Rho Signaling Pathway Targeted to Promote Spinal Cord Repair

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The Journal of Neuroscience, August 1, 2002, 22(15):6570-6577

Rho Signaling Pathway Targeted to Promote Spinal Cord Repair
Pauline Dergham¹, Benjamin Ellezam¹, Charles Essagian¹, Hovsep Avedissian², William D. Lubell², and Lisa McKerracher¹
Départements de ¹ Pathologie et Biologie Cellulaire and ² Chimie, Université de Montréal, Montréal, Québec, H3T 1J4, Canada

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The Rho signaling pathway regulates the cytoskeleton and motility and plays an important role in neuronal growth inhibition.Here we demonstrate that inactivation of Rho or its downstreamtarget Rho-associated kinase (ROK) stimulated neurite growth inprimary cells of cortical neurons plated on myelin or chondroitinsulfate proteoglycan substrates. Furthermore, treatment eitherwith C3 transferase (C3) to inactivate Rho or with Y27632 to inhibitROK was sufficient to stimulate axon regeneration and recoveryof hindlimb function after spinal cord injury (SCI) in adult mice.Injured mice were treated with a single injection of Rho or Rho-associatedkinase inhibitors delivered in a protein adhesive at the lesionsite. Treated animals showed long-distance regeneration of anterogradelylabeled corticospinal axons and increased levels of GAP-43 mRNAin the motor cortex. Behaviorally, inactivation of Rho pathwayinduced rapid recovery of locomotion and progressive recuperationof forelimb-hindlimb coordination. These findings provide evidencethat the Rho signaling pathway is a potential target for therapeuticinterventions after spinal cordinjury.

Key words: Rho GTPase; Rho-associated kinase; C3; Y27632; corticospinal tract; regeneration; BBB behavior scale; GAP-43; mouse

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mammalian neurons do not regenerate successfully after lesion. This is explained in part by myelin-derived inhibition (Caroniand Schwab, 1988; McKerracher et al., 1994; Mukhopadhyay et al.,1994; Chen et al., 2000) and the formation of a glial scar expressinginhibitory molecules (Snow et al., 1990; McKeon et al., 1991;Asher et al., 2000). However, numerous studies in animal modelsusing methods designed to overcome the effect of growth inhibitoryproteins have confirmed the regenerative potential of the injuredspinal cord. These methods include the use of antibodies (Schnelland Schwab, 1990; Huang et al., 1999), peripheral nerve grafts(Cheng et al., 1996), transplantation of cells into the lesionsite (Howland et al., 1995; Rapalino et al., 1998; Liu et al.,1999; McDonald et al., 1999; Ramon-Cueto et al., 2000) and limitingthe formation of the glial scar (Davies et al., 1999; Moon etal., 2000).

The failure of regeneration in the adult CNS may also be caused by changes occurring in mature neurons (Li et al., 1995, 1996;Shen et al., 1999; Cai et al., 2001). Another approach to stimulateregeneration has been to target neurite growth signaling. Forexample, different neurotrophin treatments have increased theability of neurons in adult CNS to regenerate and stimulate bothaxonal growth and sprouting after injury (Schnell et al., 1994;Sawai et al., 1996; Blesch and Tuszynski, 1997; Weidner et al.,1999; Coumans et al., 2001). Neurotrophins are known to delayapoptosis, prevent atrophy of axotomized neurons, and enhancethe expression of growth-associated genes (Fournier et al., 1997;Kobayashi et al., 1997; Bregman et al., 1998; Broude et al., 1999).Recent data suggest that neurotrophins might stimulate regenerationby increasing neuronal cAMP levels to overcome inhibitory signaling(Cai et al., 1999). Therefore, the decreased ability of the matureCNS to regenerate after injury may result from both the intrinsicproperties of adult neurons and the extracellular inhibitoryenvironment.

The Rho GTPase is a key intracellular regulator of cytoskeletal dynamics and cell motility (Hall, 1998). Rho is activatedwhen growth cones collapse in response to chemorepulsive factors(Tigyi et al., 1996; Jin and Strittmatter, 1997; Kuhn et al.,1999; Wahl et al., 2000), and inhibiting Rho promotes neuriteoutgrowth in the presence of myelin (Jin and Strittmatter, 1997;Lehmann et al., 1999). Recently, Rho has been shown to regulateapoptosis (Liu et al., 2001; Trapp et al., 2001). An enzyme fromClosteridium botulinum, C3 transferase (C3), blocks Rho functionby ADP ribosylation of the effector domain (Dillon and Feig, 1995).Y27632 inhibits Rho-associated kinase (ROK), a serine-threonineprotein kinase that is activated by Rho (Ishizaki et al., 1997;Uehata et al., 1997). Inactivation of ROK with Y27632 promotesneurite outgrowth (Katoh et al., 1998; Bito et al., 2000), butit is not known whether it is sufficient to block growth inhibitionas was shown for inactivation of Rho (Lehmann et al., 1999). Inthe present study, we compare inactivation of Rho or ROK to promoteaxon growth on inhibitory substrates. We further study in fullyadult mice whether inactivation of the Rho signaling pathway promotesaxon regeneration and functional recovery after spinal cord injury(SCI). Animals treated to inactivate the Rho signaling pathwayshow significant improvement in locomotion by open field testing.Thus, inactivation of the Rho signaling pathway is an effectivemethod to improve outcome afterSCI.

  MATERIALS AND METHODS

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INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell culture. Primary cortical neurons were isolated from embryonic day (E) 15-E18 rat fetuses. The cortex was cut into smallpieces into Ca²⁺- and Mg²⁺-free HBSS, 0.3 M HEPES buffer, pH 7.3, and penicillin/streptomycin,and then dissociated with 0.25% trypsin, 0.1% DNase at 37°C for15 min. The dissociated cells were washed and diluted to 2 × 10⁵ cells per milliliter in minimal essential media (Invitrogen,Burlington, ON), N2 supplement (Invitrogen), 5% fetal bovine serum,1% ovalbumin, and 1 mM pyruvate. Cells were then triturated with25 µg/ml C3 or buffer, or with 31 or 3.1 µM Y27632. Cells wereplated in eight-well chamber slides coated with 25 µg/ml poly-L-lysineor with test substrates. Myelin substrates were made by coatingwith 8 µg purified bovine brain myelin dried overnight at roomtemperature. Chondroitin sulfate proteoglycan (CSPG) substrateswere made by incubating 0.5 µg/ml mixed CSPG solution (Chemicon,Temecula, CA) overnight in poly-L-lysine-coated chamber slides.Mixed substrate was made by coating and drying 8 µg of myelinin 150 µl of CSPG solution. The plates were fixed with 4% paraformaldehydeand 0.5% gluteraldehyde after 12, 24, or 48 hr, and neurons wereidentified by immunocytochemistry using a $beta$ III-tubulin antibody(Sigma, Oakville, ON). The longest neurite per neuron was measuredon an average of 400 cells per experiment with a minimum of threeexperiments per condition. Doses for C3 and Y27632 were chosenon the basis of previous experiments (Lehmann et al., 1999; Bitoet al., 2000; M. Winton and L. McKerracher, unpublishedobservations)

Preparation of recombinant C3 and Y27632. Recombinant C3 exoenzyme was prepared as a glutathione S-transferase-C3 fusion proteinand stored at $-$ 80°C (Lehmann et al., 1999). Y27632 was synthesizedfrom $alpha$ -methylbenzylamine and exhibited identical ¹H and ¹³C nuclear magnetic resonance spectra as reported in United StatesPatents 4,997,834 and 5,478,838. Before in vivo use, the activityof C3 and Y27632 was tested in tissue culture with retinal neuronsplated on myelin substrates (Lehmann et al., 1999).

Spinal cord injury and delivery of Rho and Rho-kinase inhibitors. BALB-c female mice (n = 70) of ~20 gm were anesthetizedwith 0.4 ml/kg hypnorm and 5 mg/kg diazepam. A segment of thethoracic spinal cord was exposed using fine rongeurs to removethe bone, and a dorsal over-hemisection was made at T7. Fine scissorswere used to cut the dorsal part of the spinal cord, which wascut a second time with a fine knife to ensure that the lesionextended past the central canal. A fibrin adhesive delivery systemwas prepared using a Tisseel VH kit (ImmunoAG, Vienna, Austria).According to manufacturer's instructions for slow polymerization,lyophilized fibrinogen was reconstituted in an aprotinin solution,thrombin was reconstituted in a calcium chloride solution, andboth solutions were warmed to 37°C. Fifty microliters of 1 mg/mlC3 or Y27632 were added to 25 µl of the thrombin solution. Thiswas mixed with 25 µl of the fibrinogen solution just before applicationto the spinal cord to allow infiltration of the mixture into thelesion site before polymerization. In some C3-treated animalsand in all Y27632-treated animals, 10 µl of the 1 mg/ml solutionwas applied to the lesion site immediately after the cord wascut. As controls, a second group of animals received fibrin adhesivewith buffer, and a third group was left untreated. C3-containingcollagen gels were formed as follows. C3 was lyophilized (40 µgper mouse) and then reconstituted in 10 µl of 7.5% NaHCO₃, andthen 25 µl of 0.7 mg/ml rat tail collagen was added. As with fibrin,10 µl of C3 was added to the lesion cavity before the C3-containingcollagen gel was applied. For retransections 3 weeks after SCI,the spinal cords were cut at T6 as described above, and the animalswere tested using the Basso-Beattie-Bresnahan (BBB) locomotorrating scale on days 1, 2, and 6 after the secondsurgery.

Anterograde labeling. Three weeks to 3 months after injury, corticospinal tract (CST) fibers were labeled by injection ofthe anterograde tracer wheat germ agglutinin-horse radish peroxidase(WGA-HRP) into the motor cortex as described (Huang et al., 1999).Two days later, the animals were perfused transcardially withsaline and then 4% paraformaldehyde, and the spinal cords andbrains were removed. Serial longitudinal cryostat sections ofthe spinal cord were cut at 30 µm, reacted for HRP (Huang et al.,1999), and counterstained with neutral red. Measurement of axonregeneration was assessed independently by two reviewers. Lesiondepth was assessed by measuring the depth of damaged tissue inthe spinal cord as a percentage of total spinal cordwidth.

In situ hybridization. GAP-43 mRNA was detected by in situ hybridization on coronal cryostat sections through the motor cortexof mice treated with PBS (n = 2) or C3 (n = 3). In situ hybridizationwas performed as described previously (Fournier et al., 1997)with an ³⁵S-labeled GAP-43 cRNA probe derived from a plasmid provided byDr. Pate Skene (Duke University Medical Center) (Basi et al.,1987). After the in situ hybridization procedure, sections wereNissl stained and bright-field and dark-field digital micrographswere taken. On the basis of Nissl staining and retrograde labelingof motor cortex by Fluorogold in previous animals, a region wascircled on bright-field micrographs to include axotomized layerV neurons. Corresponding dark-field micrographs were black andwhite inverted and thresholded in Northern Eclipse (Empix imaging,Mississauga, ON), and autoradiographic grain clusters >30 pixelsin size were counted. Background-corrected grain cluster densitieswere calculated on 4-10 sections per animal using the followingformula: [(number of counted grain clusters in circled region/areaof circled region)/(number of counted grain clusters in background/areaof background sampled].

Behavioral testing. Behavioral recovery was assessed for 1 month after SCI in an open field environment by the BBB method(Basso et al., 1995). We modified the 21 point BBB scale to a17 point score because mice do not exhibit differences in toedrag that can be monitored visually. Thus, scale points 16, 17,and 18 were removed from the scale. Mice raise their tails earlyin their recovery, and score 19 for tail up position was removed,leaving a 17 point total score. The mouse modified BBB score wasas follows: (0) no observable hindlimb (HL) movement; (1) slightmovement of one or two joints; (2) extensive movement of one jointand/or slight movement of one other joint; (3) extensive movementof two joints; (4) slight movement of all three joints of theHL; (5) slight movement of two joints and extensive movement ofthe third; (6) extensive movement of two joints and slight movementof the third; (7) extensive movement of all three joints of theHL, walking with little/no weight support; (8) extensive movementof all three joints, walking with weight support; (9) frequentto consistent dorsal stepping with weight support; (10) frequentplantar stepping with weight support; (11) consistent plantarstepping with weight support, no coordination; (12) consistentplantar stepping with consistent weight support, occasional forelimb(FL)-HL coordination; (13) consistent plantar stepping with consistentweight support, frequent FL-HL coordination; (14) consistent plantarstepping with consistent weight support, consistent FL-HL coordination;predominant paw position during locomotion is rotated internallyor externally, or consistent FL-HL coordination with occasionaldorsal stepping; (15) consistent plantar stepping with consistentweight support, consistent FL-HL coordination; predominant pawposition is parallel to the body; frequent to consistent curledtoes, trunk instability; (16) consistent plantar stepping withconsistent weight support, consistent FL-HL coordination; predominantpaw position is parallel to the body, flat toes, some trunk instability;(17) consistent plantar stepping with consistent weight support,consistent FL-HL coordination; predominant paw position is parallelto the body, flat toes and consistent stability in the locomotion.For scoring, each animal was videotaped for 3 min, and two reviewersparticipated. In the late phase of recovery, the BBB score wasdetermined from sequences of four steps or more from digitizedvideos projected on a computer screen at one-fourth speed. Detailedpatterns of front paw and foot placements were assessed, as shownin Figure 5, F and G, for untreated (n = 6) and C3-treated (n= 6)animals.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Inactivation of Rho or ROK promotes growth of primary neurons plated on complex inhibitory substrates

We tested first whether treatment of primary cortical neurons with C3 or with Y27632 was sufficient to stimulate growth oncomplex inhibitory substrates typical of the glial scar and whitematter. Neurons plated on different test substrates were examinedat 12, 24, and 48 hr, and similar results were observed at alltime points. Neurons plated on CSPG, purified myelin, or a mixtureof both did not extend long neurites and had a rounded shape (Fig.1A,B). After treatment with C3 (Fig. 1C) or Y27632 (Fig. 1D),neurons were able to extend neurites. Measurements at 24 hr showedthat treatment with either C3 or Y27632 significantly increasedthe length of neurites compared with untreated cells plated onmyelin, CSPG, or mixed myelin/CSPG substrates (Fig. 1A). Quantitationat 12 hr showed similar results (data not shown), and at 48 hrgrowth of treated neurons was too extensive to measure neuritelength. C3 was significantly better than Y27632 in promoting neuritegrowth (t test; p < 0.05). These results demonstrate that inactivationof Rho or inhibition of ROK stimulates cortical neurons to extendneurites on complex growth inhibitory substrates.

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Figure 1. Effect of Rho antagonist C3 or Rho-associated kinase inhibitor Y27632 on neurite outgrowth of primary cortical neurons plated on inhibitory substrates. A, Neurite outgrowth was analyzed quantitatively by measuring the longest neurite per cell 24 hr after plating on poly-L-lysine, myelin, CSPG, or mixed substrates and treatment with buffer (white), 25 µg/ml C3 (gray), or 31 µM Y27632 (black). Differences between treated and untreated cells were significant on all test substrates (t test; p < 0.05). B-D, Representative micrographs of cortical neurons plated on mixed inhibitory substrates either untreated (B) or treated with C3 (C) or Y27632 (D). Scale bar, 25 µm.

Treatment of injured spinal cord promotes long-distance regeneration

To assess the potential of Rho inactivation to treat SCI, we cut the spinal cord of adult mice at T7 by a dorsal over-hemisection(Huang et al., 1999). We tested C3 by local delivery either incollagen or in a fibrin adhesive that polymerizes in vivo severalseconds after injection, because both matrices have been reportedto support tissue repair (Joosten et al., 1995; Herbert et al.,1998). We used the fibrin adhesive to test Y27632 because of favorableresults with C3 (see below). Anterograde tracing with WGA-HRPof CST, a tract often used to study histological regeneration,was used to assess fiber growth in six groups of animals: animalstreated with fibrin plus C3 (n = 13), collagen plus C3 (n = 12),fibrin plus Y27632 (n = 5), fibrin alone (n = 10), collagen alone(n = 7), and SCI with no treatment (n = 13) (Fig. 3). All sectionswere counterstained with neutral red to verify that lesions extendedpast the central canal (Fig. 2I). A quantitative analysis of lesiondepth showed no significant differences between treated and controlgroups (one-way ANOVA). Without C3 or Y27632 treatment, transectedCST axons retracted back from the site of lesion by ~300 µm (Fig.2H), although in animals treated with fibrin alone some regenerativesprouts did extend from the retracted bundle (Fig. 2G). Applicationof C3 to the injured spinal cord elicited extensive sproutinginto the dorsal white matter and the lesion scar (Fig. 2A,C,E).Treated animals with Y27632 showed regenerative sprouting intothe dorsal white matter and toward the lesion site (data not shown).To assess axons distal to the lesion site, the distance of thelongest axon was measured. Axons were found up to 12 mm from thelesion site in C3-treated animals and up to 3 mm from the lesionsite in Y27632-treated animals (Fig. 3), whereas buffer-treatedanimals showed retraction from the lesion site. Therefore, aftertreatment with C3 or Y27632, axons were found to extend past thelesion into the distal white matter. These axons have a twistedcourse of growth typical of regenerated axons (Figs. 2D,F). Althoughneutral red staining showed lesions extended past the centralcanal (Fig. 2I), these experiments alone cannot rule out the possibilitythat secondary damage was reduced after injury. This could arisein the damaged CNS because C3 has neuroprotective effects (Liuet al., 2001; Trapp et al., 2001), in addition to promoting growthon inhibitory substrates (Fig. 1).

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Figure 2. Axon regeneration after SCI and treatment with C3. Shown are dark-field micrographs of spinal cord sections; rostral is to the left. A, Anterogradely labeled CST fibers in a C3-treated spinal cord 3 weeks after injury. The lesion site is between the dotted lines. B, Same section as A 12 mm caudal to the lesion site. C, Higher magnification of boxed region in A to show regenerative sprouting into lesion site and into the dorsal white matter. D, A different section from the same animal as A, showing regenerating fibers 10 mm from the lesion site. E, Anterogradely labeled CST fibers 3 months after SCI sprout into the dorsal white matter and cross the lesion site. The lesion appears as a vertical line; accumulated blood contributes to the bright appearance of the lesion. F, Same section as E taken 8 mm from the lesion site. G, Fibrin-treated control showing some sprouting of lesioned fibers, but no long-distance regeneration. H, Anterogradely labeled fibers retract from the lesion site in an untreated animal. I, Neutral red staining showing glial scar 1 month after lesion. Arrows indicate axon sprouting. Scale bars: A, B, E, G, H, 500 µm; I, 250 µm; C, D, 100 µm; F, 25 µm.

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Figure 3. Quantification of regeneration length. Longest regeneration distances after SCI alone or treatment with vehicle, Rho antagonist C3, or Rho kinase inhibitor Y27632. Each point represents one animal. The circles represent animals examined 3 weeks to 1 month after SCI; the triangles represent animals examined at 3 months. Lines indicate averages for each group. Statistical significances were evaluated with the unpaired t test: C3 + collagen versus collagen, p < 0.05; C3 + fibrin versus fibrin, p < 0.001; Y27632 + fibrin versus fibrin, p < 0.05; C3 + collagen versus C3 + fibrin, p < 0.05; C3 + fibrin versus Y27632 + fibrin, p < 0.01.

Effect of C3 on the expression of GAP-43 mRNA in the motor cortex of spinal cord injured animals

After thoracic spinal cord lesion, only axons that regenerate long distances show upregulation of GAP-43 mRNA expression (Ferandeset al., 1999). To confirm the growth response and the long-distanceregeneration after Rho inactivation, we examined the pattern ofGAP-43 mRNA expression in the motor cortex (Fig. 4A,B) of animals1 month after CST transection with or without treatment with C3.In situ hybridization using ³⁵S-labeled riboprobes on coronal brain sections revealed high levelsof GAP-43 mRNA expression in neurons of the motor cortex of C3-treatedanimals (Fig. 4D), whereas untreated animals showed GAP-43 signalsimilar to background (Fig. 4C). Quantitation of grain clusterdensities in motor cortex showed significant upregulation of GAP-43mRNA (Fig. 4E). These results indicate that C3 treatments elicitchanges in gene expression consistent with axon regeneration.

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Figure 4. Expression of GAP-43 mRNA in motor cortex. A, Photomicrograph of a cresyl violet-stained coronal section of mouse brain. Box outlines motor cortex area depicted in B-D. B, Fluorescent micrograph of same section as in A showing neurons retrogradely labeled with Fluorogold applied at the site of a dorsal hemisection at T7. C, D, Dark-field photomicrographs showing sections of motor cortex from an untreated mouse (C) or a C3/fibrin-treated mouse (D) after in situ hybridization for GAP-43. E, Quantitation showing significantly increased grain density in motor cortex after treatment with C3. Differences between C3 and background (Bkgd) were significant (t test; p < 0.05); differences between PBS and background were not significant. Scale bar: A, 1.8 mm; B, 1.2 mm; C, D, 250 µm.

Behavioral testing

To test functional recovery after SCI and C3 or Y27632 treatment, we measured HL motor function using the BBB locomotor ratingscale (Basso et al., 1995) (n = 37 animals). Because a toe clearancephase cannot be evaluated in recuperating mice, we modified therating to a 17 point scale (see Materials and Methods). Twenty-fourhours after surgery, control mice were paraplegic (Fig. 5A) andmoved by pulling themselves forward with their forelimbs (Fig.5B). Mice treated with C3 or Y27632 showed a remarkable recoverywithin 24 hr (Fig. 5A), already walking with weight support (Fig.5A,C) (movie 1; available at www.jneurosci.org). Although thisearly recovery is too rapid to be explained by long-distance regeneration,possible mechanisms include local reorganization of central patterngenerator circuitry (Giménez y Ribotta et al., 2000) that mayinclude sprouting from undamaged ventral fibers or interneurons,pharmacological activation of neurotransmitter receptors (Rossignolet al., 2000), or neuroprotection (C. Dubreuil, M. Winton, F.Yang, P. Morley, L. McKerracher, unpublished observations). Micethat had received C3 or Y27632 treatment continued to recoverover the 1 month period of observation and exhibited HL-FL coordination(Fig. 5E,G) (movie 2; available at www.jneurosci.org). By contrast,the average recovery plateau for untreated animals was limitedto unstable walking without HL-FL coordination (Fig. 5D,F) (movie2). Retransection of the spinal cord at 3 weeks (n = 8) eliminatedany difference between the C3-treated (n = 5) and control (n =3) animals (BBB at day 6, 7.6 vs 7.3, respectively).

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Figure 5. Analysis of functional recovery. A, Modified BBB scores of C3-treated (black circles; n = 11), Y27632-treated (black triangles; n = 5), fibrin-treated (gray circles; n = 11), and untreated (open circles; n = 10) mice to evaluate recovery of locomotion during the month after dorsal over-hemisection. At 24 hr, 1 week, 2 weeks, and 1 month, differences between groups of animals were evaluated by the Mann-Whitney U test. p values were similar at all four time points: C3-treated versus fibrin-treated, p < 0.001; Y27632-treated versus fibrin-treated, p < 0.05; C3-treated versus Y27632-treated, NS; fibrin-treated versus untreated, NS. B, Photograph of a spinal cord-injured mouse 24 hr after injury; HL cannot support body weight. C, Photograph of a C3/fibrin-treated mouse 24 hr after injury; body weight is supported by HL. D, E, Selected videoframes of representative untreated and C3/fibrin-treated mice, respectively, to show differences in recovery of HL-FL coordination 30 d after lesion. Although C3-treated mice alternate front paw and foot placements properly, untreated mice do not show one-to-one correspondence between HL and FL stepping. Numbers refer to elapsed time in tenths of seconds. F, G, For the mice depicted in D and E, respectively, HL-FL coordination is represented graphically. The position of the right hindpaw (solid line) and the right front paw (dotted line) on (I) or off (O) the ground was noted for each 1 of 38 sequential videoframes. The untreated mouse in D moves its forelimb twice before each HL step. NS, Not significant.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The failure of axon regeneration in the spinal cord is attributable, at least in part, to the growth inhibitory propertiesof white matter and the lesion site. The Rho signaling pathwayis known to be important both for the cell response to growthinhibition (Lehmann et al., 1999) and for neuroprotection (Trappet al., 2001), and growth-inhibitory substrates activate Rho (M.Winton and L. McKerracher, unpublished observations). We reporthere that inactivation of either Rho or Rho kinase is sufficientto allow axon growth on inhibitory substrates and leads to improvedrecovery after SCI. C3 ribosylates asparagine 41 in the effectordomain to inactivate Rho (Sekine et al., 1989); Y27632 inhibitsthe kinase activity of ROK by competing with ATP for binding tothe kinase (Ishizaki et al., 1997; Uehata et al., 1997). Our studiestarget these two different parts of the Rho signaling pathwayto demonstrate the importance of Rho signaling for CNS repair.Both C3 and Y27632 promoted axon growth, but C3 was more effectivethan Y27632. The difference between the effects of C3 and Y27632suggest the presence of other effectors of Rho that are inactivatedby C3 but not by Y27632. Rho signals not only to ROK but alsoto protein kinase N (Amano et al., 1996), rhotekin, and othertargets (Reid et al., 1996). Therefore, for CNS repair, Rho appearsto be a more efficient target thanROK.

The remarkable improvement in function within 1 d of spinal cord lesion and treatment with C3 or Y27632 may be caused by increasedneuroprotection in the lesioned spinal cord. Neuroprotection byitself is important for improved functional recovery after SCI(Pencalet et al., 1993; Gaviria et al., 2000), and a growing volumeof literature suggests that the application of C3 to ischemicCNS tissue has neuroprotective effects (Laufs et al., 2000; Trappet al., 2001). Moreover, inactivation of Rho in spinal cord reducesthe number of apoptotic cells (C. Dubreuil, M. Winton, F. Yang,P. Morley, and L. McKerracher, unpublished observations). It hasbeen demonstrated that the application of C3 after middle cerebralartery occlusion reduces infract volumes (Trapp et al., 2001).Therefore, Rho signaling pathway is a good target to both preventcell death and stimulate regeneration. The ability of C3 and Y27632to block unwanted effects of Rho activation, cell death, and neuriteretraction are likely to contribute importantly to improved outcomeafter SCI. It is also possible that C3 and Y27632 treatments affectedother cells, such as leukocytes; immediate improvement in functionalrecovery after SCI has been observed 24 hr after treatment withgabexate mesilate, a protease inhibitor that inhibits activationof leukocytes (Taoka et al., 1997). Therefore, the short-termeffects that we observe after treatment with C3 or Y27632 arelikely caused by the ability of these compounds to limit the celldamage that occurs immediately afterinjury.

It should be kept in mind that mice show important differences from rats in their response to spinal cord injury, most notablythe absence of necrotic cavitation (Steward et al., 1999). Inour experiments, we used an over-hemisection of the spinal cordto test whether Rho or ROK inactivation was able to promote repair.Many strategies that work well to promote regeneration after hemisectionare not effective after complete transection of the spinal cord.It has been shown that sparing of ventrolateral fibers may translateinto improved locomotor performance (Brustein and Rossignol, 1998)because these fibers are important in the initiation and controlof spinal central pattern generators (for review, see Rossignolet al., 2000). Sprouting of uninjured collaterals (Weidner etal., 2001) or sprouting of fibers that are part of the circuitryof the spinal cord (Giménez y Ribotta, 2000) are likely to contributeimportantly to repair. It was demonstrated recently that reorganizationof spared pathways also contributes to functional recovery (Raineteauet al., 2001). Thus, inactivation of Rho may help stimulate andenhance the spontaneous repair process that leads to limited recoveryafter SCI, in addition to its effects onregeneration.

To study the effects of C3 and Y27632 on axons in vivo, we chose to study the CST because it is one of the best characterizedtracts for studies of axon regeneration in the spinal cord. Moreover,the CST can be anterogradely labeled, and in mice, most of thefibers within the CST are located just above the central canalin the dorsal spinal cord. The dorsal over-hemisection that weused for our studies would eliminate not only the CST fibers butalso other dorsal and lateral descending pathways while sparingthe ventral pathways essential for locomotion. We demonstratedwith our in vitro studies that treatment with C3 or Y27632 canstimulate axon growth on inhibitory substrates. In vivo, we observedsprouting and long-distance regeneration. It is well documentedthat reorganization of collateral CST fibers occurs after SCI(Weidner et al., 2001). Also, dendritic remodeling of neuronscan be enhanced by inactivation of Rho (Ruchhoeft et al., 1999).Thus, inactivation of Rho, which is known to affect both axonsand dendrites, is likely to enhance spontaneous plasticity ofaxons and dendrites, leading to functional remodeling of spinalcordcircuitry.

The BBB open-field locomotor test cannot be correlated with the regeneration of specific tracts. Although the late recoveryof HL-FL coordination that we observe at 1 month is consistentwith regeneration of cut fibers, we cannot completely rule outthe possibility of protective sparing, as reported with otherstrategies that promote repair after CNS injury (Lazarov-Spiegleret al., 1996; Hauben et al., 2000). However, our observation thatGAP-43 is upregulated in the motor cortex is consistent with theinterpretation that anterogradely labeled CST fibers past theinjury site represent regenerated fibers. Increased GAP-43 expressioncorrelates with regeneration of rubrospinal neurons, and projectionneurons do not express GAP-43 after thoracic injury alone (Ferandeset al., 1999). Therefore the upregulation of GAP-43 expressionis a good indicator for long-distance regeneration. We observedlong-term improvements in BBB outcomes, even in animals in whichsubstantial CST labeling was not observed. Therefore, many factors(neuroprotection, remodeling, and regeneration) and many fibertracts (dorsal and ventral) are likely to contribute to functionalrecovery after SCI and treatment with Rho or Y27632. Notwithstandingthe possibility of multiple mechanisms, long-distance regenerationis likely to have been important for the improved function atlater stages. These treatments that potentiate spontaneous functionalrecovery in open-field tests give hope that effective treatmentfor spinal cord injury will be developed in the foreseeable future.The treatment that we have developed to promote functional recoveryand axonal regeneration after SCI is simple: an inhibitor of Rhosignaling pathway injected at the lesion site in a tissue adhesive.These studies show the potential for a new, straightforward treatmentto reduce functional impairment afterSCI.

  FOOTNOTES

Received Dec. 3, 2001; revised May 6, 2002; accepted May 8, 2002.

This work was supported by the Canadian Institutes of Health Research (CIHR), a Barbara Turnbull Foundation-CIHR Scholarship(P.D.), and a Fonds de la Recherche en Santé (FRSQ) scholarship(B.E.). L.M. is a Chercheur Boursier Senior of the FRSQ. We thankDr. Sam David for valuable discussions on spinal cord surgeryand anterograde labeling. We thank Dr. Dana Lasko for commentson this manuscript and Charles Essagian for expert technical help.We gratefully acknowledge Maxime Lehmann for help with the synthesisofC3.

Correspondence should be addressed to Dr. Lisa McKerracher, Département de Pathologie et Biologie Cellulaire, Universitéde Montréal, CP 6128, Succursale Centre-Ville, Montréal, Quebec,H3C 3J7, Canada. E-mail: mckerral{at}patho.umontreal.ca.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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