Retrograde Regulation of Growth-Associated Gene Expression in Adult Rat Purkinje Cells by Myelin-Associated Neurite Growth Inhibitory Proteins

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The Journal of Neuroscience, October 1, 1998, 18(19):7912-7929

Retrograde Regulation of Growth-Associated Gene Expression in Adult Rat Purkinje Cells by Myelin-Associated Neurite Growth Inhibitory Proteins
Marta Zagrebelsky¹, Annalisa Buffo¹, Arne Skerra³, Martin E. Schwab², Piergiorgio Strata¹, and Ferdinando Rossi¹
¹ Department of Neuroscience, University of Turin, I-10125 Turin, Italy, ² Brain Research Institute, University of Zurich, CH-8057 Zurich, Switzerland, and ³ Institute of Biochemistry, Technische Hochschule, Darmstadt, D-64289 Germany

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Axon regeneration requires that injured neurons reinitiate long-distance growth and upregulate specific genes. To addressthe question of whether inhibitory environmental cues along theaxon could exert a negative, tonic downregulation of growth-associatedgenes, we have examined adult rat Purkinje cells, which are endowedwith poor regenerative capabilities. First we have compared theirresponse to axotomy with that of neurons of the inferior olive,lateral reticular nucleus, and deep cerebellar nuclei, all ofwhich vigorously regenerate into growth-permissive transplants.These injured neurons upregulate the transcription factors c-Junand JunD, GAP-43, and NADPH diaphorase. In contrast, most axotomizedPurkinje cells fail to express any of these markers, showing thatthe strength of this response parallels the regenerative potentialof the examined neuron populations. However, strong upregulationof the same genes can be induced in Purkinje cells after colchicineinjection into the uninjured adult cerebellum, indicating thattheir expression could be controlled by retrograde signals. Toassess whether myelin-associated neurite growth inhibitory proteinscontribute to this regulation, we applied the neutralizing antibodiesIN-1 against one of the main inhibitory components of centralmyelin (NI-250) either in vivo or in vitro to organotypic cerebellarcultures. Application of IN-1 antibodies induces the upregulationof c-Jun, JunD, and NADPH diaphorase in Purkinje cells, showingthat their expression is suppressed constitutively by myelin-associatedneurite growth inhibitors. Thus, the inhibitory activity of theIN-1 antigen on axon growth is not restricted to the control ofgrowth cone motility but also involves a retrograde regulationof gene expression in adult central neurons.

Key words: axotomy; immediate early genes; growth-associated proteins; axon regeneration; intrinsic determinants; cerebellum; colchicine

  INTRODUCTION

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Axon regeneration depends on the availability of favorable environmental conditions and on the capability of injured neuronsto express a specific repertoire of growth-associated genes (Skene,1989; Fawcett, 1992; Schwab and Bartholdi, 1996). The strengthof the cell body reaction to axotomy differs among distinct neuronpopulations and correlates with their regenerative potential (Lieberman,1971; Barron, 1989; Herdegen et al., 1993, 1997), indicating thateach neuron class is endowed with peculiar regenerative properties.Nevertheless, within each neuron population the intensity andduration of this response depend on lesion conditions such asthe distance from the soma (Doster et al., 1991; Hüll and Bähr,1994a; Tetzlaff et al., 1994), the presence of uninjured collateralbranches (Leah et al., 1993), and the sectioned axon branch, aswith dorsal root ganglion neurons (Chong et al., 1991; Jenkinset al., 1993; Smith and Skene, 1997). In addition, the expressionof growth-associated genes in injured neurons can be sustainedby growth-permissive transplants (Hüll and Bähr, 1994b; Robinson,1995; Vaudano et al., 1995; Chong et al., 1996; Broude et al.,1997) or the application of neurotrophins (Kobayashi et al., 1997).These observations indicate that the reaction to injury is notdetermined exclusively by intrinsic properties of the affectedneurons, but it is influenced by environmental signals.

The nature of these signals and the mechanisms of this regulation remain to be elucidated. It has been proposed that the expressionof growth-associated genes is suppressed in adult neurons by retrogradeinhibitory cues (Skene, 1989, 1992). In the peripheral nervoussystem these signals are thought to derive from targets (Goldet al., 1993; Wu et al., 1993; Verzè et al., 1996; Smith andSkene, 1997). In the CNS, however, the reaction to injury canbe weak or absent even after complete target loss, whereas thelength of the axon stump can play a major role, suggesting thatfactors acting along the axon contribute to the regulation ofgrowth-associated gene expression (Kalil and Skene, 1986; Dosteret al., 1991; Skene, 1992). The myelin-associated neurite growthinhibitory proteins NI-35 and NI-250 (Caroni and Schwab, 1988a)are interesting candidate molecules for this function. Most invitro assays of these proteins have focused on their inhibitoryaction on growth cone motility (Schwab et al., 1993; Bandtlowet al., 1996). However, their appearance during development parallelsthe downregulation of GAP-43 (Caroni and Schwab, 1989; Kapfhammerand Schwab, 1994a), and they also control the intracellular distributionof this protein in the adult (Kapfhammer and Schwab, 1994a,b).In addition, their neutralization allows for axonal regenerationand enhances plasticity in the adult brain (Schwab and Bartholdi,1996; Thallmair et al., 1998; Z'Graggen et al., 1998).

To test the hypothesis that myelin-associated neurite growth inhibitors also could regulate the expression of regeneration-associatedgenes in central neurons, we have examined adult Purkinje cells,which show poor regenerative capabilities even in the presenceof growth-permissive conditions (Rossi et al., 1995; Bravin etal., 1997; Dusart et al., 1997). We first compared Purkinje cellresponse to axotomy with that of other cerebellar or precerebellarneurons endowed with robust regenerative capabilities, and wefound that the regenerative properties of these neuron populationsparallel the strength of their reaction to injury. Then, by blockingaxon flow, we asked whether injury-associated gene expressionin Purkinje cells is inhibited via retrograde signals. Finally,to determine whether this retrograde control is mediated by myelin-associatedneurite growth inhibitors, we applied recombinant neutralizingIN-1 antibody Fab fragments to the cerebellum.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animals and surgical procedures. All of the experiments were performed on adult Wistar rats (Charles River, Calco, Italy)deeply anesthetized by means of intraperitoneal administrationof a mixture of ketamine (100 mg/kg, Ketalar, Bayer, Leverkusen,Germany) and xylazine (5 mg/kg; Rompun, Bayer). The experimentalplan was designed according to the Italian law for care and useof experimental animals (DL116/92) and approved by the ItalianMinistry of Health.

We have studied the reaction to axotomy of four different cerebellar and precerebellar neuron populations (inferior olivaryneurons, lateral reticular nucleus neurons, deep cerebellar nucleineurons, and Purkinje cells) for which the axons were transectedeither in the cerebellar white matter (Dusart and Sotelo, 1994;Rossi et al., 1995) or in the cerebellar peduncles (Buffo et al.,1998). By the latter approach axons from the inferior olive andlateral reticular nucleus as well as the cerebellofugal projectionfrom the deep nuclei are severed. By contrast, lesions of thecerebellar white matter affect Purkinje cell axons and the afferentprojections to the cortex from the cerebellar and precerebellarnuclei. In this condition, however, olivocerebellar and mossyfiber pathways are affected only partially, and the axotomy ismade far away from the cell body.

Cerebellar lesions were obtained according to a previously described method, which allows for the transection of the axialwhite matter of several cerebellar lobules (Dusart and Sotelo,1994; Rossi et al., 1995). Briefly, the posterior surface of thecerebellum was exposed by drilling a hole in the occipital bone,and a microknife, made of a piece of a razor blade, was introducedinto the cerebellar parenchyma and moved horizontally from theright to the left side of the vermis. Then the wound was sutured,and each animal was returned to its cage. A total of 14 animalswho underwent this injury procedure and were killed at survivaltimes ranging from 1 d to 1 month after the lesion (see Table1)were considered in this study. In addition, in another set ofanimals solid specimens of embryonic cerebellum (n = 8) or neocortex(n = 5) were transplanted into the lesion track immediately afterthe surgical transection (Table 1). The preparation of the embryonictissue and the grafting procedures were performed as previouslydescribed (Rossi et al., 1995; Bravin et al., 1997). Briefly,under general anesthesia, caesarean incisions were performed onpregnant rats, the embryos were collected in 0.12 M phosphatebuffer (PB) with 0.6% glucose, and the embryos were decapitated.The cerebellar primordium [from embryonic day 14 (E14) embryos]or neocortical tissue (from E17 embryos) was reduced in morselsand then pressure-injected into the lesion cavity, using a glassmicropipette connected to a Hamilton syringe.


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Table 1. Number of animals examined for the in vivo experiments

The unilateral transection of the cerebellar peduncles was performed on 29 rats (Table 1). In these animals the atlanto-occipitalmembrane was exposed and excised, and the cerebellar pedunclesof one side was cut by inserting a microknife into the fourthventricle underneath the cerebellum. These animals belong to anexperimental set described in a previous study to which it canbe referred for details about the surgical procedures and theevaluation of lesion extent (Buffo et al., 1998).

The Purkinje cell axonal transport was blocked in vivo by injecting a colchicine solution into the cerebellar parenchyma ofuninjured rats. These animals were placed on a stereotaxic frame,the occipital bone was exposed, and a hole was drilled in thesuperior aspect to expose the cerebellar vermis. A total of 4µg of either colchicine (n = 17, Table 1) or $beta$ -lumicolchicine,as a control (n = 4, Table 1), diluted in 1 µl of saline solutionwas pressure-injected 1 mm deep within the cerebellar parenchymaaround the midline at the level of lobule VI. As an additionalcontrol, 1 µl of saline solution (n = 6, Table 1) was injectedaccording to the same method. The injection was performed by meansof a glass micropipette connected to a PV800 Pneumatic Picopump(World Precision Instruments, New Haven, CT). The frequency andduration of pressure pulses were adjusted to inject 1 µl of thesolution during ~10 min. Then, the pipette was left in situ foran additional 5 min to avoid an excessive leakage of the injectedsolution on the cerebellar surface.

In 19 intact rats (Table 1) a recombinant Fab fragment of the IN-1 antibody (produced in Escherichia coli), which neutralizesmyelin-associated neurite growth inhibitory proteins (Bandtlowet al., 1996), was injected into the cerebellar parenchyma. Inthis case three 1 µl injections of Fab fragments in saline solution(5 mg/ml) were made 1 mm deep around the cerebellar midline alongthe anterior-posterior axis. The injections were made by meansof a glass micropipette connected to a PV800 Pneumatic Picopump(World Precision Instruments). As a control an affinity-purifiedF(ab')₂ fragment mouse anti-human IgG (Jackson ImmunoResearch,West Grove, PA) was injected (n = 6, Table 1) by using the sameprocedure. In an additional set of animals (n = 7) the injectionof Fab fragment solution was associated with the surgical transectionof the cerebellar white matter (as above), which was performedduring the same surgical session. Finally, five intact animalswere examined as untreated controls.

Organotypic cerebellar cultures. Slice cultures were prepared according to the procedure described by Dusart et al. (1997).In our study postnatal day 10 Wistar rats (Charles River) wereanesthetized deeply by means of an intraperitoneal injection ofa mixture of ketamine (100 mg/kg, Ketalar, Bayer) and xylazine(5 mg/kg, Rompun, Bayer) and transcardially perfused with 5 mlof 0.12 M PB, pH 7.2-7.4, with 0.6% glucose to remove blood. Thenthe brains were dissected and placed into the same buffer, andthe meninges were removed carefully. Cerebellar parasagittal slices,400 µm thick, were cut with a McIlwain tissue chopper and separatedin 0.12 M PB containing glucose. The slices then were culturedon the membrane of a 30 mm Millipore culture insert (Millicell,Millipore, Bedford, MA; pore size, 0.4 µm) in 10 cm culture dishescontaining 3 ml of a culture medium composed of 50% basal mediumwith Earle's salts (Life Technologies, Gaithersburg, MD), 2.5%HBSS (Life Technologies), 25% horse serum (Life Technologies),22.5% water, 1 mM L-glutamine (Life Technologies), 200 U/ml penicillin/streptomycin(Life Technologies), and 5 mg/ml glucose. The cultures were keptat 37°C in a humidified atmosphere with 5% CO₂. After 1 week inculture the concentration of horse serum was lowered to 15%.

All of the slices were kept for 7 d in culture before any manipulation. To cut Purkinje cell axons, we transected a set ofslices (n = 27) by means of an ultramicrotomy glass knife undera dissecting microscope, according to a previously described approach(Dusart et al., 1997). Afterward, such injured slices were keptin culture for an additional period of time ranging from 48 hrto 4 d. To block axon flow, we placed some millicells containingcerebellar slices (n = 51) in a culture medium added with colchicine(4 ng/ml) for 15 min. Then they were removed, carefully rinsed,and incubated with the normal culture medium for another 18-24hr before being processed.

Another set of cerebellar slices, kept for 7 d in culture as previously described, were incubated with a culture medium suppliedwith hybridoma cells secreting either IN-1 antibodies (n = 116)or control anti-horseradish peroxidase (HRP; n = 107) antibodies(Caroni and Schwab, 1988b). Hybridoma cells were grown in Iscove'smodified Dulbecco's medium supplemented with 6% fetal calf serum(Life Technologies), 2 mM L-glutamine (Life Technologies), 100U/ml penicillin/streptomycin (Life Technologies), and 50 µM $beta$ -mercaptoethanol(Life Technologies) at 37°C in 5% CO₂ humidified atmosphere (seeCaroni and Schwab, 1988b). The cells were counted, spun down,and resuspended in the medium used for slice culture at a concentrationof 1 × 10⁶ cells/ml of medium. The slices were cultivated in this conditionedmedium for a period from 24 hr to 4 d. In a separate experimentsome cerebellar slices (n = 10) were incubated for 1-4 d withthe recombinant Fab fragment of the IN-1 antibody (Bandtlow etal., 1996) diluted 1:10 in the slice culture medium. Finally,another set of cultures (n = 75), which remained in vitro forthe same period of time, was processed and examined as untreatedcontrols.

Histological procedures. At different postsurgery survival times under deep general anesthesia (as above), the rats were perfusedtranscardially with 1 l of 4% paraformaldehyde in 0.12 M PB, pH7.2-7.4. The brains were dissected immediately, stored overnightin the same fixative at 4°C, and finally transferred in a 30%sucrose in 0.12 M PB at 4°C until they sank. The cerebella werecut by means of a freezing microtome in several series of 30-µm-thicksagittal sections. Subsequently, one series of sections was processedfor NADPH diaphorase histochemistry. These sections were incubatedfor 3-4 hr in darkness at 37°C in a solution composed of 1 mg/ml $beta$ -NADPH (Sigma, St. Louis, MO) and 0.2 mg/ml nitroblue tetrazolium(Sigma) in 0.12 M PB with 0.25% Triton X-100. All of the otherseries were incubated first in H₂O₂ 0.3% in PBS to neutralizeendogenous peroxidase. They were incubated for 30 min at roomtemperature and then overnight at 4°C in the different primaryantibodies: anti-calbindin D-28K (monoclonal, 1:5000; Swant, Bellinzona,Switzerland) to visualize Purkinje cells; anti-B-50/GAP-43 (rabbitimmunoglobulins, 1:7000; gift of Dr. A. B. Oestreicher, RudolfMagnus Institute, Utrecht, The Netherlands); anti-CAP-23 (polyclonal,1:700; gift of Dr. P. Caroni, F. Miescher Institute, Basel, Switzerland);anti-c-Jun (polyclonal, 1:1000; Santa Cruz Biotechnology, SantaCruz, CA); anti-junD (polyclonal, 1:8000; gift of Dr. R. Bravo,Myers Squibb Pharmaceutical Research Center, Princeton, NJ); andanti-c-Jun phosphorylated form (ser 63 and 73) (P-Jun, polyclonal,1:10,000; New England Biolabs, Beverly, MA). All of the antibodieswere diluted in PBS with 0.25% Triton X-100 added either withnormal horse serum or normal goat serum, depending on the speciesof the second antibody. Immunohistochemical staining was performedaccording to the avidin-biotin-peroxidase method (Vectastain,ABC Elite kit, Vector Laboratories, Burlingame, CA) and was revealedby using 3,3' diaminobenzidine (0.03% in Tris-HCl) as a chromogen.For c-Jun, JunD, and P-Jun the reaction was intensified by adding0.04% nickel ammonium sulfate to the diaminobenzidine solution.The reacted sections were mounted on chrome-alum gelatinized slides,air-dried, dehydrated, and coverslipped.

The organotypic cerebellar slides were fixed overnight at 4°C in 4% paraformaldehyde in 0.12 M PB, pH 7.2-7.4, and were detachedcarefully from the Millicell membrane before being processed forimmunocytochemistry. All of the slices were double-stained byanti-c-Jun (polyclonal, 1:1000; Santa Cruz Biotechnology) andanti-calbindin antibodies (monoclonal, 1:3000; Swant). Both ofthe incubations in primary antibodies were performed at 4°C overnight.The c-Jun staining was revealed according to the avidin-biotin-peroxidasemethod (Vectastain, ABC Elite kit; Vector), using 3,3' diaminobenzidine(0.03% in Tris-HCl) as a chromogen. Then the same slices wereincubated in anti-calbindin, which was revealed via fluoresceinisothiocyanate (FITC) immunofluorescence. Finally, the sliceswere mounted on chrome-alum gelatinized slides in PBS-glyceroland were coverslipped.

GAP-43 in situ hybridization. In situ hybridization histochemistry to reveal GAP-43 mRNA was performed on two intact and nineexperimental rats killed 7 d after the different lesion/injectionprocedures described above (cerebellar lesion, n = 3; peduncletransection, n = 2; colchicine injection, n = 2; IN-1 Fab application,n = 2). The rats were decapitated and brains were removed quicklyby dissection. Tissue blocks were covered with Tissue-Tek embeddingmedium (Miles, Elkhart, IN) and rapidly frozen at $-$ 40°C in 2-methyl-butane.The frozen tissue was stored at $-$ 80°C for at least 24 hr and upto several weeks. Sections 15 µm thick were cut on a cryostat,collected on Superfrost slides, and air-dried at room temperaturefor ~30 min. Then the sections were fixed in 4% paraformaldehyde(freshly prepared in 0.1 M PBS and stirred for 1 hr at 70°C todissolve) for 10 min, washed in PBS, and permeabilized for 10min in PBS with 0.1% Triton X-100. Next the sections were acetylatedby a 10 min incubation in a solution made of 250 ml of autoclaveddistilled water with 3.5 ml of triethanolamine (Sigma) and 625µl of acetic anhydride (Sigma) added dropwise. Prehybridizationwas performed at room temperature in a humid chamber in 500 µlof the hybridization buffer (50% formamide, 5× SSC, and 2% blockingreagent; Boehringer Mannheim, Mannheim, Germany). The hybridizationmixture was prepared by adding 50 ng/ml of a full-length digoxigenated(DIG) riboprobe synthesized from GAP-43 containing plasmid (akind gift of Dr P. Caroni, F. Miescher Institute, Basel, Switzerland)(Kapfhammer et al., 1997) that was heated first for 5 min at 85°Cto denature the probe and then chilled on ice. Hybridization mixturewas spread over the sections and coverslipped to maintain theconcentration of formamide and salts. The hybridization was doneovernight at 68°C in a hybridization mixture humidified chamber.Slides were washed by placing them vertically in a rack immersedin 5× SSC, and the coverslips were allowed to slide off. Stringencywashing was performed in 0.2× SSC at 68°C for 60 min. For theimmunological detection of DIG-labeled hybrids the slides wereincubated for 1 hr at room temperature in 1% blocking reagentmade in maleic acid, incubated for 1 hr in anti-DIG antibody (BoehringerMannheim) diluted 1:5000 in 1% blocking reagent, and finally washedtwice for 30 min in maleic acid. To perform the color reaction,we incubated the slides with 2.4 mg of levamisole (Sigma), 45µl of 4-nitroblue tetrazolium (Sigma), and 35 µl of 5-bromo-4-chloro-3-indolyl-phosphate(Sigma) diluted in 10 ml of a buffer made of (in M) 0.1 Trizmabase, 0.1 NaCl, and 0.005 MgCl, pH 9.5. The color reaction wasdeveloped in the dark for 1-24 hr and stopped when the desiredintensity was reached. Sections were mounted immediately in aglycerol solution made in PBS, and the coverslips were sealedwith nail polish.

Quantitative analysis. Quantitative estimations of reactive Purkinje cells in the different in vivo experiments were madeby estimating the neurons labeled by c-Jun antibodies or NADPHdiaphorase histochemistry. For each treated animal three sectionslabeled for either marker were chosen according to the followingcriterion: only vermal sections close to the cerebellar midline,which contained the surgical injury track or the injection site(in the case of drug or antibody applications) were considered.Cell counts made on nine calbindin-immunolabeled vermal sectionsfrom three intact animals showed that each section contained onthe average of 2061 ± 116 (SD) Purkinje cells. The selected sectionsfrom treated animals were reproduced by the Neurolucida software(Microbrightfield, Colchester, VT) connected with an E-800 Nikonmicroscope, and the position of every single labeled cell wasmarked carefully (see Figs. 3, 5, and 8 for several examples ofsuch sections). Then the number of labeled cells present in thethree reproduced sections was averaged to calculate the valuefor every single animal, which was represented individually inthe plots of Figures 3, 5, and 8.

For in vitro experiments the number of c-Jun-immunolabeled Purkinje cells was estimated on nonaxotomized cerebellar slicestreated for 1-4 d with hybridoma cells secreting IN-1 antibodies(n = 13), hybridoma cells secreting anti-HRP antibodies (n = 13),IN-1 Fab fragment (n = 10), or no treatment (n = 11). The analyzedcultures were selected randomly from parallel experimental runs,which were performed and processed simultaneously, to minimizedifferences caused by culture or histological processing. On eachselected culture the total number of Purkinje cells, visualizedby anti-calbindin immunofluorescence, was counted directly atthe light microscope. The number of Purkinje cells displayinganti-c-Jun-labeled nuclei was estimated simultaneously. The identificationof such double-labeled Purkinje cells was checked carefully byfrequently shifting from immunofluorescence to bright-field microscopy.The value calculated from each slice was represented individuallyin the plot of Figure 6 as the percentage of double-labeled Purkinjecells over the total number counted in the same culture. Statisticalanalysis was performed by Student's t test.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The response to axotomy of adult Purkinje cells and other cerebellar or precerebellar neurons parallels their different regenerative capabilities

The different cerebellar axon populations are peculiar for their different regenerative properties. Olivocerebellar (Rossiet al., 1995; Bravin et al., 1997) and mossy fiber axons (Munzet al., 1985; Armengol et al., 1989) vigorously regenerate intogrowth-permissive grafts. Also, the axons from deep nuclear neuronscan elongate into peripheral nerve implants (Dooley and Aguayo,1982). In contrast, in the same experimental conditions adultPurkinje cell neurites are never able to grow (Dooley and Aguayo,1982; Rossi et al., 1995; Bravin et al., 1997; Buffo et al., 1997;Dusart et al., 1997). Thus, we first asked whether such differentregenerative capabilities also are paralleled by differences inthe response to axotomy of these neuron populations. To this aimwe examined the cellular changes occurring in injured Purkinjecells, deep cerebellar nuclei, lateral reticular nucleus, andinferior olive (see also Buffo et al., 1998) after unilateraltransections of the cerebellar peduncles or lesions of the cerebellarwhite matter. In these injured neurons we investigated the expressionof several well known injury-associated markers, including theimmediate early genes c-Jun, JunD, and the phosphorylated formof c-Jun (P-Jun; Herdegen and Zimmermann, 1994; Herdegen et al.,1997; Yang et al., 1997), the growth-associated protein GAP-43(Doster et al., 1991; Schaden et al., 1994; Tetzlaff et al., 1994),and the activity of NADPH diaphorase, which is known to be relatedto nitric oxide synthase (Herdegen et al., 1995). The base levelof expression of these markers in intact animals was consistentwith previous reports: no immunolabeling for immediate early genes(Herdegen et al., 1995) or NADPH diaphorase histochemistry (Saxonand Beitz, 1994, 1996) was observed in the examined neuron populations.Similarly, no GAP-43 mRNA could be detected in Purkinje cells,whereas in the deep cerebellar and lateral reticular nucleus onlya few faintly labeled neurons were seen occasionally. By contrast,inferior olivary neurons throughout the whole extent of the nuclearcomplex displayed a clear constitutive expression (Kruger et al.,1993; Console-Bram et al., 1996). However, no GAP-43-immunolabeledcell bodies were ever encountered in any of these nuclei.

A consistent response to axotomy was observed in the lateral reticular nucleus, deep cerebellar nuclei, and inferior olive(see also Buffo et al., 1998); after the unilateral transectionof the cerebellar peduncles, numerous neurons in these nucleibecame reactive for all of the examined markers (representativeresults from the lateral reticular nucleus are shown in Fig. 1a-d).Immediate early gene expression started from the very first daysafter injury (Fig. 1a,b), and GAP-43 and NADPH diaphorase activityincreased during the second half of the first week (Fig. 1c,d).These changes were maintained substantially for the whole examinedperiod, up to 1 month after lesion.

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Figure 1. a-l, Response to axotomy of cerebellar and precerebellar neurons. The plate illustrates the expression of injury-associated markers in the lateral reticular nucleus (LRN, a-d) after unilateral transections of the cerebellar peduncles and in the deep cerebellar nuclei (DCN, e-h) and inferior olive (IO, i-l; dotted line indicates midline) after surgical injuries of the cerebellar white matter. The response to axotomy in these nuclei is consistent: numerous injured neurones become immunoreactive for c-Jun (a, e, i), for JunD (b, f, j), and for NADPH diaphorase histochemistry (NADPHd, c, g, k) within all three nuclei. In addition, GAP-43 mRNA upregulation in these nuclei is revealed by in situ hybridization histochemistry (GAP-43, d, h, l). Arrowheads in l point to inferior olivary neurons displaying a labeling intensity clearly above the basal level. Survival times, 7 d. Scale bar, 50 µm.

A similar response pattern and time course were observed after lesions in the cerebellar white matter. Numerous reactive neuronsfor all of the markers were present in the deep cerebellar nuclei(Fig. 1e-h). In addition, some neurons showing upregulation ofimmediate early genes, GAP-43, and NADPH diaphorase were foundconsistently in the medial regions of the inferior olive (Fig.1i-l), which are known to project to the posterior vermal cortex(Voogd et al., 1985) where the lesion was made. The limited numberof reactive nerve cells found in the latter nucleus is consistentwith the facts that only part of the olivocerebellar axons actuallywere touched by these lesions, the affected nerve cells were injuredfar from the cell body, and the collateral branches directed tothe deep cerebellar nuclei likely were spared. Thus, these cerebellarand precerebellar neuron populations respond to axotomy by expressingthe same repertoire of markers that also are upregulated in otherbrain regions (Doster et al., 1991; Herdegen and Zimmermann, 1994;Schaden et al., 1994; Tetztlaff et al., 1994). This indicatesthat the reaction to axotomy involves the expression of a stereotypedset of genes common to most nerve cells.

When Purkinje cells were examined in the same animals, completely different results were obtained: most of the Purkinje cellsdid not show any detectable c-Jun (Fig. 2a), P-Jun, and JunD expression(Fig. 2b). The only exception was a few neurons localized in theclose proximity of the injury (Figs. 2a,b, 3). Quantitative estimationof c-Jun-positive Purkinje cells (plot in Fig. 3) showed thatthe average number of reactive neurons per section never exceededa few dozen cells of 2061 (± 116 SD) Purkinje cells that wereestimated on similar sections from intact cerebella, and the numbertended to decrease over time. A similar result was obtained byNADPH diaphorase histochemistry (see Fig. 2c): reactive Purkinjecells were restricted to the immediate vicinity of the lesionand first appeared 3 d after lesion. Their number increased duringthe following days, but they never exceeded a few dozen labeledneurons per section (plot in Fig. 3) (see also Chen and Aston-Jones,1994; Saxon and Beitz, 1994, 1996). Consistent with previous resultsin the mouse (Buffo et al., 1997), we never observed GAP-43-immunoreactivePurkinje cell bodies or axons along the axial white matter ofthe transected folia, nor could we detect any GAP-43 mRNA expressionin these axotomized neurons (see Fig. 2e). However, a few Purkinjecells in the vicinity of the lesion became immunoreactive forCAP-23 (see Fig. 2d), a protein that shares some functional homologywith GAP-43 (Caroni, 1997). Thus, despite the large transections,which are known to induce the axotomy of virtually all Purkinjecells in the affected lobuli (Dusart and Sotelo, 1994; Rossi etal., 1995), only a few of these neurons, located close to theinjury, reacted by expressing the cellular markers that are widelyexpressed by the other cerebellar or precerebellar neurons. Hence,the very poor regenerative behavior of Purkinje cells is paralleledby an inability to upregulate growth-associated genes in responseto injury.

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Figure 2. a-g, Response to axotomy of Purkinje cells. Micrographs a-d show the expression of c-Jun (a), JunD (b), CAP-23 (d), and NADPH diaphorase histochemistry (c) in Purkinje cells after cerebellar lesions. Note that for all of these markers only a few labeled Purkinje cells (arrowheads in a-d) are present and that they are always localized in the proximity of the injury track (dotted line in a-e), whereas more distant Purkinje cells for which the axons also have been transected are nonreactive. In situ hybridization histochemistry that is used to reveal GAP-43 mRNA is shown in e; the granular layer as well as interneurons in the molecular layer are stained, whereas no labeled Purkinje cells can be seen (dotted line points to lesion site). Similar results are obtained when embryonic cerebellar or neocortical grafts are placed into the lesion site (f, g display c-Jun immunolabeling and NADPH diaphorase histochemistry, respectively). Also, in these cases the few labeled neurons (arrowheads in f, g) are localized exclusively in the close vicinity of the lesion track, which now corresponds to the host-graft interface (marked by the dotted line in f, g). Survival times: 1 d in a, b; 7 d in e-g; 14 d in d; 30 d in c. Scale bars: 50 µm in b, d, f; 100 µm in a, c, e, g.

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Figure 3. Spatial distribution and quantitative evaluation of c-Jun and NADPH diaphorase-positive Purkinje cells after axotomy. Neurolucida reconstructions of representative cerebellar sections labeled by c-Jun antibodies or NADPH diaphorase histochemistry at different survival times after lesion are shown. Note that reactive Purkinje cells (indicated by black dots) invariably are localized in the vicinity of the lesion track (dotted line). Only the portion of the section distal to the lesion is represented at 1 and 3 d survival times, because in these short-term cases the two halves of the sections separated during the histological procedures. The average number of labeled neurons per section is shown in the plots at the bottom of the plate. Each point represents the value obtained from a single animal. c-Jun-labeled neurons (left plot) are already present 1 d after injury, and their number gradually decreases thereafter. By contrast, NADPH diaphorase-reactive Purkinje cells (right plot) first appear at 3 d and progressively increase in number during the following weeks. Note, however, that in both instances only a very small number of Purkinje cells are present in each section.

The expression of growth-associated genes can be enhanced in different neuron populations by the presence of growth-permissive/promotingtissues, such as peripheral nerve implants or embryonic grafts(Hüll and Bähr, 1994b; Robinson, 1995; Vaudano et al., 1995;Chong et al., 1996; Broude et al., 1997). Hence, we asked whetherthe expression of axotomy-associated genes in Purkinje cells couldbe enhanced by embryonic neural transplants. The grafts of E14cerebellum or E17 neocortex placed into the injury track filledthe lesion cavity being directly apposed to the transected folia.However, despite the proximity of the embryonic tissue, the patternof marker expression in the injured Purkinje cells did not change(see Fig. 2f-g); only sparse neurons were reactive, and they werealways located close to the injury site, now represented by thehost-graft interface. This inability of the grafted tissues toinduce or enhance the expression of growth-associated genes inPurkinje cells is consistent with the well established notionthat such transplants cannot induce adult Purkinje axon growtheither in vivo (Rossi et al., 1995; Bravin et al., 1997; Buffoet al., 1997) or in vitro (Dusart et al., 1997). In conclusion,the results of these experiments show that Purkinje cells do notupregulate growth-associated genes in response to axon injuryas the other cerebellar or precerebellar neurons do, and thiscellular behavior parallels the poor regenerative capability displayedby this nerve cell population even when confronted with growth-permissiveenvironmental conditions.

The expression of axotomy-associated genes can be induced in Purkinje cells by blocking axonal flow

The observation that at least a few Purkinje cells display a cell body response after axotomy indicates that they are notintrinsically unable to express the injury-associated genes. Rather,the consistent localization of such reactive neurons in the closeproximity of the injury site suggests that the distance from thelesion, and possibly the length of the axon stump, is a crucialparameter to determine whether they will respond or not. To elucidatethis point further, we examined c-Jun expression of Purkinje cellsafter axotomy in organotypic slice cultures in which the relationbetween the cell body reaction and the length of the axon stumpcan be assessed directly. These experiments, described below,clearly showed that the only reactive Purkinje cells were thoseundergoing a very proximal injury, which left a short axon stump(see Fig. 6a,b). Thus, the response of Purkinje cells to injuryis conditioned by the length of the remaining axon segment, indicatingthat their expression of growth-associated genes is inhibitedby retrogradely transported signals.

To test this hypothesis, we blocked axonal transport with colchicine. Colchicine injection into the intact cerebellum in vivoinduced a strong expression of c-Jun (Fig. 4b), P-Jun (Fig. 4d),and JunD (Fig. 4c) in numerous Purkinje cells distributed throughoutseveral lobules around the injection site (Fig. 5). Quantitativeestimation of c-Jun expression showed that several hundreds ofreactive Purkinje cells per section were present from the veryfirst days after lesion (Fig. 5). This expression was maintainedfor several weeks, and values returned to control levels after2 months. Colchicine application also induced a strong NADPH diaphorasereactivity (see Fig. 4e,f) and CAP-23 immunolabeling (see Fig.4g,h) in the same cerebellar lobuli. In contrast, Purkinje cellsdid not show GAP-43 immunostaining or GAP-43 mRNA upregulation(data not shown). The appearance of CAP-23 expression and NADPHreactivity was delayed with respect to the immediate early genesbut was well evident at 7 and 14 d (Fig. 5). At 2 months afterinjection, NADPH diaphorase-reactive cells were absent from threeof the four examined animals, although one of them still displayedsparse labeled cells. CAP-23-immunoreactive neurons (see Fig.4g,h) were consistently present between 1 and 2 weeks after injury,although their number was always far fewer than that of neuronslabeled for the other markers. As a control experiment we injected $beta$ -lumicolchicine, which did not induce any expression of the examinedmarkers in Purkinje cells except for a few neurons located aroundthe injection cannula track (Fig. 5). Similarly, upregulationof immediate early genes, NADPH diaphorase, and GAP-43 also wasobserved in the examined cerebellar and precerebellar nuclei afterapplication of colchicine, but not of $beta$ -lumicolchicine (data notshown).

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Figure 4. a-h, Response of Purkinje cells after intracerebellar injections of colchicine. Micrograph a shows the morphological alterations of anti-calbindin-immunolabeled Purkinje cells, which mostly involve the formation of axonal torpedoes (arrowheads). Starting from the very first days after injection, numerous Purkinje cells (arrowheads in b-d) show a strong nuclear staining for c-Jun (b), P-Jun (d), and JunD (c) immediate early genes. In addition, c-Jun expression is increased in granule cells (b). A survey picture of a cerebellar section labeled for NADPH diaphorase histochemistry 14 d after colchicine injection is shown in e. The arrow points to the area of cortical atrophy around the injection site. Note, however, (Figure legend continues) that numerous labeled Purkinje cells are present over several cerebellar lobules. The morphology and labeling intensity of these reactive neurons are better appreciated in the higher magnification picture f. g, h show anti-CAP-23-immunolabeled Purkinje cells 7 d after colchicine application. Purkinje cell somata, dendrites, and axons (arrowhead in g) are decorated by the immunoreaction product. Survival times: 2 d in a-d; 7 d in g, h; 14 d in e, f. Scale bars: 20 µm in g, h; 50 µm in a, d, f; 100 µm in b, c; 200 µm in e.

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Figure 5. Spatial distribution and quantitative evaluation of c-Jun and NADPH diaphorase-positive Purkinje cells after colchicine or $beta$ -lumicolchicine applications. Neurolucida reconstructions of representative cerebellar sections labeled by c-Jun antibodies or NADPH diaphorase histochemistry at different survival times after injection are shown. After $beta$ -lumicolchicine injections only rare Purkinje cells (black dots) localized around the injection site become reactive for either marker. In contrast, numerous labeled Purkinje cells distributed over several cerebellar lobules are present in the colchicine-treated cerebella. Note the similar distribution of reactive neurons for either marker in the corresponding sections. (Figure legend continues)The average number of labeled neurons per section is reported in the plots on the bottom right corner of the plate. Each point represents the value obtained from a single animal. Several hundreds of c-Jun-labeled neurons (top plot) are already present 2 d after injection, and this number essentially is maintained during the first weeks after injection. A considerable number of NADPH diaphorase-reactive neurons (bottom plot) can be found from 7 d after the injection onward. However, their number is constantly lower than that of c-Jun-positive Purkinje cells. At 60 d after injection, the number of reactive neurons for either marker is again at control level. Note the very small number of labeled neurons counted in the $beta$ -lumicolchicine-treated cerebella (indicated by filled triangles in the plots).

As previously reported (Pioro and Cuello, 1988), colchicine treatment induced structural abnormalities in Purkinje cell axons,mostly involving the appearance of torpedoes (see Fig. 4a). Inaddition, because of its well established neurotoxic effect (Goldschmidtand Steward, 1982) an area of cortical atrophy and neuronal degenerationwas evident around the injection site (Fig. 4e). However, thisarea was much smaller than the area in which marker expressionwas induced. Indeed, the distribution of reactive Purkinje cellsin the treated cerebella was consistent with a diffusion of colchicinealong the axial white matter of several cerebellar lobuli aroundthe injection site (Fig. 5). In addition, the comparison of thecerebella from animals killed at different survival times clearlyshowed that, although the effects of colchicine application onPurkinje cells (i.e., alterations of axonal morphology and geneexpression) persisted for several weeks, in most of the affectedcortical regions they were fully reversible and not associatedwith neuronal death (Fig. 5).

In conclusion, most of the markers that are expressed by cerebellar or precerebellar neurons after axon injury can be inducedin Purkinje cells by colchicine treatment. The comparison withthe application of $beta$ -lumicolchicine, which shares some of thebiological actions of colchicine but is not able to depolymerizemicrotubules (Dasheff and Ramirez, 1985), indicates that thiseffect of colchicine may be attributed to the blockade of theaxonal transport of retrograde signals that regulate gene expressionin Purkinje cells. The Purkinje cell axon is myelinated startingat 40-50 µm from the cell body, and the myelin sheath also coversall of the thin recurrent collateral ramifications (Palay andChan-Palay, 1974). Thus, myelin-associated factors may be candidatemolecules to regulate Purkinje cell gene expression.

The application of IN-1 antibodies on organotypic cerebellar cultures induces c-Jun expression in Purkinje cells

To test the hypothesis that myelin-associated neurite growth inhibitors regulate gene expression in Purkinje cells, we firstexamined organotypic cerebellar cultures. The cerebellar sliceswere dissected from P10 animals and kept in vitro for 7 d beforeexperimental manipulations were started. In intact cultures thatremained 7-11 d in vitro, c-Jun was expressed only in 4% (± 1.9SD; Fig. 6i) of Purkinje cells, randomly scattered throughoutthe slice. When a cut was made across the slice, some c-Jun-labeledneurons consistently appeared along the edge of the lesion track.All of these reactive neurons underwent very proximal axotomies,which only spared a few hundred micrometer long axon stumps (Fig.6a,b). Furthermore, a 15 min addition of colchicine to the culturemedium of intact slices induced a strong immunoreactivity in Purkinjeand granule cells all over the slice (Fig. 6c). Thus, in linewith a previous report (Dusart et al., 1997), these in vitro experimentsfaithfully reproduced the results obtained on adult Purkinje cellsin vivo.

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Figure 6. a-i, c-Jun expression in Purkinje cells in organotypic cerebellar cultures. c-Jun expression in axotomized Purkinje cells in vitro is shown in a (anti-calbindin immunofluorescence) and b (anti-c-Jun immunoperoxidase labeling). Two Purkinje cells (small arrows in a) localized close to the injury site (dotted line in a, b) display c-Jun-immunoreactive nuclei (arrowheads in b); these cells are characterized by short axon stumps that measure a few hundred micrometers long. Another Purkinje cell (large arrow in a) displaying a longer axon stump does not express c-Jun (Figure legend continues)(arrow in b points to the position of this cell). Micrograph c shows a cerebellar culture treated for 15 min with colchicine and fixed 24 hr later; note the strong nuclear labeling in Purkinje cells (large nuclei) and granule cells (small nuclei). Micrographs d-g show the double-immunolabeling pattern of two slices cultured for 2 d in the presence of hybridoma cells secreting anti-HRP (d, e) or anti-IN-1 (f, g) antibodies. In the anti-HRP-treated culture only a few Purkinje cells display dimly c-Jun-immunolabeled nuclei (arrowheads in e), whereas the IN-1-treated slice displays numerous strongly stained Purkinje cell nuclei (arrowheads in g point to some). No granule cell labeling is evident in these cultures. Note also that this antibody treatment does not induce any overt morphological change in Purkinje cells and, especially, in their axons (d, f). A survey picture of another slice incubated for 1 d with the Fab fragment of the IN-1 antibody is shown in h; arrowheads point to the numerous labeled Purkinje cell nuclei aligned along the granular-molecular layer interface. The percentage of c-Jun-positive Purkinje cells over the whole population is plotted in i; every point in the graph represents the value obtained from a single slice. Only a few labeled cells are found in untreated cultures (control), whereas a higher number is present in the anti-HRP-treated slices (HRP). However, a much larger number of labeled cells is present in the cultures treated with IN-1-secreting hybridoma cells (IN-1) or IN-1 Fab fragments (Fab). Scale bars: 20 µm in b; 50 µm in c, e, g; 100 µm in h.

We then examined the effect of neutralizing antibodies against myelin-associated neurite growth inhibitors. After 7 d in vitro,hybridoma cells secreting the IN-1 antibody, or an anti-HRP antibodyas a control, were added to the culture medium in parallel setsof uninjured slices. The treated cultures contained the same numberof Purkinje cells as the untreated ones (no treatment: 502 ± 166SD, n = 11; IN-1 hybridoma: 537.1 ± 229.1 SD, n = 13; HRP hybridoma:644 ± 338.2 SD, n = 13; IN-1 Fab fragment: 463.1 ± 139 SD, n =10). In addition, Purkinje cells did not show any visible morphologicalalteration that could be attributed to cell damage or degeneration(Fig. 6f).

The application of anti-HRP antibody led to a slight increase of c-Jun-labeled Purkinje cell nuclei (14.7% ± 7.7 SD; Fig.6d,e,i), which was statistically different from untreated cultures(4% ± 1.9 SD; Student's t test, p < 0.0001). Interestingly, inthe IN-1-treated cultures numerous c-Jun-positive Purkinje cellnuclei were distributed rather uniformly over the whole slice(Fig. 6f,g). No clear granule cell labeling was observed (Fig.6g). Quantitation of c-Jun-positive Purkinje cells showed thatIN-1 treatment induced the expression of this gene in 49.8% (±9.2 SD, Fig. 6i) of Purkinje cells. This value was very differentfrom that obtained from anti-HRP treated cultures (Student's ttest, p < 0.0001), thus showing that the application of the IN-1antibody was effective in inducing c-Jun expression in Purkinjecells. To validate this result further, we added the recombinantFab fragment of the IN-1 antibody to the medium in another setof slices (Fig. 6h). The result of this experiment showed that63% (± 8 SD; Fig. 6i) of Purkinje cells expressed c-Jun. Thisnumber was statistically different from that obtained from IN-1hybridoma-treated cultures (Student's t test, p = 0.001). Thisdifference may be attributed to the fact that the smaller-sizedFab fragments more easily penetrate into the slice than the hybridoma-secretedIgM. Thus, c-Jun expression is induced in Purkinje cells in vitroby the application of neutralizing antibodies against the myelin-associatedneurite growth inhibitors, indicating that these proteins areinvolved in the regulation of growth-associated genes in Purkinjecells.

Injection of the Fab fragment of the IN-1 antibody induces the expression of axotomy-associated genes in Purkinje cells in vivo

To assess whether myelin-associated neurite growth inhibitors regulate Purkinje cell gene expression in vivo, we injectedthe Fab fragment of the IN-1 antibody, or a mouse anti-human IgGFab fragment as a control, into the intact adult cerebellum. Injectionof the control Fab fragment, like that of saline solution, inducedthe expression of the different markers in only a few Purkinjecells located around the cannula track (see Fig. 8). In contrast,the application of IN-1 Fab fragments induced a strong expressionof several markers in large cerebellar areas (Figs. 7a-e, 8).Immediate early gene expression already was evident in numerouscells at 2 d, the shortest survival time that was examined (Fig.7a-d). As shown in Figures 7a and 8, labeled Purkinje cells weredistributed over large areas of the cerebellum around the injectionsite. Most interestingly, no labeling was observed in granulecells, except for a few neurons exclusively localized in the closeproximity of the cannula track, for which the axons most likelyhad been injured during the penetration of the injection pipette(Fig. 7a). Similarly, the expression in other cortical interneuronsdid not exceed basal levels.

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Figure 7. a-g, In vivo response of Purkinje cells to intracerebellar injections of the Fab fragment of the IN-1 antibody. The injection of the Fab fragment of the IN-1 antibody induces a strong expression of several markers in Purkinje cells. Immediate early genes are upregulated already at 48 hr after the injection in several cerebellar lobuli all around the injection site. a, b, c-Jun expression is shown. Positive Purkinje cells are distributed over several cerebellar lobules (arrowheads in a). Note that granule cell labeling is restricted to a small area along the cannula track (marked by the arrow in a) where granule cell axons most likely have been injured by the injection pipette. Similarly, numerous Purkinje cell nuclei are stained by anti-P-Jun (c) and anti-JunD (d) antibodies. Micrograph e shows NADPH diaphorase-reactive Purkinje cells 5 d after injection. Anti-calbindin (Figure legend continues)immunostaining (f) shows the normal morphological features of Purkinje cells in such treated cerebella. A transected cerebellar lobule (dotted line points to the lesion track) that also received the Fab fragment injection is shown in g; arrowheads point to the numerous c-Jun-immunoreactive Purkinje cell nuclei, which also are located distantly from the lesion. Survival times: 2 d in a-d, g; 5 d in e, f. Scale bars: 20 µm in d, e; 50 µm in b, c, f; 100 µm in a, g.

At 5 d after the injection, numerous Purkinje cells still expressed the immediate early genes (see Fig. 8 for c-Jun distributionand quantification). In addition, at this survival time the Purkinjecells, distributed over the same areas as the other markers, becamestrongly reactive for NADPH diaphorase histochemistry (Figs. 7e,8). The number of such reactive neurons was variable among theexamined animals. A high number of positive Purkinje cells (~100per section) were present in the two animals with the highestnumber of c-Jun-positive cells. In the other cases only a fewtens of Purkinje cells were observed, but they were always morenumerous than those in time-matched controls (Fig. 8). Finally,at 7 d the number of labeled Purkinje cells for all of the examinedmarkers returned almost to control levels (Fig. 8), indicatingthat the single Fab injections exerted a transitory effect, whichfaded within 1 week after application. No labeling for GAP-43or CAP-23 was observed in Purkinje cells during this period. Itis worth mentioning also in these in vivo experiments that theanalysis of anti-calbindin-immunolabeled cerebella at all survivaltimes did not show signs of regressive or dystrophic changes inPurkinje cells or in their axons (see Fig. 7f).

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Figure 8. Spatial distribution and quantitative evaluation of c-Jun and NADPH diaphorase-positive Purkinje cells after the application of the Fab fragment of the IN-1 antibody or of the mouse-anti-human control Fab fragment. Neurolucida reconstructions of representative cerebellar sections labeled by c-Jun antibodies or NADPH diaphorase histochemistry at different survival times after injection are shown. After mouse-anti-human control Fab fragment injections (control Fab), only a few Purkinje cells (black dots) that are localized around the injection site become reactive for either marker. By contrast, numerous labeled Purkinje cells distributed over several cerebellar lobules are present in the IN-1 Fab (Figure legend continues)fragment-treated (IN-1 Fab) cerebella. Note the similar distribution of reactive neurons for either marker in the corresponding sections. The average number of labeled neurons per section is reported in the plots on the right side of the plate. Each point represents the value obtained from a single animal. A large number of c-Jun-labeled neurons (top plot) are present 2 d after injection. Their number gradually decreases thereafter and returns almost to basal levels at 7 d. NADPH diaphorase-reactive Purkinje cells (bottom plot) are evident at 5 d; two animals have ~100 cell per sections, whereas the others show a smaller number of labeled cells. Also, in this case the number of reactive neurons is close to control values at 7 d. Note, however, that both the control Fab (filled squares) or saline injections (filled triangles) yielded only a small number of labeled cells per section, which was consistently lower than that counted in time-matched IN-1 Fab fragment-treated cerebella.

Finally, to test whether the neutralization of myelin-associated neurite growth inhibitors also affected gene expression inaxotomized Purkinje cells, the IN-1 Fab fragment was injectedinto the transected lobuli of injured cerebella. The results ofthese experiments were essentially similar to those from injectionsinto intact cerebella: numerous Purkinje cells distributed overthe whole transected folia and also far away from the lesion site(see Fig. 7g) were immunoreactive for the immediate early geneswithin 2 d after the lesion/injection procedure; NADPH diaphorasereactivity appeared a few days later. Again, these markers disappearedat 7 d.

In conclusion, these results show that the expression of several axotomy-associated genes in Purkinje cells can be inducedin vivo when the activity of 250 kDa myelin-associated neuritegrowth inhibitor is neutralized by the Fab fragment of the specificblocking antibody IN-1. Thus, these molecules effectively regulatethe expression of these genes in intact and injured Purkinje cells.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

We have studied the expression and regulation of injury-associated markers in adult Purkinje cells to assess whether theirpoor regenerative capabilities can be related to a weak cell bodyreaction to axotomy. Then we asked whether this lack of reactivitydepends on intrinsic features of these neurons or is determinedby environmental influences. We show that (1) different neuronpopulations respond to injury by expressing a common set of markers,including several immediate early genes, GAP-43, CAP-23, and NADPHdiaphorase reactivity; (2) the strength of this response parallelsthe regenerative capabilities of the different neuron types, beingmost weak or absent in Purkinje cells; (3) however, Purkinje cellsupregulate these genes when their axonal flow is blocked or whenthe axotomy occurs very close to the perikaryon, indicating thattheir expression is controlled by retrogradely transported signals;and (4) a similar upregulation is induced by applying IN-1 antibodiesthat neutralize myelin-associated neurite growth inhibitory proteins.Thus, the expression of injury or growth-associated genes in Purkinjecells is prevented constitutively by the latter proteins, andthis inhibition likely accounts, at least in part, for the weakregenerative response of Purkinje cell bodies and the constantfailure of these neurons to regenerate their axons (Rossi et al.,1995; Bravin et al., 1997; Buffo et al., 1997; Dusart et al.,1997).

The cell body reaction and its relation to axon regeneration

Axon regeneration requires that the injured neurons undergo specific metabolic changes (Lieberman, 1971; Barron, 1989), andseveral genes expressed during this response recently have beenidentified (Doster et al., 1991; Herdegen and Zimmermann, 1994;Schaden et al., 1994; Tetzlaff et al., 1994; Caroni, 1997; Herdegenet al., 1997). The cellular changes as well as the repertoireof molecules induced after axotomy are similar in most neuronpopulations. However, the intensity of this response differs amongdistinct nerve cell categories and also according to injury conditions,usually being correlated to the regenerative potential shown bythe affected neurons when confronted with a growth-permissivemilieu (Doster et al., 1991; Jenkins et al., 1993; Schaden etal., 1994; Tetzlaff et al., 1994). Observations made in this studyfor the cerebellar and precerebellar neurons confirm these concepts:the pattern of axotomy-induced gene expression in these neuronsis similar to that shown by other neuron populations except forthe lack of GAP-43 upregulation in Purkinje cells. However, thelatter neurons do not express GAP-43 during development (Console-Bramet al., 1996), and this protein might be substituted by the relatedprotein CAP-23 (Caroni, 1997), which could be induced in our experiments.Thus, the cell body reaction to axotomy involves the upregulationof a stereotyped gene set common to most nerve cells, includingthe examined cerebellar and precerebellar neurons.

It has been proposed that adult neurons respond to injury by suppressing genes involved in signal processing, typical of theirmature phenotype, and upregulating growth-associated genes, characteristicof developmental processes (Hökfelt et al., 1994). However, despitethe relationship existing between the expression of injury-inducedgenes and regenerative phenomena, to date their precise role inaxon growth is still unclear, if not controversial, because manyof them also have been related to cell death processes (Herdegenet al., 1997; Isenmann and Bähr, 1997). On the other hand, neurondegeneration and axon growth share, at least in part, common cellularpathways (Herdegen et al., 1997). Hence, pharmacological blockof c-Jun kinase-1 in primary neurons prevents apoptosis but alsoinhibits axon growth (Markus et al., 1997). Overexpression ofthe bcl-2 gene prevents axotomy-induced degeneration (Bonfantiet al., 1996; Cenni et al., 1996) and enhances the regenerativecapacity of retinal ganglion cells (Chen et al., 1997). MousePurkinje cells that overexpress GAP-43 show enhanced growth capabilities,together with a reduced resistance to axotomy-induced cell death(Buffo et al., 1997). These observations indicate that the cellbody response to axon injury may result in very different outcomesranging from cell death to regeneration. However, it is clearthat it is required to initiate axon growth; hence, the associatedcellular changes can be taken as a reliable index of the regenerativepotential of a neuron.

Environmental control of growth-associated gene expression in adult neurons

The constitutive capability for axon growth gradually declines as neurons mature (Skene, 1989, 1992); coincidentally, theirregenerative potential is reduced also (Woodhams et al., 1993;Chen et al., 1995; Dusart et al., 1997). This phenomenon may beattributable either to intrinsic modifications associated withthe acquisition of the adult neuronal phenotype (Bates and Meyer,1997) or to the progressive appearance of growth inhibitory signalsor the disappearance of growth-promoting factors (Kalil and Skene,1986; Skene, 1989, 1992).

After axotomy, adult neurons often react by attempting to reexpress the growth-associated gene program. This response, however,may not be induced by injury per se but, rather, by the consequentremoval of retrograde inhibitory signals. In the peripheral nervoussystem such signals are derived primarily from peripheral targets(Baizer and Fishman, 1987; Skene, 1989, 1992). Indeed, growth-associatedgenes can be upregulated in the absence of injury by target loss(Verzé et al., 1996) or block of the axon flow (Wu et al., 1993).Furthermore, the response to a distal axotomy is delayed but isnot weaker than that induced by a proximal injury (Kenney andKocsis, 1998), suggesting that influences acting along the axondo not contribute significantly to this regulation. In the CNS,in contrast, complete target deprivation is not necessarily followedby a cell body reaction (Skene, 1989). However, the strength ofthis response depends on the distance between the injury and thecell body. The observation that retinal ganglion cells react equallywell to an intraorbital optic nerve transection, irrespectiveof their distance from the optic disk, indicates that the crucialfactor is not the actual distance of axon injury from the somabut, rather, the length of the remaining myelinated axon segment(Doster et al., 1991; Meyer et al., 1994). Thus, it has been proposedthat growth-associated gene expression in the adult CNS is regulatedby cues produced by non-neuronal elements present along maturewhite matter tracts (Skene, 1989, 1992; Doster et al., 1991; Meyeret al., 1994). The intimate nature of these cues has remainedelusive up to date.

The behavior of adult Purkinje cells described here is fully consistent with these concepts: they react only to very proximalinjuries, and a vigorous response can be elicited by blockingaxonal flow. Interestingly, we found that injury-associated geneexpression also can be induced by applying neutralizing antibodiesagainst myelin-associated neurite growth inhibitory proteins inthe absence of any lesion. The mechanism of action of the antibodyas well as its actual ability to penetrate between myelin andaxon to disrupt their interaction remains to be established. However,the specificity of this effect is supported by the observationthat the neutralizing antibodies do not induce a similar responsein granule cells or cortical interneurons in which the axons areunmyelinated (Palay and Chan-Palay, 1974). Thus, our results stronglysupport the conclusion that myelin-associated neurite growth inhibitoryproteins are among the signaling molecules exerting a retrogradenegative control on growth-associated gene expression in adultcentral neurons.

The discovery of NI-35 and NI-250 proteins has led to the notion that constitutive growth inhibitory mechanisms are activein the adult mammalian brain. The role of these proteins in preventingaxon regeneration or sprouting after injury has been establishedin numerous experimental conditions (Schwab et al., 1993; Schwaband Bartholdi, 1996). As to their constitutive function in theintact brain, it has been proposed that the myelin-associatedneurite growth inhibitory proteins could stabilize mature centralfiber tracts and prevent adult axon sprouting, thus contributingto the maintenance of specific connections (Schwab et al., 1993;Colello and Schwab, 1994; Thallmair et al., 1998; Z'Graggen etal., 1998). This concept is supported by their time course ofexpression during development (Caroni and Schwab, 1989), theirreciprocal distribution with GAP-43 (Kapfhammer and Schwab, 1994a,b),and the effects of their neutralization in developing uninjuredwhite matter tracts (Schwab and Schnell, 1991). The present resultsprovide evidence for a new additional function of these proteins:the active suppression of growth-associated gene expression. Thus,they may contribute to the developmental regulation of the axongrowth program and, thereafter, may maintain adult neurons inthe mature "nongrowing" condition by inhibiting growth cone motilityand regulating gene expression.

After injury in the adult brain the amount of NI-35 and NI-250 protein remaining along the axon stump proximal to the lesioninfluences the strength of the reaction of the affected neurons.As a consequence, the specific regenerative capabilities of eachneuron population do not depend solely on its intrinsic potentialto express the growth-associated program but also on its degreeof sensitivity to these environmental influences. Indeed, thereare neuron populations with myelinated axons, such as inferiorolivary neurons, that constitutively express growth-associatedgenes and are able to react and regenerate even after a distalaxotomy. Thus, understanding the molecular mechanisms responsiblefor these interactions will be of major importance to improvesubstantially the reparative processes in the adult brain.

  FOOTNOTES

Received May 27, 1998; revised July 6, 1998; accepted July 13, 1998.

This work was supported by grants from Ministero dell'Università della Ricerca Scientifica e Tecnologica, Consiglio Nazionaledelle Ricerche, and European Community Biotechnology Programme(ERBBIO4-CT96-0774). We are grateful to Drs. Pico Caroni, AnneB. Oestreicher, and Rodrigo Bravo for the kind gift of differentantibodies and mRNA probes. We thank Mrs. Luisella Milano fortechnical help and Miss Graziella Milano for secretarial assistance.
M.Z. and A.B. contributed equally to this paper.

Correspondence should be addressed to Dr. Ferdinando Rossi, Department of Neuroscience, University of Turin, Corso Raffaello30, I-10125 Turin, Italy.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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