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The Journal of Neuroscience, February 15, 2003, 23(4):1424
Neurotrophin-3 Expressed In Situ Induces Axonal Plasticity in the Adult Injured Spinal Cord
Lijun Zhou1, 2, Brian J. Baumgartner1, Sandra J. Hill-Felberg1, Leonard R. McGowen1, 2, and H. David Shine1, 2, 3, 4 1 Department of Neurosurgery, 2 Center for Cell and Gene Therapy, 3 Division of Neuroscience, and 4 Department of Molecular and Cellular Biology, Baylor College of Medicine, Houston, Texas 77030
ABSTRACT
TOP
ABSTRACT
Introduction
The mammalian CNS lacks the ability to effectively compensate for injury by the regeneration of damaged axons or axonal plasticity of intact axons. However, reports suggest that molecular or cellular manipulations can induce compensatory processes that could support regeneration or plasticity after trauma. We tested whether local, sustained release of the neurotrophic factor neurotrophin-3 (NT-3) would support axonal plasticity in the spinal cord distal to the site of injury in rats. The corticospinal tract (CST) was cut unilaterally at the level of the medulla. This avoided excessive inflammation, secondary cell death, vascular disruption, and the release of inhibitory molecules in the lumbar spinal cord. A replication-defective adenoviral vector (Adv) carrying the NT-3 gene (Adv.EF
-NT3) was delivered to the spinal motoneurons by retrograde transport through the sciatic nerve. Retrograde transport of the adenoviral vectors avoided the inflammatory response that would be associated with direct injection into the spinal cord. Transduction of spinal motoneurons with Adv.EF
Key words: neurotrophin-3; axonal plasticity; adenoviral vectors; spinal cord injury; regeneration; NT-3
Introduction
The robust anatomical and functional plasticity of the embryonic and perinatal mammalian CNS is lost soon after birth, so that regeneration or compensation after injury is all but absent in adults. The lack of a supportive environment and the presence of inhibitory molecules prevent the regeneration of damaged axons and compensatory growth of intact axons. This inability of the adult CNS to regenerate or effectively compensate after injury leads to permanent and many times to devastating functional deficiencies after injury. Nevertheless, there is emerging evidence that the adult CNS retains some capacity for plasticity and may, under the right conditions, be able to regenerate (Schwab, 2002
). Manipulation of the CNS environment will support sprouting of undamaged axons into areas denervated by lesions. Neutralization of the myelin-associated neurite growth inhibitor Nogo with a monoclonal antibody (IN-1) resulted in extensive sprouting of axons from an intact corticospinal tract (CST) to the denervated side of the spinal cord after the other tract was cut at the level of the pyramids (Thallmair et al., 1998
We have demonstrated previously that the retrograde transport of adenoviral vectors (Advs) expressing neurotrophic factor genes (Adv.RSV-nf) from the periphery to CNS motoneurons results in the local expression of neurotrophic factors that block axotomy-induced motoneuron death in the facial nucleus and spinal cord (Baumgartner and Shine, 1997
Materials and Methods
Preparation of an adenoviral vector carrying the NT-3 gene. To express NT-3 locally in the rat spinal cord, we constructed a replication-defective Adv carrying the cDNA sequence of rat NT-3, the nerve growth factor (NGF) signal sequence, and the FLAG marker sequence driven by the mammalian elongation factor
Western blot and ELISA analyses of NT-3-FLAG expressed by HeLa cells transduced with Adv.EF
Analysis of biological activity of conditioned medium from HeLa cells transduced with Adv.EF
Pyramidotomy for unilateral lesion of the CST. In the rat, most CST fibers decussate at the level of the pyramids in the brainstem and project to the contralateral side of the spinal cord via the dorsal funiculus. The CST was cut at the level of the pyramids above the decussation, resulting in an almost complete denervation of the right CST in the spinal cord (Fig. 1). Severing the CST unilaterally at the pyramids permitted us to denervate the CST to the full extent of the length of the spinal cord, thus avoiding vasculature disruption and inflammation that would be associated with a lesion in the spinal cord. Adult Sprague Dawley female rats (250-300 gm) were anesthetized with halothane followed by continuous isoflurane using a vaporizing system (Vip 3000; Matrx Medical Inc., Orchard Park, NY). A midline incision was made in the ventral neck region. The trachea and paratracheal musculature were retracted to expose the basioccipital portion of the skull. The left CST was exposed by a 2 mm craniotomy performed with a burr drill just lateral to the midline ridge. Taking the basal artery as the landmark of midline, a 1.5-mm-wide and 0.5-mm-deep incision was made into the medulla. To ensure that all of the CST was completely transected, we aspirated the incision site with a fine-tipped glass suction pipette. The exposed brain tissue was covered with gel foam, and the skin was closed with sutures. Animal experiments and animal care were performed in accordance with approved protocols of the Baylor College of Medicine.
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Figure 1. Schematic of the experimental protocol. A, One CST was lesioned at the level of the hindbrain. B, After 10 d, the neuronal tracers BDA and Fluoro-ruby were injected into opposite sensorimotor cortices. C, Four days after the tracer injection, Adv.EF
Anterograde tracing of CST projections. Ten days after CSTL, the rats were anesthetized with isoflurane and fixed in a sterotaxic frame. Biotinylated dextran amine (BDA; lysine fixable, MW 10,000; Molecular Probes, Eugene, OR) at a concentration of 10% in PBS was injected into 12 sites (146 nl per site) in two rows of six sites spaced 0.5 mm apart caudorostrally and 1 mm apart mediolaterally at a depth of 1.2 mm in the sensorimotor cortex on the side that innervated the intact CST (Grill et al., 1997
Retrograde delivery of adenoviral vectors. Two weeks after CSTL and 4 d after BDA cortical injection, the rats were anesthetized with continuous isoflurane, and an incision was made posterior and parallel to the femur on the right side to expose the sciatic nerve within its surrounding connective tissue and superficial blood vessels. The sciatic nerve was transected ~2 mm proximal to the bifurcation of the common peroneal and tibial branches. The proximal end of the cut nerve was placed in a small chamber fashioned from a 1.5 cm length of polyethylene tubing (1.4 mm inner diameter; Intramedic; Becton Dickinson, Sparks, MD) with one end sealed with a 2-mm-diameter glass bead and filled with 1 × 109 infectious units of either Adv.EF
Adenoviral vector-mediated expression of NT-3 in vivo. Adv.EF
80°C. The frozen tissue was homogenized in a lysate buffer consisting of 137 mM NaCl, 20 mM Tris-HCl, pH 7.6, 1% Igepal CA-630, 10% glycerol, 1 mM PMSF, 10 µg/ml aprotinin, 1 µg/ml leupeptin, and 0.5 mM sodium vanadate (all reagents from Sigma) and centrifuged at 13,000 × g at 4°C for 30 min to remove the nonsoluble fraction. The concentration of NT-3 in the supernatant was determined by ELISA (Promega).
Histochemistry. Three weeks after vector delivery, the animals were heavily anesthetized with halothane and perfused intracardially with heparinized PBS followed by 4% paraformaldehyde (PFA) in PBS. The lumbar region of the spinal cords (L3-L6) was removed and postfixed in the same buffered fixative for 3 hr, washed briefly in PBS, and infiltrated with 21% sucrose in PBS. Cross sections of spinal cord 40 µm thick were cut on a cryostat and collected in PBS. Every sixth section was put in one well of a 96 well culture plate. One section per two wells was picked randomly for BDA staining. A total of 14 sections between lumbar segments L3 and L6 were analyzed for each animal. For BDA staining, sections were washed in PBS three times, for 15 min each, followed by treatment with 0.3% H2O2 for 30 min at room temperature. After three washes in PBS containing 0.1% Triton X-100 (PBST), BDA was detected with ABC reagent (Vector Laboratories) and diaminobenzidine (DAB). CST axons containing the anterograde marker BDA developed a dark-brown reaction product that was readily visible against the unstained spinal cord tissue.
To examine the completeness of the CSTL, BDA was detected with Alexa Fluor 488-conjugated streptavidin (Molecular Probes). Lumbar spinal cord sections were washed in PBST, incubated with Alexa Fluor 488-conjugated streptavidin (1 µg/ml in PBST) overnight, washed in PBS, and mounted with SuperMount (BioGenex, San Ramon, CA). Standard immunocytochemical techniques were used to detect macrophages in the lumbar spinal cord using ED1 antibody (Serotec, Oxford, UK) and a goat anti-mouse secondary antibody linked to Alexa Fluor 568 dye (Molecular Probes). To demonstrate the expression of LacZ in motoneurons after the retrograde delivery of Adv.EF
-galactosidase (
To determine the survival of motoneurons after the retrograde delivery of adenoviral vectors, five sections from three rats from each group were stained with hematoxylin and eosin. Large, multipolar cells located in the ventral horn of the spinal cord were identified as motoneurons and counted. The number of motoneurons on the lesioned and unlesioned sides of the spinal cords were compared within each group using a paired t test. The ratio of the number of motoneurons on the lesioned side to the number of motoneurons on the unlesioned side was compared; this compensated for variability between animals.
Quantification of CST axons. Photomicrographs of the spinal cord sections were taken with a digital camera (AxioCam; Carl Zeiss, Jena, Germany) at 100× magnification under dark-field illumination. Five vertical lines, M, N1, N2, L1, and L2, were drawn on the photographs (see Fig. 7a), where M passed through the midline, N1 was just lateral to the funiculus of the normal side of the CST parallel to M, and N2 was parallel to N1 and twice the distance of N1 to M. On the lesioned side of the spinal cord, L1 and L2 corresponded to lines of N1 and N2. Lines A and B were drawn perpendicular to the dorsoventral axis of the cord. Line A was drawn just below the dorsal columns, and line B was drawn just above the ventral columns. Axons that crossed the five lines between lines A and B were counted on the computer screen. To compensate for any variability in the degree of BDA staining, we calculated the ratios of M, L1 and L2 to N1 + N2 (M/N1 + N2, L1/N1 + N2, L2/N1 + N2).
Statistical analysis. ANOVA followed by the appropriate parametric and nonparametric post hoc tests were used for multiple group comparisons and Student's t test for paired comparisons using SigmaStat software (SPSS Inc., Chicago, IL). Significance was assigned at p < 0.05.
Results
HeLa cells transduced in vitro with Adv.EF
In previous reports we used the Rous sarcoma virus (RSV) promoter to control the expression of neurotrophic factors in Adv constructs (Adv.RSV-nf) (Baumgartner and Shine, 1997
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Figure 2. Analysis of NT-3 protein produced by cells transduced with Adv.EF
Transgene expression after retrograde transport of adenoviral vectors from sciatic nerve to the spinal cord
Adv.EF
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Figure 3.
ELISA analysis (Fig. 4) of the concentration of NT-3 in the lumbar spinal cord on the side that received vector showed that the animals receiving Adv.EF
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Figure 4. Expression of NT-3 in the L3-L6 lumbar spinal cord 3 weeks after the retrograde delivery of Adv. The concentration of NT-3 in the spinal cord was determined by ELISA (Promega). Values are means ± SD; *p < 0.05; n = 4 per group (ANOVA followed by the Student-Newman-Keuls test).
To determine whether the retrograde delivery of Adv affected motoneuron survival, we counted the number of motoneurons present in sections of lumbar spinal cord 5 weeks after CSTL and 3 weeks after the sciatic nerve was cut and the Adv delivered. Large, multipolar cells located at the ventral horn of the spinal cord were identified as motoneurons. Comparison of the numbers of motoneurons in the lumbar region sections taken from the lesioned versus the unlesioned side of the spinal cord did not show a statistically significant difference (p = 0.596; Student's t test; df = 16; t = 0.541). Nor was there a significant difference (p = 0.989; ANOVA; df = 2; F = 0.0115) among the numbers of motoneurons present on the lesioned side in groups treated with Adv.EF
Completeness of CST lesion
As shown in Figure 5A, the left CST was completely removed at the pyramidal lesion site. The completeness of the CSTL was further examined in sections of lumbar spinal cord. In animals without CSTL or with incomplete CSTL, Fluoro-ruby was visible in the right CST in the lumbar spinal cord, as shown in Figure 5C. For animals with complete CSTL, Fluoro-ruby was not present in the right CST (Fig. 5E). BDA efficiently labeled the unlesioned CST (Fig. 5B,D).
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Figure 5. A, Photomicrograph at the level of the lesion site in the pyramids showing the extent of the lesioned CST. The nonlesioned CST is demarcated by the anterograde marker BDA stained with ABC reagent (Vector Laboratories) and DAB. B-E, Completeness of the CST lesion demonstrated by anterograde markers in the lumbar spinal cord of unlesioned (B, C) and lesioned (D, E) animals. The unlesioned CST was traced with BDA and visualized with Alexa Fluor 488-conjugated streptavidin; the lesioned CST was traced with Fluoro-ruby. B, Section from a normal rat (sham surgery) showing the unlesioned CST labeled with BDA. C, The same section as B, showing the CST positive for Fluoro-ruby. D, Section from an animal with a complete CSTL, showing the unlesioned side of CST positive for BDA. E, Same section as D showing absence of Fluoro-ruby in the lesioned CST, indicating that the CSTL was complete.
Sprouting of contralateral CST axons after in situ expression of NT-3
In the rat, most CST fibers cross the midline at the pyramidal decussation within the brainstem and project into the contralateral dorsal funiculus of the spinal cord (Fig. 1); however, a small number of fibers do not cross at the pyramidal decussation and project ipsilaterally into the ventral and dorsal funiculi (Brosamle and Schwab, 1997
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Figure 6. Sprouting of CST axons across the midline in the spinal cord after CSTL and Adv.EF
Quantification of sprouting of contralateral CST axons after in situ expression of NT-3
The number of CST axons that projected across the midline from the unlesioned CST was measured in sections taken from the seven experimental groups listed above. It is likely that the efficiency of anterograde labeling of CST axons with BDA varied among animals, which in turn would result in a variable amount of axons visible in spinal cord sections. Thus, simply counting the axons that passed through the midline would not represent the actual degree of sprouting in the experimental groups. To compensate for variable labeling, we counted the number of BDA-labeled axons in two regions of the unlesioned side (N1 + N2) as well as the number of axons crossing the midline (M) in sections taken from the lumbar region of the spinal cord (see Materials and Methods) (Fig. 7a). Because the value for N1 + N2 represented the degree of BDA labeling for each animal, M/N1 + N2 represented the number of axons crossing the midline relative to the BDA labeling. Axons lateral to the midline on the lesioned side (L1 and L2) (Fig. 7a) were also counted, so that the ratios of L1/N1 + N2 and L2/N1 + N2 represent the axons that crossed the midline and reached the lines of L1 and L2 relative to the degree of BDA labeling. There was no difference in the M/N1 + N2 ratio among groups that did not receive a CSTL lesion (ANOVA followed by the Student-Newman-Keuls test; p < 0.01; F = 6.313; df = 6; power(
= 0.05) = 0.984) (Fig. 7b), demonstrating that in the absence of denervation, in situ expression of NT-3 had no effect on axonal sprouting. The CSTL plus NT-3 group had a significantly greater M/N1 + N2 ratio compared with all other groups (ANOVA followed by the Student-Newman-Keuls test; p < 0.01; F = 6.313; df = 6). There was a slight, statistically insignificant reduction in the number of axons that crossed the midline in the CSTL plus LacZ animals. It is not clear whether this represents a true treatment effect within the spinal cord or in the periphery or whether it is attributable to the variation in animals. The L1/N1 + N2 and L2/N1 + N2 ratios in the CSTL plus NT-3 group were not statistically different from those of the CSTL plus LacZ and CSTL plus PBS groups (data not shown). These findings demonstrate that local expression of NT-3 will elicit and support sprouting of CST axons into a region of traumatically denervated spinal cord, but not when both CSTs are intact.
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Figure 7. a, Method for quantification of axonal sprouting from the CST across the midline in the spinal cord. Dark-field photomicrographs were taken of each spinal cord section. Five vertical and two horizontal lines were drawn on each photomicrograph of a spinal cord section as reference points for counting axons. M was drawn through the midline, N1 was drawn just lateral to the funiculus of the CST and parallel to M, and N2 was drawn parallel to M and two times the distance between N1 and M. L1 and L2 were drawn on the lesioned side of the spinal cord and corresponded to lines N1 and N2. Lines A and B were drawn perpendicular to the dorsoventral axis of the cord. A was drawn just below the dorsal columns, and B was drawn just above the ventral columns. Axons that crossed M, N1, N2, L1, and L2 within the boundaries of A and B were counted. b, Quantification of CST axons crossing the midline in response to the local expression of NT-3. BDA-positive axons were counted at the midline (M) and at two sites (N1 and N2) in the lateral gray matter of the spinal cord on the side of the unlesioned CST (see Materials and Methods). The ratio of the axons that crossed the midline (M) to those that crossed the two sites in the lateral gray matter (N1 + N2) was computed (M/N1 + N2) to compensate for any variation in the degree of anterograde labeling of the CST. The ratios of the treatment groups were normalized to the ratio of the normal animal group, which was set to zero. A positive value indicates that more axons crossed the midline compared with normal, unlesioned animals; a negative value indicates that fewer axons crossed the midline compared with normal animals. Values are means ± SD; **p < 0.01 (ANOVA followed by the Student-Newman-Keuls test). Numbers in parentheses represent the number of animals per group.
Discussion
Adenovirus-mediated expression of biologically active NT-3 in vitro
Conditioned medium from HeLa cells transduced with Adv.EF
Retrograde transport of Adv.EF
ELISA analyses of spinal cord tissue showed a threefold greater concentration of NT-3 at 1 week and a twofold greater concentration at 3 weeks on the side of the spinal cord on which motoneurons had been transduced with Adv.EF
To avoid vector-associated inflammation, we exploited the fact that Adv is transported from the periphery to the CNS by retrograde transport (Ridoux et al., 1994
In our previous research, we targeted neurotrophic factors to the motoneurons of neonatal rats by injecting them with Adv.RSV-nf directly into muscle, where the vectors were efficiently taken up by peripheral nerves and transported to motoneurons (Baumgartner and Shine, 1997
Histochemical staining for
Sprouting from the intact CST is induced by local expression of NT-3
The principal observation of our experiments is that the local expression of NT-3 by motoneurons induced and supported the sprouting of axons from the contralateral CST. It is notable that the sprouting was (1) observed, suggesting that overexpression of NT-3 induced the axons to overcome or evade any negative factors that may inhibit axonal growth; (2) induced in uninjured axons, demonstrating that these observations represent neurotrophic factor-induced plasticity rather than regeneration; and (3) present only when the ipsilateral CST was lesioned, suggesting that other factors play a role in the observed plasticity.
Lesioning the CST at the level of the pyramids avoided conditions associated with other spinal cord lesion models, such as inflammation, secondary cell death, vascular disruption, and connective-tissue disruption, which could confound analysis of the effect of NT-3 on axonal plasticity. Because the lesion was distal to the region of analysis, no trauma-associated inhibitory molecules such as Nogo or myelin-associated glycoprotein were released or upregulated (such as chondroitin sulfate proteoglycans) that could have blocked axonal projection from the CST (Schwab, 2002
That we observed axonal plasticity only when the ipsilateral motoneurons were denervated by lesioning the ipsilateral CST suggests that NT-3 alone is insufficient to elicit and support this axonal plasticity. Additional factors present in the denervated side of the spinal cord may signal the intact CST to either sprout collaterals or grow toward the denervated side and that NT-3 acts in concert with these signals to establish the contralateral axonal projections. Because we measured the degree of sprouting at only one time point (5 weeks after CSTL and 3 weeks after the beginning of NT-3 overexpression), it is not clear whether the number of axons crossing the midline is stable or are increasing or decreasing. Nor is it known whether CST axons would respond differently if NT-3 were expressed at other times after CSTL.
Conclusions
These data demonstrate that local, sustained expression of NT-3 by motoneurons will support sprouting of intact CST axons after they have lost their normal CST innervation. In addition, they suggest that CNS neurons have the capacity to respond to trauma-induced denervation through axonal plasticity. Hence, it is possible that interventions based on gene delivery would promote limited functional recovery from neural trauma by eliciting plasticity changes in intact nervous system tissue in addition to regenerating damaged tissue.
FOOTNOTES Received Sept. 16, 2002; revised Nov. 20, 2002; accepted Nov. 21, 2002.
This work was supported by National Institutes of Health Grant NS35280 and by Mission Connect, a project of The Institute for Rehabilitation and Research Foundation. We thank our colleagues of Mission Connect helpful discussion of this work; D. Bui, T. Chacko, and R. Rosado for technical assistance; R. J. Gill for immunocytochemical analysis; S. L. C. Woo and Z. S. Guo for the pXCJL.1 plasmid; and John Gilbert for editorial assistance.
Correspondence should be addressed to Dr. H. David Shine, Department of Neurosurgery, Baylor College of Medicine, One Baylor Plaza, Houston, TX 77030. E-mail: hshine{at}bcm.tmc.edu.
B. J. Baumgartner's present address: Department of Biology, Trinity Valley Community College, Athens, TX 75751.
S. J. Hill-Felberg's present address: Department of Medicine, Tulane University Health Sciences Center, New Orleans, LA 70112.
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