A Changing Pattern of Brain-Derived Neurotrophic Factor Expression Correlates with the Rearrangement of Fibers during Cochlear Development of Rats and Mice

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The Journal of Neuroscience, April 15, 1999, 19(8):3033-3042

A Changing Pattern of Brain-Derived Neurotrophic Factor Expression Correlates with the Rearrangement of Fibers during Cochlear Development of Rats and Mice
Barbara Wiechers¹, Glikeria Gestwa¹, Andreas Mack², Patrick Carroll³, Hans-Peter Zenner¹, and Marlies Knipper¹
Departments of ¹ Oto-Rhino-Laryngology and ² Anatomy, University of Tübingen, D-72076 Tübingen, Germany, and ³ Institut National de la Santé et de la Recherche Médicale, Institut National de la Santé et de la Recherche Médicale, Unit 382, 13288 Marseille Cedex 09, France

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The reorganization of specific neuronal connections is a typical feature of the developing nervous system. It is assumed thatthe refinement of connections in sensory systems requires spontaneousactivity before the onset of cochlear function and selective sensoryexperience during the ensuing period. The mechanism of refinementthrough sensory experience is currently postulated as being basedon the selective reinforcement of active projections by neurotrophins.We studied a presumed role of neurotrophins for rearrangementof afferent and efferent fibers before the onset of sensory functionin the precisely innervated auditory end organ, the cochlea. Weobserved a spatiotemporal change in the localization of brain-derivedneurotrophic factor (BDNF) protein and mRNA, which correlatedwith the reorganization of fibers. Thus, BDNF decreased in targethair cells during fiber retraction and was subsequently upregulatedin neurons, target hair cells, and adjacent supporting cells concomitantwith the formation of new synaptic contacts. Analysis of the innervationpattern in BDNF gene-deleted mice by immunohistochemistry andconfocal microscopy revealed a failure in the rearrangement offibers and a BDNF dependency of distinct neuronal projectionsthat reorganize in control animals. Our data suggest that, beforethe onset of auditory function, a spatiotemporal change in BDNFexpression in sensory, epithelial, and neuronal cells may guidethe initial steps of refinement of the innervationpattern.

Key words: BDNF; fiber rearrangement; innervation pattern; cochlea; development; rat; knock-out mouse

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activity-dependent rearrangement of fibers is a general property of the developing nervous system commonly studied in thevisual cortex and in neuromuscular junctions (Van Essen et al.,1990; Hockfield and Kalb, 1993; Cramer and Sur, 1995). In thevisual system, the refinement of patterning, subsequent to theonset of visual function, is presumed as being primarily dependenton visual experience (Antonini and Stryker, 1993) and as beinginfluenced by neurotrophins (Cabelli et al., 1995; Kwon and Gurney,1996).

Neurotrophins, including nerve growth factor (NGF), brain-derived neurotrophic factor (BDNF), neurotrophin-3 (NT-3), and neurotrophin-4(NT-4), act through their appropriate high-affinity receptorstrkA, trkB, and trkC (for review, see Bothwell, 1991), as wellas through the low-affinity neurotrophin receptor p75^NGFR (Chao, 1994). In addition to their role as mediators of selectiveneuronal survival (Barde, 1989), neurotrophins have potent abilitiesfor enhancing the efficacy of synaptic transmission (Lohof etal., 1993; Knipper et al., 1994a,b; Kang and Schuman, 1995; Figurovet al., 1996), as well as for influencing the patterning and stabilityof synaptic contacts (Cabelli et al., 1995; Wang et al., 1995).

Before the onset of auditory function, spontaneous activity contributes to the development of orderly connections (Meisteret al., 1991; Penn et al., 1994; for review, see Shatz, 1996).The mechanisms that determine the selectivity of the early reorganizationof fibers are still unknown. In the cochlea, a rearrangement ofnerve projections occurs before the onset of hearing. At the outerhair cell (OHC) level, transitory radial afferent type I collateralsretract and are exchanged by spiral afferents type II and efferentsfrom the medial olivocochlear complex (MOC efferents) (Lenoiret al., 1980; Hafidi and Romand, 1989; Sobkowicz, 1992; Knipperet al., 1995). At the inner hair cell (IHC) level, efferents originatingin the lateral olivocochlear complex (LOC efferents) lose theircontacts with the soma and form new synapses with dendrites ofafferent type I fibers, which project to IHCs (Lenoir et al.,1980; Pujol, 1986; Echteler, 1992).

Manifold studies demonstrated the crucial role of BDNF and NT-3 for the survival of the distinct sets of cochlea neurons (Pirvolaet al., 1994; Ernfors et al., 1995; Fritzsch et al., 1997). Recently,a transient expression of the neurotrophin receptor trkB in haircells has been observed during the rearrangement of fibers (Knipperet al., 1996, 1997). To elucidate the presumed functional involvementof trkB ligand BDNF in the reorganization of connectivities beforeauditory experience, we analyzed the BDNF expression in postnatalrat and mice cochlea and correlated our results with the rearrangementof fibers in control and BDNF null mutantmice.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. Wistar rats were purchased from Interfauna (Tuttlingen, Germany). BDNF +/ $-$ mice, heterozygous for a deletion of theBDNF gene, were kindly provided by Patrick Carroll and Hans Thoenen(Max-Planck-Institut, Martinsried, Munich, Germany). BDNF $-$ / $-$ null mutant mice were obtained by mating of heterozygous mice.The offspring was genotyped by PCR according to Korte et al. (1995).Homozygous +/+ littermates were used ascontrols.

Tissue preparation. BDNF +/+ and $-$ / $-$ mice and Wistar rat pups of ages postnatal day 1 (P1) to P17 were used for this study.The day of birth was defined as P0. Cochleae were prepared asdescribed by Knipper et al. (1997). Tissues were cryosectionedat 10 µm for in situ hybridization and immunohistochemistry andat 25 µm for laser scanning confocal microscopy and stored at $-$ 20°C. For mRNA and protein preparations, tissues were immediatelyfrozen in liquid nitrogen and stored at $-$ 70°C beforeuse.

Immunohistochemical staining for fluorescence microscopy. For staining with rabbit polyclonal anti-BDNF antibody (2 µg/ml;Chemicon, Temecula, CA), rat cochlea sections were permeabilizedwith 0.1% saponin (Sigma, Deisenhofen, Germany) in PBS, pH 7.4,for 10 min at room temperature and blocked with 5% goat serumin PBS before overnight incubation with antibody at 4°C. For neutralizationof BDNF immunoreaction, the anti-BDNF antibody was preincubatedwith either recombinant human BDNF (rhBDNF) (100 ng/ml; RegeneronPharmaceuticals, Tarrytown, NY) or recombinant human NT-3 (rhNT-3)(100 ng/ml; Regeneron Pharmaceuticals) before immunohistochemicalstaining. Mouse cochlea sections were permeabilized with 0.1%Triton X-100 in PBS, blocked with 1% bovine serum albumin in PBS,and incubated overnight at 4°C with monoclonal antibody to GAP-43(1:50, clone GAP-7B10; Sigma) or rabbit polyclonal antibodiesto GluR4 (1:50; Chemicon), GluR2/3 (1:50; Chemicon), NF-200 (1:1000;Sigma), or synaptophysin (1:10; Chemicon). Primary antibodieswere detected with Cy3- (0.35 µg/ml; Jackson ImmunoResearch, WestGrove, PA) or FITC-conjugated secondary antibodies (1:100; Sigma).Sections were mounted with Vectashield (Vector Laboratories, Burlingame,CA) and viewed using an Olympus (Tokyo, Japan) AX70 microscopeequipped with epifluorescenceillumination.

Immunohistochemical staining for laser scanning confocal microscopy. Sections (25-µm-thick) of BDNF +/+ and $-$ / $-$ mice wereimmunostained with rabbit polyclonal anti-synaptophysin antibody(1:10; Chemicon) and Cy3-conjugated secondary antibody (0.35 µg/µl;Jackson ImmunoResearch). Sections were viewed using a confocallaser scanning microscope [Zeiss (Oberkochen, Germany) LSM 410with an Axiovert 135 M]. Stacks of images 0.5 µm apart were takenon the z-axis of the hair cells and reconstructed using VoxelViewsoftware (Vital Images, Fairfield,IA).

Western blot analysis. Cochleae were collected from postnatal rats and mice, homogenized in electrophoresis sample buffer(250 mM Tris-HCl, pH 6.8, 15% sodium dodecylsulfate, 40% sucrose,5 mM EDTA, and 15% $beta$ -mercaptoethanol), and heated at 90°C for5 min. The protein equivalent of four (rats) or six (mice) cochleaand recombinant human neurotrophins (Regeneron Pharmaceuticals)were separated on 15% acrylamide gels, and the protein was transferredto 0.2 µm nitrocellulose membranes (Amersham, Buckinghamshire,UK) as described by Towbin et al. (1979). Membranes were blockedwith 5% dry milk powder in PBS and incubated with anti-BDNF antibody(1 µg/µl; Chemicon). Bound antibodies were visualized with theenhanced chemiluminescence detection system(Amersham).

Riboprobe synthesis. pBluescript II SK( $-$ ) vectors containing full-length sequences of rat trkB (pSK-rTrkB(C1); 3.3 kb) andrat BDNF (pSK-rB(C1); 1.1 kb) were supplied by Regeneron Pharmaceuticals.Complementary strands for sense or antisense were transcribedfrom T7 or T3 promotor sites in the presence of digoxigenin labelingmix (Boehringer Mannheim, Mannheim, Germany) to obtain labeledriboprobes or, in the presence of nonlabeled nucleotide triphosphates,to obtain nonlabeled riboprobes. Nonlabeled RNA probes were usedin cohybridization assays to test the specificity of theriboprobes.

In situ hybridization. Riboprobes were diluted to appropriate concentrations in hybridization buffer (RPN3310; Amersham) containing50% formamide and were denatured for 10 min at 68°C. Riboprobeswere applied to sections for overnight hybridization in a 50%formamide chamber at 55°C. Sections were washed twice in 0.1×SSC (300 mM sodium chloride and 30 mM sodium citrate, pH 7.0)at 55°C for 30 min. To analyze the specificity of the riboprobes,digoxigenin-labeled riboprobes were cohybridized with a 100-foldexcess of a nonlabeled riboprobe of the same or the related gene.After a brief wash in Tris buffer (0.1 M Tris-HCl and 0.15 M sodiumchloride, pH 7.5), sections were blocked in Tris buffer containing0.5% blocking reagent (catalog #1096176; Boehringer Mannheim)and 0.3% Triton X-100 and incubated with anti-digoxigenin antibodyconjugated to alkaline phosphatase (1:750; Boehringer Mannheim).Sections were exposed to staining solution containing nitrobluetetrazolium salt and 5-bromo-4-chloro-3-indolyl phosphate forup to 20 hr and viewed with Normarski optics using an OlympusAX70microscope.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Spatiotemporal expression pattern of BDNF in the developing cochlea

In a first step, we studied the spatiotemporal expression of BDNF protein in mice and rat cochlea (data not shown) duringthe first 2 postnatal weeks by immunohistochemistry. The alterationof the expression profile of BDNF was found to be similar in bothspecies. In mice, however, all processes occurred ~1 or 2 d inadvance to rats. For a better understanding of the specific termsused to describe the cellular structures in the organ of Cortiduring this time, see Figure 1, which illustrates the typicalmorphological and cellular details of a postnatal organ of Corti,shown for mice cochlea. At P1, BDNF was expressed in hair cellsin the more apical, but not basal, cochlea turns, as shown forthe medial turn in Figure 2 (P1, Organ of Corti, IHC, OHC). NoBDNF expression was detected in spiral ganglion cells (Fig. 2,P1, Spiral Ganglion). Between P2 and P4, BDNF was absent in theorgan of Corti in the apical to basal cochlea turn (Fig. 2, P3,Organ of Corti). During this time, BDNF gradually appeared indistinct spiral ganglion cells, as shown for P3 (Fig. 2, P3, SpiralGanglion). At approximately P5-P6, the number of immunopositivespiral ganglion neurons reached a maximum and, in addition tocell bodies, neuronal projections were BDNF-immunopositive (Fig.2, P6, Spiral Ganglion). These immunopositive fibers seemed tobe afferents but not efferents, because BDNF was not detectedin the intraganglionic spiral bundle (data not shown). From P4onward, BDNF reappeared in the organ of Corti of the apical tomidbasal, but not basal, cochlea turn. BDNF appeared in outerhair cells and supporting cells that are in contact with haircells as pillar, Deiters', and border cells (Fig. 2, P6, Organof Corti). Whereas BDNF expression persisted in Deiters' and bordercells at least up to P12 (Fig. 2, P6, P10, Organ of Corti), BDNFdisappeared from hair and pillar cells from P8 onward, as shownfor P10 (Fig. 2, P10, Organ of Corti). Beyond P8, BDNF could nolonger be detected in neuronal fibers but only in neuronal cellbodies (Fig. 2, P10, Spiral Ganglion). The antibody to BDNF nonspecificallystained the tectorial membrane (Fig. 2, Organ of Corti, TM). Thisalteration of the expression pattern of BDNF protein during thefirst 2 postnatal weeks was observed with similar results in triplicateexperiments in mice and rats.

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Figure 1. Toluidine blue stained section of an organ of Corti of a mouse at P5, indicating the typical cellular details of an organ at that age. SC, Supporting cells; TM, tectorial membrane. Scale bar, 20 µm.

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Figure 2. Localization of BDNF protein in spiral ganglion cells and organ of Corti in mice cochleae (BDNF +/+) at P1, P3, P6, and P10 by immunohistochemistry. In IHCs (arrowhead) and OHCs (vertical arrows) of the organ of Corti, BDNF was expressed at P1, was absent at P3, reappeared at P6, and was downregulated again at P10. At P6, BDNF was also detected in supporting cells as pillar cells (PC), Deiters' cells (DC), and border cells (BC). In the spiral ganglion (SG), no BDNF staining was detected at P1, single neurons expressed BDNF at P3 (arrowhead), and the maximal number of immunopositive neuronal cell bodies was reached between P4 and P6 (P6, filled arrowheads). During this time, we observed BDNF in neuronal fibers (P6, open arrowheads). The experiment was repeated in triplicate with similar results. The staining of the tectorial membrane (TM) was nonspecific. Scale bar, 20 µm.

Specificity and sensitivity of the anti-BDNF antibody was examined by immunoblot analysis. The antibody recognized only recombinantBDNF protein but not NT-3, NT-4, or NGF (Fig. 3A). The minimumamount of rhBDNF detected by the antibody was 5 ng (Fig. 3B).Thus, the anti-BDNF antibody used in the present study did notcross react with neurotrophins other than BDNF and revealed asimilar sensitivity as other anti-BDNF antibodies used in previousstudies (Zhou und Rush, 1996). In addition, we analyzed the reactionof the anti-BDNF antibody with cochlear proteins (Fig. 3C, Cochlea)and used rhBDNF as control (Fig. 3C, rhBDNF). A protein closeto the molecular weight of mature BDNF protein was detected inrat cochlea at P5 (Fig. 3C, arrow). Furthermore, proteins of ~20and 30 kDa were labeled, which may correspond to the unprocessedprecursor proteins of BDNF, and a ~45 kDa protein of unknown identity(Fig. 3C, Cochlea). To further test the specificity of the antibody,we performed preabsorption experiments (Fig. 3D). BDNF immunoreactivityin hair cells of mice (data not shown) and rat (Fig. 3D, Anti-BDNF)cochlea was completely abolished by preincubation of the anti-BDNFantibody with an excess of rhBDNF (Fig. 3D, Anti-BDNF+rhBDNF),whereas a preincubation of the antibody with rhNT-3 had no effecton the immunoreactivity (Fig. 3D, Anti-BDNF+rhNT-3). The stainingof the tectorial membrane was nonspecific (Fig. 3D, TM).

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Figure 3. Characterization of anti-BDNF antibody. A, Cross-reactivity of anti-BDNF antibody with neurotrophins NT-3, NT-4, and NGF was tested in Western blot analysis. Anti-BDNF recognized only rhBDNF but not rhNT-3, rhNT-4, or rhNGF. B, Sensitivity of anti-BDNF antibody was tested in Western blot using indicated concentrations of BDNF. The minimal amount rhBDNF recognized by anti-BDNF antibody was 5 ng. C, In a Western blot with rat cochlear protein, anti-BDNF antibody recognized a protein (arrow) close to the molecular weight of rhBDNF, which is likely to be the mature BDNF protein. Anti-BDNF antibody also recognized proteins of ~20 and ~30 kDa, probably BDNF precursor proteins. D, Anti-BDNF immunoreaction (Anti-BDNF) in hair cells (arrowheads and vertical arrows) was completely abolished by preabsorption of the antibody with rhBDNF (Anti-BDNF+rhBDNF) but not with rhNT-3 (Anti-BDNF+rhNT-3). Immunoreaction in the tectorial membrane (TM) was nonspecific. Scale bar, 20 µm.

Because the localization of BDNF protein may be caused by either a local BDNF synthesis or by an uptake of BDNF synthesizedin other cells, we studied BDNF expression at the mRNA level byin situ hybridization. The distribution of BDNF mRNA was similarin rats and mice and is shown for rats in Fig. 4. Using in situhybridization, BDNF signals were detected in hair cells of themost apical cochlea turn at P1 only in rats but not in the earlierdeveloped mice (data not shown). The detection of BDNF mRNA atP1 in rats did depend on the size of the litter, with positiveresults in younger P1 specimens and negative results in olderP1 specimens. From P1 onward, BDNF mRNA was not detected in theorgan of Corti, as shown for P3 (Fig. 4, P3, IHC, OHC), but reappearedin hair and supporting cells as pillar, Deiters', and border cellsin mice at approximately P4 (data not shown) and in rats at approximatelyP5, as shown for P6 (Fig. 4, P6). From P8 onward, BDNF mRNA disappearedfrom hair and pillar cells but lasted in Deiters' and border cells(Fig. 4, P8, DC, BC). We repeatedly observed that, in rat andmice species, the disappearance of BDNF mRNA precedes the disappearanceof BDNF protein by ~1 or 2 d. The detection of BDNF protein inspiral ganglia cells could also be confirmed on mRNA level (n> 10) (Fig. 4, SG) and was demonstrated on parallel improvementof the specificity of the BDNF riboprobe. A possible cross-reactionof BDNF riboprobe with NT-3 mRNA was scrutinized in competitionexperiments. BDNF signal was completely abolished by a cohybridizationwith an excess of nonlabeled BDNF antisense riboprobe (Fig. 4,SG, BDNF+nlBDNF), whereas an excess of nonlabeled NT-3 antisensedid not diminish the intensity of the signal (Fig. 4, SG, BDNF+nlNT-3).Furthermore, we localized high-affinity neurotrophin receptortrkB mRNA in spiral ganglion neurons during the whole postnataldevelopmental period (data not shown). Thus, the spatiotemporalpattern (Fig. 4) of BDNF mRNA expression in the organ of Cortiand in the spiral ganglion changed in a manner similar to theexpression pattern of BDNF protein (Fig. 2).

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Figure 4. Localization of BDNF mRNA in the organ of Corti and the spiral ganglion of rats by in situ hybridization. Although no BDNF mRNA was detected at P3, BDNF mRNA was localized in OHCs (vertical arrows), pillar cells (PC), Deiters' cells (DC), and border cells (BC) of the organ of Corti at P6. At P8, BDNF mRNA was noted restrictively in Deiters' and border cells. In the spiral ganglion (SG), BDNF hybridization signal in neurons was not effected by cohybridization with an excess of nonlabeled NT-3 antisense (BDNF+nlNT-3) but was completely abolished by cohybridization with an excess of nonlabeled BDNF antisense (BDNF+nlBDNF). Scale bars, 20 µm.

Correlation between BDNF expression and rearrangement of fibers

To scrutinize a possible correlation between BDNF expression and the rearrangement of fibers, we examined the expression ofBDNF protein and marker proteins for efferent and afferent projectionsin control and BDNF gene-deleted mice. We used antibodies to thedistinct glutamate receptor subtypes GluR2/3 and GluR4, whichare expressed in afferent type I collaterals and afferent typeI fibers, respectively (Knipper et al., 1997). We further usedantibodies to the 200 kDa neurofilament protein NF-200, whichspecifically stains afferents (Berglund and Ryugo, 1986;). Furthermore,we used antibodies to the growth-associated protein GAP-43 andto synaptophysin for staining of efferents (Knipper et al., 1995,1997).

Reorganization of presynaptic specializations at the outer hair cell level

First, we will focus on the innervation at the OHC level. The analysis of synaptic vesicle proteins in synaptic specializationsin hair cells and in efferent fibers at the OHC level was performedusing an anti-synaptophysin antibody. In control mice, the absenceof BDNF immunoreactivity in hair cells at P2 (Fig. 5, P2, Synaptophysin)was associated with strong synaptophysin-immunoreactive outerhair cells (Fig. 5, P2, Synaptophysin), indicating the existenceof presynaptic specializations in OHCs during this time. Withthe reappearance of BDNF in hair and supporting cells at P4, synaptophysindisappeared from OHCs and appeared in efferent projections oppositeto OHCs. This aspect is shown for the basal cochlea turn at P6for BDNF (Fig. 5, BDNF; see similar illustration in Fig. 2) andsynaptophysin (Fig. 5, P6, Synaptophysin). Aiming to clarify therole of BDNF for the reorganization of presynaptic specializations,we studied synaptophysin staining in BDNF gene-deleted mice.

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Figure 5. Localization of BDNF protein and synaptophysin protein in the midbasal cochlea turn of mice (BDNF +/+) by immunohistochemistry. The absence of BDNF protein in the organ of Corti at P2 (P2, BDNF) is associated with a detection of synaptophysin-immunopositive presynaptic specializations in OHC soma (P2, Synaptophysin). The appearance of BDNF in outer hair cells and supporting cells as pillar cells (PC), Deiters' cells (DC), and border cells (BC) between P4 and P6 occurs parallel to the loss of synaptophysin-immunopositive presynaptic specializations in outer hair cells and the appearance of synaptophysin immunoreactivity in MOC efferents (P6, Synaptophysin). Scale bar, 10 µm.

Synaptophysin immunoreactivity in outer hair cells was observed in control mice and BDNF gene-deleted mice at P2 (Fig. 6,P2), indicating the existence of presynaptic specializations independentfrom the presence of BDNF. In control mice, synaptophysin immunoreactivitywas lost from the soma of OHCs from P4 onward, when at the sametime, synaptophysin-immunoreactive MOC efferents gradually appearedat the base of OHCs, as shown for the midbasal cochlea turn atP6 (Fig. 6, P6, BDNF +/+, diagonal arrow). In contrast, in BDNF $-$ / $-$ mice, synaptophysin-immunoreactive presynaptic specializationswere noted in outer hair cells still at P6 and MOC efferents wereabsent at that time (Fig. 6, P6, BDNF $-$ / $-$ , diagonal arrow). Witha delay of ~3 d (from P8 onward), however, we noticed that synaptophysindeclined from OHCs in BDNF $-$ / $-$ mice, revealing the reorganizationof presynaptic specializations that now occurred coincident withthe gradual appearance of MOC efferents. Nevertheless, MOC efferentsremained reduced in BDNF $-$ / $-$ mice, even at later developmentalstages in comparison to BDNF +/+ mice, as shown for the midbasalcochlea turn at P17 (Fig. 6, P17, diagonal arrow). The BDNF $-$ / $-$ mice exhibited a nearly total destruction of efferents from OHCsin the usually less innervated apical cochlea turns and a retardedefferent innervation of OHCs in the usually more innervated midbasalcochlea turns. In presumptive relation to the near absence ofBDNF expression in the most basal cochlea turn, the efferent innervationof OHCs in the basal turn of BDNF $-$ / $-$ mice, however, exhibitedan innervation density that was close to normal (n = 4; no deviation).

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Figure 6. Localization of presynaptic specializations in outer hair cells and efferents innervating outer hair cells in the midbasal cochlea turn in control and BDNF gene-deleted mice analyzed by immunohistochemistry using an anti-synaptophysin antibody. At P2, synaptophysin immunoreactivity was observed in BDNF +/+ and $-$ / $-$ mice in OHC soma (OHC, vertical arrows), implicating a BDNF-independent existence of synaptophysin-immunopositive presynaptic specializations in outer hair cells. In control mice at P6, synaptophysin immunoreactivity was restricted to fibers below outer hair cells (BDNF +/+, P6, OHC, vertical arrows), indicating the loss of synaptophysin-immunopositive presynaptic specializations in outer hair cells and the appearance of synaptophysin immunoreactivity in MOC efferents. In BDNF $-$ / $-$ mice, the MOC fiber population was absent at P2 and P6 (BDNF $-$ / $-$ , P2, P6, diagonal arrow), whereas synaptophysin-immunoreactive presynaptic specializations persisted in outer hair cells at both ages (P2, P6, vertical arrows). At P17, presynaptic specializations were lost in BDNF $-$ / $-$ mutants, whereas MOC efferents were still retarded in comparison to controls (compare diagonal arrows below outer hair cells in both specimens at P17). The experiment was repeated in quadruplicate with similar results. Arrowheads, IHC. Scale bar, 20 µm.

Afferent type I collaterals to outer hair cells

In BDNF +/+ mice, GluR2/3-immunopositive projections were detected below OHCs until P3 (Fig. 7, P2, GluR2/3, diagonal arrow)but were lost since then, as shown for the medial turn at P6 (Fig.7, P6, GluR2/3, diagonal arrow). In BDNF $-$ / $-$ mice, however, GluR2/3-immunopositiveprojections were neither observed at P2 nor at later stages inany cochlea turn, as shown for the medial turn at P6 (n = 3, withoutdeviation) (Fig. 7, P2, P6, GluR2/3, diagonal arrow), demonstratingthe loss of afferent type I collaterals in mutant mice. Consideringthat the loss of afferent type I collaterals from basal cochleaturns may occur before birth, we cannot exclude, however, thatin BDNF $-$ / $-$ mutants some afferent type I collaterals may neverthelessinnervate outer hair cells in the basal turn in analogy to a conceptof a trophic gradient along the tonotopic axis of the cochlea(Bianchi et al., 1996; Fritzsch et al., 1997).

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Figure 7. Afferent innervation of outer hair cells in the medial turn of control and BDNF gene-deleted mice analyzed by immunohistochemistry. GluR2/3-immunopositive fibers, presumptive afferent type I collaterals, were observed below outer hair cells in BDNF +/+ mice at P2 but not at P6 (BDNF +/+, GluR2/3, OHC, diagonal arrows). These GluR2/3-immunoreactive fibers were absent in BDNF $-$ / $-$ mice at both ages (BDNF $-$ / $-$ , GluR2/3, diagonal arrows). Anti-NF-200 stained presumptive afferent type II projections to OHCs in BDNF +/+ mice at P6 and P13 (BDNF +/+, NF-200, OHC, diagonal arrows), whereas BDNF $-$ / $-$ mice lacked this fiber population at both postnatal ages (BDNF $-$ / $-$ , NF-200, OHC, diagonal arrows). The experiment was repeated in triplicate with similar results. Arrowheads, IHC. Scale bar, 20 µm.

Afferent type II fibers to outer hair cells

Afferent type II projections were detected below OHCs in BDNF +/+ mice using anti-NF-200 antibody, as shown for P6 and P13(Fig. 7, BDNF +/+, NF-200). In BDNF $-$ / $-$ mice, this fiber typewas absent at all analyzed ages in the midbasal, medial, and apicalturns, although some fibers remained in the basal cochlea turn(data not shown), confirming the data of Bianchi et al. (1996)and Fritzsch et al. (1997). The loss of NF-200-immunopositiveafferent type II fibers in the absence of BDNF is shown for themedial turn at P6 and P13 (Fig. 7, BDNF $-$ / $-$ , NF-200). These observationswere made in triplicate experiments with similarresults.

Efferent fibers to inner hair cells

BDNF downregulation in inner hair cells and the subsequent BDNF upregulation in spiral ganglion neurons appeared to correlatetemporally with the retraction of LOC efferents from the somaof IHC and the formation of new LOC synapses with dendrites ofafferents, respectively (Knipper et al., 1995, 1997). We thereforeanalyzed the innervation at the IHC level during the time of rearrangementof LOC efferents in control and BDNF-deficient mice. Until P3-P4,we could not observe any difference in the innervation patternof synaptophysin- and GAP-43-immunopositive LOC efferents at thebase of the IHC in BDNF +/+ and $-$ / $-$ mice, as shown for synaptophysin-immunoreactiveLOC efferents in the medial cochlea turn at P4 (Fig. 8A, Syn).From P3-P4 onward, however, in control mice, synaptophysin- andGAP-43-immunopositive LOC efferent synapses gradually moved awayfrom IHC bases to a more distant level, indicating to the switchof LOC synapses to afferent dendrites. This aspect is demonstratedfor the GAP-43-immunopositive LOC efferents in the medial cochleaat P15, which are localized at that age distant from the IHC soma(Fig. 8B, BDNF +/+, asterisks) and distant from double-stainedGluR4 receptors in afferent type I fibers at the base of IHCs(Fig. 8B, BDNF +/+, compare GluR4, GAP-43). In contrast, in BDNF $-$ / $-$ mice, presumptive GAP-43-immunopositive LOC terminals persistedat the base of IHCs (n = 3, no deviation) (Fig. 8B, BDNF $-$ / $-$ ,compare GluR4, GAP-43). To obtain more detailed information abouta presumed difference of the innervation pattern at the IHC levelin control and mutant mice, we analyzed synaptophysin-immunopositivesynaptic contacts of LOC efferents below single IHCs by confocalmicroscopy. In BDNF +/+ mice at P15, a scattered elongated synaptophysin-immunopositivepattern below the IHC was observed (Fig. 8C, BDNF +/+, Syn), whereasin BDNF $-$ / $-$ mice, synaptophysin staining was restricted to thebase of the IHC (n = 3, no deviation) (Fig. 8C, BDNF $-$ / $-$ , Syn),confirming the data obtained with anti-GAP-43 antibody at thatage (Fig. 8B).

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Figure 8. Innervation of inner hair cells in control and BDNF gene-deleted mice in the midbasal turn at P4 and P15 analyzed by immunohistochemistry. A, Staining of the immature synaptophysin-immunopositive efferent innervation at P4. Note the close localization of the efferent projections at the base of the IHCs in both mice specimens (compare the distance of the arrowhead and asterisk in BDNF +/+ and $-$ / $-$ mice at P4). B, Immunostaining of the afferent and efferent fibers by double-labeling at P15. GluR4-immunopositive afferent nerve endings were observed at the base of inner hair cell of BDNF +/+ and $-$ / $-$ mice (GluR4, filled arrowheads). In BDNF +/+ mice, GAP-43-immunopositive presumptive LOC terminals (GAP-43, open arrowheads) were localized in a distance to the base of the inner hair cell (filled arrowheads). In contrast to control, in BDNF $-$ / $-$ mice, GAP-43-immunopositive presumptive LOC terminals (GAP-43, open arrowheads) were observed at the hair cell base (filled arrowheads), indicating the persistence of axosomatic LOC synapses in BDNF $-$ / $-$ mice. Note the distance between the two arrowheads in BDNF +/+ and $-$ / $-$ mice. Asterisks mark the hair cell nucleus. The experiment was repeated in triplicate with similar results. C, Comparison of efferent innervation of inner hair cells in control and BDNF gene-deleted mice at P15 by laser scanning confocal microscopy using an anti-synaptophysin antibody. In BDNF +/+ mice, a scattered elongated synaptophysin-immunopositive pattern was observed below the inner hair cell base (filled arrowheads), whereas in BDNF $-$ / $-$ the synaptophysin staining was concentrated at the base of inner hair cell (filled arrowheads). Differences in colors from blue to green to red mirror an intensity gradient of immunoreactivity. Asterisks mark the hair cell nucleus. Scale bars, 10 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The data in the present study demonstrate a remarkable change in the expression pattern of BDNF protein (Fig. 2) and mRNA(Fig. 4) in the auditory end organ in mice and rats. Using a highlyspecific and sensitive antibody (Fig. 3), we observed a decreaseof BDNF protein from inner and outer hair cells at approximatelyP1, followed by a reappearance of BDNF in hair cells and supportingcells as pillar, Deiters', or border cells at approximately P4(mice) and P5 (rats), respectively. A successive downregulationof BDNF from hair cells and pillar cells is noted at approximatelyP8-P9 (Fig. 2).

The early downregulation of BDNF from hair cells at P1 agrees with the results of Wheeler et al. (1994), who quantitativelyanalyzed BDNF expression in the organ of Corti at the mRNA level.Furthermore, BDNF mRNA expression in outer hair cells of 1-week-oldrats was reported by Ylikoski et al. (1993) but was not detectedby Wheeler et al. (1994). The unusual downregulation and upregulationof BDNF reported in the present study could have been overlookedin less detailed analyses and may explain current variations inthe documented expression pattern of BDNF mRNA in the organ ofCorti in the postnatal ratcochlea.

During the downregulation of BDNF in hair cells, we also observed an upregulation of BDNF in spiral ganglion cells. BDNF expressionhas not yet been described for spiral ganglion neurons but hasbeen reported for other sensory neurons during development (forreview, see Davies and Wright, 1995). In addition, as with recentfindings in the vestibular system (Montcouquiol et al., 1998),BDNF was expressed in supporting cells of the organ ofCorti.

Correlation of BDNF expression with the change in innervation pattern

When the spatiotemporal change of BDNF expression was compared with the course of the reorganization of early connectivitiesin the cochlea of control and BDNF gene-deleted animals, a causalrelationship between the alteration of the expression patternand the refinement of connectivities became evident. This is discussedin thefollowing.

Reorganization of presynaptic specializations at the outer hair cell level

The upregulation of BDNF in OHCs in mice cochlea at approximately P4 occurred simultaneously with the disappearance of presynapticspecializations from OHCs and the synaptogenesis of MOC efferents(Fig. 5). In BDNF gene-deleted mice, MOC efferents formed synapticcontacts with OHCs (Ernfors et al., 1995), indicating that othertrophic factors regulate this process. Considering the reportedexpression profile of the glial-derived nerve growth factor duringthis time period (Ylikoski et al., 1998), this factor may be aninteresting candidate for the control of MOC synaptogenesis. Asshown in the present study, however, when compared with controls,the synaptogenesis of MOC efferents in BDNF mutant mice occurswith a delay of several days (Fig. 6), suggesting that BDNF, nevertheless,has an indirect or redundant effect on this process. Because thesynaptogenesis of MOC efferents and the reorganization of synapticspecializations in OHCs in BDNF $-$ / $-$ mice occurred with the samedelay, these processes seem causally related and timed by BDNF.Recently, a transient appearance of the trkB full-length receptorin hair cells was suggested as influencing the reorganizationof synaptic specializations (Knipper et al., 1996, 1997). In supportof this hypothesis, we here observed the upregulation of the trkBligand BDNF coincident with the transient receptor expressionin haircells.

Afferent type I collaterals to outer hair cells

The retraction of transitory afferent type I collaterals from OHCs (Echteler, 1992; Knipper et al., 1997) and IHCs (Sobkowicz,1992) during the first postnatal week coincides with the downregulationof BDNF from hair cells shortly after birth, as observed in thepresent study (Fig. 2, P3). The absence of afferent type I collateralsin BDNF null mutants below OHCs (Fig. 7, GluR2/3) implies thatthese fibers are BDNF-dependent and, as a consequence, retractin control animals when BDNF disappears from target hair cellsafter P1. Considering the predicted differential trophic gradientof BDNF and NT-3 along the tonotopic axis of the cochlea (Bianchiet al., 1996; Fritzsch et al., 1997), our data cannot excludethe possibility that BDNF might have fewer effects on afferenttype I collaterals in basal than in the apical cochlea turn, becauseGluR2/3-immunoreactive afferent type I collaterals retract frombasal cochlea turns before birth. In addition, further studiesare required for analyzing whether collaterals to IHCs are BDNF-dependentas well, and, as a result, become reduced in number because ofthe disappearance of BDNF from inner hair cells. The retractionof BDNF-dependent afferent type I collaterals as a consequenceof the disappearance of BDNF from the target outer hair cellssuggests a new withdrawal mechanism for these fibers. This contrastswith the earlier notion that afferent type I collaterals retractbecause of the competition with innervating afferent type II orMOC efferents (Pujol, 1986; Sobkowicz, 1992).

Afferent type II fibers to outer hair cells

In agreement with previous studies (Ernfors et al., 1995; Bianchi et al., 1996; Fritzsch et al., 1997), we report the absenceof afferent type II fibers in BDNF gene-deleted mice (Fig. 7),thus confirming BDNF dependency of these fibers. Afferent typeII fibers were, however, still noted in basal cochlea turns inBDNF $-$ / $-$ mice (data not shown), in line with the absence of BDNFin these cochlea turns and consistent with the predicted BDNFgradient along the tonotopic axis of the cochlea (Bianchi et al.,1996; Fritzsch et al., 1997). Thus, the data indicate a cochleargradient in the BDNF dependency of afferent type IIfibers.

After BDNF downregulation in target hair cells in control animals, single spiral ganglion neurons synthesize their own BDNF(Figs. 2, 4). This suggests that BDNF-dependent afferent typeII fibers may grow and mature through an autocrine mechanism untilBDNF is supplied again by target and supporting cells. A transientautocrine loop for neurotrophin action during development hasalso been proposed for other sensory neurons (Schecterson andBothwell, 1992; for review, see Davies and Wright, 1995).

At the time when BDNF reappears in outer hair cells and supporting cells (Fig. 2, P6), afferents type II make synaptic contactswith OHCs (Hafidi and Romand, 1989; Echteler, 1992; Knipper etal., 1997). The expression of BDNF in supporting cells as pillar,Deiters', and border cells, in addition to hair cells during thisperiod, may either serve to transiently enlarge the target fieldand/or to ensure the innervation of supporting cells (Burgesset al., 1997). Because it has been suggested that BDNF is involvedin the maturation of the neuromuscular synapses and in the developmentof synapses in the visual system (for review, see Lu and Figurov,1997), we propose that in the auditory system, target-derivedBDNF, in addition to supporting cell-derived BDNF, may inducesynaptogenesis of afferent type II fibers. The disappearance ofBDNF from OHCs and pillar cells subsequent to presumptive synaptogenesisof afferent type II fibers at approximately P8-P10 (Fig. 2) mayimply that, as in other systems (Acheson et al., 1995; Daviesand Wright, 1995), these fibers may lose their BDNF dependencyagain after maturation of the innervation pattern. This processwould occur later for the innervation pattern of Deiters'cells.

Efferent fibers to inner hair cells

In conjunction with a maximum BDNF expression in spiral ganglion neurons (Fig. 2, P5), BDNF was found in axons and dendrites,suggesting that BDNF may be transported and released by axonsand dendrites, as has been shown for visual projections by vonBartheld et al. (1996). BDNF was localized in afferent dendriteswhen LOC efferents form axodendritic contacts with afferent typeI projections (Lenoir et al., 1980; Pujol, 1986; Knipper et al.,1995). Because in BDNF null mutant mice LOC efferents fail toform axodendritic contacts (Fig. 8), we assume that BDNF is involvedin the reorganization of LOC projections. Thus, we propose thatBDNF, which is synthesized, transported, and released by afferents,may attract LOC fibers and stabilize new axodendritic synapses.A similar role of BDNF for the stabilization of synapses has beenshown for neuromuscular junctions (Kwon and Gurney, 1996). Thepresence and persistence of axosomatic contacts of LOC efferentsin BDNF gene-deleted mice (Fig. 8) indicate that other factorsbesides BDNF may regulate the formation of axosomatic contactsor that BDNF is redundant for the guidance and maintenance ofLOC efferents. In control animals, however, the decline of BDNFfrom IHCs observed at approximately P1 may cause the retractionof BDNF-dependent LOC efferents, as has been suggested by Wheeleret al. (1994).

Conclusion

In conclusion, and for the first time, the data in the present study suggest that, before the onset of auditory function,BDNF may have a controlling role for the refinement of the innervationpattern. In particular, the retraction of fibers may be causedby the disappearance of BDNF from target hair cells, whereas thesuccessive upregulation of BDNF in hair cells, supporting cells,and spiral ganglion cells appears to be related to the formationof new synaptic contacts. Indeed, the innervation density andpatterning have been shown to be influenced by the experimentalmodulation of the BDNF level (Cohen-Cory and Fraser, 1995; Causinget al., 1997). Because the synthesis of neurotrophins is regulatedby neuronal activity (for review, see Thoenen, 1995) and neuronalactivity is increased by neurotrophins (Lohof et al., 1993; Knipperet al., 1993a,b, 1994a,b; Le $beta$ mann et al., 1994; Kang and Schuman,1995; Figurov et al., 1996), it has been suggested that a reciprocalinteraction between neurotrophins and neuronal activity may beinvolved in the innervation patterning after the onset of thefunction of sensory organs (for review, see Shatz, 1996; Knipperand Rylett, 1997). Before the onset of visual function, spontaneousNMDA-mediated activity of retinal ganglion cells is assumed toregulate the refinement of early neuronal connections in the visualsystem (for review, see Shatz, 1996). Because NMDA receptors havebeen localized during transient trkB (Knipper et al., 1997) andBDNF expression (present study), coincident to the fiber rearrangementin the developing cochlea, the next challenge will be to investigatewhether or not BDNF and NMDA-mediated spontaneous activity actin concert to determine the refinement of fibers before the transmissionof sensoryinformation.

  FOOTNOTES

Received Aug. 3, 1998; revised Feb. 2, 1999; accepted Feb. 8, 1999.

This work was supported by Deutsche Forschungsgemeinschaft Grants Ze 149/6-1, Kni 316/2-1, and SFB 430/Kni-B3. We thank HansThoenen (Max-Planck-Institut, Martinsried, Munich, Germany) forthe generous supply of BDNF mutant mice. Furthermore, we thankRegeneron Pharmaceuticals, Inc. (Tarrytown, NY) for placing cDNAprobes of BDNF and trkB at ourdisposal.
Drs. Wiechers and Gestwa contributed equally to thiswork.

Correspondence should be addressed to Dr. Marlies Knipper, University of Tübingen, Department of Oto-Rhino-Laryngology, Laboratoryof Molecular Neurobiology, Röntgenweg 11, D-72076 Tübingen,Germany.

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