BDNF and NT-4/5 Prevent Atrophy of Rat Rubrospinal Neurons after Cervical Axotomy, Stimulate GAP-43 and Talpha 1-Tubulin mRNA Expression, and Promote Axonal Regeneration

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Volume 17, Number 24, Issue of December 15, 1997

BDNF and NT-4/5 Prevent Atrophy of Rat Rubrospinal Neurons after Cervical Axotomy, Stimulate GAP-43 and T $alpha$ 1-Tubulin mRNA Expression, and Promote Axonal Regeneration

Nao R. Kobayashi¹^,², Da-Peng Fan², Klaus M. Giehl¹, Annie M. Bedard¹, Stanley J. Wiegand³, and Wolfram Tetzlaff¹^,²
¹ Department of Physiology, University of Ottawa, Ontario, Canada KIH 8M5, ² Departments of Zoology and Surgery, University of British Columbia, Vancouver, British Columbia, Canada V6T 1Z4, and ³ Regeneron Pharmaceuticals Inc., Tarrytown, New York 10591-6707

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Rubrospinal neurons (RSNs) undergo a marked atrophy in the second week after cervical axotomy. This delayed atrophy is accompaniedby a decline in the expression of regeneration-associated genessuch as GAP-43 and T $alpha$ 1-tubulin, which are initially elevated afterinjury. These responses may reflect a deficiency in the trophicsupport of axotomized RSNs. To test this hypothesis, we firstanalyzed the expression of mRNAs encoding the trk family of neurotrophinreceptors. In situ hybridization revealed expression of full-lengthtrkB receptors in virtually all RSNs, which declined 7 d afteraxotomy. Full-length trkC mRNA was expressed at low levels. UsingRT-PCR, we found that mRNAs encoding trkC isoforms with kinasedomain inserts were present at levels comparable to that for theunmodified receptor. TrkA mRNA expression was not detected inRSNs, and the expression of p75 was restricted to a small subpopulationof axotomized cells. In agreement with the pattern of trk receptorexpression, infusion of recombinant human BDNF or NT-4/5 intothe vicinity of the axotomized RSNs, between days 7 and 14 afteraxotomy, fully prevented their atrophy. This effect was stillevident 2 weeks after the termination of BDNF treatment. Moreover,BDNF or NT-4/5 treatment stimulated the expression of GAP-43 andT $alpha$ 1-tubulin mRNA and maintained the level of trkB expression.Vehicle, NGF, or NT-3 treatment had no significant effect on cellsize or GAP-43 and T $alpha$ 1-tubulin expression. In a separate experiment,infusion of BDNF also was found to increase the number of axotomizedRSNs that regenerated into a peripheral nerve graft. Thus, inBDNF-treated animals, the prevention of neuronal atrophy and thestimulation GAP-43 and T $alpha$ 1-tubulin expression is correlated withan increased regenerative capacity of axotomized RSNs.
Key words: axotomy; spinal cord injury; neurotrophin; regeneration, red nucleus; gene expression; neuronal atrophy; cell body response; peripheral nerve transplant

INTRODUCTION

Within the CNS, axons usually fail to regenerate after injury, whereas successful axonal regeneration occurs in the peripheralnervous system (PNS) (Ramon y Cajal, 1928/1991). This failurehas been attributed to the presence of inhibitory molecules inthe mature CNS (Caroni and Schwab, 1988; Bovolenta et al., 1993;McKerracher et al., 1994; Mukhopadhyay et al., 1994; Schachneret al., 1994), and in addition to the death or atrophy of theparent cell body (Barron et al., 1989; Aguayo et al., 1991; Giehland Tetzlaff, 1996) and to intrinsic factors (Barron et al., 1989;Chen et al., 1995), such as the failure of the injured CNS neuronsto express regeneration-associated genes (Skene, 1989; Tetzlaffet al., 1991, 1994). For example, we have shown that after axotomyat the cervical level of the spinal cord, GAP-43 and T $alpha$ 1-tubulinexpression are increased transiently in rubrospinal neurons (RSNs)(Tetzlaff et al., 1991). This observation correlates with thegrowth of a small percentage (1-2%) of RSN axons into the permissiveenvironment of peripheral nerves implanted into the cord at thelevel of transection (Richardson et al., 1984; Houle, 1991; Tetzlaffet al., 1994). However, the very limited regeneration of RSN axonsinto the grafts may reflect an impaired regenerative propensityof these neurons, which is likely related to the severe atrophythat occurs during the second week after cervical axotomy (Eganet al., 1977; Barron et al., 1989; Tetzlaff et al., 1991). Concomitantwith this massive neuronal atrophy, the number of axotomized RSNsthat express GAP-43 and T $alpha$ 1-tubulin decreases markedly duringthe second week after injury (Tetzlaff et al., 1991). Here, wetest the hypothesis that the atrophy and decline in regeneration-associatedgene expression observed in axotomized RSNs are caused by a lackof trophic support, and that these effects may be prevented bythe application of exogenous trophic factors. The trophic dependencyof RSNs in adult rats is not well understood, and in this studywe focused on the family of neurotrophins and their receptors.

The neurotrophin family of factors, comprising nerve growth factor (NGF), brain-derived neurotrophic factor (BDNF), neurotrophin-3(NT-3), and neurotrophin-4/5 (NT-4/5), has been shown to influenceneuronal survival and differentiation during development, as wellas maintenance of neuronal phenotype and modulation of synapticefficacy in the adult nervous system (for review, see Korsching,1993; Davies, 1994; Lindholm et al., 1994; Lindsay et al., 1994;Bonhoeffer, 1996; Lewin and Barde, 1996). The trk family of receptortyrosine kinases has been identified as the high-affinity, signal-transducingreceptor for the neurotrophins (for review, see Kaplan and Stephens,1994; Barbacid, 1995; Bothwell, 1995). Based largely on in vitrotransfection studies in PC-12 cells and fibroblast cell lines,NGF is considered to be the primary ligand for TrkA, BDNF, andNT-4/5 for TrkB, and NT-3 for TrkC (Klein et al., 1991a,b, 1992;Lamballe et al., 1991; Soppet et al., 1991; Squinto et al., 1991;Ip et al., 1993). Insertions in the tyrosine kinase domain ofthe TrkC alter the signaling capacity of this receptor in responseto NT-3 binding (Tsoulfas et al., 1993, 1996; Valenzuela et al.,1993; Guiton et al., 1995). Thus, the cellular responsivenessto NT-3 is likely influenced by the presence of the various receptorisoforms.

In the present study, we report that RSNs express mRNA for full-length trkB and low levels of noninserted and inserted trkCbut no trkA receptors. Application of BDNF or NT-4/5, but notNGF or NT-3, fully prevented the atrophy of axotomized RSNs andalso stimulated the expression of GAP-43 and T $alpha$ 1-tubulin. Infusionof BDNF also was found to increase the number of axotomized RSNsthat regenerated into grafts of sciatic nerve implanted into thecervical cord at the level of spinal transection.

MATERIALS AND METHODS
Animals and surgery. Male Sprague Dawley rats (Charles River Laboratories, Wilmington, MA) (220-250 gm; n = 112) were usedfor this study. They were kept in a 12 hr light/dark cycle andfed a standard rodent diet ad libitum. All experiments were performedin accordance with the guidelines of the Canadian Council forAnimal Care and approved by the local animal care committee. Allsurgery was performed under anesthesia with sodium pentobarbital(32 mg/kg) plus chloral hydrate (150 mg/kg) in sterile conditions.

Spinal cord hemisection. The neck musculature was split in the midline, and left hemilaminectomy was performed at C3/C4. Afterthe dura was opened, the dorsolateral funiculus of the spinalcord was cut with a pair of iris scissors, and the incision wasverified with a fine Dumont no. 5 forceps. In some animals, asmall piece of gelfoam (Upjohn, Kalamazoo, MI) soaked with 0.5-1.0µl of 2% FluoroGold (FG) (Fluorochrome Inc., Eaglewood, CA) wasapplied to the injury site. The muscles were sutured with prolene(6-0) (Ethicon, Somerville, NJ), and the skin was closed withwound clips. Rats used for the in situ hybridization (ISH) andRT-PCR study of neurotrophin receptor expression (n = 14) werekilled by an overdose of chloral hydrate 7 d after axotomy, andthe fresh midbrains were immediately frozen on dry ice. In allother experiments, rats were injected with an overdose of chloralhydrate and perfused transcardially with PBS followed by freshlyhydrolyzed paraformaldehyde (4% in 10 mM phosphate buffer.

Neurotrophin application. RSN atrophy and the expression of GAP-43 and T $alpha$ 1-tubulin were assessed in animals that were treatedwith recombinant human (rh) NGF, rhBDNF, rhNT-3 or rhNT-4/5, orvehicle. On day 7 postaxotomy, rats were anesthetized, and cannulae(28 ga, 8 mm; Plastic One Inc., Roanoke, VA) were inserted stereotaxicallyinto the vicinity of the red nucleus at the following coordinates:anterior-posterior 6.3 mm posterior to Bregma, medial-lateral $-$ 1.7 mm (to the right of midline), and dorsal-ventral $-$ 6.5 mm(from the cortical surface). The cannulae were anchored in positionwith two watchmaker screws and dental cement. Osmotic minipumps(Alzet no. 2001) (1 µl/hr) were filled with either vehicle alone[20 mM sterile PBS supplemented with 100 U penicillin/streptomycinand 0.5% rat serum albumin (no. A-6272; Sigma, St. Louis, MO)],rhNGF, rhBDNF, rhNT-3, or rhNT-4/5 at a concentration of 500 ng/µl.Pumps were connected to the infusion cannulae with 6-8 cm of SILASTICtubing (no. 508-003, VWR Canlab), and the entire assembly waspreincubated for 4-12 hr in sterile 20 mM PBS at 37°C before implantation.Thus, each treated animal received 12 µg of rhNGF, rhBDNF, rhNT-3,or rhNT-4/5 per day in a total volume of 168 µl over a periodof 7 d (between day 7 and 14 postaxotomy).

Peripheral nerve implants. To evaluate the effect of BDNF treatment on the regenerative capacity of axotomized RSNs, segmentsof peripheral nerve were implanted into the hemisected spinalcord. The right sciatic nerve was transected at the level of theobturator tendon and left in situ to allow Wallerian degenerationof the distal stump. Ten days later, a 30-35 mm segment of thepredegenerated nerve was resected, and its proximal end was insertedinto a C4 left spinal cord hemisection site. It was held in placewith two Prolene 10-0 sutures (Ethicon, Somerville, NJ), and thedistal free end was marked with a Prolene 6-0 suture (Ethicon)and left in the subcutaneous tissue. The spinal column from C3to C5 was immobilized by placing three watchmaker screws intothe right vertebral pedicles of C3, C4, and C5 and stabilizedwith bone cement (Ethicon, Peterborough, ON, Canada). During thesame surgical session, an osmotic minipump was implanted as describedabove to administer BDNF into the vicinity of the RSNs. The rationaleto apply BDNF for 7 d at the time of spinal cord injury and transplantationwas based on the animal care regulation that recommends the numberof surgical interventions (three instead of four operations).We documented a prolonged effect of BDNF beyond the period ofapplication, which further justifies our design. Ten weeks afterspinal cord injury, pump implantation, and transplantation, therats were anesthetized again, and the free end of the nerve transplantwas identified and mobilized. The distal end (1-3 mm) of the nervegraft was resected, and the freshly exposed end of the nerve wasplaced into a small polyethylene tubing filled with 5% FG for1 hr. Fourteen days later, the rats were overdosed with chloralhydrate and perfused with paraformaldehyde, as described above.After post-fixation overnight in the same fixative, the midbrainsand cervical spinal cords were cryoprotected in 16% and 22% sucrosein 10 mM PBS and frozen in dry ice-cooled isopentane. The midbrainswere cut in series at 14 µm thickness. FG-labeled neuronal profileswere counted throughout the caudal 1 mm of the red nucleus. Carewas taken to avoid double counting in adjacent sections. Student'st test was used to compare the number of retrogradely filled,i.e., regenerating, neurons in BDNF-treated versus untreated rats.

RT-PCR. Fresh frozen midbrains from 10 rats at 7 d after spinal cord hemisection at the cervical level were used for RT-PCRanalysis of trkB and trkC receptor expression. FG-filled axotomizedRSNs were visualized with a fluorescent microscope and microdissectedfrom 70- to 80-µm-thick serial sections through the caudal pole(400 µm) of the red nucleus containing the magnocellular population.The contralateral red nuclei were identified and dissected underdark-field illumination. We determined in earlier experimentsthat retrograde-labeling of RSNs with FG had little effect onRNA expression (W. Tetzlaff, B. Tsui, A. M. Bedard, and S. Cassar,unpublished observation). Total RNA was extracted from red nucleipooled from 2× five animals using Trizol (Life Technologies, Gaithersburg,MD) according to a standard protocol provided by the manufacturer,followed by DNase treatment. The procedures for RT-PCR and controlexperiments were essentially the same as in our previous study(Kobayashi et al., 1996). PCR for cyclophilin was included asa control, using the primers published in Mearow et al. (1993)to ensure that equivalent amounts of input cDNA were analyzed(data not shown). The trkB primers used have been described previouslyin Kobayashi et al. (1996). The trkC primers were previously usedby Offenhauser et al. (1995) and designed to bracket the potentialinsertion site within the tyrosine kinase domain to reveal differenttrkC insertion isoforms. After 30 amplification cycles, trkC PCRproducts were run on a 5% polyacrylamide gel stained with ethidiumbromide and visualized under UV light and photographed. For trkBserial dilution PCR, 25, 12.5, and 6.75 ng of input cDNA wereamplified for 25 PCR cycles, and trkB PCR products were run on1% agarose gel, followed by Southern transfer to a nylon membrane(Zeta-probe, Bio-Rad, Hercules, CA). The membrane was subsequentlyhybridized with ³⁵S-labeled trkB oligonucleotide probe internal to and not overlappingwith the respective PCR primers according to the standard protocol(Sambrook et al., 1989). The PCR of input cDNA serial dilutionsfollowed by Southern blotting were within the linear range asdetermined by phosphoimaging (Molecular Dynamics, Sunnyvale, CA)when 25 amplification cycles were used for trkB and 30 amplificationcycles were used for trkC (noninserted trkC isoform at 299 bp;data not shown), respectively. These 50 mer were also used inour trkB and trkC in situ hybridization study (see ISH section)and had little homology to other trk receptors.

Immunocytochemical assessment of the neurotrophin distribution. Perfusion-fixed sections containing red nuclei were immunostainedusing antibodies for NGF, BDNF, NT-3, or NT-4/5. The specificityof the antibodies for their respective neurotrophin has been describedpreviously (Anderson et al., 1995; Alderson et al., 1996). Theconcentrations of the primary antibodies were adjusted so thatthey exhibited equivalent levels of detection of the homologousneurotrophin on slot blots (0.5-1.0 ng/8 mm²); 1:7500 for the turkey anti-BDNF antibody, 1:5000 for the turkeyanti-NT-3 antibody, 1:15,000 for the goat anti-NGF antibody, and1:10000 for the chicken anti-NT-4/5 antibody. No cross-reactivitywith heterologous neurotrophins was apparent on slot blots orin perfusion-fixed midbrain sections taken from animals that hadbeen injected with 1 µg of the neurotrophins (data not shown).Primary antibody omission or preabsorption with the appropriatebut not related neurotrophins also abolished specific immunostaining(data not shown). Primary antibodies bound to tissue were localizedusing an appropriate biotinylated secondary antibody (1:1500)and the avidin-biotin-peroxidase complex (Vectastain, Vector Laboratories,Burlingame, CA).

Histology and cell size measurements. Most neurotrophin-treated and vehicle-treated rats were killed on day 14, except forsix rats that were left beyond the cessation of neurotrophin applicationi.e., until day 21 or 28. These rats were overdosed with chloralhydrate, followed by perfusion as described above. Frozen sectionswere cut coronally at 12 µm through the midbrain and mounted ontoSuperfrost Plus slides (Fisher Scientific, Houston, TX). Eachslide contained a section from two control animals that receivedno pump or a vehicle pump and from one or two animals treatedwith a neurotrophin. The order in which they were cut and positionedonto the slide was randomized. The midbrains were cut from caudalto cranial, and collection of sections was begun when 6-10 RSNsappeared at the caudal pole of the red nucleus and the following35 sections were gathered. Sections 15, 25, and 35 were stainedwith 0.2% cresyl violet for cell profile measurement and photography.The remaining sections were stored at $-$ 80°C for ISH analysis.

The cell profile sizes were measured using a computerized image analysis system. Two techniques involving computerized digitizationof the cell image and profile measurement were used. In the firstmethod, a 16× oil immersion objective (Zeiss) was used to cropthe images, and the contour of each neuron containing a visiblenucleus was traced. This contour was filled in, and the numberof pixels was measured to obtain an arbitrary value for the cross-sectionalcell area. In the second technique, a field comprising about halfthe red nucleus was digitally captured using a 10× objective.Subsequently the density threshold was determined to discriminatethe stained neurons from the background. Only those cell profilesthat were twice the size of an average glial cell were includedin our analysis. Confluent neurons were separated with a digitizedpaintbrush. In both procedures, the operator was blinded to thetreatment condition. Because both procedures yielded very similarresults, the latter technique was used routinely. The size ofneurons within the red nucleus is heterogeneous, and smaller neuronsare located predominantly toward the cranial end of the nucleus;hence, axotomized neurons at the caudal pole of the red nucleushave a size similar to the uninjured neurons in the rostral portionof the magnocellular red nucleus. Thus, the average cell sizeof axotomized RSNs was normalized to that of its contralateralcounterpart in sections 15, 25, and 35, and values were expressedas a percentage of contralateral control for each level of thenucleus. These percentages from individual animals were subjectedto statistical analysis (see Statistical Analysis), and the medianpercentage from the individual treatment groups plus the 25th-75thpercentiles are presented. We also provided the actual cell profilesize measurements at the level of section 25 obtained from perfusion-fixedmidbrains of different animal groups (see Table 1).

Table 1. Mean cell profile sizes (µm²) of RSN 14 d after axotomy, with or without neurotrophin treatment

Mean cell size (mm²)

Group Contralateral Axotomized

No pump (n = 6) 444.6 ± 36.5 297.2 ± 20.4

Vehicle (n = 5) 449.6 ± 29.1 307.2 ± 33.6

BDNF (n = 6) 494.3 ± 15.8 545.6 ± 59.7^*

NT-4/5 (n = 4) 517.5 ± 12.8 603.1 ± 35.2^*

NGF (n = 4) 437.3 ± 30.8 338.1 ± 17.3

NT-3 (n = 5) 495.3 ± 39.5 368.2 ± 41.3

There is no significant difference in the contralateral profile sizes among different animal groups. The RSNs treated withBDNF or NT-4/5 are significantly larger than all the other groups(*p < 0.05), whereas NGF- or NT-3-treated RSNs are not differentfrom the control groups. ^* p < 0.05; Newman-Keuls test.

ISH. The protocol given in Verge et al. (1992) was used with some modification. The trkA probe was complementary to bases1198-1245 and was used previously by Verge et al. (1992). Thefull-length trkB probe was described in Kobayashi et al. (1996)and is complementary to bases 1363-1407 (Middlemas et al., 1991).The trkC probe (Giehl and Tetzlaff, 1996) was complementary tobases 2109-2272 (excluding 2134-2250), bridging the insertionsite in the cytoplasmic tyrosine kinase domain (Valenzuela etal., 1993). The T $alpha$ 1-tubulin probe was a 50 mer oligonucleotidecomplementary to the 3 $'$ -untranslated sequence of T $alpha$ 1-tubulin 5 $'$ -AAACCCATCAGTGAAGTGGACGGCTCGGGTCTCTGACAAATCATTCA-3 $'$ , and the GAP-43 probe was complementary to bases 220-270(Basi et al., 1987). For all probes, no similarities were foundfor other molecular sequences at a 75% cutoff level in a BLASTNdatabase search at the National Center for Biotechnology Information(Altschul et al., 1990). These oligonucleotide probes were end-labeledwith ³⁵S-ATP using deoxynucleotide terminal transferase according toa standard protocol (Ausubel et al., 1987). For trk receptor ISH,sections collected from fresh frozen midbrains were hybridizedto 10⁶ cpm of the respective probe in 100 µl of hybridization mixturefor 16-18 hr at 43°C [for details of the mixture, hybridizationconditions, and washes, see Verge et al. (1992)]. For GAP-43 andT $alpha$ 1-tubulin ISH, perfusion-fixed sections (14 µm) were pretreatedand hybridized to 10⁶ cpm of probe for 16-18 hr at 43°C [for details, see Giehl andTetzlaff (1996)]. The slides were dipped in Kodak NTB-2 emulsionand were exposed for 2 d for T $alpha$ 1-tubulin, 7 d for GAP-43, 3 weeksfor trkB, and 7-9 weeks for trkA and trkC. For trk receptor ISH,the sections were stained with 0.2% cresyl violet, dehydrated,and embedded in DePex (BDH Chemicals, Poole, UK). We confirmedthat GAP-43 and T $alpha$ 1-tubulin probes gave a single band of expectedsize in Northern blots of RNA from facial nuclei under identicalor less stringent hybridization conditions (Tetzlaff et al., 1991)Equivalent data were obtained for the oligonucleotide probes (datanot shown). We performed RT-PCR for trkB and trkC, followed bySouthern blotting. The trkB and trkC probes recognized the bandsof expected size (see RT-PCR section). We obtained essentiallythe same results for GAP-43 and T $alpha$ 1-tubulin ISH in no-pump controlanimals and our previous study using cDNA probes of several hundredbase pairs (Tetzlaff et al., 1991), except that the oligonucleotideprobes in this study detected the low levels of GAP-43 and T $alpha$ 1-tubulinin the contralateral control RSNs because of their higher sensitivity.

Quantification of GAP-43 and T $alpha$ 1-tubulin ISH signals. The Northern Exposure Image Analysis system (EMPIX, Mississauga, Ontario,Canada) equipped with a frame grabber for the integration of multipleframes was used, allowing us to capture pictures of the fluorescentFG-filled RSNs. This integration allowed us to visualize furtherthe contours of the unstained contralateral neurons. RSNs (50-100)from each animal (two to four slides per animal) were analyzedfor each probe. To obtain this number, we collected and analyzedthree to five digitized images of the FG-filled RSNs from eachsection through the red nucleus. The fluorescent pictures of RSNswere loaded into one frame buffer, and corresponding dark-fieldimages of the silver grains representing the ISH signal were capturedinto another frame buffer. The contours of the fluorescent-labeledcells were traced with a digitized mouse, and this contour wasused as a mask in the other frame buffer, which contained thedark-field-illuminated silver grains. The area fraction occupiedby the silver grains within this mask was measured and correctedfor a background of the tissue. This corrected fraction was subsequentlymultiplied by the estimated volume of the neuronal cell body (assumingthat the latter is spherical) to generate the "ISH signal/cell."The ISH signal/cell values of the axotomized RSNs were expressedas multiples of the mean ISH signal/cell of the contralateralRSNs. Only perfusion-fixed brain tissues were included in ISHquantification, because fixation was needed to retain FG-labelingafter ISH procedures. Therefore, the numbers of animals for ISHquantification were smaller than those included in the cell sizestudy.

Statistics. Because the cell size data as well as ISH quantification data were normalized and expressed as percentage of ormultiples of contralateral values, we used Kruskal-Wallis one-wayANOVA on ranks to test the differences in median values amongthe different treatment groups. This test does not assume normaldistribution or equal variance of data. To identify the groupsthat differ significantly from the control group (vehicle-treatedgroup), Dunn's multiple comparison procedure was performed atthe significance level of p < 0.05. The actual cell profile sizesof the axotomized and contralateral RSNs within the same groupwere compared using paired t test (p < 0.05). Groupwise comparisonsof the contralateral RSNs as well as the axotomized RSNs amongdifferent groups were performed using Newman-Keuls test at thesignificance level of p < 0.05.

RESULTS

Neurotrophin receptor expression
The expression of the trk family of neurotrophin receptors in RSNs 7 d after axotomy was studied by ISH to predict the possibleresponsiveness of RSNs to neurotrophins. TrkA ISH signal was notdetectable in either unlesioned or axotomized RSNs (Fig. 1a,b).However, interpeduncular neurons in the same sections as wellas cholinergic basal forebrain neurons (Figueiredo et al., 1995)showed strong expression of trkA, ruling out technical problems(data not shown). In contrast, expression of full-length trkBmRNA was seen in virtually all uninjured RSNs, in agreement withthe recent immunocytochemical study of Yan et al. (1997) (Fig.1d). This expression was decreased to 0.7× the contralateral level7 d after axotomy (Fig. 1c) and declined further thereafter asthese neurons became atrophic during the second week after axotomy(data not shown). The expression of trkB in the red nucleus wasconfirmed by serial dilution RT-PCR (amplification of 25, 12.5,and 6.75 ng cDNA), followed by Southern blotting using a trkBprobe internal to the PCR primers (Fig. 1g). This analysis alsoconfirmed the ISH observation that the trkB expression was decreasedin axotomized RSNs compared with the contralateral, intact RSNs(Fig. 1g).
Fig. 1. Expression of trkA, trkB, and trkC receptors in RSNs. trkA ISH signal is undetectable in axotomized as well as contralateralRSNs (a, b). Expression of full length trkB (c,d) as well as full-lengthnoninserted trkC in RSNs (e, f) at 7 d after axotomy (c, e) andin contralateral RSNs (d, f). 700× magnification. Scale bar, 20µm. RT-PCR for trkB (25 cycles, visualized by Southern blotting)using serial dilutions of the input cDNA (25.0, 12.5, 6.75 ng)obtained from axotomized ("a") and contralateral ("c") red nuclei(g). Note the decrease in trkB mRNA 7 d after axotomy seen byISH (c,d) and RT-PCR (g). RT-PCR (30 cycles, ethidium bromidestaining) for trkC isoforms in axotomized ("a") and contralateral("c") red nuclei (h). Note the predominant expression of the noninsertedtrkC isoform (299 bp) as well as the isoforms with 14 amino acids(341 bp) and the weak expression of the isoforms with 25 (374bp) and 35 (416 bp) amino acids insertions.
[View Larger Version of this Image (109K GIF file)]

TrkC isoforms having 14, 25, or 39 amino acids insertions in the kinase domain are commonly present in neural tissues (Tsoulfaset al., 1993; Valenzuela et al., 1993). Because these isoformsappear to be limited in their signaling capability (Guiton etal., 1995; Tsoulfas et al., 1996), we used an oligonucleotideprobe bridging the insertion site to study the expression of thefull-length, noninserted trkC receptor. Weak expression of noninsertedtrkC mRNA was detected in uninjured and axotomized RSNs only afterprolonged autoradiographic exposure (6-8 weeks) (Fig. 1f,e). Similarexposure times produced strong hybridization signals in corticospinalneurons (Giehl and Tetzlaff, 1996) and in facial motoneurons (K.L. Fernandes, N. R. Kobayashi, and W. Tetzlaff, unpublished observations).To further study the expression of trkC isoforms, we used trkCPCR primers bracketing the insertion site within the tyrosinekinase domain (Offenhauser et al., 1995). RT-PCR results revealedthat both axotomized and contralateral RSNs expressed the noninserted(299 bp) as well as the known inserted isoforms (341, 374, and416 bp) of the trkC receptor (Fig. 1h). The noninserted and 14amino acid insert forms of trkC were the predominant types expressedin uninjured RSNs, and there was no apparent change in isoformcomposition 7 d after axotomy (Fig. 1h). The ISH analysis of thep75 neurotrophin receptor showed no signal in unlesioned RSNs.However, at 7 d, but not 3 weeks postaxotomy, we found detectablep75 mRNA expression in the occasional axotomized RSNs (<10%; datanot shown). Taken together, these observations suggest that axotomizedRSNs may be responsive to BDNF and NT-4/5, cognate ligands forthe trkB receptor, and to NT-3, which preferentially binds tothe trkC receptor.

Distribution of infused neurotrophins
The receptor expression profiles of RSNs provided the rationale for the application of the neurotrophins. These were infusedbetween days 7 and 14 postaxotomy because acute axotomy-inducedatrophy and concomitant decline in regeneration-associated geneexpression occur in axotomized RSNs during this period (Tetzlaffet al., 1991). Figure 2 shows a diagram of an infusion cannulainserted into the vicinity of the red nucleus, which is connectedto an osmotic minipump via SILASTIC tubing to apply 500 ng · µl¹ · hr¹ of the appropriate neurotrophin. To assess the extent of factordistribution within the target tissue, midbrain sections werestained with antibodies to the various neurotrophins at the endof the 7 d infusion period. Immunostaining for rhNGF, rhNT-3,and rhNT-4/5 (Fig. 3a,c,d) revealed that these factors diffusedover most of the midbrain tegmentum ipsilateral to the side ofinfusion, filling a sphere of tissue ~4 mm in diameter. In contrast,the diffusion of rhBDNF (Fig. 3b) was confined to an area within1.0-1.5 mm of the cannula. These finding are consistent with thestudy of Anderson et al. (1995). Given the relatively limiteddiffusion of rhBDNF, for all of the factors we limited our analysisto those cases in which the cannulae were located within 0.5-1.0mm of the lateral margin of the red nucleus. Cannula placements<0.5 mm from the nucleus were excluded to rule out dendritic damageand nonspecific effects of trauma.
Fig. 2. Schematic diagram showing the midbrain at the level of the red nucleus and the cervical spinal cord. The approximate insertionsite of the application cannula connected to an osmotic minipumpcontaining either vehicle alone or neurotrophins is illustratedin the coronal midbrain section. The hatched area in the spinalcord indicates the extent of transection at the cervical level(C3), which includes the rubrospinal tract.
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Fig. 3. Immunohistochemistry for NGF(a), BDNF (b), NT-3 (c), and NT-4/5 (d) infused lateral to the red nucleus. NGF immunostaining(a) reveals good tissue penetration of rhNGF covering almost anentire half of the midbrain in the coronal plane. In contrast,rhBDNF (b) diffusion is limited around the center of the applicationneedle within ~1 mm of the cannula. Penetration of rhNT-3 (c)and rhNT-4/5 (d) is comparable to that of rhNGF as shown by theirrespective immunostaining. 10× magnification. Scale bar, 1.5 mm.
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Effects of neurotrophin infusion on RSN size
Consistent with earlier findings (Egan et al., 1977), atrophy of RSNs was prominent 14 d postaxotomy. We found that the medianof cell profile size of axotomized untreated RSNs decreased to62.8% (25th-75th percentile: 59.6-66.6%; n = 12) of their uninjuredcontralateral counterparts. The infusion of BDNF or NT-4/5 completelyprevented this axotomy-induced reduction in atrophy (Fig. 4b vsc, d vs e), whereas infusion of NGF, NT-3, or vehicle alone (Fig.4a vs b) did not affect the size of the axotomized RSNs. Interestingly,axotomized RSNs in BDNF- or NT-4/5-treated animals continued toexhibit classic signs of retrograde reaction to axotomy, includingchromatolysis and a pronounced eccentricity of the nucleus. ANOVAon ranks (Kruskal-Wallis test) revealed significant differences(p < 0.0001) in the median cell profile size expressed as percentageof contralateral between the treatment groups. The median percentageof the BDNF- (105.2%; 25th-75th percentile: 92.3-129.1%; n = 9)and NT-4/5-treated (107.0%; 25th-75th percentile: 96.8-111.3%;n = 7) groups was significantly different (p < 0.05; Dunn's test)from the median percentage of the vehicle-treated group (68.8%;25th-75th percentile: 62.4-75.3%; n = 15). Neither infusion ofNGF (72.1%; 25th-75th percentile: 67.6-75.5%; n = 6) nor of NT-3(84.6%; 25th-75th percentile: 65.6-90.3%; n = 9) increased thesize of axotomized RSNs compared with vehicle treatment.
Fig. 4. Cresyl violet staining of vehicle- or neurotrophin-treated RSNs 14 d after axotomy (a, c, e) and their contralateral counterparts(b, d, f). Note the severe atrophy of vehicle-treated RSNs (avs b). This atrophy is fully prevented in axotomized RSNs treatedwith BDNF (c) or NT-4/5 (e), displaying the cell profile sizescomparable to the contralateral RSNs (d, f). Note that the axotomizedand neurotrophin-treated RSNs are chromatolytic. 400× magnification.Scale bar, 50 µm.
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To gain more insight into the cell size changes after axotomy with or without neurotrophin treatment, the cell profile sizemeasurements were taken from the equivalent level of red nucleusfrom different groups (Table 1). This confirms that there wereno differences in mean cell profile sizes of contralateral RSNsamong these groups and that BDNF- and NT-4-treated axotomizedRSNs were significantly larger than the axotomized RSNs of allother treatment groups (p < 0.05; Newman-Keuls test). The axotomizedRSNs treated with BDNF and NT-4/5 displayed cell profiles sizesthat were not different from their contralateral counterparts,whereas the axotomized RSNs of all other groups were significantlysmaller (p < 0.01; except for NT-3 treatment, p < 0.05). The cellprofile sizes of the untreated intact RSNs were comparable tothe study by Mori et al. (1997).

Interestingly the effect of the BDNF application lasted beyond the 7 d period of infusion. In BDNF-treated animals, the mediansize of axotomized RSNs was 79% and 83% of the contralateral,intact RSNs on days 21 and 28, respectively (7 and 14 d aftercessation of the BDNF treatment). The corresponding values fromvehicle controls were 60 and 56%, indicating a continuing declinein cell size over time (data not shown). As mentioned above, thesedata are based on infusions through cannulae positioned within0.5-1.0 mm from the lateral border of the red nucleus. BDNF infusionhad no effect on neuronal soma size if the cannula was placedfurther away, reflecting the limited diffusibility of this factor(see above).

Effects of neurotrophin infusion on GAP-43 and T $alpha$ 1-tubulin expression
Because infusion of BDNF and NT-4/5 into the vicinity of axotomized RSNs fully prevented their atrophy (Fig. 4, Table 1),we wished to determine whether infusion of neurotrophins mightalso prevent the decline in GAP-43 and T $alpha$ 1-tubulin mRNA expressiontypically observed during the second week after axotomy (Tetzlaffet al., 1991). The histogram of GAP-43 ISH quantification obtainedfrom representative animals (marked by arrows in Fig. 6b) showedthat on day 14 postaxotomy, only a subpopulation (50%) of axotomizedRSNs treated with vehicle displayed increases in GAP-43 hybridization,whereas the remainder showed signals near intact, control levels(Figs. 5a, 6a). In contrast, when treated with BDNF or NT-4/5the majority (>90%) of axotomized RSNs expressed increased levelsof GAP-43 mRNA (Figs. 5b,c, 6a). Furthermore, vehicle-infusedand no-pump animals exhibited only a two- to threefold mean increasein GAP-43 mRNA expression, whereas treatment with BDNF or NT-4/5typically produced mean increases of four- to sevenfold (Fig.6b). In three cases, the increases were much higher (9- to 13-fold).GAP-43 expression in NGF- and NT3-treated animals was similarto that seen in controls. The differences among treatment groupswere statistically significant (p < 0.01; Kruskal-Wallis). Subsequentgroupwise comparisons (Dunn's test) revealed that the median increasein GAP-43 ISH signal in the BDNF-treated (5.3×, 25th-75th percentile:5.1-6.5×; n = 6) and NT-4/5-treated (7.6×, 25th-75th percentile:5.1-9.8×; n = 4) groups were significantly different from thatof the vehicle control group (2.4×, 25th-75th percentile: 2.3-2.8×;n = 5) (p < 0.05). In contrast, neither treatment with NGF (3.0×,25th-75th percentile: 2.2-4.3×; n = 4) nor with NT-3 (2.7×, 25th-75thpercentile: 2.3-3.2×; n = 5) produced increases in GAP-43 expressionthat were significantly different from that of the vehicle control.
Fig. 6. Histograms of the percentage of cells displaying GAP-43 (a) or T $alpha$ 1-tubulin (c) expression in multiples of their contralateralexpression level, obtained from representative animals infusedwith vehicle, BDNF, or NT-4/5 (marked by arrows in b and d). Thelabels of x-axis (multiples of contralateral) indicate an upperlimit value of the bin category. Note the apparent shift to theright (increased expression) for both genes in the numbers ofRSNs treated with BDNF or NT-4/5 compared with those treated withvehicle. Each symbol in b and d represents the mean (±SEM) ofISH signals/cell normalized to that of contralateral RSNs, i.e.,expressed as multiples of contralateral derived from an individualanimal. Dashed lines indicate the expression level of contralateral(=1). Note the increased expression of GAP-43 (b) as well as T $alpha$ 1-tubulin(d) in the animal groups treated with BDNF or NT-4/5 comparedwith the vehicle or no-pump control groups.
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Fig. 5. GAP-43 and T $alpha$ 1-tubulin ISH in axotomized RSNs treated with vehicle, BDNF, or NT-4/5. The FG-labeled, axotomized RSNs are visualizedunder fluorescent illumination, superimposed with autoradiographicsilver grains representing the ISH signals in dark-field illumination.Note that only a subpopulation of axotomized RSNs display GAP-43ISH signal with vehicle treatment (a); in contrast, the majorityof axotomized RSNs treated with BDNF (b) or NT-4/5 (c) expresshigh levels of GAP-43 mRNA. Moreover, an increase in T $alpha$ 1-tubulinexpression is also observed in axotomized RSNs treated with BDNF(e) or NT-4/5 (f) compared with those RSNs treated with vehicleonly (d). 360× magnification. Scale bar, 40 µm.
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Axotomized RSNs also exhibited higher T $alpha$ 1-tubulin expression in BDNF- and NT-4/5-treated animals compared with vehicle-treatedcontrols (Fig. 5d-f). The histogram of representative animals(marked by arrows in Fig. 6d) illustrated that by 14 d after axotomy,~60% of the RSNs displayed T $alpha$ 1-tubulin ISH signals at levels belowtheir contralateral counterparts, whereas <20% showed increasedlevel of expression (Fig. 6c). In marked contrast, T $alpha$ 1-tubulinexpression was higher on the lesioned side in more than half ofthe RSNs treated with BDNF or NT-4/5 (Fig. 6c). Mean T $alpha$ 1-tubulinISH signals, expressed as multiples of contralateral values, rangedfrom 0.4 to 1.1× in both "no-pump" and vehicle control groups(Fig. 6d). In BDNF- and NT-4/5-treated animals, values were between1.3 and 2.3×. Infusion of NGF or NT-3 produced mean values thatdid not differ from that of controls (range, 0.4-1.4×). Thesedifferences among groups were statistically significant (p < 0.01;Kruskal-Wallis), and subsequent groupwise comparisons demonstratedthat the median increases in T $alpha$ 1-ISH signal of the BDNF- (1.6×,25th-75th percentile: 1.3-1.8×; n = 6) and the NT-4/5-treated(1.6×, 25th-75th percentile: 1.3-1.9×; n = 4) groups were significantlydifferent (p < 0.05) from that of the vehicle-treated controlgroup (0.67×, 25th-75th percentile: 0.57-0.76×; n = 6). Neithertreatment with NGF (0.75×, 25th-75th percentile: 0.69-0.98×; n= 4) nor with NT-3 (0.87×, 25th-75th percentile: 0.65-1.1×; n= 5) resulted in median T $alpha$ 1-tubulin ISH signals different fromthose of the vehicle-treated controls.

Stimulation of rubrospinal regeneration into peripheral nerve transplants
Predegenerated sciatic nerve segments of 30-40 mm length were inserted into C4 lesions of the rubrospinal tract, and regenerationwas assessed by retrograde labeling with FG 2 months later. Typicallythese experiments resulted in a mean of 43 ± 9.3 regeneratingneurons in control rats (n = 6) (Fig. 7c, open symbols). Animalsreceiving BDNF infusions into the vicinity of the red nucleus,however, had a mean number of 131 ± 19.7 regenerating RSNs (n= 6) (Fig. 7c, filled symbols), which was significantly differentfrom the untreated controls (p < 0.01; t test). Representativesections through the red nucleus for both groups (marked by arrowsin Fig. 7c) are shown in Figure 7a,b.
Fig. 7. Photomicrographs of FG-labeled RSNs regenerated into a peripheral nerve transplant obtained from an animal without treatment(a; c, marked by arrow) and of a BDNF-treated animal (b; c, markedby arrow). c shows the numbers of FG-labeled, i.e., regenerated,RSNs of individual animals without treatment (open symbols) andwith BDNF treatment (filled symbols). Note a severalfold increasein the number of FG-positive neurons in BDNF-treated animals comparedwith the animals without treatment (p < 0.01; t test). 160× magnification.Scale bar, 100 µm.
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DISCUSSION
In the present study, we have shown that uninjured and axotomized RSNs express mRNA for the full-length trkB receptor. TrkAmRNA expression was not detected in the intact red nucleus, althoughlike p75 it was expressed in a few cells after axotomy at thecervical level of the spinal cord. Full-length trkC, includingisoforms bearing amino acid inserts in the kinase domain, wereexpressed at only very low levels in intact or axotomized RSNs.In accordance with the observed pattern of receptor expression,infusion of the TrkB ligands BDNF or NT-4/5 during the secondweek after spinal cord transection fully prevented the atrophyof axotomized RSNs, which remained chromatolytic. Moreover thisinfusion also maintained the axotomy-induced increase in GAP-43and T $alpha$ 1-tubulin mRNA expression. In contrast, NGF and NT-3 treatmentwere without effect. In a subsequent experiment, BDNF treatmentproduced a severalfold increase in the number of axotomized RSNsregenerating into peripheral nerve grafts implanted into the cervicaltransection site. Taken together, these findings support the hypothesisthat neuronal atrophy and the concomitant failure of injured cellsto maintain expression of regeneration-associated genes are importantfactors that limit the regenerative capacity of axotomized CNSneurons. Furthermore, these effects of axotomy can be attenuatedby application of appropriate trophic factors, thereby enhancingthe capacity of the injured cell to sustain regrowth of its axon.

Interestingly, the prevention of reduction in cell size after axotomy by BDNF and NT-4/5 did not include a normalization ofthe neuronal morphology, which remained chromatolytic. Becausethe cell size could be maintained by the application of trophicfactors, we feel justified to use the term atrophy, which impliesthe lack of some trophic support. It is difficult to evaluatethe persisting chromatolytic response after neurotrophin application.Various degrees of chromatolysis are seen in both regeneratingand nonregenerating neurons, as well as within the same neuronalphenotypes (for review, see Lieberman, 1971; Goldstein et al.,1987). Thus, the significance of a chromatolytic response forthe regenerative success of a neuron is incompletely understood,and we therefore focused on the more prominent representativesof regeneration-associated genes.

Receptor expression and effects of neurotrophins on atrophy
The expression of neurotrophin receptors in uninjured RSNs is reminiscent of spinal cord and brainstem motoneurons, whichalso predominantly express full-length trkB receptors (Koliatsoset al., 1994; Piehl et al., 1994; Kobayashi et al., 1996). However,RSNs and lower motoneurons respond differently to injury. Axotomyproduces an increase in trkB expression as well as de novo expressionof the p75 neurotrophin receptor in motoneurons (Piehl et al.,1994; Kobayashi et al.,1996). In contrast, trkB expression decreasedin axotomized RSNs, and p75 expression became detectable in onlya small number of cells. The decline in trkB mRNA expression wasprevented in axotomized RSNs by BDNF infusion (data not shown),suggesting that RSNs remain responsive to BDNF and NT-4/5, whichwas consistent with the observed prevention of their axotomy-inducedatrophy.

The effect of NT-3 on the atrophy of axotomized RSNs did not reach statistical significance. This is reminiscent of the moderateeffect of NT-3 in contrast to BDNF on survival of axotomized facialmotoneurons of newborn rats (Sendtner et al., 1992; Koliatsoset al., 1993; Yan et al., 1993). Moreover, NT-3 application toaxotomized motoneurons of adult rats has little effect on cellsize (Fernandes et al., 1995; Tuszynski et al., 1996). We areconfident that this marginal effect of NT-3 is not attributableto technical deficiencies, because immunostainings for NT-3 demonstratedgood penetration of this factor through the relevant tissue. Inaddition, in parallel experiments infusions of NT-3 fully preventthe axotomy-induced cell death of adult corticospinal neurons(Giehl and Tetzlaff, 1996). In this context, it is important tonote that trkC isoforms with insertions in the kinase domain arelimited in their downstream signaling capacities (Tsoulfas etal., 1993, 1996; Guiton et al., 1995). In contrast to RSNs, corticospinalneurons express high levels of full length trkC, and the noninsertedisoform is predominant (N. R. Kobayashi and W. Tetzlaff, unpublishedobservation). Therefore, the marginal effect of NT-3 on axotomizedRSNs may be attributable not only to the lower level of expressionof full length trkC but also to coexpression at comparable levelsof isoforms carrying amino acid insertions in their kinase domains.Although in the present study, axotomized RSNs in the adult ratdid not appear to be responsive to NT-3, axotomized RSNs are rescuedfrom cell death by application of exogenous NT-3 in newborn rats(Diener and Bregman, 1994). Presently, it is unknown whether thisdifference might be attributable to developmental differencesin the pattern of trkC expression in RSNs. It should also be notedthat axotomized corticospinal neurons rescued by application ofNT-3 remain atrophic, in contrast to those rescued by treatmentwith BDNF (Giehl and Tetzlaff, 1996). Therefore, it is possiblethat NT-3 may be a survival factor for RSNs, even in adulthood,but may not influence cell size. This also implies that differentsignaling pathways are activated by stimulation of the TrkB andTrkC receptors, even when they are expressed contemporaneouslyin the same cell.

Effect of the neurotrophins on regeneration-associated gene expression
We show here that BDNF and NT-4/5 but not NGF, NT-3, or vehicle maintained the increased levels of GAP-43 and T $alpha$ 1-tubulinmRNA expression in axotomized RSNs. This differential responsivenessto the neurotrophins is consistent with the pattern of trk receptorexpression. In essence, the expression of full-length trkB receptorswould provide means for a direct stimulation of RSNs by BDNF orNT-4/5. Likewise, BDNF has been reported to stimulate GAP-43 andT $alpha$ 1-tubulin expression in axotomized facial motoneurons that expresstrkB (Fernandes et al., 1995), and NGF regulates the expressionof these same genes in neurons of the PNS that express trkA (Vergeet al., 1990; Miller et al., 1994; Mohiuddin et al., 1995). Furthermore,BDNF stimulates the expression of GAP-43, but not T $alpha$ 1-tubulin,in axotomized retinal ganglion cells (Fournier et al., 1997).Thus, regulation of regeneration-associated genes by BDNF is context-dependentand distinct in different neuronal systems.

We do not know, however, how directly the expression of GAP-43 and T $alpha$ 1-tubulin is controlled by BDNF- or NT-4/5-activatedsignaling pathways. We cannot rule out the possibility that theneurotrophins indirectly maintain the expression of these genesvia a pleiotrophic effect. Interestingly, we found that BDNF hadno effect on the baseline expression of GAP-43 in uninjured RSNs(N. R. Kobayashi and W. Tetzlaff, unpublished observation); thus,although GAP-43 mRNA expression can be maintained by BDNF, itsinduction appears to require additional signals associated withaxotomy. In contrast, BDNF infusion increased T $alpha$ 1-tubulin expressionin intact RSNs (N. R. Kobayashi and W. Tetzlaff, unpublished observation)as well as in axotomized RSNs, indicating that GAP-43 and T $alpha$ 1-tubulinare not strictly co-regulated.

The differential regulation of GAP-43 and T $alpha$ 1-tubulin is further evidenced by the varying effects of NT-3 on these two genesin axotomized corticospinal neurons (Giehl et al., 1995), retinalganglion cells (Kittlerova et al., 1996), and dorsal root ganglioncells (Mohiuddin et al., 1995; Gratto and Verge, 1996). Differentialresponses of these neuronal types to axotomy and distinct modesand doses of applied NT-3 may be partly responsible for thesediverse outcomes. In addition, as discussed above, both the absoluteand relative levels of trkC isoforms carrying insertions in thetyrosine kinase domain may differ in these models, contributingto the apparent discrepancies. Moreover, although NT-3 binds mostavidly to trkC, it can also bind to trkA or trkB, so that differentsignaling cascades may be activated by NT-3 on cells expressingdistinct complements of trk receptors (Davies et al., 1995; Rydenand Ibanez, 1996). Further complexity is added by emerging evidencethat the different neurotrophins may elicit distinct downstreamresponses, even if their actions are mediated through the samecognate receptor (Belliveau et al., 1997). These data underlinethe necessity for analyzing the specific effects of the differentneurotrophins in each neuronal system of interest, rather thanrelying on inference.

Neurotrophins and CNS regeneration
Several studies have demonstrated that local application of neurotrophins can enhance regenerative sprouting of various CNSaxons (Schnell et al., 1994; Tuszynski et al., 1994; Xu et al.,1995; Oudega and Hagg, 1996; Ye and Houle, 1997). In these experimentalparadigms, neurotrophins are applied to the vicinity of the axonsand may exert local trophic and/or tropic effects. This standsin contrast to the model introduced here in which applicationof neurotrophins to the parent cell bodies enhances their regenerativepropensity even after injury at greater distances. We hypothesizethat this effect is mediated through the stimulation of regeneration-associatedgenes. T $alpha$ 1-tubulin and GAP-43 are highly expressed during axonaloutgrowth in development and are re-expressed in regeneratingPNS neurons (Skene and Willard, 1981; Miller et al., 1987, 1989;Skene, 1989; Tetzlaff et al., 1989). Increased tubulin expressionafter axotomy is believed to play a role in the replacement ofthe lost axoskeleton (for review, see Bisby and Tetzlaff, 1992).GAP-43 is concentrated at the axonal growth cone where it seemsto play an important role in the transduction of growth cone guidancesignals (for review, see Benowitz and Routtenberg, 1997). In vitro,GAP-43 conveys on neurons a greater propensity to grow (Aignerand Caroni, 1995). This is consistent with the close correlationbetween GAP-43 expression and successful regeneration of CNS neuronsinto peripheral nerve transplants (Doster et al., 1991; Campbellet al., 1992; Schaden et al., 1994; Tetzlaff et al., 1994; Vaudanoet al., 1995). Ordinarily, only a very small fraction of axotomizedRSNs typically regenerate into nerve grafts (Richardson et al.,1984; Houle, 1991). This appears to be attributable to the abortiveexpression of regeneration-associated genes and the concomitantatrophy of these cells. We show here that the stimulation of GAP-43and T $alpha$ 1-tubulin expression by application of BDNF is correlatedwith an increased number of RSNs regenerating into peripheralnerve implants. It remains to be shown whether the stimulationof GAP-43 and T $alpha$ 1-tubulin expression alone is sufficient to inducethis regenerative response, or whether other growth-associatedproteins, e.g., CAP-23 (Widmer and Caroni, 1990) or microtubule-associatedproteins (Fawcett et al., 1994; Nothias et al., 1995), might playa cooperative role in this process (Caroni et al., 1995). In anyevent, the present study supports the concept that the applicationof a specific neurotrophin to the vicinity of an axotomized CNSneuron can stimulate the expression of regeneration-associatedgenes and enhance its propensity to regenerate.

FOOTNOTES

Received April 24, 1997; revised Sept. 17, 1997; accepted Sept. 25, 1997.

This study was supported by an operating grant from the Medical Research Council of Canada and the Neuroscience Network ofCanada to W.T. N.R.K. is a recipient of the Government of CanadaStudentship Award, supplemented by the Neuroscience Network ofCanada. K.M.G. was supported by a Canadian Neuroscience Networkfellowship. W.T. is a recipient of the Rick Hansen Man in MotionChair in Spinal Cord Research. BDNF, NT-3, NT-4/5, and the NT-4/5antibody were kindly provided by Regeneron Pharmaceuticals Inc.(Tarrytown, NY). We thank Dr. Eugene Johnson (University of Washington,St. Louis, MO) for providing the NGF antibody and Dr. James Miller(Amgen, Thousand Oaks, CA) for providing NGF and the antibodiesto BDNF and NT-3.

Correspondence should be addressed to Dr. Wolfram Tetzlaff, Department of Zoology, University of British Columbia, 6270 UniversityBoulevard, Vancouver, British Columbia, Canada V6T 1Z4.

Dr. Giehl's present address: Department of Anatomy, University of Saarland, D66421 Homburg, Germany.

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