice) and lesioned animals that were treated with control solutions(rats). This area was used as an anatomical mask for the otherexperimental groups to obtain the respective survival data. Bothin mice and in rats, the anterior end of the cell death area isat the frontal plane of the anterior pole of the anterior commissure(Fig. 1). Within the cell death area, percentage of survival isdefined as "number of FB-labeled CSNs on the lesion side/numberof FB-labeled CSNs contralateral to the lesion side × 100%." Thedata are based on a total of over 380,000 cells counted in ratsand over 310,000 cells counted in mice. One-way ANOVA which wasfollowed by a post hoc Newman-Keuls test (NKT) and a post hocFisher's least significance difference test (FLSD) was used todetermine the statistical significance of differences in survivalamong the individual experimental groups. As determined separatelyfor mice and rats, the differences in the mean values among theindividual experimental groups were highly significant using ANOVA(p < 0.001). For the respective NKT and FLSD, see Figurelegends.

Analysis of neurotrophin receptor expression. Abundant TrkC immunoreactivity has been shown in several cortical layers, includinglayer 5 (Miller and Pitts, 2000; Pitts and Miller, 2000), andp75 immunoreactivity is inducible by several stimuli includinglesions in many cortical areas (Botchkina et al., 1997; Roux etal., 1999; Shi and Mocchetti, 2000) and after axotomy in spinalmotoneurons (Wu et al., 1993). To examine whether the respectiveproteins localize to unlesioned and/or axotomized corticospinalneurons, we performed immunohistochemistry for the neurotrophinreceptors on sections from animals that received unilateral axotomyof FB-labeled CSNs. Satisfactory cortical immunolabeling was onlypossible with mild fixation and free-floating techniques thatare not compatible with the maintenance of FB labeling of CSNs.We, therefore, analyzed neurotrophin receptor expression withan oligonucleotide in situ hybridization technique that has previouslybeen shown to be compatible with neuronal FB label (Giehl andMestres, 1995; Giehl et al., 1998). Oligonucleotide probes forthe individual mRNAs were labeled with ³⁵S-dATP (DuPont NEN, Boston, MA), using terminal deoxynucleotidetransferase (Life Technologies, Gaithersburg, MD). The p75 probeused for the semiquantitative in situ hybridizations reportedin this paper was complementary to the nucleotides 932-971 ofthe rat p75 mRNA (Radeke et al., 1987). We repeated the experimentswith a probe complementary to nucleotides 1809-1848 of rat p75mRNA (Radeke et al., 1987), and the results were essentially thesame (data not shown). The trkC probe (Giehl and Tetzlaff, 1996)was complementary to base pairs 2109-2272 (except 2134-2250) andbridged the insertion site (2134-2250) of the TrkC tyrosine kinasedomain (Valenzuela et al., 1993). Posthybridization washes andautoradiography were performed as described elsewhere (Giehl andMestres, 1995). At the high stringency conditions used for thehybridizations and the posthybridization washes (Giehl and Mestres,1995), the trkC probe is highly specific for the noninserted full-lengthtrkC isoform (Giehl and Tetzlaff, 1996).

Quantification of mRNA expression. The procedure used for the quantification of mRNA expression in CSNs is described elsewhere(Giehl et al., 1998). For the calculation of the percentage ofCSNs expressing the respective mRNA, mRNA levels in CSNs are expressedas an x-fold of background grain density (see below). Becauseexpression of p75 and trkC mRNA in reactive glia cannot be excludedin brain tissue after experimental manipulation, background measurementswere performed over the slide. The brain tissue itself can havean unspecified chemographic effect on the grain density, whichresults in higher background values over the tissue than overthe slide (Rogers, 1979; McCabe et al., 1989). To account forthis chemographic effect, we determined a correction factor forthe above slide background measurements as follows: backgroundmeasurements have been performed over the slide and the cortexof autoradiographies obtained from the competition tests for therespective probes. Because autoradiographies of competition testsdid not contain positive label, these measurements assess solelythe chemographic component of the brain tissue without includingthe glial signal. From these measurements, we calculated a slide-to-brainratio for each probe (1.6 for p75 and 1.66 for trkC). These slide-to-brain-ratioshave then been used as correction factor for the background measurementsof the p75 and trkC ISH, respectively. The procedure and rationalefor determining the criterion for a CSN expressing the respectivemRNA (threshold in all cases more than threefold corrected background)has been described elsewhere (McCabe et al., 1989; Giehl et al.,1998). The data are based on a total of >25,000 cells. As determinedseparately for p75 and trkC, the differences in the mean valuesamong the individual experimental groups were highly significantusing ANOVA (p < 0.001). For the respective NKT and FLSD, seeFigurelegends.

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The gross anatomy of the corticospinal system is not altered in young adult BDNF and NT-3 heterozygotes

The developmental role of BDNF and NT-3 for CSNs was analyzed in young adult BDNF and NT-3 mutant mice. For this analysis,it is necessary to specifically label CSNs by injecting retrogradetracers to the corticospinal tract of the spinal cord. Becausehomozygous BDNF (Ernfors et al., 1994a; Jones et al., 1994) andNT-3 knock-out mice (Ernfors et al., 1994b; Farinas et al., 1994;Tessarollo et al., 1994) survive only a few days after birth,and the axonal connectivity of CSNs to the spinal cord developsbetween P0 and P20 (Jones et al., 1982; Oudega et al., 1994; Uematsuet al., 1996), only the respective heterozygous (+/ $-$ ) and wild-type(+/+) animals were analyzed. CSNs were labeled with RDX in 6-week-oldmice. Mapping (data not shown) and cell counts (Table 1) of RDX-labeledCSNs did not reveal any changes regarding localization or numbersof CSNs in BDNF or NT-3 (+/ $-$ ) animals, suggesting that wild-typelevels of BDNF and NT-3 are not essential for the developmentalregulation of these aspects.


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Table 1. RDX-labeled CSNs

Survival of axotomized CSNs is decreased in BDNF (+/ $-$ ) and improved in NT-3 (+/ $-$ ) mice

To examine the roles of these neurotrophins for mature CSN, we analyzed their response to axotomy in adult mice of these mutantstrains. FB-labeled CSNs of 8- to 9-week-old mice were axotomizedby an ICL (Fig. 1). One-third of the axotomized CSNs died in theBDNF and NT-3 (+/+) groups within the first week after axotomy(Fig. 2). Death was significantly increased in BDNF (+/ $-$ ) animals(Fig. 2), indicating that BDNF is a survival factor for axotomizedmurine CSNs. In contrast, survival of axotomized CSNs was muchimproved in NT-3 (+/ $-$ ) mice (Fig. 2), suggesting that endogenousNT-3 promotes CSNdeath.

Endogenous NT-3 induces death of BDNF-dependent axotomized rat CSNs

To determine whether the unexpected results in NT-3 (+/ $-$ ) animals reflect promotion of death by endogenous NT-3 or were attributableto developmental changes caused by the targeted mutation of theNT-3 allele, we acutely reduced NT-3 levels in wild-type albinorats with a monoclonal NT-3 antibody (anti-NT-3) (Barres et al.,1994). Anti-NT-3 was continuously infused into the lesioned cortexfor 7 d starting immediately after ICL, which resulted in completerescue of FB-labeled CSNs from axotomy-induced death (Fig. 3).Thus, endogenous NT-3 induces death of axotomized CSNs. The majorityof axotomized rat CSNs depend on endogenous BDNF for survival(Giehl et al., 1998). This BDNF-dependent population consistsof all CSNs that die after axotomy and, in addition, almost halfof those that survive their axotomy (Giehl et al., 1998). Togetherwith the present finding, these data demonstrate that the survivalof all CSNs that die after axotomy is antagonistically regulatedby endogenous NT-3 and BDNF.

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Figure 3. Survival of axotomized CSNs is antagonistically regulated by endogenous BDNF and NT-3. A, FB-labeled CSNs of lesion and control sides of representative animals of control groups [lesion-only (l.o.), mouse IgG1 (MIgG1), and rabbit IgG (RIgG)] and the groups receiving neutralizing neurotrophin antibodies [NT-3 antibody (anti-NT-3), BDNF antibody RAB (anti-BDNF), and anti-NT-3 plus anti-BDNF] 1 week after axotomy. In the control groups, axotomy results in death of many CSNs. This death is completely prevented after anti-NT-3 treatment and strongly increased after anti-BDNF treatment. Simultaneous application of BDNF and NT-3 (anti-NT-3 + anti-BDNF) results in complete survival of axotomized CSNs. Scale bar, 1 mm. B, Quantification of survival of axotomized rat CSNs (indicated is mean survival ± SEM). The control groups display significant death within the first week after axotomy [l.o. (n = 11), PBS (n = 12), P1 buffer (64 ± 5%; n = 5; data not shown), MIgG1 (n = 4), and RIgG (1 mg/ml; n = 5)]. Anti-NT-3 treatment completely prevents this death [n = 7, p < 0.01 vs each control group adb NKT]. In contrast, approximately two-thirds of the CSNs die after anti-BDNF treatment [n = 5, p < 0.01 vs RIgG adb NKT, p < 0.05 vs l.o. adb NKT]. Simultaneous anti-NT-3 + anti-BDNF treatment completely rescues CSNs [n = 5, p < 0.01 vs all control groups adb NKT], demonstrating that the NT-3-mediated death signal is dominant and that virtually all BDNF-dependent CSNs (see Results) underlie an antagonistic survival regulation by BDNF and NT-3. The difference in survival between l.o. group and groups receiving control solutions is statistically significant and has been discussed elsewhere (Giehl and Tetzlaff, 1996; Giehl et al., 1998).

To show whether NT-3 or BDNF is functionally dominant, we simultaneously infused for 7 d the affinity-purified neutralizingBDNF antibody RAB (anti-BDNF) (Yan et al., 1997b; Giehl et al.,1998) and anti-NT-3 to axotomized CSNs and compared it with theeffects of anti-BDNF alone. Anti-BDNF treatment alone caused deathof approximately two-thirds of the axotomized CSNs, whereas deathwas completely prevented by anti-BDNF/anti-NT-3 treatment (Fig.3). Thus, BDNF-dependent CSNs survive axotomy in the absence ofBDNF if NT-3 is neutralized. This finding further shows that thetwo neurotrophins have opposing effects on the survival of allBDNF-dependentCSNs.

Axotomized rat CSNs express p75 and trkC mRNA, and trkC expression is suppressed by high-dose NT-3 treatment

Although survival promotion of neurotrophins is mediated by Trk receptors, their death-inducing activity is thought to bemediated via p75^NTR receptor in the absence of signaling by the respective Trk receptor(Dechant and Barde, 1997; Kaplan and Miller, 1997). We have shownrecently that virtually all lesioned CSNs express trkB mRNA (Giehlet al., 1998), consistent with the survival promotion of endogenousBDNF. To show whether axotomized CSNs display a neurotrophin receptorexpression pattern compatible with the death promotion of endogenousNT-3, we analyzed the expression of p75 mRNA (Radeke et al., 1987)and trkC mRNA lacking an insert in the tyrosine kinase domain(Valenzuela et al., 1993) with semiquantitative in situ hybridizationswithin the first week after axotomy. Axotomy-induced death ofCSNs occurs between days 3 and 4 after ICL, reaches a plateauby day 5 (Giehl and Tetzlaff, 1996), and does not further proceedlater on (Giehl and Tetzlaff, 1996; Giehl et al., 1997). Thus,the receptor mRNA expression was assessed at days 1, 3, and 7after axotomy. Virtually all CSNs expressed trkC at any time point(Fig. 4). Figure 4 further shows that many non-CSN cells expresstrkC mRNA. As revealed by cresyl violet staining (data not shown),this expression is mainly localized to pyramidal cells of corticallayer 5, but some of the label appeared to be derived from glia.In contrast to the robust expression of trkC, p75 was barely detectablein unlesioned CSNs or in CSNs at day 1 after axotomy, but it wasclearly upregulated in axotomized CSNs at postlesion day 3 andlater (Fig. 4). The time course of p75 expression suggests thatp75^NTR receptor may be involved in the death induction of CSNs. Noncorticospinalcells of cortical layer 5 on the lesion side have higher p75 levelsthan CSNs, indicating that ICL leads to a general increase ofp75 expression on the axotomy side (Fig. 4). As revealed by cresylviolet counterstaining (data not shown), this p75 expression ismainly localized to pyramidal-shaped neurons of cortical layer5, suggesting that these noncorticospinal cells are subcorticallyprojecting neurons that have been axotomized by the internal capsulelesion. Whether these cells contribute to the death of CSNs isnot clear.

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Figure 4. Expression of p75 and trkC mRNA in unlesioned and axotomized vehicle- and NT-3-treated CSNs. A, Double exposures of FB-labeled CSNs and autoradiograms of p75 and trkC ISHs at days 3 and 7 after axotomy. p75 expression is barely detectable in unlesioned CSNs but clearly upregulated by days 3 and 7 after axotomy. Infusion of NT-3 at a dose of 12 µg/d does not have an effect on p75 expression. Virtually all unlesioned and axotomized CSNs express trkC mRNA. Treatment with 12 µg/d NT-3 strongly suppresses trkC expression in axotomized CSNs at postlesion day 3. Scale bar, 50 µm. The p75 expression data were obtained with a probe complementary to nucleotides 932-971 of the rat p75 mRNA. The same experiments (data not shown) have been performed with a probe complementary to nucleotides 1809-1848 of the rat p75 mRNA, which yielded essentially the same results. B, Quantification of p75 and trkC mRNA expression in CSNs (indicated is mean percentage of CSNs expressing a mRNA ± SEM). Very few unlesioned CSNs (n = 6) express p75 mRNA. This expression pattern is not altered at day 1 after axotomy (n = 4). In contrast, the expression of p75 mRNA is induced in more than one-third of axotomized CSNs at day 3 [n = 6, p < 0.01 vs control adb NKT] and day 7 [n = 4, p < 0.05 vs control adb NKT] after axotomy. There is a trend of reduced p75 mRNA expression in axotomized CSNs after NT-3 treatment at day 3 (n = 4, NS vs control adb FLSD at p < 0.05) and day 7 (n = 4, NS vs control adb FLSD at p < 0.05). Virtually all CSNs express trkC mRNA in unlesioned animals (n = 6) or vehicle-treated animals at days 1 (n = 3), 3 (n = 5), and 7 (n = 5) after axotomy. NT-3 application significantly reduced the proportion of axotomized CSNs expressing trkC at day 3 [n = 4, p < 0.01 vs control adb NKT] but not at day 7 [n = 5, NS adb FLST at p < 0.05] after axotomy. Black bars, Axotomized CSNs on the lesion sides of the cortices (l); gray bars, unlesioned animals or unlesioned CSNs of the control sides of the cortices (c).

Treatment with exogenous recombinant NT-3 at doses of 12 µg/d promotes survival (Giehl and Tetzlaff, 1996), whereas endogenousNT-3 induces death of axotomized CSNs. The survival-promotingeffect of NT-3 treatment may be explained by mimicking BDNF actione.g., through TrkB activation caused by the unphysiologicallyhigh dose of NT-3 (Davies et al., 1995; Ryden and Ibanez, 1996)and/or increasing cortical BDNF expression. Alternatively, theseinfusions might alter the expression of the receptor or receptorsinvolved in survival and/or death signaling in axotomized CSNs.The first possibility is supported by previous findings that theeffects of NT-3 infusions are at least partially mediated by endogenousBDNF (Giehl et al., 1998) and that NT-3 treatment clearly increasesBDNF mRNA expression in cortical layers 2-4, whereas trkB expressionin CSNs is unaffected (Schütte et al., 2000). To show whetherNT-3 treatment affects the expression of neurotrophin receptorspotentially involved in the NT-3-mediated survival regulationof lesioned CSNs, we analyzed the expression of p75 and trkC inaxotomized CSNs treated with 12 µg/d of recombinant NT-3. Althoughp75 expression was not significantly altered by this NT-3 treatment,the portion of CSNs expressing trkC was clearly decreased at day3 and largely recovered by day 7 (Fig. 4). These data suggestthat the survival-promoting effect of high-dose NT-3 treatmentis not mediated by TrkC but is also not explained by the downregulationof p75. We wondered whether changes in the relative levels oftrkC isoforms might be relevant for trkC-dependent neuronal deathin NT-3 and vehicle-treated animals. RT-PCR with primers on bothsides of the kinase insert demonstrated the presence of all kinaseinsert forms (14, 25, and 39 amino acids) together with the insertlesskinase, but failed to reveal any alterations in the relative levelsof these isoforms (data not shown). We finally directly assessedTrkB activation by exogenous NT-3 by directly measuring corticalTrkB phosphorylation after high-dose NT-3 treatment. Indeed, intracorticalinjections of high doses of NT-3 induce TrkB phosphorylation asearly as 1 hr after administration (Fig. 5A). Together, thesefindings suggest that the effects of our previously reported NT-3treatment (Giehl and Tetzlaff, 1996) do not reflect the physiologicalrole of NT-3 for CSNs but rather a mimicry of endogenous BDNFfunction.

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Figure 5. A, Intracortical high-dose NT-3 injections induce cortical TrkB phosphorylation. TrkB Western blots of electrophoresed anti-phosphotyrosine immunoprecipitates of homogenates of vehicle (V)- or 500 ng/µl NT-3 (N)-treated rat cortices 30, 60, 120, and 360 min after 10 µl injection of the respective solution. The arrowheads indicate the position of TrkB. B, TC89 specifically binds to TrkC. In Western blots of 50 (lanes labeled 50) or 500 ng (lanes labeled 500) of the extracellular domains of each recombinant Trk protein per lane, TC89 recognizes TrkC, and there was no cross-reactivity to TrkA or TrkB. The arrowheads indicate the position of the encoded recombinant Trk proteins (Yan et al., 1997a). C, TC89 inhibits NT-3-induced phosphorylation of TrkC. TrkC-transfected NIH 3T3 cells were exposed to NT-3 (+), TC89 (+), or both for 10 min. TrkC phosphorylation was seen after NT-3 treatment but completely abolished by TC89. Also, TC89 alone had no effect on TrkC phosphorylation. The arrowhead indicates the position of the trkC product.

Death of axotomized rat CSNs depends on cosignaling of p75 and trkC receptors

The p75 and trkC mRNA expression patterns in untreated and NT-3-treated lesioned CSNs suggest a mechanism of NT-3-mediateddeath induction different from previous reports (Frade et al.,1996; Bamji et al., 1998) in which a neurotrophin mediates neuronaldeath via p75^NTR receptor in the absence of its Trk receptor. To determine whichreceptors are involved in the death induction, we treated axotomizedrat CSNs with monovalent Fab fragments of the rabbit REX antibody(REX-Fab) (Weskamp and Reichardt, 1991) against p75^NTR and with the rabbit TrkC antibody TC89. REX has been shown tospecifically bind to and block the p75 receptor (Weskamp and Reichardt,1991). Similarly, TC89 only recognizes the extracellular domainof TrkC, but not of TrkA and TrkB and completely blocks NT-3-inducedTrkC phosphorylation without having detectable agonist-like effectson this receptor (Fig. 5B,C). The intracortical treatment of lesionedanimals with these antibodies started immediately after ICL andlasted for 7 d. Axotomy-induced death of CSNs was prevented inanimals treated either alone with REX-Fab or alone with TC89 (Fig.6). These data argue that both p75^NTR and TrkC signaling are essential for the induction of CSN death.

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Figure 6. Death of axotomized CSNs is mediated via essential coactivation of TrkC and p75 receptors. A, FB-labeled CSNs of lesion and control sides of representative animals of a control group [rabbit monovalent Fab fragments, 1 mg/ml (RFab-1)] and the groups receiving receptor-blocking antibodies [p75 antibody, 0.3 mg/ml (REX-0.3); TrkC antibody; 4 mg/ml (TC89-4)]. Application of control rabbit Fab (RFab-1) results in death of CSNs comparable with other control solutions (Fig. 3). Treatment with either REX-Fab or TC89 IgG alone prevents axotomy-induced death of CSNs. Scale bar, 1 mm. B, Quantification of survival of axotomized CSNs (indicated is mean survival ± SEM). One-third of the CSNs of the control groups [monovalent rabbit Fab, 1 mg/ml (RFab-1; n = 2) and 0.15 mg/ml (RFab-0.15; n = 4); rabbit IgG, 1 ml/ml (RIgG-1; n = 5) (Fig. 1), and 16 mg/ml (RIgG-16; n = 2); P2 buffer (69 ± 2%; n = 3; data not shown)] die within the first week after axotomy. This death is completely prevented by application of either REX-Fab [0.15 mg/ml (REX-0.15, n = 5, p < 0.01 vs P2 and RFab-0.15 adb NKT, p < 0.05 vs RFab-1 adb NKT) and 0.3 mg/ml (REX-0.3, n = 3, p < 0.05 vs all control groups adb NKT)] or TC89 [2 (TC89-2l n = 3), 4 (TC89-4l n = 4), 8 (TC89-8; n = 4), and 16 mg/ml (TC89-16; n = 3), p < 0.01 vs all control groups adb NKT)]. The data in this figure argue that activation of both p75 and TrkC is required for the induction of death in CSNs.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study shows that endogenous BDNF and NT-3 antagonistically regulate survival of lesioned adult CSNs in vivo. Death isinduced by endogenous NT-3 and requires activation of TrkC andcosignaling of p75^NTR, demonstrating that mature central neurons can integrate multipleneurotrophin-dependent signals for death and survivaldecisions.

Although previous reports have not found gross morphological alterations of the cortex or the corticospinal tract in micemutant for BDNF, NT-3, and their receptors (Klein et al., 1993;Ernfors et al., 1994a,b; Farinas et al., 1994; Jones et al., 1994;Klein et al., 1994), several aspects of cortical development areregulated by endogenous BDNF and NT-3. BDNF has been implicatedin the development of cortical lamination (Ringstedt et al., 1998),and NT-3 influences axonal growth of cortical neurons (Castellaniand Bolz, 1999). In addition, both neurotrophins regulate thedendritic development of cortical pyramidal neurons (McAllisteret al., 1997). We found that neither the number nor the localizationof corticospinal neurons was altered in young adult heterozygousBDNF and NT-3 mutants. Thus, the reduced levels of these neurotrophinsin heterozygotes (Ernfors et al., 1994a,b; Korte et al., 1995;Airaksinen et al., 1996) (C. Helbig and M. Meyer, unpublisheddata) appear to be sufficient for normal development. To furtherexclude the possibility that results from axotomized mutant miceare obscured by developmental alterations, we also acutely depletedneurotrophins using antibodies in rats. Conclusions from bothtypes of experiments are verysimilar.

These data confirm our previous notion that endogenous BDNF is crucial for survival promotion of the majority of lesionedadult CSNs (Giehl et al., 1998). In contrast, endogenous NT-3is a critical component of lesion-induced death signaling in axotomizedCSN, despite our earlier work showing that exogenous NT-3, aswell as BDNF, promote their survival (Giehl and Tetzlaff, 1996).How can these results be reconciled? Most importantly, there isan obvious difference in the experimental approach. Here, endogenousNT-3 was depleted, whereas in the previous study, high doses ofNT-3 were intracortically infused. High concentrations of NT-3are known to evoke effects similar to BDNF by activating TrkBas a nonpreferred receptor (Davies et al., 1995; Ryden and Ibanez,1996) or by inducing BDNF release (Canossa et al., 1997; Kruttgenet al., 1998). We have previously shown that the complete rescueof lesioned CSNs by NT-3-infusions (Giehl and Tetzlaff, 1996)depends on endogenous BDNF (Giehl et al., 1998) and that theseinfusions increase cortical BDNF mRNA expression (Schütte etal., 2000). In addition, we show here that a high dose of exogenousNT-3 reduces the number of trkC-expressing CSNs and results incortical TrkB phosphorylation. Thus, high-dose NT-3 treatmentmay promote survival by evoking BDNF-like effects and stimulatingendogenous BDNF, and, at the same time, also counteract deathby reduced expression of death-mediating receptor or receptors.The prediction that low NT-3 concentrations will enhance deathof axotomized CSNs is valid only if the effects of endogenousNT-3 are submaximal. We have tested this possibility in a limitednumber of experiments (data not shown), and even NT-3 treatmentat doses as low as 0.06 ng/hr did not yield lower survival thanvehicle application. This result is compatible with the assumptionthat endogenous NT-3 levels are sufficient for a maximal effect.However, limited diffusion or stability of NT-3 at very low dosesmay have hindered its effects. Furthermore, the function of NT-3may depend on the way of its presentation as previously demonstratedin the chick visual system (Frade and Barde, 1998). A clear answerto this specific question requires administration of NT-3 aloneand in combination with anti-BDNF into the cortex of animals devoidof endogenous NT-3 and, therefore, has to await the availabilityof cortex-specific conditionalmutants.

According to the classical neurotrophin hypothesis, survival of neurons is regulated by their limited access to survival-promotingsubstances (Lewin and Barde, 1996). This hypothesis has been significantlymodified by the recent findings that endogenous NGF (Frade etal., 1996, 1997; Frade and Barde, 1998; Davey and Davies, 1998)and BDNF (Bamji et al., 1998) can induce neuronal death via p75^NTR receptors during development. Previous evidence that exogenoustrophic factors promote survival of neurons that are killed byanother endogenous neurotrophin (Frade et al., 1997; Davey andDavies, 1998) suggests that a neurotrophin antagonism might regulateneuronal survival. The present finding of opposite effects ofendogenous NT-3 and BDNF on the survival of one neuronal populationdemonstrates that endogenous neurotrophins can indeed antagonisticallyregulate neuronal survival in vivo. In addition, our data provideevidence that neurotrophins can induce neuronal death in the matureCNS.

The observation that axotomized CSNs survive simultaneous depletion of BDNF and NT-3 suggests that the NT-3-mediated deathsignal is functionally dominant. It is unlikely that other neurotrophinscan substitute for BDNF in this situation. Of the known neurotrophins,NT-4/5 is, like BDNF and NT-3, expressed in the mature cortex(Timmusk et al., 1993). It acts via TrkB and has higher affinityto this receptor than NT-3 (Barbacid, 1995). Because BDNF neutralizationalone clearly enhances death of axotomized CSN, it is unlikelythat endogenous NT-4/5 significantly promotes their survival.The question arises why there should be a survival-supportingsignal if the amount of cell death can be determined by endogenousNT-3? Considering the pleiotrophic roles of BDNF and NT-3 forcortical neurons (Schnell et al., 1994; McAllister et al., 1997;Castellani and Bolz, 1999), endogenous NT-3 may regulate additionalaspects of CSN biology and, therefore, its effects on survivalhave to be regulated in accordance with theseroles.

There are three striking features of the NT-3-dependent death pathway for axotomized CSNs in vivo. First, NT-3 controls survivalof virtually all BDNF-dependent CSNs. This single factor couldin principle be altered to precisely titrate the number of dyingneurons. Second, the essential players for cell death promotionare locally present before and after lesion: NT-3 is expressedin the unlesioned and lesioned cortex (Ernfors et al., 1990; Altaret al., 1994; Zhou and Rush, 1994) (K. Giehl and W. Tetzlaff,unpublished observation), and virtually all unlesioned (Giehland Tetzlaff, 1996) and lesioned CSNs express trkC. Similarly,the BDNF-TrkB pathway is also present in cortex and CSNs and notaltered by axotomy (Giehl et al., 1998; Schütte et al., 2000).In addition to their neuronal expression in the cortex, thereare other potentially relevant sources of endogenous BDNF andNT-3, e.g., cortical astrocytes (Rubio, 1997), the cortical whitematter and the internal capsule, and several brainstem areas (Ernforset al., 1990; Altar et al., 1994; Zhou and Rush, 1994). Finally,significant p75 expression in CSNs is only observed at day 3 andlater after axotomy. Thus, the onset of p75 expression may controlthe timing of CSN death. The p75^NTR signal is probably ligand-induced because REX antibody has beendescribed to inhibit ligand binding to p75^NTR (Weskamp and Reichardt, 1991). Because exogenous (Giehl and Tetzlaff,1996) as well as endogenous (S. Röhrig, M. Meyer, and K. Giehl,unpublished data) NGF does not seem to play a role in this context,NT-3 is the most likely ligand for the p75^NTR-mediated death induction of CSNs. We can, however, not excludethat constitutive p75^NTR signaling (Majdan et al., 1997) contributes to thiseffect.

How does the NT-3-TrkC pathway relate to known neurotrophin-mediated death mechanisms? To our knowledge, there is no previousreport involving an action of NT-3 via TrkC in cell death promotionin vivo. There is, however, an intriguing account of death inductionof NT-3 via TrkC in medulloblastomas (Kim et al., 1999). Interestingly,death induction in medulloblastomas can also be triggered by NGFthrough TrkA (Muragaki et al., 1997), suggesting that this effectis not specific for TrkC. Thus, there is apparently no need toinvoke the induction of specific TrkC receptor isoforms (Valenzuelaet al., 1993; Tsoulfas et al., 1996) as being more prone to deathsignaling. This conclusion is supported by our analysis of theexpression of these isoforms in lesionedcortex.

The necessity of p75^NTR and TrkC cosignaling for death induction could be explained by two principally different models. Bothreceptors could be involved in death signaling, and the observedinterdependence could be accounted for by a threshold for efficientdeath induction, which is not reached by p75^NTR or TrkC signaling alone. This is in line with the observationthat TrkC and p75^NTR receptors can be coimmunoprecipitated (Bibel et al., 1999). Alternatively,one of the receptors may be required as a conditioning signal.Because endogenous NT-3 induces neuronal differentiation of corticalprecursors which, after adopting a neuronal phenotype, are dependenton endogenous BDNF for survival (Ghosh et al., 1994; Ghosh andGreenberg, 1995), one conceivable scenario states that NT-3 signalingvia TrkC is constantly required to maintain BDNF dependence ofCSNs. In this case, p75^NTR signaling would induce death of those CSNs that do not receivesufficient BDNF to allow survival. Our observation that CSNs arerescued from axotomy-induced death by simultaneous depletion ofendogenous BDNF and NT-3 is in accordance with this possibility.It will be important to unravel the mechanisms underlying thisregulation in subsequent studies. In this context, it will beof central interest to determine whether the BDNF-NT-3-mediatedantagonism on CSN survival represents a pure and direct trophicaction on CSNs or involves additional molecules and/or celltypes.

  FOOTNOTES

Received Aug. 2, 2000; revised Feb. 15, 2001; accepted Feb. 23, 2001.

This work was supported by grants from the Deutsche Forschungsgemeinschaft (SFB 530 C6 to K.M.G. and DFG Gi 271/3-1 to K.M.G.and P.M.). We thank Birgit Kunkel and Andrea Steinberg for excellenttechnical assistance, Dr. Miriam Bibel for advice on the phosphorylationassay and gift of reagents, and Dr. Georg Dechant for providingthe TrkC-expressing cell line. We are also grateful to Drs. Y.-A.Barde and H. Thoenen for helpful suggestions and discussion andDr. Clare J. Menzel-Dowling for helpful discussion and proofreadingof the manuscript. NT-3 has been generously supplied by Amgen/Regeneronpartnership.
Correspondence should be addressed to Dr. Klaus Giehl, University of Saarland, Department of Anatomy, 66421 Homburg/Saar,Germany. E-mail: k.giehl{at}rz.uni-sb.de.

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DISCUSSION
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