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Anterograde tracing of the sensory and motor CST. Locations of forelimb sensory and motor cortices were determined by measuring positions on the skull relative to bregma (Neafsey et al., 1986
The Journal of Neuroscience, August 15, 2002, 22(16):7097-7110
Long-Lasting Sprouting and Gene Expression Changes Induced by the Monoclonal Antibody IN-1 in the Adult Spinal Cord
Florence M. Bareyre, Brigitte Haudenschild, and Martin E. Schwab Brain Research Institute, Department of Biology, University of Zürich, ETH Zürich, 8057 Zürich, Switzerland
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Lesion-induced plasticity of the rat corticospinal tract (CST) decreases postnatally, simultaneously with myelin appearance. In adult rats, compensatory sprouting can be induced by the monoclonal antibody (mAb) IN-1 raised against the growth inhibitory protein Nogo-A. In this study, we examined separately the fate of sensory and motor corticospinal fibers after mAb IN-1 application. Intact adult rats treated with the IN-1 antibody exhibited an increase of aberrant CST projections, i.e., sensory fibers projecting into the ventral horn and motor fibers projecting dorsally. Unilateral lesion of the CST [pyramidotomy (PTX)] in the presence of mAb IN-1 triggered a progressive reorganization of the sprouting of the remaining CST across the midline, with sensory fibers projecting gradually into the denervated dorsal horn and motor fibers projecting into the denervated ventral horn. In unilaterally denervated spinal cords, aberrant sprouts were only transient and disappeared by 6 weeks, whereas midline crossing fibers ending in the appropriate target region were stabilized and persisted over the entire study period. Within the spinal cord, IN-1 antibody treatment was associated with upregulation of growth factors (BDNF, VEGF), growth-related proteins (actin, myosin, GAP-43), and transcription factors (STATs), whereas pyramidotomy induced an enhanced expression of guidance molecules (semaphorins and slits) as well as neurotrophic factors (BDNF, IGFs, BMPs). These gene expression changes may contribute to attraction, guidance, and stabilization of sprouting CST fibers.
Key words: corticospinal tract; GAP-43; gene expression; Nogo-A; plasticity; pyramidotomy; sprouting
INTRODUCTION
The pyramidal tract, originating in the sensory and motor cortex, is the only direct cortical pathway to the spinal cord. In cats (Fetz, 1968
), primates (Coulter and Jones, 1977
The present data show that, also in the rat, projections of the sensory and motor cortex terminate precisely within the spinal dorsal and ventral horn, respectively. The mAb IN-1 triggers sprouting of CST fibers in intact rats that is aberrant but transitory. After unilateral PTX, mAb IN-1 induces compensatory sprouting across the midline that is target specific and mostly stable, suggesting lesion-induced CST sprouting and rewiring. The sprouting effect of the IN-1 antibody was associated with increased growth-related protein expression (among others), whereas the PTX-driven compensatory reorganization was paralleled by enhanced expression of certain guidance molecules.
MATERIALS AND METHODS
Male adult Lewis rats (200-220 gm) were used in this study. Anatomical and histochemical data were obtained from 120 animals with successful labeling of the corticospinal axons, and gene expression data were obtained from 30 animals.
Anatomical organization and reorganization of CST projections
Pyramidotomy and antibody application. Rats were anesthetized using a combination of Hypnorm (0.3 mg/kg, s.c; Roche, Basel, Switzerland) and Dormicum (0.6 mg/kg, s.c.; Roche). A right unilateral lesion of the CST at the level of the medulla oblongata was performed by using a ventral approach (Thallmair et al., 19984 mm caudal, 5 mm lateral to bregma, 5 mm depth). Cyclosporin A (5 mg/kg body weight, i.p.; Sandimmun, Novartis, Basel, Switzerland) was given daily during the first 5 d postoperatively to allow the transplant to grow and secrete the antibody. Pyramidotomized animals receiving no cells were also generated as a control baseline as well as intact animals without pyramidotomy but with antibody transplant only. After surgery, all animals were kept on a heating plate (38°C) until fully awake and received Carpofen (Rimadyl, 5 mg/kg, i.m.; Pfizer, Karlsruhe, Germany) for 2 d.
Gene expression changes after IN-1 treatment and pyramidotomy
Pyramidotomy and antibody application. A first group of rats underwent a right-side pyramidotomy as described above. Sham animals with a laminectomy only were generated in parallel. A second group of rats received hybridoma cells secreting either the mAb IN-1 or the anti-HRP control antibody as described above (no lesion). Control animals receiving no cells were generated in parallel as a baseline. A third group of rats were pyramidotomized, and hybridoma secreting either IN-1 or anti-HRP antibodies were implanted. At 48 hr, 1 week, or 4 weeks after injury (n = 3 per group) rats were decapitated, and the spinal cords were quickly dissected on a cold plate. Three millimeter transverse sections were taken at the cervical enlargement, and for the lesion experiments, the lesioned side was separated from the unlesioned side. Samples of three rats per group were pooled, and the tissue was immediately frozen in isopentane (-actin, GADPH, hexokinase, 5S rRNA) which served as internal controls. Several human, murine, and yeast probe sets on each chip served as negative controls, and externally spiked bacterial bioB, bioC, bioD, and Cre served as positive hybridization controls. The gene chips were scanned with a probe array scanner, and the results were subsequently analyzed using the Affymetrix GeneChip analysis followed by the DNA-Chip Analyzer (dChip) software from Harvard University (Li and Wong, 2001
Validation of the gene chip data: RNase protection assay
The same total RNA extracted previously from spinal cords of IN-1 or anti-HRP-treated rats or control rats for the gene chip analysis was used. Cloning of rat STAT1, GAP43, vimentin, neurofilament light, and TIMP1 PCR probes. The rat cDNA sequences of STAT1, GAP43, vimentin, neurofilament light (NFL), and TIMP1 were analyzed by using the program Oligo (Primer Analysis Software, Cascade, CO) with regard to their suitability for primer selection. The following primers were used and synthesized (Microsynth, Balgach, Switzerland): GAP43, sense: 5'-CAG CCA CCA GCC CTA AGG-3', antisense: 5'-TCA GTG ACA GCA GCA GGC-3'; STAT1, sense: 5'-CCA TCC GCT TCC ATG ACC-3', antisense: 5'-GTT TCT GGT CGC TCT TCG-3'; vimentin, sense: 5'-CCG CAC CTA CAG CCT AGG-3', antisense: 5'-TCT GCT GCT CGA GGA AGC-3'; TIMP1, sense: 5'-AGC TTC CTG GTT CCC TGG-3', antisense: 5'-GGT AGC CCT TCT CAG AGC-3'; NFL, sense: 5'-TCG ACC TCC TAC AAG CGG-3', antisense: 5'-ACC AAC AGC TCG GCT TCC-3'. Riboprobes were transcribed from linearized templates prepared in Bluescript plasmid using the T7 in vitro transcription system (Stratagene) and labeled with 32P uridine triphosphate. Isolation and analysis of RNA. Ribonuclease protection assays were performed using the Ribo Quant Kit (PharMingen). For each reaction, probes (4.6 105 cpm) were hybridized against 10 µg of spinal cord RNA and RNase-treated according to the manufacturer's instructions. tRNA was used as negative control. GAPDH was used as an internal standard for the amount and integrity of the RNA preparations. Protected fragments were separated on a 5% sequencing gel. Radioactivity in each band was quantified using a PhosphorImager (Amersham Biosciences). The level of expression of each RNA was calculated as a ratio of the protected RNA fragment to the intensity of the protected GAPDH fragment. The intensity of the GAPDH fragment was roughly equivalent in all the samples, showing that GAPDH expression was independent of any treatment applied. Relative expression values (fold changes) were calculated by dividing the level in antibody-treated rats by the level in control untreated rats. Experiments were performed three to six times.GAP-43 immunohistochemical staining and analysis
Spinal cord sections were collected and mounted as explained previously. Primary antibodies were used at a dilution of 1:1000 (GAP-43, Chemicon) and 1:40 (vimentin, Chemicon). Immunohistochemistry for each antibody was performed on all sections at the same time. Sections were incubated in methanol containing 5% H2O2 to quench endogenous peroxidases, washed in 0.1 M Tris buffer, pH 7.4, and blocked in TBS-T × 5% normal horse serum. All antibodies were diluted in TBS-T × 5% normal horse serum and AB complex in 0.1 M Tris buffer. Sections were incubated overnight with primary antibody at 4°C and incubated at room temperature for 1 hr with appropriate biotinylated secondary antibodies [biotin-SP donkey anti-rabbit IgG (Jackson ImmunoResearch; West Grove, PA; dilution, 1:1000) for polyclonal GAP-43; biotin-SP rabbit anti-goat IgG (Vector Laboratories; dilution, 1:300) for vimentin]. Sections were then incubated at room temperature for 1 hr with AB reagent (Vector Laboratories) and developed with 3,3'-diaminobenzidine (Sigma). Sections were dehydrated and coverslipped. Application of control serum instead of primary antibody on selected sections of rat tissue provided a negative control. Intensity of the stainings was quantified by trained personnel blinded to treatment and injury status of the animals. Under low-power light microscopy, an image of the whole cervical cord was captured by video camera, and the borders of the spinal cord were traced manually. The pixels per area were then automatically calculated using an image analysis software routine (MCID/M4, Imaging Research, St. Catherines, Ontario, Canada) after defining a threshold for the background that was kept identical throughout the analysis. A ratio between animals treated with IN-1 and anti-HRP antibodies was then calculated.Statistical evaluation
All data were analyzed using a nonparametric Kruskall-Wallis test in cases of multiple comparisons followed by nonparametric Mann-Whitney tests in cases of paired comparisons. Significance was taken at p < 0.05 and indicated with an asterisk.
RESULTS
Specific topographic organization of sensory and motor corticospinal projections in normal rats
Both forelimb sensory and motor cortex give rise to corticospinal axons that reach their target in the gray matter of the cervical enlargement. Most of the corticospinal fibers cross in the pyramidal decussation and enter the ventral region of the dorsal columns (O'Leary and Koester, 1993
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Figure 1. Photomicrographs and camera lucida reconstructions of corticospinal projections to the cervical spinal cord. A, Projections of sensory CST fibers to the dorsal horn as shown by injections of BDA into the sensory cortex. B, Projections of motor CST fibers to the intermediate layers and the ventral horn as shown by injections of BDA into the motor cortex. Scale bar, 250 µm.
Sprouting of corticospinal fibers after monoclonal antibody IN-1 administration in intact adult animals
Animals sustaining a laminectomy without lesion of the pyramid were implanted with either IN-1 or anti-HRP antibody secreting cells, and sensory or motor corticospinal projections in the cervical enlargement were analyzed by comparison to control rats receiving no cells. Quantification of sprouting fibers was conducted 2 weeks after antibody application in two ways: (1) fibers topographically projecting across the midline and (2) fibers aberrantly sprouting across lamina V (i.e., motor fibers entering laminas III and IV and sensory fibers entering laminas VI and VII). When BDA was injected into the sensory cortex, no midline-crossing fibers could be detected in any of the treatment groups. In particular, animals implanted with anti-HRP or IN-1 antibodies were not statistically different (p > 0.05) from control animals (Fig. 2A). Similarly, when BDA was injected into the motor cortex, no midline-crossing fibers were observed after anti-HRP antibody treatment (p > 0.05) (Fig. 2B). However, the number of midline-crossing fibers was slightly higher after IN-1 monoclonal antibody treatment (p < 0.05; IN-1 antibody-treated rats vs anti-HRP antibody-treated rats or control rats) (Fig. 2B).
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Figure 2. Percentage of CST fibers sprouting across lamina V or across the midline in the cervical spinal cord in nonlesioned animals. A, Sensory CST projections. B, Motor CST projections. Monoclonal antibody IN-1 induced both sensory and motor fibers to sprout across lamina V when compared with anti-HRP mAb treatment. In addition, IN-1 induced motor fibers to cross the midline of the spinal cord. *IN-1 or HRP antibody-treated rats significantly different from control non-treated rats (p < 0.05). #IN-1 antibody-treated animals significantly different from anti-HRP antibody-treated rats (p < 0.05). Black diamonds indicate individual values.
When invasion of the ventral horn by sensory fibers was evaluated, no statistical differences were seen between anti-HRP antibody-treated rats and control rats. Conversely, IN-1 antibody-treated rats demonstrated significantly more sensory fibers entering the ventral horn than anti-HRP antibody-treated rats and control rats (p < 0.05 and p < 0.01, respectively (Figs. 2A, 3A,B). When motor CST fibers were observed for their ability to invade the dorsal horn, anti-HRP and IN-1 antibody-treated animals showed significantly more ectopic fibers than control animals (p < 0.05 in both cases) (Fig. 2B). In addition, IN-1 antibody-treated animals demonstrated a significantly higher (p < 0.05) (Figs. 2B, 3C,D) number of motor CST fibers invading the dorsal horn than anti-HRP antibody-treated animals. These observations show that monoclonal antibody IN-1 induces sprouting of sensory and motor CST fibers in the noninjured adult rat spinal cord.
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Figure 3. Photomicrographs of fibers sprouting across lamina V in nonlesioned animals. A, No invasion of the ventral horn by sensory fibers after anti-HRP treatment. B, Invasion of the ventral horn by sensory fibers (arrows) after IN-1 treatment. C, No invasion of the dorsal horn by motor fibers after anti-HRP treatment. D, Pronounced invasion of the dorsal horn by motor fibers (arrows) after IN-1 treatment. Scale bar, 250 µm.
Long-term topographic reorganization of adult corticospinal fibers after pyramidotomy and implantation of monoclonal antibody IN-1 secreting cells
The CST was removed unilaterally by transection at the entry into the pyramidal decussation (pyramidotomy). Reorganization of the fibers was assessed 1, 2, and 6 weeks after pyramidotomy in rats implanted with IN-1 or anti-HRP antibody-secreting cells or in control rats (lesion only). As previously, quantification of the sprouting fibers was conducted by counting (1) fibers topographically projecting across the midline and (2) fibers aberrantly sprouting into the inappropriate horn (i.e., motor fibers entering laminas III and IV and sensory fibers entering laminas VI and VII). Because we counted only fibers visibly crossing the midline, we did not include ipsilateral ventral fibers that were also reported by Weidner et al. (2001)
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Figure 4. Long-term reorganization of motor (A, B) or sensory (C, D) CST fibers in pyramidotomized animals. IN-1 treatment induced more motor fibers to sprout dorsally (A) and more sensory fibers to invade the ventral horn on the intact side 2 weeks after pyramidal tract lesion than anti-HRP antibody treatment (C). IN-1 also induced motor and sensory fibers to cross the midline 1 and 2 weeks after pyramidal tract lesion, in contrast to anti-HRP treatment (B, D). Sensory sprouts retracted, but motor fibers grew across the midline to the denervated cord and were stable at 6 weeks after injury (B). *Anti-HRP-treated rats significantly different from control nontreated rats (p < 0.05). #IN-1 antibody-treated rats significantly different from anti-HRP-treated rats (p < 0.05).
At 2 weeks after injury, anti-HRP antibody-treated animals showed an increased number of sprouting fibers when compared with control animals in all parameters examined (p < 0.05 in all cases) except for ectopic sensory CST projections. IN-1 antibody-treated animals showed significantly more midline crossing fibers than control animals in all parameters examined (p < 0.05 in all cases) (Fig. 4). In addition, IN-1 antibody-treated rats exhibited significantly more sensory and motor fibers topographically crossing the midline to invade the contralateral dorsal and ventral horn, respectively, than anti-HRP antibody-treated animals (p < 0.01) (Fig. 5A-D). When aberrant sprouting of sensory fibers (into the ventral horn) was considered, a small but statistical increase was also shown after IN-1 antibody treatment when compared with anti-HRP antibody treatment 2 weeks after pyramidotomy.
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Figure 5. Photomicrographs of fibers sprouting across the spinal cord midline 2 weeks after pyramidotomy. A, Topographic sprouting of a sensory CST fiber (arrow) into the contralateral, denervated dorsal horn after IN-1 mAb treatment. B, Absence of sprouting of sensory fibers after anti-HRP treatment. C, Topographic sprouting of motor CST fibers into the contralateral ventral horn (arrows) after IN-1 mAb treatment. D, Virtual absence of sprouting (very rare fibers) of motor fibers in anti-HRP treatment. Scale bar, 250 µm.
At 6 weeks after injury, animals treated with anti-HRP antibody were similar to control animals in all parameters examined. Conversely, IN-1 antibody-treated animals exhibited a significantly higher sprouting index when compared with control animals (p < 0.05) in all cases. In addition, IN-1 antibody-treated animals exhibited significantly more motor fibers topographically crossing the midline than anti-HRP antibody-treated animals (p < 0.01), indicating that the sprouts triggered by the antibody IN-1 at 1 or 2 weeks after the lesion were stable over an extended period of time.
Motor corticospinal fibers persist over time and arborize
We estimated the arborization complexity of motor CST fibers grown across the midline into the denervated ventral horn by a 0-4 point score (0, no branches/4, highly branched terminal arbors) at 1, 2, and 6 weeks after pyramidotomy and anti-HRP or IN-1 antibody application. We observed that at 1 and 2 weeks, scores were low, and the branching complexity after IN-1 treatment was not statistically different from the complexity of the rare fibers seen after anti-HRP treatment. Conversely, 6 weeks after the injury, a significantly higher arborization complexity was detected in IN-1 antibody-treated animals when compared with the very few fibers seen after anti-HRP treatment (p < 0.05) (Fig. 6), indicating that the persisting fibers acquired a more pronounced complexity (Fig. 6A,B).
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Figure 6. Photomicrographs of the arbor complexity of motor fibers grown across the midline into the denervated ventral horn at 2 weeks (A) and 6 weeks (B) after pyramidotomy and monoclonal IN-1 antibody treatment. C, Complexity of axonal arbors of motor CST fibers 1, 2, and 6 weeks after pyramidotomy and antibody treatment. Six weeks after the injury, IN-1-treated animals had higher scores than anti-HRP-treated animals. Scores are described in Materials and Methods. *IN-1-treated rats significantly different from anti-HRP-treated rats (p < 0.05). Black and white diamonds represent individual values. Scale bar, 200 µm.
Gene expression changes in the cervical spinal cord after pyramidotomy and IN-1 monoclonal antibody application
Of 8784 oligonucleotide probe sets present on the Affymetrix U34A chips, 3601-4589 (41-52%) were identified as present in control as well as in injured or antibody-treated rats. Replicate chips, done for each experimental point, gave extremely similar results (R2 above 0.95 after paired comparison analysis).
Gene expressions changes in the cervical spinal cord after pyramidotomy: 48 hr and 1 week
In the denervated cervical spinal cord, at 48 hr after pyramidotomy, the major upregulated genes were IGFII, IGF receptor, and binding protein, BMP-2, components of the pro-apoptotic cascade (BAD/caspases/c-jun), some extracellular matrix (ECM) proteins (laminin/decorin/collagen), and enzymes of the cell metabolism (Table 1). Some metabolic genes were also downregulated (lipooxygenase/acyl-coA synthase). At 1 week after pyramidotomy, we found prominent upregulation of growth factors and their receptors (trkB/VEGF receptor/BDNF), the axonal guidance molecules (semaphorin 3/slit1), and ECM proteins (decorin/lumican/collagens). Cytoskeletal proteins (actin/myosin/MAP2), GABA receptors, and several ion transporters (Cl/HCO3
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Table 1. Differential gene expression in the cervical cord when the denervated side was compared with the intact side of the cervical spinal cord (3-mm-thick sections; three rats pooled) 48 hr and 1 week after pyramidotomy Gene expressions altered in the cervical spinal cord after monoclonal antibody IN-1 treatment: 48 hr and 1 week
In the cervical spinal cord, at 48 hr, when unlesioned animals treated with IN-1 were compared with animals treated with anti-HRP antibody, the major upregulated genes were for cytoskeletal proteins (actin/myosin), creatin kinase, and calcium-binding proteins, genes related to inflammation and collagens (Table 2). At 1 week, when animals treated with monoclonal antibody IN-1 were compared with animals treated with anti-HRP antibody, cytoskeletal proteins (actin/myosin/troponin), the growth-associated protein GAP-43, and the growth factors (BDNF/VEGF) were upregulated several-fold as were transcription factors (STAT1/MRP14), the SNARE protein VAMP1, synapsin3a, creatine kinase, the inhibitor of metalloproteinases TIMP1, and collagens (Table 2). The major downregulated genes were related to immune functions and components of the complement system (Table 2).
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Table 2. Differential gene expression in the cervical cord 48 hr and 1 week after IN-1 or anti-HRP antibody application in intact adult rats Genes altered in the cervical spinal cord after pyramidotomy and IN-1 or anti-HRP antibody treatment: 1 and 4 weeks
At 1 week, when the denervated spinal cord of animals treated with monoclonal antibody IN-1 were compared with the denervated spinal cord of animals treated with anti-HRP antibody, the major upregulated genes were cytoskeletal proteins (MAP2/actin), the growth-associated protein GAP-43, growth factors/receptors (BDNF/TrkB/IGFI and II/GDNF receptor/glia maturation factor/endothelin receptor), semaphorin 3a, ECM, and membrane proteins (NCAM/F3/APP/collagen/laminin/TIMP1), and transcription factors (STATs) (Table 3). The major downregulated genes were immune response-related molecules such as MHC Class II and components of the complement system (Table 3). At 4 weeks, when the denervated spinal cord of animals treated with monoclonal antibody IN-1 were compared with the denervated spinal cord of animals treated with anti-HRP antibody, only very few gene expression changes were observed. The major upregulated gene was BDNF. Actin and collagen were downregulated (Table 3).
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Table 3. Non-exhaustive differential gene expression in the cervical cord 1 week and 4 weeks after both pyramidotomy and IN-1 or anti-HRP antibody application RNase protection assays
RNase protection assays confirmed the increased expression of GAP-43, TIMP1, and STAT1 and the unaltered expression of NFL and vimentin in rats treated for 7 d with mAb IN-1 compared with anti-HRP antibody (Fig. 7). The magnitude of the changes between control antibody and IN-1 antibody-treated rats were in the same range as those found with the gene chip technology for most of the studied genes.
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Figure 7. Results from RNase protection assays done on cervical spinal cord tissue and compared with results from the analysis with the Affymetrix gene chip. Five different genes were similarly expressed using both assays in rats treated with mAb IN-1 for 7 d compared with rats treated with an anti-HRP antibody.
Immunoreactivity of GAP-43 after pyramidotomy and IN-1 and anti-HRP antibody treatments
We quantified the immunoreactivity of the growth-related protein GAP-43 and of vimentin in the cervical cord after IN-1 or anti-HRP treatments in unlesioned rats and in rats 1, 2, and 6 weeks after pyramidotomy. IN-1 antibody-treated animals exhibited a twofold increase in GAP-43 immunoreactivity in unlesioned animals as well as 1 and 2 weeks after the lesion and IN-1 antibody treatment when compared with their matching controls (Fig. 8). No differences in GAP-43 immunoreactivity were found 6 weeks after the lesion when IN-1 antibody-treated animals were compared with anti-HRP animals. Vimentin immunoreactivity was unchanged for the entire study period when IN-1 antibody-treated animals were compared with anti-HRP antibody-treated animals.
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Figure 8. Photomicrographs of GAP-43 immunoreactivity in the denervated cervical spinal cord. IN-1 antibody treatment (B) increased GAP-43 immunoreactivity (twofold by densitometry) in unlesioned animals when compared with unlesioned animals treated with anti-HRP antibody (A). GAP-43 immunoreactivity was also increased (2.5-fold) 2 weeks after pyramidotomy and IN-1 antibody treatment (D) compared with lesioned anti-HRP antibody-treated rats (C). Scale bar, 850 µm.
DISCUSSION
The present results show that the monoclonal antibody IN-1 induces transitory sprouting of CST fibers in the normal adult rat spinal cord associated with enhanced gene expression in particular of cytoskeletal and growth-related proteins and transcription factors. The IN-1 antibody combined with a discrete unilateral pyramidal tract lesion further enhanced the sprouting, especially of motor CST fibers, which formed stable, highly branched projections in the denervated ventral horn. This reorganization was associated with an upregulation of genes such as growth factors/receptors and guidance molecules.
The corticospinal tract is topographically organized
Electrophysiological mapping of the rat sensorimotor cortex has shown a clear topographic organization of somatosensory and motor areas (Donoghue and Wise, 1982
The monoclonal antibody IN-1 enhances sprouting in normal adult spinal cord
The monoclonal antibody IN-1, raised against the growth inhibitory protein Nogo-A (Caroni and Schwab, 1988a
The mAb IN-1 enhances long-term compensatory sprouting after unilateral lesion of the pyramidal tract
After unilateral pyramidotomy in adult rats and subsequent treatment with the mAb IN-1, sprouting of the remaining, intact corticospinal tract has previously been observed (Thallmair et al., 1998
The presence of specific molecular cues appearing in the spinal cord as a consequence of the denervation was fully confirmed by the Affymetrix gene chip analysis. In addition to growth-related proteins (GAP-43), growth factors (BDNF, VEGF), and transcription factors (STATs) that were upregulated after IN-1 treatment alone, guidance molecules from the semaphorin (3 and 6) and slit family, additional growth factors and receptors (IGFs, BMPs, GDNF receptor) were upregulated after a pyramidotomy. As reflected by the gene expression pattern after combined pyramidotomy and IN-1 cell implantation, it seems likely that two mechanisms must be present for a meaningful compensatory reorganization of CST fibers across the midline of the spinal cord: the more general growth promoting effects of the IN-1 antibody and the denervation-induced modulation of guidance molecules and growth factors that allow fibers to reinnervate denervated target in an organized manner. In this plasticity model, the appearance of target-specific guidance information generated by the lesion seems to channel sprouting axons to reinnervate denervated targets as previously reported in regeneration studies (Wizenmann et al., 1993
In conclusion, we demonstrated the clear endogenous sprouting effect of IN-1 antibody that, in combination with a unilateral lesion of the pyramids, greatly enhances the compensative capacity of adult motor CST fibers to reorganize in a target-specific manner. Such processes will be of importance for long-term functional recovery after CNS lesion.
FOOTNOTES Received March 19, 2002; revised May 21, 2002; accepted May 29, 2002.
This work was supported by the Swiss National Foundation (Grant 31-63633.00) and the Christopher Reeve Paralysis Foundation (Spinal Cord Consortium, Springfield, NJ). We thank Dr. J. Del Rio and A. Garcia (Salk Institute, La Jolla, CA) for technical support with the Affymetrix gene chip. We also thank Dr. M. Gesemann (University of Zürich) for advice with the RNase Protection Assay. We acknowledge Dr. Raineteau for the guidance provided during this work.
Correspondence should be addressed to Florence Bareyre, Brain Research Institute, University of Zürich and Department of Biology, ETH Zürich, Winterthurerstrasse 190, 8057 Zürich, Switzerland. E-mail: florence.bareyre{at}access.unizh.ch.
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