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In vivo and in vitro characterization of novel neuronal plasticity factors identified
following spinal cord injury
Simone Di Giovanni1, 2∗, Andrea De Biase2∗, Alexander Yakovlev1, Tom Finn1, Jeanette
Beers1, Eric P. Hoffman2, Alan I. Faden1
∗These authors equally contributed to this work
Abbreviated Title: Neuronal plasticity after spinal cord injury
1Department of Neuroscience Georgetown University Medical Center Washington DC 20057 Telephone: (202) 687-0492
2Center for Genetic Medicine Children’s National Medical Center Washington DC 20010 Telephone: (202) 884-6011
Correspondence: Alan I. Faden, MD, or Simone Di Giovanni, MD Department of Neuroscience Georgetown University School of Medicine 3900 Reservoir Road, NW Washington, DC 20057 e.mail: [email protected] or [email protected] Number of figures and tables: 10 Number of pages: 33 Keywords: spinal cord, microarray, plasticity, coronin 1b, rab13, ninjurin Acknowledgments: This work was supported by the National Institute of Health contract NIH-NINDS-01 (NS-1-2339) (to AIF and EPH), and an NIH Programs in Genomic Applications grant U01 HL66614 HOPGENE (to EPH). We would like to thank Bogdan Stoica for assistance using confocal microscope.
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JBC Papers in Press. Published on November 1, 2004 as Manuscript M411975200
Copyright 2004 by The American Society for Biochemistry and Molecular Biology, Inc.
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SUMMARY Following spinal cord injury, there are numerous changes in gene expression that appear
to contribute to either neurodegeneration or reparative processes. We utilized high
density oligonucleotide microarrays to examine temporal gene profile changes after
spinal cord injury in rats with the goal of identifying novel factors involved in neural
plasticity. By comparing mRNA changes that were coordinately regulated over time with
genes previously implicated in nerve regeneration or plasticity, we found a gene cluster
whose members are involved in cell adhesion processes, synaptic plasticity and/or
cytoskeleton remodeling. This group, which included the small GTPase rab13 and actin
binding protein coronin 1b, showed significantly increased mRNA expression from 7 - 28
days after trauma. Over-expression in vitro using PC-12, neuroblastoma, and DRG
neurons demonstrated that these genes enhance neurite outgrowth. Moreover, RNAi
gene silencing for coronin1b or rab13 in NGF treated PC-12 cells markedly reduced
neurite outgrowth. Coronin 1b and rab13 proteins were expressed in cultured DRG
neurons at the cortical cytoskeleton, and at growth cones along with the pro-
plasticity/regeneration protein GAP-43. Finally, coronin 1b and rab13 were induced in
the injured spinal cord, where they were also co-expressed with GAP-43 in neurons, and
axons. Modulation of these proteins may provide novel targets for facilitating restorative
processes after spinal cord injury.
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INTRODUCTION
Traumatic injury to the spinal cord induces delayed biochemical responses that affect
both cell loss and subsequent repair. Modulation of reparative processes includes factors
involved in either facilitating or inhibiting neurite outgrowth, which are often regulated at
the gene and protein levels after injury. Collectively, these factors likely determine in part
the degree of anatomical and functional recovery after injury.
“Regeneration-associated proteins” (RAGs) appear to play a role in plasticity and
regeneration following SCI. These include transcription factors (c-jun), cytoskeletal
components (Tα1), microtubule associated proteins, growth associated proteins (GAP-43,
CAP-23), cell adhesion molecules (N-CAM, L1, TAG1), neurotrophic factors, cytokines
and extracellular matrix components (SNAP25, munc13, and cpg15/neuritin) (1-10). In
some cases, these factors share common molecular pathways. GAP-43 and CAP-23 bind
downstream to the cofactor PI(4,5)P(2), at plasmalemmal rafts, contributing to the
regulation of actin and modulating neurite outgrowth in neuronal-like cell lines (11, 12).
In other instances, a common downstream effector, such as neurotrophin dependent
intracellular cAMP, may serve to facilitate axonal regeneration by overcoming inhibition
from factors such as myelin associated glycoprotein (MAG) (13-15).
Microarray technology provides a powerful tool for identifying molecular
pathways involved in either endogenous neurotoxicity or regeneration/plasticity after SCI
(16-19). It allows concurrent analysis of thousands of genes and the identification of
clusters of coordinately regulated transcripts sharing similar functions.
Previously we reported early changes following spinal cord injury in rats,
showing induction of specific cell cycle genes (gadd45a, c-myc, cyclin D1 and cdk4,
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pcna, cyclin G, Rb, and E2F5) that were closely associated with post-traumatic apoptosis
(18). Here, we focused on later time points to identify genes potentially associated with
neuronal plasticity and neurite outgrowth after SCI, by evaluating temporal gene profiles
that were coordinately regulated with expression profiles of known pro-plasticity factors.
A stringent temporal correlation analysis of the profiles and subsequent functional
classification allowed identification of 6 genes belonging to a specific gene cluster, which
was over-expressed between 7 and 28 days after injury, and whose members are involved
in neuronal plasticity, neurite outgrowth, and synaptogenesis. Over-expression of these
genes in PC-12, SH-SY5 neuroblastoma cell lines, or DRG neurons in vitro significantly
promoted neurite outgrowth. Novel members of this cluster: coronin 1b and rab13, were
further characterized in vivo, and in vitro, and their role in neuronal differentiation and
neurite outgrowth was studied using RNAi gene silencing. Based upon these in vitro and
in vivo observations, we propose a role for these genes in neuronal plasticity after injury.
EXPERIMENTAL METHODS
Experimental spinal cord injury and expression profiling
Mild contusion spinal cord injury was performed in rats, as previously described
(18). Briefly, male Sprague-Dawley rats (275-325 gm) were anesthetized with sodium
pentobarbital (65mg/Kg, i.p.). Injury was induced using a weight drop method (10 g
dropped from 17.5 mm). Animals with this injury level show mild motor impairment on
the Basso, Beattie, Breshnahan scale, averaging 12±1, 14±1, and 17±1 respectively at 7,
14, and 28 days after injury. Animals were fully anesthetized with sodium pentobarbital
(67 mg/Kg) during the operative procedures and experiments complied fully with the
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principles set forth in the “Guide for the Care and Use of Laboratory Animals” prepared
by the Committee on Care and Use of Laboratory Animals of the Institute of Laboratory
Resources, National Research Council (DHEW Pub. No. (NIH) 85-23, 2985).
A 1 cm section of the spinal cord, centered at T-9, was dissected, and immediately
frozen in liquid nitrogen. Spinal cords were collected from 4 injured and 2 sham-operated
rats (receiving only laminectomy) for each time point (4 hours, 24 hours, 7, 14, and 28
days (3 animals) and two naïve controls (rats that did not undergo any surgical procedure)
for a total of 31 animals. Seven micrograms of total RNA was used for complementary
DNA (cDNA) and biotinylated complementary RNA (cRNA) synthesis. Expression
profiling analysis was performed using the Affymetrix rat U34 A, B, and C arrays. Each
genechip was used for a single hybridization with RNA isolated from one spinal cord
sample from a single animal. Total of samples was 31.
Expression profiling was performed as described previously (18). Briefly, RNA
was extracted from each cord sample individually using TRIzol reagent (Invitrogen) and
processed for chip hybridization using the manufacturers protocol (Affymetrix).
Microarray (genechip) quality control and normalizations
We employed stringent quality control methods as previously published and
detailed on our Web site: (http://pepr.cnmcresearch.org/browse.do). Expression profiles
utilized for analysis fulfilled all quality control measures as detailed in previous papers
(18, 21). We used two normalization processes: one for chip-chip comparisons (scaling
factors), and one for temporal analysis (normalization to the average of the naïve signal
intensities for each gene). The scaling factors determinations were done using default
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Affymetrix algorithms (MAS 5) with a target intensity of chip sector fluorescence to 800.
Both pre-amplification (s1) and post –amplification with streptavidin/phycoerythrin (s2)
scans were done, and the scans compared by scatter plots and correlation coefficients.
Those probe sets showing evidence of saturation of the PMT in s2 were flagged.
Data scrubbing and statistical analysis
We have recently shown that use of Affymetrix MAS 5.0 signal intensity values,
together with a “present call” noise filter achieves an excellent signal/noise balance
relative to other probe set analysis methods (dchip, RMA) (39) . Data analyses were
limited to probe sets that showed 1 or more “present” (P “calls”) in the 79 genechip
profiles in our complete dataset. Experiment normalization was performed by
normalizing gene chips from injured and sham controls to the mean of the two chips from
naïve animals considered as the baseline gene expression level. Normalized data were
then compared for differential gene expression analysis across time points between sham
and injured groups. Genes that showed a Welch ANOVA t-test p value < 0.05 between
sham and injured groups for at least one time point were retained for further analysis.
Initial data analysis also included a fold change filter of >1.5 (50% difference) increase or
decrease relative to sham operated animals (Affymetrix MAS 5.0). While a p value of
<0.05 alone would give many false positives, the combination of present call filters, fold
change thresholds, and p values thresholds, eliminates most false positives that are
obtained with only p<0.05.
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Real time-RT-Multiplex-PCR
We studied selected transcripts by real time PCR using cDNAs extracted from cords of
rats subject to spinal cord trauma and sham controls in parallel experiments, at the time
point 14 days, to validate our microarrays findings. Fluorophore-labeled LUX primers
(forward) and their unlabeled counterparts (reverse) were provided by Invitrogen. LUX
primers were designed matching the probe sets sequences for ninjurin, rap1b, rab13 and
coronin 1b and all primers were designed using the software called LUX Designer
(Invitrogen, www.invitrogen.com/lux). Each primer was chosen matching the target
probe set sequence for the gene of interest. More in detail, primer sequences were:
ninjurin (forward: caccttTCCTGTTCACAGCCCAAGG5G), reverse:
(TCTTCATGGCTTTGCATCCAG), rab13 (forward:
cacactgAGACAAGTGCCAAATCCAGTG5G), (reverse:
TCAGTGCTTGAGGGCTTGCT), rap1b (forward: cacgaCTCCCTTGCTTGCTCG5G),
(reverse: TTCCCACATTCACATCCACA), and coronin 1b (forward:
caccaTAGAGGACTGCACTGTCATGG5G), (reverse: GCACATTTCGGGCTGTGG).
We performed multiplex PCR using each experimental gene with the housekeeping gene
GAPDH. For each sample, as previously detailed, 50 µl PCR contained 2 µl cDNA,
10 µM of each gene-specific primer (two pairs for multiplex PCR) and 1X Platinum
Quantitative PCR SuperMix-UDG (Invitrogen). Reactions containing fluorogenic LUX
primers included 1X SuperMix and were incubated at 25°C for 2 min, 95°C for 2min, and
then cycled (45×) using 95 C for 15s, 55 C for 30s, and 72 C for 30s, and reactions were
incubated at 40°C for 1min and then ramped to 95°C over a period of 19min followed by
incubation at 25°C for 2min (ramp for melting-curve analysis). Reactions were conducted
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in a 96-well spectrofluorometric thermal cycler (ABI PRISM 7700 Sequence detector
system, Applied Biosystems). Fluorescence was monitored during every PCR cycle at the
annealing or extension step and during the post-PCR temperature ramp. Fold changes
were calculated following manufacture instructions (Invitrogen).
Immunoblotting
Cords used for immunoblotting included samples from three injured and two
sham spinal cords at the time points 7 and 14 days after injury. For E14 DRGs, 500-600
DRG were isolated for each time point, and cultured in six well plates. Frozen tissues
were washed once with ice-cold phosphate-buffered saline and lysed on ice in a solution
containing 50 mM Tris-HCl, pH 7.5, 150 mM NaCl, 1 mM EGTA, 1 mM PMSF, 0.5%
NP-40, 0.25% sodium deoxycholate (SDS), leupeptin (5 µg/ml), and aprotinin (5 µg/ml).
After removal of cell debris by centrifugation, the protein concentration of the cell lysate
was determined with the BioRad protein assay reagent. A portion of the lysate (30-50 µg
of protein) was then resolved by SDS-polyacrylamide gel electrophoresis (PAGE), and
the separated proteins were transferred to a nitrocellulose filter. The filter was stained with
Ponceau S to confirm equal loading and transfer of samples, and was then probed with
specific antibodies. Immune complexes were detected with appropriate secondary antibodies
and chemiluminescence reagents (Pierce). β-Actin protein abundance was used as controls
for gel loading and transfer.
The following primary antibodies were used: rabbit polyclonal anti-coronin 1b (1:1000,
custom antibody from Betyl Laboratories), and rabbit polyclonal anti-Rab13 (1:1000,
custom antibody from Betyl Laboratories). Omission of the primary antibodies or their
replacement by pre-immune sera was used for control experiments. Immunocomplexes
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were visualized with ECL chemiluminescence (Amersham).
Immunocytochemistry
Spinal cords
12 µm frozen sections from three injured and two sham spinal cords were
collected between 0.4 and 0.5 cm below or above the injury site epicenter, as previously
reported (18). Sections were incubated under the same coverslip and processed for
immunocytochemistry. They were first dried at room temperature, fixed in 4%
paraformaldehyde, rinsed in PBS and incubated with 10% normal serum and 0.2% Triton
X in PBS (goat or rabbit depending on the secondary antibodies used) for 60 min to mask
non-specific adsorption sites. Sections were then incubated overnight at 4° C with one or
more of the following primary antibodies: rabbit polyclonal anti-coronin 1b (1:100,
custom antibody from Betyl Laboratories), and rabbit polyclonal anti-Rab13 (1:100,
custom antibody from Betyl Laboratories).
Omission of the primary antibodies or their replacement by pre-immune sera was
used for control experiments. After several rinses in PBS, the sections were incubated
with the appropriate rhodamine – Alexa 488, 568 or 647-coupled secondary antibodies
(goat anti-mouse or goat anti-rabbit) for 1 hour at room temperature, and washed in PBS
before mounting the slides with aqueous medium. Double labeling was also performed
combining mouse monoclonal anti-rat neuN (1:100, Chemicon, Temecula, CA), mouse
monoclonal anti-rat beta III tubulin (1:200, Promega, Madison, WI), or mouse
monoclonal or rabbit polyclonal anti-GFAP (1:200, Chemicon, Temecula, CA); mouse
monoclonal anti-rat Myelin/Oligodendrocyte O4 (1:100, US Biological); mouse anti-rat
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CD11b (1:100, Serotec, Oxford, UK), and mouse monoclonal or rabbit polyclonal anti-
GAP-43 (1:200, Chemicon, Temecula, CA), with each of the above antibodies.
Immunofluorescence was detected using confocal microscopy (Zeiss Inc.)
Dorsal Root Ganglia neurons
E14 dorsal root ganglia cells cultured in Neurobasal medium onto glass coverslips
(circular, 13 mm in diameter) coated with poly-D-lysine and laminin (Biomedical
Technologies Inc.) in 24-well plates at a density of 2.5 × 104 cells/well, were fixed after
three, five, seven, nine and fourteen days in culture, and processed for
immuncytochemistry as described above for spinal cord tissue.
Primary antibodies used included coronin 1b, and rab13, (same dilutions as
above). Each one of them was combined in double immunostaining experiments with
either mouse monoclonal or rabbit polyclonal GAP-43, or with Alexa Fluor 568
phalloidin for detection of F-actin (Molecular Probes, OR). The same secondary
antibodies used for spinal cord sections were employed in these experiments.
Immunofluorescence was detected using deconvolution microscopy (Zeiss Inc.). Clones and transfection experiments
Ninjurin, rab13, rap1b, synaptogyrin, synaptotagmin, and coronin 1b, full length
cDNA expression constructs in pCMV SPORT6 were purchased from Invitrogen Inc.
(respectively IMAGE LLAM clones #2596463; 3908502; 6150381; 5173992; and
GATEWAY Human clones #CSODG004YH12; CSODD003YH09).
PC-12 and SH-SY5 neuroblastoma cells were cultured in DMEM plus 10% FBS.
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Embryonic day 14 DRG neurons were removed and dissociated as previously described
(40). Briefly, E14 embryos were collected and placed in cold L-15 medium, the head and
tail removed, and skin overlaying the spinal cord cut. The spinal cord with DRG attached
was removed using fine curved forceps, the ganglia isolated, and excess meninges
trimmed. Ganglia were suspended in L-15 medium containing 0.25% trypsin and
incubated at 37 degrees for 15 minutes, fetal bovine serum was added to 10% final
concentration, washed, then dissociated by titration with a fire polished pipette. DRG
neurons were cultured in Neurobasal medium (Gibco-BRL) supplemented with B-27, 2
mM L-glutamine, 50 units penicillin-streptomycin, and 50 µg/ml of NT3. Some cultures
were treated with 1 x 10-5 flurodeoxyuridine-1 x 10-5 uridine 24 hours after plating for 2
days to reduce non-neuronal cells. Cells were transfected after 7 days in culture. For
transfection, cells were seeded onto glass coverslips (circular, 13 mm in diameter) coated
with poly-D-lysine and laminin (Biomedical Technologies Inc.) in 24-well plates at a
density of 2.5 × 104 cells/well and cultured for 72 h. Transfection experiments were
performed using the NeuroPORTER Transfection Kit (Sigma) for DRGs, and using
Lipofectomine 2000 for PC-12 and SH-SY5 cells (Invitrogen). Recombinant plasmid
DNA encoding GFP was included in transfections to monitor transfected cells. Cells were
stained with both beta III tubulin and GAP-43 (Chemicon, Temecula, California)
antibodies to identify both cell body and processes of neurons undergoing plasticity.
Neurite outgrowth was evaluated measuring the neurite length of the longest neurite per
cell counting only processes positive for GFP, beta III tubulin and GAP-43 for DRGs,
and measuring the number of PC-12 and SH-SY5 cells with neurites at least 2 times the
length cell body. Measurements were conducted in three different experiments by two
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different operators. Cells were viewed using a CCD camera and analyzed with image
analysis software AxioVision 3.1 (Zeiss).
RNA interference experiments
Complementary hairpin oligonucleotides were designed using the "siRNA
Converter" Internet tool (Ambion), annealed, and cloned between BamHI and HindIII
restriction sites in pSilencerTM 3.1-H1/neo (Ambion) according to the manufacturer's
recommendations. The oligonucleotide sequences were as follows (sense and antisense,
respectively): rat coronin 1b 5'-
GATCCCAAGTTGTGCGGCAGAGCAATTCAAGAGATTGCTCTGCCGCACAACT
TTTTTTTGGAAA A-3' and 5'-
GCTTTTCCAAAAAAAAGTTGTGCGGCAGAGCAATCTCTTGAATTGCTCTGCCG
CACAACTTGG -3'; and rat rab13 5'-
GATCCCGATCCGAACTGTGGAAATATTCAAGAGATATTTCCACAGTTCGGAT
CTTTTTTGGAAA-3', and 5'-
AGCTTTTCCAAAAAAGATCCGAACTGTGGAAATATCTCTTGAATATTTCCACA
GTTCGGATCGG-3'. Oligonucletides were transfected along with eGFP plasmid DNA
using Lipofectomine 2000 (Invitrogen) for experimental samples, and with eGFP plus
naked DNA for control cells. We also employed scrambled siRNA sequences to control
for the specificity of the silencing effect (data not shown, Silencer™ Negative Control,
Ambion). Inhibitory effect of RNA interference on expression of coronin 1b was tested in
transiently transfected PC-12 cells during NGF treatment (50 ng/ml) by Western blotting
and immunofluorescence staining using anti-rat coronin antibodies (custom antibodies,
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Betyl Laboratories). Cells positive for eGFP and negative for coronin or rab13 staining
were compared to control cells positive for both eGFP and coronin or rab13, and were
selected for evaluation of neurite outgrowth, measuring the length of the longest neurite
per cell as detailed in previous section.
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RESULTS Identification of putative pro-plasticity gene cluster induced between 7 and 28 days
following SCI
Approximately 24,000 probe sets were examined using Affymetrix high density
oligonucleotides arrays (U34 A, B, and C chips) at 4 hrs, 24 hrs, 7 days, 14 days, or 28
days after SCI. We applied a “present call” noise filter (1 in 79 arrays), fold change
thresholds (>1.5), and p value of less than 0.05 as our initial data set for preliminary
analysis and pathway identification. This analysis led to further consideration of about
6000 transcripts, of which 5% would be expected to be false positives. Files from all 79
arrays are available from our website, including .dat, .cel, and .txt files
(http://pepr.cnmcresearch.org/browse.do). This website includes an on-line time series
query tool of this data set (http://pepr.cnmcresearch.org/jsp/searchForm.jsp). The
spreadsheets showing all genes profiling preliminary analysis criteria is also available on
the website. A more complete analysis of the global gene changes have also been
previously reported by us (18).
Among the significantly altered transcripts, we searched for transcripts previously
implicated in neuronal-axonal repair and plasticity after injury. We identified a transcript
corresponding to ninjurin (nerve injury-induced protein), a cell adhesion molecule that is
up-regulated after axotomy in neurons and in Schwann cells surrounding the distal nerve
segment, and promotes neurite extension of dorsal root ganglion neurons in vitro (20).
We then used ninjurin as “anchor gene” to fish out a cluster of temporally correlated
genes that could potentially have a similar function that is involved in neuronal plasticity
after SCI. We used the gene array analysis software GeneSpring (as previously detailed,
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18, 21) that allows identification of gene profiles with similar temporal regulation, and
identified a cluster of temporally correlated genes (correlation coefficient, R2=0.98) over-
expressed between 7 and 28 days after injury, that included 20 transcripts. Functional
classification showed that this group of genes was variably associated with immune
response, cell adhesion, axon migration, polarity, growth, guidance, dendrite elaboration,
plasticity and synapse formation (table 1). To further narrow the field to identify a more
specific group of temporally correlated transcripts, we performed a more stringent
correlation analysis using both Standard and Pearson correlation (R2=0.99), which
identified 5 genes other than ninjurin: coronin 1b, rab13, synaptogyrin, and
synaptotagmin (figure 1). Synaptic vesicles associated proteins synaptotagmin and
synaptogyrin have been localized at the synaptic terminals in several neuronal types and
in PC-12 cells, and play a role in synaptic plasticity, neurotransmitter release and neurite
outgrowth (for review, 22-24). Rap1 is a small GTPase involved in several signal
transduction pathways, and is induced by NGF in PC12 cells and is necessary for neurite
outgrowth (25, 26). Coronin 1b is an actin binding protein involved in cytoskeleton
remodeling (for review, 27), rab13 is another small GTPase, belonging to the rab family
of proteins, which plays a role also in cytoskeleton dynamics and vesicle transport (for
review, 28). Analogs of coronin 1b (cilpin C) and a rab family member (Rab8) have also
been localized at cellular protrusions, and neurite tips in PC-12 and SH-SY5 cells (29,
30). Therefore, based upon their temporal co-regulation with the other members of the
cluster, and upon their known or putative biological function, coronin1b, and rab13
appeared to be factors involved in neurite outgrowth and differentiation.
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Real time PCR confirmed microarray results
Real time PCR experiments using cDNAs from a parallel set of animals at 14
days after SCI was performed on several members of the gene cluster to validate results
obtained by microarrays. The transcripts included ninjurin, rap1b, synaptotagmin,
coronin1b, and rab13. PCR experiments confirmed that all mRNAs were increased after
injury (table 2). Gene changes ranged between about 1.5 to 2.6 fold changes in
microarray experiments, while a wider range of changes was present after real time PCR,
due to the extreme sensibility of this technique, from about 2 to 7.6 fold changes.
In vitro overexpression of selected gene cluster members in PC-12, SH-SY5
neuroblastoma and DRG cells promotes neurite outgrowth
In order to evaluate whether gene cluster members ninjurin, rap1b, synaptogyrin,
synaptotagmin, coronin 1b, and rab13 were involved in neuronal plasticity, we tested
them using in vitro assays. We transfected plasmid cDNAs for each gene and
overexpressed them in the neuronal like cell lines PC-12, and SH-SY5 neuroblastoma
cells, as well as in rat primary dorsal root ganglia cells (DRGs), evaluating neurite
outgrowth by measuring the longest neurite per cell, and the number of neurite branches.
Percentage of cells with neurites lengths at least two times the cell bodies were evaluated
in PC-12 and SH-SY5 neuroblastoma cells. Neurite length as percentage of length in
control cells was measured in DRGs transfected cells. Transfected genes promoted
neurite outgrowth in the two cell lines (figure 2, A, and B), as well as in DRGs (figure 2,
C). These data confirmed and extended previous findings for ninjurin, rap1,
synaptotagmin and synaptogyrin, which suggested a possible role for these factors in
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neurite extension and neuronal differentiation; they also suggested a novel function for
coronin 1b, and rab13 in neurite outgrowth. The greatest effect on neurite outgrowth was
achieved with ninjurin, rab13, and coronin 1b. Ninjurin increased the number of cells
with extended neurites by 2.3 fold in PC-12 cells and by 5.2 fold in SH-SY5
neuroblastoma cells. Rab13 overexpression resulted in 2.7 and 9 fold increase
respectively in PC-12 and SH cells. Coronin 1b induced a 2.4 fold increase in PC-12 and
5.4 in SH cells. Experiments in primary neuronal cells, such as DRGs, also confirmed the
significant effect of these genes on neurite outgrowth. Ninjurin increased neurite length
by 52%, rab13 by 54%, and coronin 1b by 63% (figure 2). The number of neurite
branches was not affected by transfections.
Expression of rab13 and coronin 1b in cultured DRG neurons
Further in vitro and in vivo experiments were conducted for coronin 1b and rab13,
whose role in the nervous system is still largely unknown. To verify if coronin 1b and
rab13 protein expression were regulated during neurite outgrowth in cultured DRG
neurons, we performed immunoblotting experiments in E14 DRG cells from days one to
seven. Coronin 1b and rab13 expression were strongly induced between one and three
days (figure 3). Immunofluorescence experiments at days one, three, five, seven, nine and
fourteen in culture showed expression for coronin 1b and rab13 in the cytoplasm, and in
particular at the cortical cytoskeleton as shown by co-localization with F-actin (data not
shown); they were also found at the neurite terminals and growth cone, where staining
pattern suggested co-localization with the pro-plasticity / regeneration marker GAP-43
(figure 4). Consistent with immunoblot experiments, an increased immunofluorescence
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signal was detected for both proteins between day one and three. No difference in the
intensity of the staining was observed beyond day three (data not shown).
RNA interference experiments show that coronin 1b and rab13 repression inhibit
neurite extension in PC-12 cells after NGF
To examine whether members of this gene cluster were involved in neurite
outgrowth during differentiation, we performed gene silencing experiments using RNAi
(RNA interference) for coronin 1b and rab13 in PC-12 cells treated with NGF. Coronin
1b and rab13 RNAi gene silencing, which resulted in strong reduction of protein
expression (figure 5, panel A, and C), significantly reduced the extent of neurite
outgrowth in PC-12 cells after NGF treatment, by 53% and 44% respectively (figure 5,
panel B, and D).
Coronin 1b, and rab13 protein expression is induced after SCI preferentially in
neurons and axons undergoing plasticity
The combination of the gene expression changes in vivo and the findings from the
experiments in vitro suggested that these genes and proteins may modulate neural
plasticity in the spinal cord after injury. In accordance with gene array experiments, we
examined changes in protein expression by immunoblotting for coronin 1b and rab13 in
injured spinal cord at 7 and 14 days post-trauma and compared them to corresponding
sham samples. Both proteins were similarly increased after injury at these time points
(figure 6). We then studied expression of these proteins at the cellular level by
immunofluorescence in sham and injured spinal cords 14 days after injury. The proteins
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were co-examined with cell specific markers for neurons (anti-NeuN, and anti beta III
tubulin antibody), astrocytes (anti-GFAP), oligodendrocytes (anti-O2), and microglia
(anti-CD11). Increased expression for coronin 1b and rab13 were found after injury
(figure 7, panels A, and B), primarily in the cell membrane and cytoplasm, and showed a
preferential localization in neurons. Only weak expression was detected in astrocytes or
in microglial cells (data not shown).
To study the possible involvement of these proteins in neuronal and axonal
plasticity, we examined the degree of coronin 1b, and rab13 co-expression and co-
localization with the well established pro-plasticity /regeneration protein GAP-43. Using
confocal microscopy, immunofluorescence experiments showed that the proteins were
highly expressed in GAP-43 positive neurons and axons after injury, including expression
in dorsal root ganglia, and each likely co-localized with GAP-43 (figure 8).
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DISCUSSION
Using a hypothesis driven approach, combined with specific bioinformatics tools
to analyze coordinated gene expression profiles, we have identified a cluster of genes
induced between 7 and 28 days after experimental rat SCI, which appear to play a role in
neuronal plasticity and neurite outgrowth. These genes include ninjurin, coronin 1b,
rab13, synaptogyrin, synaptotagmin 1, and rap1b (Figure 1), which can be classified into
several functional classes: cytoskeleton remodeling, growth cone formation, axonal
plasticity, cell adhesion activity, and synaptogenesis. We have validated and quantified
the mRNA levels for a subset of these genes (ninjurin, rab13, Coronin 1b, rap1b, and
synaptogyrin) by real time RT-PCR in vivo at 14 days after injury, confirming microarray
results (table 2).
Certain of these genes - ninjurin, synaptotagmin, synaptogyrin, and rap1b -have
already been partially characterized in vitro and/or in vivo, and have been implicated in
axonal outgrowth, synaptic plasticity, and regeneration (20, 22-26, 33). Synaptotagmin,
and synaptogyrin are active throughout the entire synapse formation process- being
involved in vesicle docking, exocytosis, and endocytosis of synaptic vesicles- and
contribute to neurite extension (22, 33). Rap1b is a small GTPase belonging to Ras
superfamily of proteins, whose members may be involved in growth cone elongation, are
induced by NGF, and can promote neurite outgrowth (34). Rap1 itself plays a role in the
activation of the NGF dependent ERK pathway, leading to axonal elongation in PC-12
cells (26). The cell adhesion molecule ninjurin has also been reported to be induced by
peripheral nerve injury, and promotes axonal and neurite outgrowth in sciatic nerve and
DRG neurons following injury (20, 35).
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Neither coronin 1b nor Rab13 have been studied in the nervous system, nor have
they been implicated in plasticity or neurite sprouting. Rab13 is a small GTPase, a ras
superfamily member, which regulates intracellular vesicle trafficking to and from the
plasma membrane, and mediates exocytosis within the trans-Golgi network (TGN) (28).
Interestingly, rab 8, an analog to rab13, also belonging to TGN network, has been found
on cellular protrusions at the cortical cytoskeleton, and is co-localized with actin
filaments (30). Coronin 1b is an actin binding protein, belonging to the coronin family,
and may bind also to tubulin (27). It is important in cytoskeleton remodeling,
lamellipodia extensions and mitosis; moreover, coronin 1b and is localized to the cortical
cytoskeleton, where it is co-localized with F-actin (36, 37). It is known that cytoskeletal
organization and remodeling are essential cellular modifications during sprouting and
axonal elongation (for review, 38). Importantly, cilpin C, a human coronin-like homolog
protein, which is highly expressed in brain, has been identified in stress fibers and neurite
tips in SH-SY5 neuronal cells during neurite outgrowth (29).
Based upon these functional features of the identified gene cluster, transfection
experiments were performed in PC-12, SH neuroblastoma neuronal like cell lines, as well
as in DRG neurons, in order to examine whether expression of these genes promote
neurite elongation or sprouting. While expression of each of these genes enhanced
neurite outgrowth, ninjurin, rab13, and coronin 1b were most effective. Moreover,
coronin 1b, and rab13 RNAi experiments in PC-12 cells showed that inhibition of
coronin 1b, and rab13 protein expression reduced neurite outgrowth after NGF treatment.
While rab13 gene knock out has never been reported before, previous work in
Dictyostelium discoideum, showed that mutant cells lacking coronin grow and migrate
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more slowly than wild-type cells, probably by affecting cytokinesis (31). Also, in
vertebrate cells coronin expression at lamellipodia was disrupted by overexpression of
truncated mutants, inhibiting cell spreading and locomotion (32).
In cultured DRG neurons, coronin 1b, and rab13 were also co-expressed with
GAP-43 at neurite terminals and growth cones, and their expression increased during the
first days in culture along with the increase in neurite outgrowth. Parallel studies in vivo
demonstrated that coronin 1b, and rab13 protein expression were increased at both 7 and
14 days after rat SCI. They were primarily expressed in neurons, although low level of
expression was also present in astrocytes. Moreover, they were co-expressed and likely
co-localized with the pro-regeneration marker GAP-43 in neurons and axonal membranes
throughout the spinal cord, as well as in DRGs. The possible functional relationship
between cytoskeleton and membrane bound proteins coronin 1b, rab13 with GAP-43 is
also supported by the fact that GAP-43 itself accumulates in the pseudopods of spreading
cells and interacts with cortical actin-containing filaments and the cell membrane at the
growth cones (11).
Taken together, these data support a role for coronin 1b and rab13 in neuronal and
axonal plasticity. For most effective regeneration to occur after injury, multiple molecular
pathways may need to operate together in a coordinated fashion. These include the ability
of the damaged axons to extend the growth cone, to make cell-contacts with the extra-
cellular matrix (guidance), to form connections with nearby cells, and to achieve
functional synapses. The genes and proteins in the gene cluster here described play a
known or putative role in several of the above mechanisms; together their coordinated
action may induce more effective plasticity and regeneration than that resulting from
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expression of a single protein.
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FIGURE LEGENDS
Table 1. Table showing comparison of expression levels between sham and injured
cords for ninjurin cluster transcripts induced 14 days after SCI. These transcripts
represent genes that are temporally co-regulated with ninjurin gene based upon a
Standard correlation coefficient R2: 0.98. Genebank, gene names, fold changes and p
values are reported for each transcript.
Figure 1. Dendogram showing temporally co-regulated transcripts induced between
7 and 28 days after SCI.
Shown is a dendogram (gene tree) obtained using ninjurin as anchor gene to
nucleate co-regulated transcripts based upon a correlation coefficient R2: 0.99 (both
Standard and Pearson correlation). Expression levels in sham and injured cords at
different time points after SCI are represented with a specific color code. Bar graph on
the right shows the color code for gene expression level from low (blue) to high (red).
These transcripts are up-regulated between 7 and 28 days after SCI (asterix indicates a
Welch t test p value <0.05 between sham and injured at the corresponding time point).
Table 2. Table shows comparison of mRNA changes by Affymetrix and real time
RT-PCR for several transcripts up-regulated 14 days following SCI.
Figure 2. Over-expression of ninjurin cluster members in PC-12, neuroblastoma SH-
SY5 cells and DRG neurons promotes neurite outgrowth.
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Shown are bar graphs documenting increased neurite length of eGFP positive
cells after co-transfection with eGFP, and respectively with ninjurin; rab13; coronin 1b;
rap1b; synaptogyrin; synaptotagmin in PC-12 cells (panel A), in SH-SY5 neuroblastoma
cells (panel B), and DRG neurons (panel C). Bar graphs show difference in neurite
outgrowth between cells transfected with eGFP plus naked DNA, and eGFP plus each
experimental gene 72 hours after transfection (panel A-C). Number of transfected cells
with neurites at least 2X the diameter of the cell body is reported for PC-12 (panel A),
and SH-SY5 neuroblastoma cells (panel B). Length of the longest neurite per cell was
measured for DRG neurons and neurite length in ninjurin, coronin, and rab13 transfected
cells was compared to control GFP transfected cells and expressed as percentage of
control (panel C). For all experiments asterix represents significant t test p values <0.01.
Figure 3. DRG neurons time course shows increased neurite outgrowth and
increased protein expression from day one to three, and seven for coronin 1b and
rab13.
Panels A, B, C. Phase contrast images of representative DRG neurons in culture at day
one, three, and seven. Shown is increased neurite outgrowth in DRG neurons from day
one, to day three and seven.
Panel D. Shown is immunoblotting for coronin 1b and rab13 in E14 DRG neurons in
culture in the time course 1, 3, and 7 days.
Expression for coronin 1b and rab13 is strongly increased by day 3 in culture in DRG
neurons. Thirty micrograms of proteins were run on a 12% polyacrilamide gel for each
sample. Beta-actin is shown as loading control.
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Figure 4. Immunocytochemistry shows expression and localization of rab13 and
coronin 1b in GAP-43 positive cultured DRG neurons.
Shown is co-localization for coronin 1b (A, D) with GAP-43 (B, E), merged (C,
F), and for rab 13 (G, J) with GAP-43 (H, K), merged (I, L) in 7 days old DRG neurons
in culture. Staining for both coronin 1b, rab 13 and GAP-43 shows cytoplasmic
localization in the cell body, and expression in neurites, including at the growth cone
(labeled with G: A-C, and G-I). Panels D-F, and J-L are magnification of the growth cone
(G) from panels A-C, and G-I. Visible is the typical dotted staining at the growth cone for
GAP-43, as well as for coronin 1b and rab13. Original magnification: 400x (A-C, G-I);
850x (D-F, G-L)
Figure 5. RNA interference shows reduction of coronin 1b and rab13 protein levels,
and inhibition of neurite outgrowth in PC-12 after NGF.
Shown is the effect of coronin 1b and rab13 RNAi upon coronin and rab13
protein expression and neurite elongation in PC-12 cells after NGF.
Immunoblotting shows strong reduction of coronin 1b (panel A), and rab13 (panel
C) expression after siRNA delivery in PC-12 cells. β-actin is shown for protein
normalization.
Bar graphs show the inhibitory effect of coronin 1b (panel B), and rab13 (panel D)
siRNA delivery upon neurite length during NGF treatment (72 hours). Bar graphs
represent neurite length (measuring the length of the longest neurite per cell) expressed as
percentage of neurite length in control transfected cells (eGFP). Experimental cells were
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transfected with either coronin or rab13 siRNA and eGFP. Cells considered in the
measurements were cells positive for GFP, and with no immunoreactivity for coronin 1b
or rab13 staining, due the gene silencing effect, compared to control cells positive for
GFP and either coronin 1b or rab13 (asterix, t test p values <0.01). Neurite lenghts are
reduced to 53% of control in coronin 1b silenced cells, and to 44% in rab13 RNAi
experiments.
Figure 6. Immunoblotting shows induction of coronin 1b, and rab13 protein
expression at 7 and 14 days following SCI.
Immunoblotting at 7 and 14 days after SCI in sham and injured cords in duplicate
shows increased expression for coronin 1b, rab13 and ninjurin in injured cords. Fifty
micrograms of protein were loaded on a 12% polyacrilamide gel for each sample. β-actin
is shown for protein normalization.
Figure 7. Immunocytochemistry shows induction of coronin 1b, and rab 13 protein
expression in neurons at 7 and 14 days following SCI.
Double immunofluorescence in cross sections of spinal cord (ventral horns, 0,4-
0.5 cm below the injury site epicenter ) shows staining for coronin 1b (panel A), and rab
13 (panel B), and neuronal marker NeuN. Coronin 1b, and rab 13 (B, E) co-localize with
NeuN (A, D), merged (C, F) in sham (A-C) and injured cords (D-E) 14 days after SCI.
Coronin 1b, and rab 13 expression in neurons is much more intense in injured than in
sham cords. Original magnification: 125x
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Figure 8. Immunocytochemistry shows co-localization of coronin 1b, and rab13 with
GAP-43 in neurons and axons in dorsal root ganglia and dorsal horns in injured
cords 14 days after SCI.
Confocal microscopy immunofluorescence images show expression of coronin 1b
and rab13 along with pro-plasticity marker GAP-43 in dorsal root ganglia, and dorsal
horns of spinal cord 14 days following SCI (0.4-0.5 cm below the injury site epicenter).
Panel A. Cross sections of dorsal root ganglia fibers are positively stained for
coronin 1b (A), and for GAP-43 (B), and show membrane co-localization in all fibers
(merged, C). Cross sections of spinal cord (dorsal horns) show expression of coronin 1b
plus NeuN (D, red nuclear staining for NeuN and green cytoplasmic and membrane
staining for coronin 1b), GAP-43 (E), and coronin 1b plus GAP-43 (merged, F). Coronin
1b, and GAP-43 co-expression and co-localization is shown in neurons (arrowhead, F)
and axons (arrows, F) in cytoplasm and membrane. Immunostaining for neuronal
membrane specific marker beta III tubulin was also performed, and showed an identical
ring-like expression pattern (F, arrows) in the same cross sections (not shown).
Panel B. Cross sections of dorsal root ganglia fibers are positively stained for
rab13 (A), and for GAP-43 (B), and merged (C). Rab13 shows membrane co-localization
with GAP-43 in fibers (arrows, C), and cytoplasmic and membrane co-expression in a
cell body (arrowhead, C). Cross sections of spinal cord (dorsal horns) show expression of
rab13 plus NeuN (D, red nuclear staining for NeuN and green cytoplasmic and membrane
staining for rab13), GAP-43 (E), and rab13 plus GAP-43 (merged, F). Rab13, and GAP-
43 co-expression and co-localization are shown in neurons (arrowhead, F) and axons
(arrows, F) in cytoplasm and membrane. Original magnification: 400x
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Figure 4
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Figure 8
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Eric P. Hoffman and Alan I. FadenSimone Di Giovanni, Andrea De Biase, Alexander Yakovlev, Tom Finn, Jeanette Beers,
following spinal cord injuryIn vivo and in vitro characterization of novel neuronal plasticity factors identified
published online November 1, 2004J. Biol. Chem.
10.1074/jbc.M411975200Access the most updated version of this article at doi:
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