Schwann Cell But Not Olfactory Ensheathing Glia Transplants Improve Hindlimb Locomotor Performance in the Moderately Contused Adult Rat Thoracic Spinal Cord

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The Journal of Neuroscience, August 1, 2002, 22(15):6670-6681

Schwann Cell But Not Olfactory Ensheathing Glia Transplants Improve Hindlimb Locomotor Performance in the Moderately Contused Adult Rat Thoracic Spinal Cord
Toshihiro Takami¹, Martin Oudega¹^,², Margaret L. Bates¹, Patrick M. Wood¹^,², Naomi Kleitman¹^,², and Mary Bartlett Bunge¹^,²^,³
¹ The Chambers Family Laboratory of Electron Microscopy, The Miami Project to Cure Paralysis, and the Departments of ² Neurological Surgery and ³ Cell Biology and Anatomy, University of Miami School of Medicine, Miami, Florida 33136

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cultured adult rat Schwann cells (SCs) or olfactory ensheathing glia (OEG), or both, were transplanted in the adult Fischerrat thoracic (T9) spinal cord 1 week after a moderate contusion(10 gm, 12.5 mm, NYU impactor). Rats received either a total of2 × 10⁶ cells suspended in culture medium or culture medium only (controls).At 12 weeks after injury, all grafted animals exhibited diminishedcavitation. Although in medium-injected rats 33% of spinal tissuewithin a 5-mm-long segment of cord centered at the injury sitewas spared, significantly more tissue was spared in SC (51%),OEG (43%), and SC/OEG (44%) grafted animals. All three types ofglial grafts were filled with axons, primarily of spinal origin.SC grafts contained more myelinated axons than SC/OEG and OEGgrafts. Both types of SC-containing grafts expressed more intensestaining for glial fibrillary acidic protein and chondroitin sulfateproteoglycan compared with OEG-only grafts. Retrograde tracingdemonstrated that the number of propriospinal and brainstem axonsreaching 5-6 mm beyond the grafted area was significantly higherwith SC and SC/OEG grafts but not with OEG-only grafts comparedwith controls. Corticospinal fibers terminated closer to the lesionepicenter in all grafted animals than in controls. With SC-onlygrafts, a modest but statistically significant improvement inhindlimb locomotor performance was detected at 8-11 weeks afterinjury. Thus, in addition to this functional improvement, ourresults show that an SC graft is more effective in promoting axonalsparing/regeneration than an SC/OEG or OEG graft in the moderatelycontused adult rat thoracic spinalcord.

Key words: spinal cord injury; transplantation; contusion injury; axonal sparing; axonal regeneration; propriospinal axons; corticospinal tract; brainstem axons; neuroprotection

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Injury to the adult mammalian spinal cord results in progressive tissue damage, which causes permanent functional deficits(for review, see Amar and Levy, 1999). Acute treatment with anti-inflammatoryagents such as methylprednisolone (for review, see Oudega et al.,1999; Takami et al., 2002) or interleukin-10 (Bethea et al., 1999;Takami et al., 2002) limits injury-induced tissue damage. However,despite application of neuroprotective treatments, severe functionaldeficits are still observed, and in fact, at present, spinal cordinjury (SCI) has very poor clinicalprospects.

Experimental strategies aimed at promoting axonal sparing/regeneration and restoring functional deficits suggest that theremay be a window of opportunity for repair after SCI (for review,see Bunge, 2001; Jones et al., 2001). Several cellular graftingstrategies result in some behavioral improvements of experimentallyinduced paralysis (Iwashita et al., 1994; Cheng et al., 1996;Grill et al., 1997; Li et al., 1997; Liu et al., 1999; McDonaldet al., 1999; Ramón-Cueto et al., 2000; Coumans et al., 2001).

An amply researched and reputable cell type for spinal cord repair is the Schwann cell (SC), the myelin-forming glial cellof the peripheral nervous system (for review, see Bunge, 1994;Bunge and Kleitman, 1999). An SC graft bridging a transected adultrat thoracic spinal cord promotes regeneration and myelinationof propriospinal axons (Xu et al., 1995a, 1997, 1999). The combinationof an SC graft with methylprednisolone (Chen et al., 1996) orwith neurotrophic factors (Xu et al., 1995b; Menei et al., 1998)promotes axonal regeneration from brainstem neurons aswell.

Another glial type that has shown promise in SCI repair is olfactory ensheathing glia (OEG) (for review, see Franklin andBarnett, 2000; Kleitman and Bunge, 2000; Ramón-Cueto, 2000; Plantet al., 2001; Raisman, 2001). OEG grafts promote axonal growthand functional improvements in different SCI models (Li et al.,1997, 1998; Ramón-Cueto et al., 1998, 2000). Moreover, combiningan SC graft with OEG placed into the transected cord stumps promotesregeneration of descending and ascending axons into the caudaland rostral cord, respectively (Ramón-Cueto et al., 1998).

The repair abilities of SCs and OEG in the adult cord have been studied in complete or partial transection models (for review,see Kleitman and Bunge, 2000; Ramón-Cueto, 2000; Bunge, 2001;Plant et al., 2001) and in demyelination models (for review, seeBlakemore et al., 2000) (see also Imaizumi et al., 1998, 2000).Although a common type of damage to the human spinal cord is acontusive injury (Bunge et al., 1997; Kakulas, 1999), studieson the repair capacity of SCs (Martin et al., 1991, 1996) andOEG in clinically relevant contusion models are sparse. In thepresent study, the effects of purified adult rat SCs or OEG, orboth, on spinal tissue sparing, axonal sparing/regeneration, andbehavioral improvement were assessed in moderately contused adultFischer rat thoracic spinal cord. We used the term "sparing/regeneration"in this paper because spared and regenerated axons could not bedistinguished. To our knowledge, this study is the first to comparethe reparative capacity of SCs and OEG in a clinically relevantcontusive SCImodel.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Schwann cell purification. Highly purified SC cultures were obtained from sciatic nerve of adult female Fischer rats (CharlesRiver Laboratories, Wilmington, MA) as described previously (Morrisseyet al., 1991). To determine the purity of the SCs used for grafting,samples of the harvested SCs were plated onto culture dishes,cultured for 3 hr, stained for S100, and then coverslipped withCitifluor (UKC Chemical Laboratory, Canterbury, England) containing100 µM Hoechst nuclear dye (Sigma, St. Louis, MO) to compare numbersof S100-positive cells with Hoechst-labeled cells. The purityof the SCs used for implantation was 95-98%.

Olfactory ensheathing glia purification. Highly purified cultures of OEG were obtained from the nerve fiber layer of the olfactorybulb of adult female Fischer rats as described previously (Ramón-Cuetoet al., 1998). Care was taken to minimize the inclusion of non-nervefiber layer bulb tissue, and the pia was removed. The tissue wasdissected in Leibovitz-15 (L-15) medium (Invitrogen, Gaithersburg,MD), washed twice with HBSS (Invitrogen), diced into small fragments,and incubated in HBSS with 0.25% trypsin (Worthington Biochemical,Lake Wood, NJ) and 50 µg/ml DNAase (Sigma) at 37°C for 60 min.Trypsinization was stopped by adding DMEM/Ham's/F-12 (Invitrogen)(1:1 mixture) supplemented with 10% FBS and 50 µg/ml gentamicin(df-10S). The dissociated cells were washed twice, resuspendedin df-10S plus 2 µM forskolin and 20 µg/ml pituitary extract,and then plated onto poly-L-lysine-coated culture dishes. Oneweek later, OEG were separated from other cell types by immunopanningusing an antibody against p75, the low-affinity nerve growth factorreceptor (gift of Dr. Eric Shooter, Stanford University), usinga modification of the published protocol (Ramón-Cueto et al.,1998). Cells were detached with 0.05% trypsin and 0.02% EDTA (Invitrogen),centrifuged, washed two times, resuspended in L-15, and then platedon antibody-treated dishes for 30 min at 4°C. Before use, thesedishes had been incubated overnight at 4°C with anti-mouse IgGA,M antibody (1:100 in Tris buffer) (0.05 M, pH 9.5; Jackson ImmunoResearch,West Grove, PA), washed three times with ice-cold L-15, incubatedwith antibodies against p75 (1:5 in L-15 medium with 5% FBS) for2 hr at 4°C, and finally washed three times with ice-cold L-15medium. The unattached cells were removed, and the dishes werewashed gently five times with ice-cold L-15 medium. The attachedcells were fed df-10S plus 2 µM forskolin and 20 µg/ml pituitaryextract for 2 d at 37°C in 6% CO₂. Next, the cells were detachedfrom the dishes with 0.05% trypsin and 0.02% EDTA and washed twicewith df-10S. Finally, the cells were resuspended in DF-10S plus2 µM forskolin and 20 µg/ml pituitary extract, plated onto poly-lysine-coatedculture dishes, allowed to grow to confluency, and then harvested(in DMEM/F-12) fortransplantation.

Animals. Adult female Fischer rats (n = 68; 160-180 gm; Charles River Laboratories) were housed according to National Institutesof Health and United States Department of Agriculture guidelines.The Institutional Animal Care and Use Committee of the Universityof Miami approved all animal procedures. Before surgery, the ratswere anesthetized with 1-2% halothane in a mixture of 70% nitrousoxide and 30% oxygen. An adequate level of anesthesia was determinedby monitoring the corneal reflex and withdrawal to painful stimulifor the hindlimbs. The back region was shaved and asepticallyprepared with betadine. Bicillin (0.02 ml/100 mg body weight,300 U/ml, i.m.) was administered before surgical procedures wereperformed. During surgery, the rats were kept on a heating padto maintain the body temperature at 37 ± 0.5°C.

Contusion injury. Contusion injury was induced by the weight drop device developed at New York University (Gruner, 1992).Without disrupting the dura mater, the ninth thoracic (T9) spinalcord segment was exposed by removing the dorsal part of the T8vertebra. The exposed cord was then moderately contused by a 10gm weight that was dropped from a height of 12.5 mm. The contusionimpact velocity and compression were monitored to guarantee consistencybetween animals. After injury, the muscles were sutured in layersand the skin was closed. The rats were returned to their partlywarmed cages with ad libitum access to water and food. Bicillinwas administered 2, 4, and 6 d after the contusion injury. Therats were maintained for a total of 12 weeks afterinjury.

Glia transplantation. One week after injury, the injury site was exposed, and a total of 2 × 10⁶ SCs, OEG, or SC/OEG (1 × 10⁶ each) in 6 µl DMEM-F12 medium (G. W. Plant, E. P. Cuervo, M.L. Bates, M. B. Bunge, and P. M. Wood, unpublished observations)was injected into the contused area using a 10 µl Hamilton syringeheld in a micromanipulator. Control rats were injected with 6µl of DMEM-F12 medium. After injections, the muscle layers andthe skin were closed separately. Sixty-eight rats were transplantedwith medium (n = 21), SCs (n = 15), OEG (n = 21), or SC/OEG (n= 11). The rats in each experimental group were randomly dividedinto subgroups for retrograde and anterogradetracing.

Anterograde axonal tracing and retrograde neuronal tracing. For anterograde axonal tracing, 9 weeks after contusion, the ratswere anesthetized and biotinylated dextran amine (BDA; MolecularProbes, Eugene, OR) was injected stereotactically into the hindlimbarea of the motor cortex (2 × 0.5 µl, bilateral), dextran coupledto fluorescein (D/Fl; Molecular Probes) into the reticular formation(2 × 0.3 µl, bilateral), and dextran coupled to rhodamine (D/Rho;Molecular Probes) into the lateral vestibular nuclei (2 × 0.2µl,bilateral).

For retrograde neuronal tracing, 11 weeks after the contusion injury, the injury site was exposed, and a total of 0.6 µl ofa 2% aqueous fast blue solution (FB; Sigma) was injected 7 mmdistal to the distal laminectomy edge (in between vertebra T10and T11) using a glass needle (diameter, 200 µm) attached to a1 µl Hamilton syringe held in a micromanipulator (Takami et al.,2002). All injections was performed over a 3 min period, and theinjection needle was kept in place for an additional 3 min tominimize leakage on withdrawal. After the injection, the musclesand skin were closed inlayers.

Histological procedures. At 12 weeks after injury, all rats were anesthetized (2.57 mg ketamine, 0.51 mg xylazine, and 0.09mg acepromazine per 100 gm body weight) and transcardially perfusedwith phosphate-buffered, 4% paraformaldehyde (0.1 M, pH 7.4) (Takamiet al., 2002). The T7-9 thoracic segments, which included thecontusion injury, were dissected and embedded in gelatin (Oudegaet al., 1994). Using a sliding freezing microtome, the embeddedcord segments were cut into 40-µm-thick horizontal sections. TheT2, C6, and C2 spinal cord segments and the brainstem and cerebralcortex were cut into 40-µm-thick transverse sections. All sectionswere collected in PBS (0.1 M, pH 7.4) and kept at 4°C until furtherprocessing.

For electron microscopic analysis, a 6-mm-long piece of the spinal cord with the epicenter in the middle was dissected anddivided into three 2-mm-long pieces. These pieces were preparedfor analysis as described previously (Xu et al., 1995a).

Estimation of the number of myelinated axons and blood vessels in transplants. Estimated total numbers of myelinated axonsand blood vessels as well as the density of myelinated axons inthe contusion lesion-transplant area were determined by systematicrandom sampling (West, 1993). In toluidine blue-stained, 1-µm-thicktransverse plastic sections, the injured-transplanted area wasoutlined and than scanned using a fractionator grid, which rangedin size from 35 to 70 µm². The objective lens used for all counts was 100× with oil immersion.In the center of the fractionator grid, a 15 µm² dissector probe was present. All myelinated profiles within thisdissector probe were counted. In this way a fraction of the lesion-transplantarea was analyzed (optical fractionator method) (West, 1993).For proper use of this technique, a minimum number of 150-300myelinated axons is required per lesion-transplant area. In ourcounts, the number for myelinated axons was between 159 and 484,with the exception of 67 in a medium-injected control animal,which contained a very large cavity. The estimation of the totalnumber of myelinated axons and blood vessels was done with theStereoinvestigator software (MicroBrightfield, Inc., Colchester,VT).

Quantitative assessment of anterograde and retrograde tracing. For quantitative analysis of the anterograde tracing, BDA-labeledcorticospinal axons were examined in every fifth section of theT7-9 cord segments. Within these sections, the labeled axons werevisualized using a Ni-enhanced avidin-biotin-peroxidase staining(Oudega et al., 1999). The number of BDA-labeled corticospinalaxons was determined by counting all labeled axons crossing animaginary line placed perpendicular to the rostral-caudal axisof the spinal cord at 1 and 2 mm rostral to and at the lesionepicenter. The numbers of each section were summed per rat andthen multiplied by 5 to obtain the final number of labeled corticospinalaxons. In addition, from the T7-9 segments, every fifth sectionwas mounted onto gelatin-coated glass slides, coverslipped withCitifluor (UKC Chemical Laboratory) containing the nuclear dye,Hoechst (100 µM, Sigma), and used to examine the D/Fl-labeledreticulospinal axons and the D/Rho-labeled vestibulospinalaxons.

For quantitative analysis of the retrograde tracing, every third horizontal section of the T7-9 cord was mounted on gelatin-coatedglass slides and coverslipped with Citifluor (UKC Chemical Laboratory).For the T2, C6, and C2 cord segments, every 5th transverse sectionand, from the brainstem and cerebral cortex, every 10th transversesection was mounted onto gelatin-coated slides and coverslippedwith Citifluor (UKC Chemical Laboratory). For each rat, the numberof FB-labeled neurons was determined in each section. These numberswere summed per rat and multiplied by 3 (T9-T7), 5 (T2, C6, andC2), or 10 (brainstem and cerebral cortex) to obtain the finalnumber of labeledneurons.

Assessment of spinal tissue sparing. Every fifth horizontal section from the T7-9 segment was mounted onto gelatin-coatedglass slides, stained with cresyl violet, dehydrated, and coverslippedin Pro-Texx (Baxter Diagnostics, Deerfield, IL) to determine thevolume of spared spinal tissue using an image analysis computersystem (Universal Imaging, West Chester, PA). In each section,the total area of a 5-mm-long cord segment with the lesion epicenterin the middle and the area of damaged spinal tissue were determined.The border of the damaged area was defined as an obvious discontinuityin density of small cells, i.e., transplanted cells and inflammatorycells, and the absence of healthy-looking spinal neurons. Occasionally,this area contained small cysts. The measurements of each sectionwere summed per rat and multiplied by 5 (every fifth section wasanalyzed) to give the total area of the 5-mm-long cord segmentand of damaged spinal tissue. The volumes were then calculatedby means of numerical integration. The volume of spared spinaltissue within the 5-mm-long segment was determined by subtractingthe volume of damaged tissue from the volume of the whole segment.Finally, this value was expressed as the percentage of the totalvolume of a 5-mm-long segment from the same cord level from normal,uninjured rats (n =4).

Immunohistochemical procedures. Every sixth horizontal section was immunohistochemically stained with mouse monoclonal orrabbit polyclonal antibodies, or both, following an earlier describedprotocol (Takami et al., 2002). The polyclonal antibodies usedwere anti-serotonin (5-HT, 1:200; Incstar Corp., Stillwater, MN),anti-dopamine- $beta$ $-$ hydroxylase (D $beta$ H, 1:200; Incstar Corp.), anti-calcitoningene-related peptide (CGRP; 1:100; Cappel, Aurora, OH), and anti-glialfibrillary acidic protein (GFAP, 1:400; Dako, Carpinteria, CA).The monoclonal antibodies used were anti-low-affinity nerve growthfactor receptor [p75 (192IgG), 1:1; gift from Dr. E. Shooter,Stanford University], anti-neurofilament (RT-97, 1:10; DevelopmentalHybridoma Bank), anti-chondroitin sulfate proteoglycan (CS-56,1:100; Sigma), and anti-growth associated protein-43 (GAP-43,1:500; Boehringer Mannheim, Mannheim, Germany). The secondaryantibodies used were Alexa 488-conjugated goat anti-rabbit (1:200;Molecular Probes) and Alexa 594-conjugated rabbit anti-mouse (1:200;Molecular Probes). The sections were mounted onto gelatin-coatedglass slides and coverslipped in Citifluor (UKC Chemical Laboratory)containing 100 µM Hoechst dye(Sigma).

Open field locomotor test. Hindlimb performance was evaluated using the open field locomotor test developed by Basso et al.(1995, 1996). Two observers, unaware of the experimental procedures,performed the test once a week for 9 weeks (for rats that receivedanterograde tracing) or 10 weeks (all otherrats).

Statistical analysis. One-way ANOVA followed by Fisher's protected least-significant difference test was used to determinestatistical differences between the average number of axons andneurons as determined for each group. However, in case of unequalvariance (F test), a nonparametric analysis (Kruskal-Wallis testfollowed by Mann-Whitney U test) was used. The latter test wasalso used to determine whether differences between the averageBasso, Beattie, and Bresnahan (BBB) score per group were statisticallysignificant. A statistically significant difference was acceptedat p < 0.05.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

SC and OEG transplants promote tissue sparing

In medium-injected animals, 12 weeks after a moderate contusion injury, large cysts were present extending in the rostral-caudaldirection (Fig. 1A). These cysts were widest at the lesion epicenter.In transplanted animals, the glial grafts were continuous withhost spinal tissue (Fig. 1B-D), although some small cavities couldbe observed (Fig. 1C,D). The effect of SC and OEG grafts on tissuesparing was assessed by subtracting the volume of damaged tissue(including cavities and transplant) within a 5-mm-long cord segment(with the epicenter in the middle of the section) from the totalvolume of this segment. This value was expressed as a percentageof the volume of the comparable (T9) segment in uninjured rats.The volume of a 5-mm-long spinal cord segment of a normal, uninjuredrat at the T9 level was 21.2 ± 0.9 mm³ (SEM; n = 4). In control medium-injected animals, the volumeof spared tissue was 6.9 ± 0.7 mm³ (n = 8), or 33 ± 3% of the volume of the comparable segment ofan uninjured rat (Fig. 1E). With an SC or OEG graft, the volumeof spared tissue was 10.8 ± 1.5 mm³ (n = 5) and 9.1 ± 0.8 mm³ (n = 9), or 51 ± 7 and 43 ± 4%, respectively, of the volume ofthe comparable segment in a normal, uninjured cord (Fig. 1E).These values were significantly greater than the volume of sparedtissue in medium-injected animals. Grafting the combination ofSCs and OEG resulted in a volume of 9.4 ± 1.1 mm³ (n = 5) of spared tissue, or 44 ± 5% of the comparable segmentin an uninjured cord (Fig. 1E), which was also significantly (p< 0.05) greater than in the medium-injected control animals. Theseresults demonstrate that implantation of SC or OEG grafts, orboth, into a 1-week-old moderate contusion lesion promotes spinaltissue sparing.

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Figure 1. Glial grafts limit contusion-induced spinal tissue damage. Cresyl violet-stained horizontal sections of T9 thoracic spinal cord 3 months after a moderate contusion injury and injection of medium (A), SCs (B), OEG (C), or SCs/OEG (D) 1 week after injury. Arrowheads indicate the contusion impact site. Black stars indicate cystic cavities, and white stars indicate coagulated blood between the dura mater and the spinal cord. GM, Gray matter; OEG, olfactory ensheathing glia transplant; SC, Schwann cell transplant; SC/EOG, transplant of Schwann cells and olfactory ensheating glia; WM, white matter. Scale bar, 50 µm. E, Bar graph showing the volume of spared spinal tissue represented as the percentage (±SEM) of a 5-mm-long analyzed spinal segment (T9 cord segment) in an uninjured spinal cord. Asterisks indicate a significant difference (p < 0.05) from the medium-injected control animals.

All grafts contain myelinated axons

At 12 weeks after injury, i.e., 11 weeks after implantation, toluidine blue-stained, 1 µm plastic cross-sections of the lesionepicenter were prepared to examine the presence of myelinatedaxons within and around the transplants. In medium-injected controlanimals, some tissue usually was found within the large cavities(Fig. 2A). This tissue contained axons surrounded by typical peripheral-type(SC) myelin (Fig. 2B). The criteria to recognize peripheral-typemyelin in plastic cross sections were the presence of a signetring configuration (myelin ring with the proximate SC nucleus)and the presence of space between the myelinated axons, whichis caused by the formation of extracellular matrix (Bunge et al.,1994). In contrast, central-type myelin profiles do not exhibitadjacent nuclei and have little or no space between them. In controlsas well as in grafted animals, a rim of preserved spinal whitematter that contained axons with typical central-type (oligodendrocyte)myelin was observed. In the dorsal aspect of this rim, both peripheraland central types of myelin were found, indicating the presenceof SCs that had migrated from the dorsal roots into the damagedspinal cord.

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Figure 2. Schwann cell transplants contain numerous myelinated axons in the middle of the graft. All panels show toluidine blue-stained, 1-µm-thick plastic sections. A, Control, medium-injected animal. Stars indicate cystic cavities. B, Higher magnification of boxed area in A, demonstrating that SCs have migrated into the lesion area, as evidenced by the presence of peripheral-type myelin (arrows). C, SC-transplanted animal. D, Higher magnification of boxed area in C. Numerous myelinated axons (arrows) are present within the SC transplant. E, OEG-transplanted animal. F, Higher magnification of boxed area in E, demonstrating a few myelinated axons (arrows) within the OEG transplant. DR, Dorsal root; LC, lateral white column; VC, ventral white column. Scale bars: A, C, E, 300 µm; B, D, F, 20 µm.

All types of grafts contained axons surrounded by peripheral-type myelin (Fig. 2B,D,F). However, the SC graft clearly containedmore axons than the other types of grafts (Fig. 2, compare D,F; Table 1). We estimated the total number of myelinated axonsand blood vessels in the contusion lesion area by image analysisusing the optical fractionator method (West, 1993) (Stereoinvestigatorprogram). In SC-injected animals (Fig. 2C,D), the number of myelinatedaxons was 5212 ± 1783 (mean ± SEM; n = 2) compared with 2125 ±697 (n = 3) in medium-injected animals (Table 1). In OEG-injectedanimals (Fig. 2E,F), the number of axons with peripheral-typemyelin was 2965 ± 1110 (n = 3), and in SC/OEG grafts, 3884 ± 711(n = 3). The density of myelinated axons was 75.8 ± 31.9 myelinatedaxons per 0.1 mm² in SC grafts, 32.3 ± 7.01 in OEG grafts, 40.2 ± 21.5 in SC/OEGgrafts, and 26.9 ± 12.2 in medium-injected animals. The numberof blood vessels was similar in all groups (Table 1).


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Table 1. Estimated numbers of myelinated axons and blood vessels in contusion lesion areas

In electron micrographs, peripheral-type myelin is recognized by the presence of an external collar of SC cytoplasm, a basallamina, and collagen fibers that run parallel to the myelin sheath.Central-type myelin does not exhibit these features. The electronmicrograph in Figure 3A illustrates central- and peripheral-typemyelin in tissue next to a cavity. Although in this area froma control animal there is little glial limiting membrane evident,in other areas it was much more prominent at the interface betweencentral tissue and invading SCs. A wide range in degree of gliallimiting membrane (basal lamina and highly filamentous astrocyticprocesses) was observed also in grafted animals. Fasciculationand perineurium formation were not evident in the SC area in Figure3A. In all animals examined, perineurium was only minimally developedat 12 weeks. This was surprising in comparison with other lesionmodels such as the photochemical lesion, where fasciculation andperineurial development in SC areas are prominent (Bunge et al.,1994). SC-related axons were often clustered around blood vessels.Occasional macrophages were seen in all samples. Near the lesionor transplant, thin central myelin was observed, suggestive ofremyelination by oligodendrocytes.

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Figure 3. SC-containing grafts contain more myelinated axons than OEG-only grafts. A, SC-myelinated axons (at the right of the dashed line) are found in the cord near the cavity in a control animal, showing that host SCs migrated into the spinal cord as well as into the lesion site. B, After grafting of SCs, numerous SC-myelinated axons were observed in the lesion area at 12 weeks. In addition, many axons of small diameter (arrows) were typically ensheathed by nonmyelinating SCs. C, A few cells that resemble OEG were found after SC/OEG grafting in areas near the lesion where central myelin was evident. These are tentatively identified as OEG because, despite numerous naked axons nearby, only meandering (arrows) rather than clearly ensheathing processes extended from the cells. The cells exhibited patches of basal lamina (asterisks) indicating that these cells were not oligodendrocytes. All panels show electron micrographs. Scale bars: A, B, 4 µm; C, 1 µm.

Figure 3B illustrates at the electron microscopic level the presence of many axons with typical SC myelin in the middle ofan SC graft. Both myelinated and unmyelinated axons were present,and the SCs were surrounded by basal lamina. Axons varied considerablyin diameter. In both SC- and SC/OEG-grafted animals, the myelinin the grafts was of the peripheral type. In most SC/OEG- andOEG-grafted animals, it was not possible to identify the OEG.Moreover, in OEG grafts, the myelin was so typical of SCs thatit was not possible to determine whether the myelin had been formedby OEG or host SCs. In one area of an SC/OEG graft, however, cellsconsidered likely to be OEG were observed. They exhibited patchesof basal lamina and extended processes that meandered among clustersof axons but did not encircle them as SCs do (Fig. 3C). Thesecells were found only in an area of central myelinated axons nearthe site of implantation and were not seen in SC-onlygrafts.

Transplanted glia survive and support axonal sparing/regeneration

The glial transplants were identified using immunostaining for p75, the low-affinity nerve growth factor receptor, which stainsboth SCs and OEG. In control rats, p75 immunoreactivity was foundin strands of tissue within the damaged area (Fig. 4A). In animalswith an SC (Fig. 4B), OEG (Fig. 4C), or SC/OEG graft, p75 immunoreactivitywas observed within the transplanted area. Generally, the p75staining appeared more intense and extensive in SC grafts thanin OEG or SC/OEG grafts.

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Figure 4. Transplanted glia survive, express CSPG, and promote sparing/regeneration of axons. All panels show photographs taken from horizontal sections of the T9 cord segment 3 months after injury. The presence of p75-positive cells is shown in medium- (A), SC- (B), and OEG- (C) injected animals. Note the presence of p75-positive cells in the trabecula of spinal tissue in the cavity (asterisks) in the medium-injected animal. A rim of GFAP-positive reactive astrocytes was present within the spinal cord tissue surrounding the SC (D), OEG (E), or SC/OEG (F) graft. Stars indicate the transplants. GFAP staining was also present within the SC (G), OEG (H), and SC/OEG (I) grafts. G, H, and I are higher magnifications of the boxed areas in D, E, and F, respectively. Generally, GFAP staining was more intense in SC-containing grafts than in OEG-only grafts. The presence of CSPG is demonstrated in an SC (J), OEG (K), or SC/OEG (L) graft but was most intense in the SC graft. Also, CSPG was present in the surrounding spinal tissue in animals receiving SC-containing grafts. All transplants contained many neurofilament-positive axons as demonstrated in M, an SC graft. Some of the axons within the grafts were CGRP positive as shown in an SC transplant (N). Serotonergic axons were present within gray matter just rostral to an SC graft (O), with some penetrating the transplant (arrows). GM, Gray matter; WM, white matter; OEG, olfactory ensheathing glia transplant; SC, Schwann cell transplant; SC/OEG, transplant containing Schwann cells and olfactory ensheathing glia. Scale bars: A, 350 µm; B-F, J-M, 400 µm; G-I, 100 µm; N, O, 200 µm.

The presence of reactive astrocytes within the transplanted cord segment was evaluated using antibodies against GFAP. In controlanimals, a rim of GFAP staining along the surrounding spinal cordtissue delineated the injury area. Similarly, GFAP staining wasobserved within the spinal cord surrounding the SC (Fig. 4D),OEG (Fig. 4E), and SC/OEG grafts (Fig. 4F). Some GFAP reactivitywas found within the transplants. Generally, GFAP staining wasmore intense in SC-containing grafts (Fig. 4G,I) than in OEG grafts(Fig. 4H).

The presence of chondroitin sulfate proteoglycan (CSPG) within the grafted cord segment was studied using the CS-56 antibody.In control animals, some CSPG staining was found within the injuryarea. All three types of glial grafts and the surrounding spinaltissue displayed CSPG immunoreactivity. Generally, SC grafts (Fig.4J) displayed more intense CSPG immunostaining than OEG (Fig.4K) or SC/OEG grafts (Fig. 4L).

Intense neurofilament (Fig. 4M) and GAP-43 immunostaining, indicating the presence of numerous axons, was present in SC (Martinet al., 1991, 1996), OEG, and SC/OEG grafts. Different antibodieswere used to examine phenotypes of these axons. Anti-CGRP antibodiesrevealed that ascending sensory axons (Gibson et al., 1984) hadgrown into and across, but not beyond, the grafts (Fig. 4N). CGRP-positiveaxons were also found within the surrounding white matter. Anti-5-HTantibodies revealed that some serotonergic axons, from the raphenuclei in the brainstem (Newton and Hamill, 1988), had grown intothe grafts (Fig. 4O). 5-HT-positive axons were also present inthe rostral gray matter and in the lateral white matter (Fig.4O). Adrenergic axons, most likely originating from locus ceruleusneurons and identified with anti-D $beta$ H-antibodies (Newton and Hamill,1988), were found in spared white matter but not in the transplantsor beyond the distal interface. These observations indicate thatthe transplants contain some sensory and serotonergic axons, butmost of the axons appear to originate from spinal cordneurons.

More axons are present beyond the lesion level with SC-containing than OEG grafts

Retrograde neuronal tracing analysis
Axonal sparing/regeneration of propriospinal and supraspinal projections was examined using retrograde FB neuronal tracing.Figure 5, A and B, shows representative examples of FB-labeledneurons in the T8-7 cord segment in control and SC-grafted rats,respectively. The number of FB-labeled neurons in the T8-7, T2,C6, and C2 cord segments in SC and SC/OEG transplanted animals,but not in OEG-only grafted animals, was significantly higher(p < 0.05) than in controls (Fig. 5C). Figure 5, D and E, demonstratesFB-labeled cells within the reticular formation of control andSC/OEG-grafted animals, respectively. Within the brainstem, thetotal number of FB-labeled neurons was significantly higher (p< 0.05) in animals receiving SC or SC/OEG, but not OEG, graftscompared with controls (Fig. 5F). Although FB-labeled neuronswere also found within the cerebral cortex of control (Fig. 5G)and grafted (Fig. 5H) animals, no significant difference was foundin the total number of FB-labeled neurons in any of the groups(Fig. 5I). These results indicate that SC and SC/OEG grafts butnot OEG grafts placed within a 1 week moderately contused thoracicspinal cord promote the sparing/regeneration of propriospinaland supraspinal axons. None of the grafts appeared by this measureto affect sparing/regeneration of corticospinal axons.

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Figure 5. SC-containing grafts promote the most sparing/regeneration of propriospinal and supraspinal axons. FB-labeled neurons were present in the T8-7 cord segment in medium- (A) and SC- (B) injected animals. C, Bar graph showing the total number of FB-labeled neurons (±SEM) in different levels of the spinal cord. FB-labeled neurons in the reticular formation in medium- (D) and SC/OEG- (E) injected animals. F, Bar graph showing the total number of FB-labeled neurons (±SEM) in the brainstem. FB-labeled neuron in the cerebral cortex in medium- (G) and OEG- (H) injected animals. I, Bar graph showing the total number of FB-labeled neurons (±SEM) in the cerebral cortex. Single asterisks indicate a significant difference of p < 0.05 from the medium-injected control animals; double asterisks indicate a significant difference of p < 0.01 from the medium-injected control animals. CC, Central canal. Scale bar: A, B, 100 µm; D-H, 50 µm.

Anterograde axonal tracing analysis
The presence of corticospinal axons in the grafted area was evaluated using anterograde axonal tracing. At 12 weeks afterinjury, most of the corticospinal axons were present rostral tothe grafted area and had formed axonal end bulbs, indicating ongoingdegeneration (Tator, 1995). In all groups, corticospinal axonshad extended thin sprouts into the nearby gray matter and intothe transplants (Fig. 6A). Quantification revealed that a significantlyhigher number of corticospinal sprouts was present at 2 mm rostralto the lesion epicenter in grafted animals compared with controlanimals (Fig. 6B). The numbers found at 1 mm rostral to the epicenterand at the epicenter did not significantly differ between groups(Fig. 6B).

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Figure 6. Glial grafts promote corticospinal axon sparing/regeneration. All panels except B show photographs taken from horizontal 40-µm-thick sections. A, BDA-labeled corticospinal axons in an OEG transplant (outlined). B, Bar graph showing the number of BDA-labeled axons (±SEM) at different levels within the glial transplants. Single asterisks indicate a significant difference of p < 0.05 from the medium-injected control animals; double asterisks indicate a significant difference of p < 0.01 from controls. C, Dextran-rhodamine-labeled vestibulospinal axons in the lateral white matter columns (LC) at the level of the lesion epicenter. D, Dextran-fluorescein-labeled reticulospinal axons in the lateral white matter columns (LC) at the level of the lesion epicenter. Scale bars, 100 µm.

Axonal sparing/regeneration of reticulospinal and vestibulospinal fibers was examined using anterograde axonal tracing. Incontrol and grafted rats, reticulospinal (Fig. 6C) and vestibulospinal(Fig. 6D) axons were observed in the peripheral spinal white matterbut rarely in thegrafts.

Transplantation of SC or SC/OEG 1 week after moderate contusion improves hindlimb performance

All animals exhibited a gradual improvement in hindlimb locomotor function during the 11 week period after cell transplantation(Fig. 7). In all experimental groups, most rats recovered to aBBB score of 10-11; they exhibited occasional (10) or frequentto consistent (11) weight-supported plantar stepping. Frequentto consistent weight-supported plantar stepping with occasionalto frequent forelimb-hindlimb coordination (BBB score of 12) wasobserved only in SC-only grafted animals. Statistical analysisindicated that the open field locomotor scores of the SC-transplantedgroup at 8, 9, 10, and 11 weeks after injury and of SC/OEG at8 weeks after injury were significantly higher (p < 0.05) thanthe control group.

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Figure 7. Transplantation of SC or SC/OEG 1 week after moderate contusion improves hindlimb performance. Bar graph shows the average open-field BBB score at different times after injury. Locomotor function of the hindlimbs was evaluated blindly once a week for 11 weeks. Data are presented as means ± SEM. Single asterisks indicate a significant difference (p < 0.05) from the medium-injected control animals. Compared with the control group, the SC-transplanted group had a significantly higher BBB score at 8-11 weeks after grafting. The SC/OEG group had a significantly higher score only at one time point, 8 weeks, after grafting.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The axonal growth-promoting effects of SCs (for review, see Bunge, 2001; Plant et al., 2001) and OEG (for review, see Franklinand Barnett, 2000; Kleitman and Bunge, 2000; Ramón-Cueto, 2000;Plant et al., 2001; Raisman, 2001) have been studied in differentadult rat spinal cord injury models. Here, we have investigatedand compared the restorative abilities of SC and OEG transplantsgrafted into a 1-week-old moderate contusion lesion in the adultrat thoracic spinal cord at 12 weeks after injury. All graftsdiminished injury-induced cavitation. The results indicate thata SC graft is more effective in promoting spinal tissue sparingand SC-containing grafts are more effective in promoting sparing/regenerationof spinal and supraspinal axons than an OEG graft. All graftspromoted axonal growth, but SC grafts exhibited the greatest numberof myelinated axons. Moreover, with an SC graft but not with anOEG graft, hindlimb performance of the contused rats was significantlyimproved 8 weeks aftertransplantation.

Retrograde neuronal tracing demonstrated that with SC and SC/OEG grafts, but not with OEG-only grafts, more propriospinaland brainstem neurons projected distal to the graft. We do notknow whether the grafts promoted axonal sparing, i.e., reducedinjury-induced axonal dieback, or axonal regeneration, or both.Certainly, some regeneration had occurred because axons were presentin the lesion epicenter where the glia had been injected 1 weekafter injury. Also, because a contusion injury generally obliteratesthe corticospinal tract (Hill et al., 2001), the presence of corticospinaltract fibers in the graft implies regeneration, with the caveatthat there could be sprouting from spared lateral and ventralcorticospinalfibers.

All three types of implants were found to promote spinal tissue sparing at 12 weeks after injury. The SC graft appears tobe more effective in reducing spinal tissue damage than the SC/OEGor OEG-only graft. SC-induced tissue sparing may have led to lessdamage to spinal white matter, which could explain the presenceof more propriospinal and brainstem projections distal to thegraft. SCs produce various growth factors such as nerve growthfactor (Bandtlow et al., 1987), brain-derived neurotrophic factor(Acheson et al., 1991; Meyer et al., 1992), ciliary neurotrophicfactor (Friedman et al., 1992; Meyer et al., 1992; Rende et al.,1992), and glial cell line-derived neurotrophic factor (Widenfalket al., 2001). Although OEG share many properties with SCs, theyare believed to be a distinct cell type (Lakatos et al., 2000).At present, convincing evidence that OEG harvested from the adultolfactory bulb produce neurotrophic factors is meager (Ramón-Cuetoand Avila, 1998; Kleitman and Bunge, 2000). Although reports havediffered on the production of neurotrophic factors by OEG (forreview, see Kleitman and Bunge, 2000), it is now clear that thesecells express several factors and their receptors (Boruch et al.,2001; Woodhall et al., 2001). We speculate that in the presentexperiment, SCs produced more supportive factors than OEG, whichmay have caused the observed difference in tissuesparing.

The secretion of various axonal growth-promoting factors has made the SC a widely used successful cellular substrate for repairstrategies in the adult spinal cord (Martin et al., 1991, 1996;Paino et al., 1994; Xu et al., 1995a,b, 1997, 1999; Chen et al.,1996; Montgomery et al., 1996; Guest et al., 1997; Oudega et al.,1997). OEG have also been shown to promote regeneration in differentinjury models in the adult rat spinal cord (Ramón-Cueto and Nieto-Sampedro,1994; Li et al., 1997, 1998; Ramón-Cueto et al., 1998, 2000).With OEG implanted in the cord beside a transection (Ramón-Cuetoet al., 2000) or a transection filled with an SC graft (Ramón-Cuetoet al., 1998), axons were found to cross the injury site and growinto the spinal cord. This finding may be related to the abilityof OEG to migrate away from the injury site into the spinal nervoustissue. SCs do not have such migratory ability (Xu et al., 1995a,1997; Iwashita et al., 2000).

In our transplantation model, the SCs and OEG were injected into a 1 week moderate contusion injury. Ongoing cytotoxic processeswithin the contusion environment may be harmful to the graftedcells. These processes include excitotoxic, inflammatory, proteolytic,and anoxic events, which are all components of progressive secondaryinjury (Tator and Fehlings, 1991; Anderson and Hall, 1993; Amarand Levy, 1999). Our results suggest that OEG may have been moresusceptible to these cytotoxic events than SCs. We were not ableto assess survival of OEG by morphological means because of thedifficulty in definitively identifying OEG without a specificlabel. Both SCs and OEG are stained by p75 antibody. OEG havebeen reported to closely resemble SCs when they remyelinate axonsin demyelinated cord (Imaizumi et al., 1998, 2000). We found onlya few cells that might be identified as OEG on the basis of thepattern of ensheathment of axon bundles observed in the electronmicroscope. At 12 weeks after injury, SC transplants were generallyin better continuity with the spinal tissue than OEG transplants.These observations may explain why SC transplants were more effectivein limiting injury-induced tissue damage, in promoting axonalsparing/regeneration, and in forming more myelin than an OEG transplant.Also, it should be kept in mind that the SC graft contained twiceas many SCs as the SC/OEGgraft.

It was not possible to decide whether the axons with peripheral-type myelin in the transplant area were myelinated by SCsor OEG. Axons with peripheral myelin were found in the nontransplantedanimals in this study as well as in several previous studies conductedin our laboratory as well as others, showing that SCs migrateinto lesion areas and myelinate axons there. In SC/OEG transplants,cells located in areas of central-type myelin near the implantationsite exhibited patches of basal lamina and extended processesthat meandered among clusters of axons but did not encircle themas SCs typically do (Fig. 3C). This type of ensheathment moreclosely resembles that of OEG in vivo (for review, see Kleitmanand Bunge, 2000). Possibly, these cells are OEG that migratedinto spinal tissue. Many papers have reported myelination by OEGin vivo (Franklin et al., 1996; Li et al., 1997, 1998; Imaizumiet al., 1998, 2000; Barnett et al., 2000; Kato et al., 2000).Possibly, less myelin was formed in OEG transplants in our studybecause the environment of the contusion cavity had damaged them.However, a recent study from our laboratory has shown that OEGdo not form myelin under the same culture conditions that arefavorable for SC myelination (Plant, Cuervo, Bates, Bunge, andWood, unpublished observations). In future studies, transplantationof labeled OEG is needed to prove the ability of OEG to producemyelin.

Both types of SC-containing grafts improved hindlimb function, but the SC-only graft was the only group consistently statisticallygreater than controls. This finding is in agreement with our observationthat SC grafts resulted in a higher number of spinal and supraspinalaxons reaching spinal segments distal to the grafted area comparedwith OEG grafts. It was shown previously that hindlimb recoveryafter an incomplete SCI depends on the number of spared and regenerateddescending axons from brainstem nuclei and cerebral cortex (Saruhashiand Young, 1994; Basso et al., 1996) and from local propriospinalaxons (Goldberger, 1988a,b; Helgren and Goldberger, 1993). Interestingly,it appears that only a small percentage of the descending brainstemaxons is needed to drive the segmental circuits involved in thegeneration of basic locomotion patterns (Helgren and Goldberger,1993; Basso et al., 1996; Ribotta et al., 2000). Thus the increasedsparing of tissue seen in the present study could explain theobserved improvement in functional recovery. Alternatively, theimprovement in behavioral outcome may have been caused, at leastin part, by remyelination of spared axons by the transplantedSCs. It was suggested previously that functional recovery seenin rats transplanted with embryonic stem cells was caused by remyelinationof axons by oligodendrocytes deriving from the grafted stem cells(McDonald et al., 1999). In the present study, it was not possibleto address this question because the transplanted cells were notprelabeled; even if the cells had been prelabeled, it would nothave been possible to identify the myelinated axon as spared orregenerated.

Both SCs and OEG have emerged as important candidates for future cell transplantation strategies in the injured adult spinalcord because of their axonal growth-promoting and myelinatingproperties. The present study directly compared these cell typesindividually and in combination and shows that SC grafts havethe greatest effect on protecting contused spinal tissue. Anotherclinically relevant advantage is that SCs can be obtained froma spinal cord injured person's peripheral nerve and produced invery large numbers in culture, which might allow autologous transplantationinto the injured human cord. A potential limitation of SC graftsis that they do not promote reentry of axons into the spinal cord,which is necessary for reestablishing axonal circuits that areinvolved in locomotion. OEG have shown promise in improving suchreentry, but we show here that they may be less effective in promotingaxonal growth and myelination than SCs when transplanted intothe contusion lesion. An alternative approach that would takeadvantage of the regeneration-promoting characteristics of bothcell types is to graft SC into the contusion lesion and OEG intothe adjacent spinal tissue. The restorative ability of this combinationstrategy in promoting axonal regeneration/sparing and improvinghindlimb function is currently being investigated in ourlaboratory.

  FOOTNOTES

Received Feb. 15, 2002; revised April 23, 2002; accepted May 9, 2002.

This work was funded by the Christopher Reeve Paralysis Foundation, National Institute of Health Grants NS09923 and PO1NS38665,and The Miami Project. M.O. is a Werner Heumann Memorial InternationalScholar. We are grateful to Andrew B. Weber and Pratik P. Desaifor histology; Annemarie N. Ali for help with image analysis;Roland Garcia-Rojas, Paulo Diaz, and Dr. Alexander E. Marcillofor inducing the contusion injury; and Yelena Pressman for cellculture. Lyudmila Rusakova, Rosemary Abril, and Kim Loor are thankedfor their help with animal care and behavioral testing, and RobertCamarena for assistance in photography. The gift of the 192 hybridomacell line from Dr. Eric Shooter (Stanford University) is gratefullyacknowledged.

Correspondence should be addressed to Dr. Mary Bartlett Bunge, The Miami Project to Cure Paralysis, University of Miami Schoolof Medicine, P.O. Box 016960, R-48, Miami, FL 33101. E-mail: mbunge{at}miami.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Acheson A, Barker PA, Alderson RF, Miller FD, Murphy RA (1991) Detection of brain-derived neurotrophic factor-like activity in fibroblasts and Schwann cells: inhibition by antibodies to NGF. Neuron 7:265-275[Web of Science][Medline].
Amar AP, Levy ML (1999) Pathogenesis and pharmacological strategies for mitigating secondary damage in acute spinal cord injury. Neurosurgery 44:1027-1039[Web of Science][Medline].
Anderson DK, Hall ED (1993) Pathophysiology of spinal cord trauma. Ann Emerg Med 22:987-992[Web of Science][Medline].
Barnett SC, Alexander CL, Iwashiti Y, Gilson JM, Crowther J, Clark L, Dunn LT, Papanastassiou V, Kennedy PGE, Franklin RJM (2000) Identification of a human olfactory ensheathing cell that can effect transplant-mediated remyelination of demyelinated CNS axons. Brain 123:1581-1588[Abstract/Free Full Text].
Bandtlow CE, Heumann R, Schwab ME, Thoenen H (1987) Cellular localization of nerve growth factor synthesis by in situ hybridization. EMBO J 6:891-899[Web of Science][Medline].
Basso DM, Beattie MS, Bresnahan JC (1995) A sensitive and reliable locomotor rating scale for open field testing in rats. J Neurotrauma 12:1-21[Web of Science][Medline].
Basso DM, Beattie MS, Bresnahan JC (1996) Graded histological and locomotor outcomes after spinal cord contusion using the NYU weight-drop device versus transection. Exp Neurol 139:244-256[Web of Science][Medline].
Bethea JR, Nagashima H, Acosta MC, Briceno C, Gomez F, Marcillo AE, Loor K, Green J, Dietrich WD (1999) Systemically administered interleukin-10 reduces tumor necrosis factor-alpha production and significantly improves functional recovery following traumatic spinal cord injury in rats. J Neurotrauma 16:851-863[Web of Science][Medline].
Blakemore SF, Smith PM, Franklin RJ (2000) Remyelinating the demyelinated CNS. Novartis Found Symp 231:289-298[Medline].
Boruch AV, Conners JJ, Pipitone M, Deadwyler G, Storer PD, Devries GH (2001) Neurotrophic and migratory properties of an olfactory ensheathing cell line. Glia 33:225-229[Web of Science][Medline].
Bunge MB (2001) Bridging areas of injury in the spinal cord. Neuroscientist 7:325-339[Abstract/Free Full Text].
Bunge MB, Kleitman N (1999) Neurotrophins and neuroprotection improve axonal regeneration into Schwann cell transplants placed in transected adult rat spinal cord. In: CNS regeneration: basic science and clinical aspects (Tuszinski MH, Kordower J, eds), pp 631-646. San Diego: Academic.
Bunge MB, Holets VR, Bates ML, Clarke TS, Watson BD (1994) Characterization of photochemically induced spinal cord injury in the rat by light and electron microscopy. Exp Neurol 127:76-93[Web of Science][Medline].
Bunge RP (1994) The role of the Schwann cell in trophic support and regeneration. J Neurol 242:S19-21[Web of Science][Medline].
Bunge RP, Puckett WR, Hiester ED (1997) Observations on the pathology of several types of human spinal cord injury, with emphasis on the astrocyte response to penetrating injuries. Adv Neurol 72:305-315[Medline].
Chen A, Xu XM, Kleitman N, Bunge MB (1996) Methylprednisolone administration improves axonal regeneration into Schwann cell grafts in transected adult rat thoracic spinal cord. Exp Neurol 138:261-276[Web of Science][Medline].
Cheng H, Cao Y, Olson L (1996) Spinal cord repair in adult paraplegic rats: partial restoration of hindlimb function. Science 273:510-513[Abstract].
Coumans JV, Lin TT, Dai HN, MacArthur L, McAtee M, Nash C, Bregman BS (2001) Axonal regeneration and functional recovery after complete spinal cord transection in rats by delayed treatment with transplants and neurotrophins. J Neurosci 21:9334-9344[Abstract/Free Full Text].
Franklin RJM, Barnett SC (2000) Olfactory ensheathing cells and CNS regeneration: the sweet smell of success? Neuron 28:15-18[Web of Science][Medline].
Franklin RJM, Gilson JM, Franceschini IA, Barnett SC (1996) Schwann cell-like myelination following transplantation of an olfactory bulb-ensheathing cell line into areas of demyelination in the adult CNS. Glia 17:217-224[Web of Science][Medline].
Friedman B, Scherer SS, Rudge JS, Helgren M, Morrisey D, McClain J, Wang DY, Wiegand SJ, Furth ME, Lindsay RM (1992) Regulation of ciliary neurotrophic factor expression in myelin-related Schwann cells in vivo. Neuron 9:295-305[Web of Science][Medline].
Gibson SJ, Polak JM, Bloom SR, Sabate IM, Mulderry PM, Ghatei MA, McGregor GP, Morrison JF, Kelly JS, Evans RM, Rosenfeld MG (1984) Calcitonin gene-related peptide immunoreactivity in the spinal cord of man and of eight other species. J Neurosci 4:3101-3111[Abstract].
Goldberger ME (1988a) Partial and complete deafferentation of cat hindlimb: the contribution of behavioral substitution to recovery of motor function. Exp Brain Res 73:343-353[Web of Science][Medline].
Goldberger ME (1988b) Spared-root deafferentation of a cat's hindlimb: hierarchical regulation of pathways mediating recovery of motor behavior. Exp Brain Res 73:329-342[Web of Science][Medline].
Grill R, Murai K, Blesch A, Gage FH, Tuszynski MH (1997) Cellular delivery of neurotrophin-3 promotes corticospinal axonal growth and partial functional recovery after spinal cord injury. J Neurosci 17:5560-5572[Abstract/Free Full Text].
Gruner JA (1992) A monitored contusion model of spinal cord injury in the rat. J Neurotrauma 9:123-126[Web of Science][Medline].
Guest JD, Rao A, Olson L, Bunge MB, Bunge RP (1997) The ability of human Schwann cell grafts to promote regeneration in the transected nude rat spinal cord. Exp Neurol 148:502-522[Web of Science][Medline].
Helgren ME, Goldberger ME (1993) The recovery of postural reflexes and locomotion following low thoracic hemisection in adult cats involves compensation by undamaged primary afferent pathways. Exp Neurol 123:17-34[Web of Science][Medline].
Hill CE, Beattie MS, Bresnahan JC (2001) Degeneration and sprouting of identified descending supraspinal axons after contusive spinal cord injury in the rat. Exp Neurol 171:153-169[Web of Science][Medline].
Imaizumi T, Lankford KL, Waxman SG, Greer CA, Kocsis JD (1998) Transplanted olfactory ensheathing cells remyelinate and enhance axonal conduction in the demyelinated dorsal columns of the rat spinal cord. J Neurosci 18:6176-6185[Abstract/Free Full Text].
Imaizumi T, Lankford KL, Kocsis JD (2000) Transplantation of olfactory ensheathing cells or Schwann cells restores rapid and secure conduction across the transected spinal cord. Brain Res 854:70-78[Web of Science][Medline].
Iwashita Y, Kawaguchi S, Murata M (1994) Restoration of function by replacement of spinal cord segments in the rat. Nature 367:167-170[Medline].
Iwashita Y, Fawcett JW, Crang AJ, Franklin RJ, Blakemore WF (2000) Schwann cells transplanted into normal and X-irradiated adult white matter do not migrate extensively and show poor long-term survival. Exp Neurol 164:292-302[Web of Science][Medline].
Jones LL, Oudega M, Bunge MB, Tuszynski MH (2001) Neurotrophic factors, cellular bridges and gene therapy for spinal cord injury. J Physiol (Lond) 533:83-89[Abstract/Free Full Text].
Kakulas BA (1999) A review of the neuropathology of human spinal cord injury with emphasis on special features. J Spinal Cord Med 22:119-124[Medline].
Kato T, Honmou O, Uede T, Kocsis JD (2000) Transplantation of human olfactory ensheathing cells elicits remyelination of demyelinated rat spinal cord. Glia 30:209-218[Web of Science][Medline].
Kleitman N, Bunge MB (2000) Olfactory ensheathing glia: their application to spinal cord regeneration and remyelination strategies. Topics Spinal Cord Inj Rehab 6:65-81.
Lakatos A, Franklin RJM, Barnett SC (2000) Olfactory ensheathing cells and Schwann cells differ in their vitro interactions with astrocytes. Glia 32:214-225[Web of Science][Medline].
Li Y, Field PM, Raisman G (1997) Repair of adult rat corticospinal tract by transplants of olfactory ensheathing cells. Science 277:2000-2002[Abstract/Free Full Text].
Li Y, Field PM, Raisman G (1998) Regeneration of adult rat corticospinal axons induced by transplanted olfactory ensheathing cells. J Neurosci 18:10514-10524[Abstract/Free Full Text].
Liu Y, Kim D, Himes BT, Chow SY, Schallert T, Murray M, Tessler A, Fischer I (1999) Transplants of fibroblasts genetically modified to express BDNF promote regeneration of adult rat rubrospinal axons and recovery of forelimb function. J Neurosci 19:4370-4387[Abstract/Free Full Text].
Martin D, Schoenen J, Delrée P, Leprince P, Rogister B, Moonen G (1991) Grafts of syngenic cultured, adult dorsal root ganglion-derived Schwann cells to the injured spinal cord of adult rats: preliminary morphological studies. Neurosci Lett 124:44-48[Web of Science][Medline].
Martin D, Robe P, Franzen R, Delree P, Schoenen J, Stevenaert A, Moonen G (1996) Effects of Schwann cell transplantation in a contusion model of rat spinal cord injury. J Neurosci Res 45:588-597[Web of Science][Medline].
McDonald JW, Liu XZ, Qu Y, Liu S, Mickey SK, Turetsky D, Gottlieb DI, Choi DW (1999) Transplanted embryonic stem cells survive, differentiate and promote recovery in injured rat spinal cord. Nat Med 5:1410-1412[Web of Science][Medline].
Menei P, Montero-Menei C, Whittemore SR, Bunge RP, Bunge MB (1998) Schwann cells genetically modified to secrete human BDNF promote enhanced axonal regrowth across transected adult rat spinal cord. Eur J Neurosci 10:607-621[Web of Science][Medline].
Meyer M, Matsuoka I, Wetmore C, Olson L, Thoenen H (1992) Enhanced synthesis of brain-derived neurotrophic factor in the lesioned peripheral nerve: different mechanisms are responsible for the regulation of BDNF and NGF mRNA. J Cell Biol 119:45-54[Abstract/Free Full Text].
Montgomery CT, Tenaglia EA, Robson JA (1996) Axonal growth into tubes implanted within lesions in the spinal cords of adult rats. Exp Neurol 137:277-290[Web of Science][Medline].
Morrissey TK, Kleitman N, Bunge RP (1991) Isolation and functional characterization of Schwann cells derived from adult peripheral nerve. J Neurosci 11:2433-2442[Abstract].
Newton BW, Hamill RW (1988) The morphology and distribution of rat serotoninergic intraspinal neurons: an immunohistochemical study. Brain Res Bull 20:349-360[Web of Science][Medline].
Oudega M, Varon S, Hagg T (1994) Regeneration of adult rat sensory axons into intraspinal nerve grafts: promoting effects of conditioning lesion and graft predegeneration. Exp Neurol 129:194-206[Web of Science][Medline].
Oudega M, Xu XM, Guenard V, Kleitman N, Bunge MB (1997) A combination of insulin-like growth factor-I and platelet-derived growth factor enhances myelination but diminishes axonal regeneration into Schwann cell grafts in the adult rat spinal cord. Glia 19:247-258[Web of Science][Medline].
Oudega M, Vargas CG, Weber AB, Kleitman N, Bunge MB (1999) Long-term effects of methylprednisolone following transection of adult rat spinal cord. Eur J Neurosci 11:2453-2464[Web of Science][Medline].
Paino CL, Fernandez-Valle C, Bates ML, Bunge MB (1994) Regrowth of axons in lesioned adult rat spinal cord: promotion by implants of cultured Schwann cells. J Neurocytol 23:433-452[Web of Science][Medline].
Plant GW, Ramón-Cueto A, Bunge MB (2001) Transplantation of Schwann cells and ensheathing glia to improve regeneration in adult spinal cord. In: Axonal regeneration in the central nervous system (Ingoglia NA, Murray M, eds), pp 529-561. New York: Marcel Dekker.
Raisman G (2001) Olfactory ensheathing cells: another miracle cure for spinal cord injury? Nat Neurosci 2:369-373.
Ramón-Cueto A (2000) Olfactory ensheathing glia transplantation into the injured spinal cord. Prog Brain Res 128:265-272[Web of Science][Medline].
Ramón-Cueto A, Avila J (1998) Olfactory ensheathing glia: properties and function. Brain Res Bull 46:175-187[Web of Science][Medline].
Ramón-Cueto A, Nieto-Sampedro M (1994) Regeneration into the spinal cord of transected dorsal root axons is promoted by ensheathing glia transplants. Exp Neurol 127:232-244[Web of Science][Medline].
Ramón-Cueto A, Plant GW, Avila J, Bunge MB (1998) Long-distance axonal regeneration in the transected adult rat spinal cord is promoted by olfactory ensheathing glia transplants. J Neurosci 18:3803-3815[Abstract/Free Full Text].
Ramón-Cueto A, Cordero MI, Santos-Benito FF, Avila J (2000) Functional recovery of paraplegic rats and motor axon regeneration in their spinal cords by olfactory ensheathing glia. Neuron 25:425-435[Web of Science][Medline].
Rende M, Muir D, Ruoslahti E, Hagg T, Varon S, Manthorpe M (1992) Immunolocalization of ciliary neuronotrophic factor in adult rat sciatic nerve. Glia 5:25-32[Web of Science][Medline].
Ribotta MG, Provencher J, Feraboli-Lohnherr D, Rossignol S, Privat A, Orsal D (2000) Activation of locomotion in adult chronic spinal rats is achieved by transplantation of embryonic raphe cells reinnervating a precise lumbar level. J Neurosci 20:5144-5152[Abstract/Free Full Text].
Saruhashi Y, Young W (1994) Effect of mianserin on locomotory function after thoracic spinal cord hemisection in rats. Exp Neurol 129:207-216[Web of Science][Medline].
Takami T, Oudega M, Bethea JR, Wood PM, Kleitman N, Bunge MB (2002) Methylprednisolone and interleukin-10 reduce gray matter damage in the contused Fischer rat thoracic spinal cord but do not improve functional outcome. J Neurotrauma 19:653-666[Web of Science][Medline].
Tator CH (1995) Update on the pathophysiology and pathology of acute spinal cord injury. Brain Pathol 5:407-413[Web of Science][Medline].
Tator CH, Fehlings MG (1991) Review of the secondary injury theory of acute spinal cord trauma with emphasis on vascular mechanisms. J Neurosurg 75:15-26[Web of Science][Medline].
West MJ (1993) New stereological methods for counting neurons. Neurobiol Aging 14:275-285[Web of Science][Medline].
Widenfalk J, Lundstromer K, Jubran M, Brene S, Olson L (2001) Neurotrophic factors and receptors in the immature and adult spinal cord after mechanical injury or kainic acid. J Neurosci 21:3457-3475[Abstract/Free Full Text].
Woodhall E, West AK, Chuah MI (2001) Cultured olfactory ensheathing cells express nerve growth factor, brain-derived neurotrophic factor, glia cell line-derived neurotrophic factor and their receptor. Mol Brain Res 88:203-213[Medline].
Xu XM, Guenard V, Kleitman N, Bunge MB (1995a) Axonal regeneration into Schwann cell-seeded guidance channels grafted into transected adult rat spinal cord. J Comp Neurol 351:145-160[Web of Science][Medline].
Xu XM, Guenard V, Kleitman N, Aebischer P, Bunge MB (1995b) A combination of BDNF and NT-3 promotes supraspinal axonal regeneration into Schwann cell grafts in adult rat thoracic spinal cord. Exp Neurol 134:261-272[Web of Science][Medline].
Xu XM, Chen A, Guenard V, Kleitman N, Bunge MB (1997) Bridging Schwann cell transplants promote axonal regeneration from both the rostral and caudal stumps of transected adult rat spinal cord. J Neurocytol 26:1-16[Web of Science][Medline].
Xu XM, Zhang SX, Li H, Aebischer P, Bunge MB (1999) Regrowth of axons into the distal spinal cord through a Schwann cell-seeded mini-channel implanted into hemisected adult rat spinal cord. Eur J Neurosci 11:1723-1740[Web of Science][Medline].

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