1 Cardiovascular Research Institute, University of California, San Francisco, CA 94143, USA
2 Department of Pediatrics, University of California, San Francisco, CA 94143, USA
3 Cancer Center, University of California, San Francisco, CA 94143, USA
4 Life Sciences Division, Genome Sciences, Ernest Orlando Lawrence Berkeley National Laboratory, Berkeley, CA 94720, USA
* Author for correspondence (e-mail: hsbernstein{at}pedcard.ucsf.edu)
Accepted 21 September 2004
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Summary |
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Key words: Sca-1, Myoblast fusion, Cell-cycle withdrawal, Ly-6, GPI-anchored proteins, Muscle regeneration
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Introduction |
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Although signaling events during myocyte differentiation have been studied in detail, cell-surface molecules that transmit signals from the extracellular milieu to these intracellular pathways are less well understood. Recent genetic studies in Drosophila have provided the first insights into mechanisms governing myoblast fusion. The Ig-like proteins Dumbfounded and Sticks and Stones support cellular adherence, whereas the membrane- and cytoskeletal-associated proteins Myoblast City and Rolling Stone facilitate formation of the fusion complex, which also requires cytoplasmic signaling proteins Rolling Pebbles and Antisocial (Taylor, 2002).
Other cell-surface molecules have been linked to muscle differentiation in vertebrates. Antibody blockade of ligand binding to ß1 integrins in chick embryos results in a predominance of early myogenic precursors (Menko and Boettiger, 1987), and whereas ß1 integrin-null myoblasts have been shown to be capable of fusion (Hirsch et al., 1998
), mice lacking ß1 integrin specifically in muscle have poorly developed muscle fibers (Schwander et al., 2003
). By contrast, murine embryonic stem cells deficient in
4 integrin can be differentiated into myoblasts that fuse to form myotubes (Yang et al., 1996
). Antibody interference of N-cadherin during early chick embryogenesis disrupts formation of early myogenic precursors (George-Weinstein et al., 1997
), and antibodies against N-cadherin inhibit cellular adherence in cultured chick myoblasts (Knudsen et al., 1990
); however, N-cadherin-null embryonic stem cells can differentiate into myoblasts with normal fusion properties (Charlton et al., 1997
).
During a screen for regulators of myoblast differentiation, we determined that expression of stem cell antigen-1 (Sca-1/Ly-6A/E), a stem cell marker, was transiently upregulated during myoblast cell-cycle withdrawal (Shen et al., 2003). Sca-1 is a member of the Ly-6 multigene family encoding several highly homologous, glycosylphosphatidylinositol (GPI)-anchored membrane proteins that are expressed on hematopoietic and lymphoid cells. The best characterized family member is Sca-1/Ly-6A, an antigen commonly used for purification of murine pluripotent hematopoietic cells (Patterson et al., 2000
). Although the ligand for Sca-1 is not known, studies have implicated Sca-1 and related family members in cell-cell adhesion among thymocytes (Bamezai and Rock, 1995
; Classon and Boyd, 1998
). Interestingly, ligands for other superfamily members contain epidermal growth factor (EGF)-like repeats, and a ligand for Ly-6D demonstrates significant homology to the Notch family responsible for somatic patterning in Drosophila (Aposolopoulos et al., 2000
). More recently, Sca-1 has been reported as a marker for muscle-derived stem cells (Asakura et al., 2002
; Jankowski et al., 2001
), and Sca-1-positive myogenic precursor cells appear to be recruited from the circulation to sites of myocardial injury (Oh et al., 2003
). However, a specific function for the Sca-1 antigen in muscle development has not been described.
We now report a previously unrecognized role for Sca-1 in myoblast differentiation and proliferation during myogenesis in C2C12 cells. Inhibition of Sca-1 expression using antisense or interference with Sca-1 activity using blocking antibodies prevent myoblast differentiation, causing sustained myoblast proliferation and producing a defect in myotube formation. Inhibition of Sca-1 expression also causes the derepression of Fyn kinase, and Fyn mutants recapitulate the phenotype of Sca-1 antisense-expressing cells. These results suggest both a mechanism for Sca-1 action and a novel pathway from the extracellular environment to myoblast differentiation.
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Materials and Methods |
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Primary myoblast isolation
Primary skeletal myoblasts were isolated according to standard procedures (Blanco-Bose et al., 2001). Skeletal muscle harvested from the hindlimbs of 10-20 C57BL/6 neonatal (3-day-old) mice was minced in cold, sterile phosphate-buffered saline (PBS), digested with 1.5 U/ml collagenase D, 2.4 U/ml dispase II, 2.5 mM CaCl2 at 37°C, filtered through 40 µm nylon mesh, centrifuged, resuspended in 80% Ham's F-10 nutrient mixture, 20% FBS, 2.5 ng/ml basic fibroblast growth factor (bFGF), and plated on laminin-coated dishes. After 24 hours, cells were harvested with trypsin-EDTA, incubated with monoclonal rat anti-
7 integrin antibody (clone CY8; gift of R. Kramer, UCSF) (Yao et al., 1996
), selected at least 5 times with MACS goat anti-rat IgG MicroBeads on an autoMACS magnetic cell sorter (Miltenyi Biotec), and re-plated in 40% Ham's F-10 nutrient mixture, 40% Dulbecco's Modified Eagle's media, 20% FBS, 2.5 ng/ml bFGF (proliferation medium) on collagen-coated dishes. Purity was analyzed by flow cytometric detection of
7 integrin, using monoclonal rat anti-
7 integrin antibody and phycoerythrin (PE)-conjugated donkey anti-rat F(ab')2 fragment (Jackson ImmunoResearch). Sorted cells were grown in proliferation medium for 5 days, and then transferred to differentiation medium (80% Dulbecco's Modified Eagle's media, 2% horse serum) to stimulate myotube formation.
Flow cytometric analysis
C2C12 cells and primary skeletal myoblasts were detached from culture with 0.25% trypsin, 2 mM EDTA at indicated times. Cells were washed with PBS, 10% FBS and fixed with 0.4% paraformaldehyde for 30 minutes at room temperature. After fixation, cells were washed with PBS, 2% calf serum (wash buffer) and then incubated in 100 µl wash buffer, 1% goat serum, 0.1% Triton X-100 containing primary antibodies at 4°C overnight. Cells were then washed with wash buffer and incubated in 100 µl wash buffer, 2 µg/ml DNAase-free RNAse A (Sigma) containing secondary antibodies at 37°C for 1 hour. Prior to flow cytometric analysis, cells were washed with wash buffer, filtered through 40 µm nylon mesh to exclude cell clumps and large myotubes, and incubated with 5 µg/ml propidium iodide (PI) at room temperature for 30 minutes. Primary/secondary antibody combinations used included monoclonal rat anti-Sca-1 (clone E13-161.7; BD Pharmingen) with PE-conjugated donkey anti-rat F(ab')2 fragment (Jackson ImmunoResearch), and monoclonal mouse anti-desmin (DAKO), anti-myosin (MF20; University of Iowa Developmental Studies Hybridoma Bank), or anti-MyoD (BD Pharmingen) with FITC-conjugated goat anti-mouse IgG (Sigma).
A Becton Dickinson FACSCalibur with 488 nm argon-ion laser was used to acquire PI, FITC and PE signals with 630/22 mm, 530/30 mm and 575/20 mm bandpass filters, respectively. Forward and side angle light scatter plots (as indicators of cell size and granularity), and PI, FITC and PE signals (to detect DNA content, desmin, myosin or MyoD, and Sca-1, respectively), were collected for at least 10,000 cells. PI area versus width plots were used to verify that our gating strategy included cell populations ranging from mononuclear cells with 2N DNA content to small, tetraploid myotubes containing 8N DNA content (Sharpless et al., 1975) that expressed MyoD and myosin. Data were analyzed using CellQuest software (Becton Dickinson).
Generation of stable antisense Sca-1 transfectants of C2C12 cells
A 330 bp fragment encoding nucleotides -9 to +321 of the Sca-1 coding sequence (Stanford et al., 1992), and flanked by EcoRI sites, was cloned by PCR from total mouse cDNA, inserted into the EcoRI site of vector pcDNA3.1A (Invitrogen), and screened for antisense orientation. The newly generated pLy6AS or empty pcDNA3.1A were transfected into C2C12 cells with Lipofectamine Plus reagent (Invitrogen) as instructed by the manufacturer. After 10 days of incubation in medium containing 800 µg/ml G418 (Life Technologies), resistant clones numbered 1-8 were isolated, expanded and screened for attenuation of Sca-1 expression by immunostaining and immunoblot, as described below. Stable cell lines were maintained in culture medium with 500 µg/ml G418. Expression levels of Sca-1 in clones 1-8 were measured by flow cytometry as described below. Experimental results were verified in multiple clones to ensure that observations were not the result of clonal variation inherent in C2C12 myoblast lines. Typical results for clone 6, which suppressed Sca-1 expression by 75% at two days in differentiation medium, are shown.
Immunostaining and immunoblot analysis
To detect Sca-1, Myf5, MyoD and myogenin in situ, wild-type and stably transfected C2C12 cells were plated on cover slips, grown as described for the indicated lengths of time, and stained with 2.5 µg/ml monoclonal anti-Sca-1 antibody (clone E13-161.7; Pharmingen) and 4 µg/ml FITC-conjugated goat anti-rat IgG (Pharmingen), or 10 µg/ml rabbit polyclonal anti-Myf5, anti-MyoD or anti-myogenin antibody (Santa Cruz Biotechnology) and 2 µg/ml FITC-conjugated goat anti-rabbit IgG (Molecular Probes), as previously described (Liu et al., 2003).
Immunoblot analysis was performed using previously described methods (Hlaing et al., 2002). Briefly, cells were lysed by sonication in lysis buffer (50 mM Tris-HCl, pH 7.5, 150 mM NaCl, 3 mM EDTA, 3 mM EGTA, 1% SDS, 10% glycerol), boiled for 5 minutes, and centrifuged at 16,000 g for 2 minutes. Protein concentrations in supernatants were measured by BCA assay (Pierce), and equal amounts of protein (100-200 µg) were separated by SDS-polyacrylamide gel electrophoresis. Immunoblots were analyzed with 5 µg/ml monoclonal antibody against Sca-1 (Pharmingen) or ß-actin (Sigma), and 1 µg/ml horseradish peroxidase (HRP)-conjugated goat anti-mouse (Bio-Rad) IgG.
BrdU incorporation and myoblast fusion assays
Cells were plated on cover slips, cultured under conditions described above, and labeled with 5-bromo-2-deoxyuridine (BrdU) for 60 minutes using Labeling and Detection Kit I (Roche) according to the manufacturer's instructions. Cells were stained with 1:10 dilution of monoclonal anti-BrdU (Roche), followed by 4 µg/ml Alexa Fluor594-conjugated goat anti-mouse IgG in incubation buffer provided with the Labeling and Detection Kit I (Roche). Cells were co-stained with antibodies against Myf5, MyoD or myogenin as described above. Prior to mounting cover slips on slides, cells were incubated with 1 µg/ml DAPI (Sigma) for 5 minutes at room temperature. Immunofluorescence signals were acquired with a Nikon Microphot-FX fluorescence microscope and Spot imaging software. At least 1000 nuclei and 20 myotubes were counted from several random fields. Cell proliferation was calculated as percent BrdU-positive nuclei per field. Fusion index was calculated as number of nuclei in myocytes containing 2 nuclei/total number of nuclei. All experiments were performed at least three times with independent cultures, and quantification values are reported as the mean±standard error of the mean (s.e.m.).
Fyn and Src kinase assays
Cells were cultured under conditions described above, lysed in lysis buffer [25 mM Tris, pH 7.2, 150 mM NaCl, 100 µm Na3VO4, 1% NP-40, 10 mM NaF, 1:1000 Protease inhibitor cocktail (Sigma)] for 30 minutes on ice, sheared by needle passage, then centrifuged at 11,750 g for 6 minutes at 4°C. Total supernatant protein was determined by BCA assay (Pierce). One mg total protein was incubated with 2 µg monoclonal anti-Fyn or anti-Src antibody (Santa Cruz Biotechnology) for 2 hours at 4°C, and 50 µl protein-A sepharose (Sigma) for an additional 30 minutes. Immune complexes were washed with ice-cold lysis buffer, then re-suspended in 40 µl ice-cold kinase reaction buffer (100 mM Tris, pH 7.2, 125 mM MgCl2, 25 mM MnCl2, 2 mM EGTA, 25 µM Na3VO4, 2 mM DTT) with 20 µM ATP and 4 µM [-32P]ATP (6000 mCi/mmol). Reactions were incubated with 150 µmol substrate peptide [(K19) cdc2 (6-20)NH2, KVEKIGEGTYGVVKK; Upstate] for 10 minutes at 30°C with vigorous agitation. Reactions were stopped on ice and proteins precipitated with 20 µl 40% tricholoracetic acid. Precipitates were collected on phosphocellulose squares (Upstate), washed with 0.75% phosphoric acid then acetone, and dried prior to measuring incorporated radioactivity by Cerenkov counting. Counts were normalized against immunoprecipitated Fyn or Src protein determined by immunoblot with monoclonal anti-Fyn or anti-Src antibody and densitometry (Adobe Photoshop and NIH/Object-Image), and expressed as fold-increase over background (immunoprecipitation performed without primary anti-Fyn or anti-Src antibody). Experiments were performed at least three times and quantification values are reported as the mean±s.e.m.
Fyn mutant assays
A 1615 bp fragment of pCMV-FynDN (Ko et al., 2002), containing the full-length, dominant-negative K299M mutant of human Fyn, was amplified by PCR using primers 5'-TTATGCGGCCGCATGGGCTGTGTGCAATGTAAGG-3' and 5'-GCATGCATGCTTACAGGTTTTCACCAGGTTGG-3' and cloned into NotI/SphI sites in pIRES-hrGFP-1a (Stratagene). pCMV-FynDN was the kind gift of M. Resh (Sloan-Kettering Cancer Center). The 1.6 kb BamHI fragment of Fyn-Y531F (Maulon et al., 2001
), containing the full-length, constitutively active Y531F mutant of mouse Fyn, was cloned into the BamHI site in pIRES-hrGFP-1a (Stratagene). Fyn-Y531F was generously provided by P. Auberger (INSERM). Sequences for both plasmids expressing Fyn mutants and green fluorescent protein (GFP) were confirmed. Expression of mutants and GFP was determined by immunoblot of whole cell lysates from transfected C2C12 cells with anti-Fyn antibody (Santa Cruz Biotechnology), and immunofluorescence detection of GFP in live cells.
Cells were plated on cover slips and cultured under conditions described above. Transfections were performed using Lipofectamine 2000 (Invitrogen) according to the manufacturer's instructions 24 hours prior to switching cultures to differentiation conditions. Prior to mounting cover slips on slides, cells were incubated with 1 µg/ml DAPI (Sigma) for 5 minutes at room temperature. Data were acquired with a Nikon Microphot-FX fluorescence microscope and Spot imaging software. Each set of transfections with mutant Fyn constructs was performed in triplicate, with data representing the mean of 10 medium-power (20x) fields (>2000 nuclei counted per experiment). The effect of Fyn mutants on cell fusion was measured as the ratio of GFP-positive mononuclear myoblasts:GFP-positive myotubes (cells with two or more nuclei). Experiments were performed at least three times and quantification values are reported as the mean±s.e.m.
Statistical analysis
To determine significance between two groups, comparisons between means were made using the Student's t-test. Multiple group comparisons were performed by one-way ANOVA with Student-Newman-Keuls' post hoc test. Trendlines were generated by bivariate regression analysis using the Pearson coefficient. SPSS version 11 for Macintosh (SPSS) was used for all tests, with a 0.05 level of confidence accepted for statistical significance.
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Results and Discussion |
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To determine further the expression of Sca-1 on the surface of C2C12 myoblasts on a per cell basis, we performed flow cytometry on proliferating C2C12 cells, and cells grown in differentiation medium for two days, which is the time point of maximal Sca-1 expression (Fig. 1A). We observed that whereas the majority (74%) of proliferating myoblasts were Sca-1-negative, more than half of the cells (51%) were positive for Sca-1 surface expression at the time of cell-cycle withdrawal during myogenesis (P=0.008). Although immunoblot analysis suggested that Sca-1 expression declines overall by five days in differentiation medium (Shen et al., 2003), the heterogeneity of cell size in differentiated cultures precluded us from analyzing these cultures by flow cytometry. However, these data suggest that subpopulations of C2C12 cells (Sca-1-positive and Sca-1-negative) exist.
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GPI-anchored proteins are necessary for myoblast cell-cycle withdrawal and myotube formation
To investigate the role of GPI-anchored cell-surface proteins in myoblast differentiation, we used the GPI-specific phospholipase, phosphatidylinositol-specific phospholipase C (PIPLC) (Griffith and Ryan, 1999), to strip GPI-anchored proteins from the surface of C2C12 myoblasts (Fig. 1B,C). Treatment with PIPLC had a profound effect on myotube formation (Fig. 2A), resulting in primarily mononuclear myoblasts even when grown under differentiation conditions. Specifically, removal of GPI-anchored proteins from the surface of C2C12 myoblasts resulted in a decrease in myoblast fusion index (0.08±0.07 versus 0.65±0.12; P=0.004) and an increased level of BrdU incorporation (37±2% versus 3±1% BrdU-positive nuclei; P=0.003) (Fig. 2B,C) under conditions that normally would produce terminally differentiated myotubes (Shen et al., 2003
). This suggested that a GPI-anchored protein, such as Sca-1, might regulate cell-cycle withdrawal and myotube formation during myocyte differentiation.
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To test whether GPI-anchored proteins play a similar role in myogenesis in other myoblasts and across species, we performed similar experiments in Sol8 murine myoblasts (Fig. 2D-F), L6 rat myoblasts (Fig. 2G-I) and QM7 avian myoblasts (Fig. 2J-L). Consistent with our findings in C2C12 cells, we observed that PIPLC decreased myotube formation and increased BrdU incorporation in Sol8 (fusion index 0.13±0.03 versus 0.66±0.07, P=0.004; 18±2% versus 1±1% BrdU-positive nuclei, P=0.01), L6 (fusion index 0.05±0.03 versus 0.75±0.08, P=0.024; 20±2% versus 2±1% BrdU-positive nuclei, P=0.009) and QM7 (fusion index 0.06±0.03 versus 0.83±0.10, P=0.031; 48±5% versus 1±0.5% BrdU-positive nuclei, P=0.005) cells. These results in different skeletal muscle types and species suggest a general role for GPI-anchored proteins in myogenesis.
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Sca-1 inhibition results in defective myogenesis and sustained myoblast proliferation |
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Clone E13-161.7 originally was raised against BALB/c mouse `pre-T' cells (Aihara et al., 1986), whereas clone D7 was raised against the interleukin 2 (IL-2)-dependent mouse T-cell line CTL-L (Ortega et al., 1986
). Although both antibodies react with Sca-1, they recognize distinct epitopes as D7 is unable to block binding of E13-161.7 (Bamezai and Rock, 1995
). In our experiments, antibody treatment did not alter Sca-1 expression, as determined by immunoblot (data not shown). Whereas treatment with either antibody alone produced no significant difference in myoblast fusion or DNA synthesis, compared with untreated cells or cells similarly treated with anti-CD34, which is a primitive stem cell marker also found on C2C12 myoblasts (Beauchamp et al., 2000
), the two anti-Sca-1 antibodies in combination blocked myotube formation and sustained myoblast proliferation compared with untreated control cells, similar to the effects seen with PIPLC treatment (fusion index 0.30±0.06 versus 0.60±0.05, P<0.001; 11±3% versus 3±1% BrdU-positive nuclei, P<0.001) (Fig. 3A,B). These effects on myoblast differentiation and DNA synthesis could be seen as far out as at 10 days of antibody treatment, with complete reversal of these effects upon removal of antibody (data not shown).
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Previously, it has been shown that D7 antibody alone can inhibit thymocyte aggregation by 80-90% (Bamezai and Rock, 1995); however, D7 was unable to block myotube formation in our studies in the absence of E13-161.7 antibody. This suggests that the mechanism for Sca-1-mediated myoblast differentiation is different from its mechanism for aggregation in thymocytes, perhaps involving other pro-differentiation events that are myoblast specific.
To determine whether Sca-1 expression is necessary for myoblast cell-cycle withdrawal and differentiation, we made stable cell lines expressing sense and antisense versions of full-length Sca-1. Sca-1-overexpressing cells behaved no differently than sham-transfected or untransfected cells (data not shown), and were not included in subsequent experiments. This suggested that Sca-1 does not confer a gain of function in cells already expressing Sca-1. Antisense-expressing cells showed a significant downregulation of Sca-1 expression, compared with a cell line stably transfected with empty vector (Fig. 3C,D). When grown in differentiation media, Sca-1 antisense-expressing cells displayed a fusion defect with short, paucinuclear myotubes (fusion index 0.09±0.07 versus 0.65±0.05; P<0.001) (Fig. 3E), and retained a higher proliferation index (29±4% versus 3±1% BrdU-positive nuclei; P<0.001) (Fig. 3F), compared with untransfected or sham-transfected cells. These data demonstrated that Sca-1 is necessary for proper cell-cycle withdrawal and myotube formation during C2C12 differentiation.
Because others have shown that myoblasts that fail to differentiate undergo apoptosis, we also analyzed Sca-1 antisense-expressing cells for cell death and p21 expression. Compared with control C2C12 cells, which showed Sca-1 antisense-expressing cells, which continue to proliferate in differentiation medium, failed to induce p21 expression and demonstrated an increase in apoptosis (C.L.E., J.E.L. and H.S.B., unpublished). Although these data suggest that Sca-1 might influence p21 expression, and consequently protect against apoptosis, how Sca-1 couples to p21 expression remains to be determined.
Sca-1 inhibition arrests myoblast differentiation
Since experiments with blocking antibodies and antisense directed against Sca-1 suggested that Sca-1 regulates myoblast cell-cycle withdrawal and myotube formation, we wanted to determine whether blocking Sca-1 affected the expression of skeletal muscle differentiation markers. We grew C2C12 cells expressing Sca-1 antisense in differentiation medium for five days and co-stained these cells with antibodies against Myf5, MyoD and myogenin, as markers of specific stages of C2C12 differentiation (Fig. 4) (Sabourin and Rudnicki, 2000; Shimokawa et al., 1998
). Myf5 and MyoD were observed both in >90% of proliferating control and antisense-expressing cells (P>0.1), whereas MyoD and myogenin were found in differentiated control (90% and 50%, respectively) and antisense (95% and 60%, respectively) cells, with no significant difference in the percent positive cells for either myogenic regulatory factor between control and antisense-expressing cells (P>0.1) (Fig. 4A). However, expression of the earliest marker of myogenic commitment, Myf5 (Beauchamp et al., 2000
), persisted in cells expressing Sca-1 antisense grown under differentiation conditions (78%±12% Myf5-positive nuclei in antisense-expressing cells at day 5 versus 4%±3% in control C2C12 cells; P=0.019) (Fig. 4A). To determine whether the Myf5-positive, Sca-1 antisense-expressing cells grown under differentiating conditions comprised the pool of proliferating cells previously detected (Fig. 3F), we labeled cells with BrdU, and co-stained with antibodies against BrdU and Myf5. The percentages of BrdU-positive control and antisense-expressing cells in proliferating and differentiating cultures were the same as reported above (Fig. 3F). However, the majority of Sca-1 antisense-expressing, Myf5-positive cells were actively proliferating (Fig. 4B). These studies demonstrate that inhibiting Sca-1 expression results in a proliferating pool of mononuclear myoblasts that persist in an early stage of differentiation, despite culture under conditions that would result in myotube formation in wild-type cells.
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Sca-1 is necessary for appropriate regulation of Fyn activity during myogenesis
Some GPI-anchored proteins signal through Src-family tyrosine kinases (Horejsi et al., 1998; Marmor and Julius, 2000
). Specifically, Sca-1/Ly-6A/E has been shown to signal through Fyn during T-cell activation in vitro (Lee et al., 1994
). However, whereas in vitro crosslinking of Sca-1 in T cells results in Fyn autophosphorylation (Lee et al., 1994
), observations with Sca-1-null mice suggest that Sca-1 downmodulates lymphocyte responses (Stanford et al., 1997
). Recently, Fyn activity has been implicated in the regulation of anti-apoptotic pathways in differentiated myotubes, but specifically has been shown to be inactive during earlier stages of myogenesis (Laprise et al., 2002
).
To determine whether Sca-1 function in myoblasts is mediated through Fyn, we assayed Fyn and Src activity in myoblasts stimulated to form myotubes. Both wild-type and Sca-1 antisense-expressing cells demonstrated constitutive Src activity, independent of differentiation stage or Sca-1 expression (Fig. 5A, bottom). Fyn activity was elevated in wild-type cells at day 5 in differentiation medium (Fig. 5A, top), consistent with the previously demonstrated role of Fyn in protecting differentiated myotubes against apoptosis (Laprise et al., 2002). By contrast, Fyn activity was elevated in Sca-1 antisense myoblasts at day 2 in differentiation medium, compared with wild-type cells (P=0.012) (Fig. 5A, top). This time point coincides with the transient increase in Sca-1 expression observed during myoblast cell-cycle withdrawal and early differentiation (Shen et al., 2003
). This finding suggested that inappropriate Fyn activity at an earlier stage of myogenesis might provide a mechanism for the sustained proliferation and arrest in myogenic differentiation seen in Sca-1 antisense cells.
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We also tested whether anti-Sca-1 antibodies, capable of producing a similar though less-robust effect on myoblast differentiation, likewise affected Fyn activity. In contrast with the upregulation of Fyn activity in Sca-1 antisense-expressing cells at 2 days in differentiation medium, we observed no detectable difference in Fyn activity in cells treated with antibodies compared with untreated cells or cells treated with anti-CD34 antibody (data not shown). Since the alteration in Fyn activity with antisense expression was significant but modest (Fig. 5A), and antisense expression probably has a more consistent effect on Sca-1 than antibody blockade, the ability to detect an alteration in Fyn activity with antibody blockade might fall below our threshold for detection. We did observe that antisense expression had a more-significant effect on BrdU incorporation and myoblast fusion, compared with antibody treatment, as shown in Fig. 3 (fusion index 0.30±0.06 with antibody treatment versus 0.09±0.07 with antisense expression; 11±3% BrdU-positive nuclei with antibody treatment versus 29±4% with antisense expression), which is consistent with this explanation.
Why should there be such variability between antibody blockade and antisense expression? We showed that there is variability in Sca-1 expression, with Sca-1+ and Sca-1- populations present at various times during differentiation (Fig. 1A). Such `shifting' antigen concentrations might explain the incomplete effect of antibody treatment on BrdU incorporation and myoblast differentiation, and the failure to detect a measurable change in Fyn activity. To evaluate further the role of Fyn in Sca-1-mediated myogenesis, we co-expressed a dominant-negative mutant of Fyn and GFP (K299M) (Ko et al., 2002) in Sca-1 antisense-expressing cells and found that the ratio of transfected myoblasts:myotubes (as indicated by GFP expression) after five days in differentiation medium was lower in cells expressing dominant-negative Fyn compared with cells expressing GFP alone (2.3±0.7 versus 5.7±1.6; P=0.006) (Fig. 5B). Conversely, we co-expressed a constitutively active form of Fyn and GFP (Y531F) (Maulon et al., 2001
) in wild-type C2C12 cells and found that the ratio of transfected myoblasts:myotubes at five days in differentiation medium was higher in cells expressing active Fyn compared with cells expressing GFP alone (4.9±1.7 versus 1.7±0.8; P=0.044) (Fig. 5B). We also monitored BrdU incorporation in transfected cells, and observed that >90% of nuclei in mononuclear cells were BrdU positive (data not shown). These studies demonstrated that dominant-negative Fyn rescued the Sca-1 antisense phenotype, whereas active Fyn produced the Sca-1 antisense phenotype in wild-type C2C12 cells. It is important to note that whereas expression of Sca-1 antisense produced a tenfold change in myoblast fusion and BrdU incorporation, the effect of constitutively active Fyn was less pronounced. Although this may, in part, be explained by technical differences between transient transfection of mutant Fyn versus stable, constitutive expression of Sca-1 antisense, it also supports the possibility that Fyn alone may not be solely responsible for mediating Sca-1 effects. However, our observations suggest that the effects of Sca-1 in differentiating myoblasts are mediated at least in part by Fyn, that Sca-1 expression couples to the downregulation of Fyn activity during early myogenesis, and that inappropriate activation of Fyn is associated with sustained myoblast proliferation and a defect in myotube formation.
The role of Sca-1 in myoblast differentiation and cell-cycle withdrawal may be analogous to its role in T cells, where the absence of Sca-1 results in a more rapid and prolonged T-cell proliferative response (Stanford et al., 1997). Our findings also suggest that Fyn activity is temporally regulated during myoblast differentiation. Normally, Fyn activity is upregulated in differentiated myotubes, and is necessary for protecting post-mitotic muscle cells from apoptosis (Laprise et al., 2002
). Downregulation of Sca-1 by antisense leads to premature activation of Fyn, which may be responsible for sustained proliferation. This suggests a role for Sca-1 in either suppressing Fyn activity or influencing the integration of Fyn with other signaling pathways that converge on the early myogenic program.
Although a role for Fyn in cellular proliferation and survival has been established in a variety of cell types (Resh, 1998), how Sca-1 couples to Fyn is not known. Plasma membrane microdomains couple signaling in space and time between GPI-anchored proteins on the extracellular surface and signaling proteins compartmentalized in the cytoplasmic leaflet of the plasma membrane, such as non-receptor protein tyrosine kinases and G proteins (Alonso and Millan, 2001
; Matko and Szollosi, 2002
). Transmembrane-spanning coreceptors also coalesce in these microdomains, and may be required for transmitting signals from GPI-anchored proteins (Werlen and Palmer, 2002
). Whether Sca-1 signals directly through Fyn, or brings components of membrane microdomains together that ultimately regulate Fyn activation, remains to be demonstrated.
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Conclusions |
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Our findings suggest the question: is Sca-1 essential for normal muscle development in vivo? Sca-1-null mice have been reported as grossly normal, with T cells that demonstrate a more rapid and prolonged proliferative response (Stanford et al., 1997). Whether these mice have abnormal muscle phenotypes with respect to performance or regenerative capacity is not yet known. We have determined that, similar to our observations in C2C12 cells, Sca-1 is expressed on a subpopulation of primary murine skeletal myoblasts, and that this population decreases in number with myogenic differentiation and the expression of myosin (Fig. 6). Several recent studies have implicated Sca-1 as a marker of myogenic precursor cells that are recruited to a regeneration program following muscle injury (Jankowski et al., 2001
; LaBarge and Blau, 2002
; Oh et al., 2003
; Polesskaya et al., 2003
). Additional studies of muscle injury in Sca-1-null mice would be informative. Mice null for thymic shared antigen-1, another Ly-6 superfamily member, recently have been reported to exhibit growth delay at E14.5 and absorption by E16 (Zammit et al., 2002
). This was preceded by the appearance of thinned ventricular myocardium with abnormal trabeculation, in the presence of otherwise normal atrioventricular and semilunar valves, at E14 (Zammit et al., 2002
). These observations suggest a primary defect of myocardial development, and are consistent with an important role for Ly-6 family members in muscle development.
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In conclusion, our studies describe a novel pathway from the extracellular environment to cell-cycle withdrawal and myogenic differentiation in C2C12 cells, and suggest that blocking Sca-1 should be explored as a strategy for muscle regeneration.
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Acknowledgments |
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References |
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