1 Pennsylvania Muscle Institute, University of Pennsylvania Medical Center, D-700 Richards Building, 3700 Hamilton Walk, Philadelphia, PA 19104-6083, USA
2 Department of Chemical and Biomolecular Engineering, Towne Building, 220 South 33rd Street, University of Pennsylvania, Philadelphia, PA 19104-6393, USA
3 Department of Physiology, University of Pennsylvania Medical Center, 3700 Hamilton Walk, Philadelphia, PA 19104-6085, USA
4 Graduate Group in Cell and Molecular Biology, University of Pennsylvania Medical Center, 3620 Hamilton Walk, Philadelphia, PA 19104-6058, USA
* Author for correspondence (e-mail: discher{at}seas.upenn.edu)
Accepted 10 January 2005
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Summary |
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Key words: Sarcoglycan, Muscular dystrophy, Limb-girdle muscular dystrophy, Differentiation
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Introduction |
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As dystrophin and the DGC contribute to the tensile strength of muscle as well as membrane integrity and elasticity (Bradley and Fulthorpe, 1978; Grady et al., 1997
; Straub et al., 1997
),
SG was initially expected to also play a role in the strength and integrity of the sarcolemma. In work with muscle from knockout mice however, no decrease in tensile strength or membrane integrity was found in
SG-deficient muscle compared with normal muscle. Apoptosis is reported to increase (Hack et al., 1998
), but the underlying mechanism for the MD phenotype is unclear.
A possible role for SG in adhesion, and perhaps anchorage-dependent signaling, is suggested by integration of
SG into the DGC and adhesion complexes, however, connections to cytoskeletal processes are also possible. Membrane adhesion complexes generally mediate a balance between cytoskeletal tension, contractility, or `prestress' and a mechanical resistance of extracellular substrates or matrix (ECM) (Lee et al., 1998
; Stamenovic et al., 2002
). Prestress has been measured for many cell types under various conditions (Hubmayr et al., 1996
; Potard et al., 1997
; Wang et al., 1993
; Wang et al., 2002
), and various components of the cytoskeleton have been individually associated with this prestress, including actin, myosin, microtubules, and intermediate filaments. Signaling aspects of such sustained contractility are unclear, especially in relation to
SG function.
We provide initial evidence here of signaling pathways that are perturbed in SG/ muscle. First, however, we used novel micromanipulation techniques to examine the prestress and adhesion dynamics of both normal and
SG/ myotubes. In decoupling the effects of adhesion from the effects of cellular prestress, we found that
SG/ cells have similar adhesive properties to normal cells, but they appear to have enhanced prestress associated with contractility. This seems to be moderated in its effects by downregulation of apoptotic signals that contribute to the MD phenotype. The results here may suggest new approaches to influence the course of disease.
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Materials and Methods |
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Microscopy
All microscopy was done with a Nikon TE300 inverted microscope. Fluorescently labeled cells and/or nuclei were imaged with either a 40x 0.45 NA objective (TUNEL assays) or a 60x 1.45 NA oil objective (immunofluorescence). Images were recorded with a Cascade CCD camera (Photometrics, Tucson, AZ), and fluorescence intensity was measured using Scion Image (Scion Corporation, Frederick, MD). Relaxing or peeling of cells were observed through a 10x 0.17 NA phase-contrast objective and images were recorded onto video through a video-rate camera (model JE8242, Javelin Systems, Torrance, CA).
TUNEL assay
TUNEL assays were performed on formaldehyde-fixed samples using the ApopTag in situ apoptosis fluorescein detection kit (Chemicon International, Temecula, CA).
Fluorescence staining
Both C57 and SG/ cells were stained for actin, myosin,
-sarcoglycan (
SG) and
SG. Cells were rinsed with PBS and fixed in 10% formaldehyde. Cells were then permeabilized in 0.1% Triton X-100 and incubated in a 5% bovine serum albumin blocking solution at 37°C for 1 hour. After blocking, the cells were incubated overnight at 4°C in one of the following four primary antibody solutions in PBS: 1:50 mouse anti-myosin (Zymed, San Francisco, CA, 18-0105), 1:10 mouse anti-utrophin (NovoCastra, Newcastle-upon-Tyne, UK, NCL-DRP2), 1:100 mouse anti-
SG (NovoCastra, NCL-a-SARC), or 1:100 mouse anti-
SG (NovoCastra, NCL-g-SARC). Control samples were incubated in pure PBS without primary antibody. Cells were then fluorescently labeled by incubation for 1 hour at 37°C in 1:100 FITC-conjugated anti-mouse IgG (F2761; Molecular Probes, Eugene, OR) in PBS. Cells previously labeled for myosin were co-labeled for actin at this point by adding 60 µg/ml TRITC-phalloidin (Sigma) to the secondary antibody solution. Finally, the cell nuclei were labeled with 1:100 Hoechst 33342 (Molecular Probes), and the samples were mounted onto slides using Gel/Mount (Biomedia, Foster City, CA).
For quantification of fluorescence, a relative intensity RI was defined. As RI=1 means there is no increase in fluorescence over the control, the RIs are represented with a minus sign for RI1 and a single plus sign for 1<RI
1.5. An additional plus sign is added for every 0.5 increase after 1.5, so an RI of 2.7, for example, is represented as `+++'.
Single cell relaxation
Patterned myotubes were allowed to relax as previously described (Griffin et al., 2004a). In brief, one end of an isolated myotube was mechanically detached from the substrate with a micropipette pre-incubated in BSA. The myotube then recoiled or relaxed for up to 6 minutes. The relative length of the myotube during the process was monitored by video, and at times, the stage was repositioned in order to keep the cell in the field of view.
Single cell peeling
Isolated myotubes were also forcibly peeled from the substrate using the micropipette peeling technique described (Griffin et al., 2004a). Briefly, a large-bore micropipette with an inner diameter of 75 µm (Polymicro Technologies, Phoenix, AZ) was pre-incubated in BSA to minimize cell-pipette interactions. The pipette was attached to a syringe pump (model SP120p-300, World Precision Instruments, Sarasota, FL) with a flow rate that ranges from 0.001 µl/minute to 602 µl/minute. After one end of the cell was mechanically detached, the syringe pump was used to initiate a flow and cells were peeled from the substrate using a motorized stage. Because of the large size of the micropipette compared with the dimensions of the cell, the shear stress,
cell of the aspirating fluid drove the cell peeling, and the peeling tension Tpeel is simply the integral of
cell over the length of cell inside the pipette, Lasp. Peeling experiments were recorded in the same manner as relaxation experiments, and the velocity of the peel, Vpeel, was measured as a function of Tpeel.
Phosphoscreen on TA muscle
Whole cell lysates were prepared from samples of unstretched and stretched TA (tibialis anterior) muscle obtained from juvenile (8-week-old) C57 and SG/ mice according to published protocols (Pelech et al., 2003
). Stretching of
10% for 20 minutes was done after dripping calcium-free PBS on the muscle. 300 µg of these protein lysates were separated by SDS-PAGE and were immunoblotted in a 20-lane Immunetics multiblotter using commercially available antibodies as recently described for the Kinexus KPSS5.0-phospho and KPSP-1 phosphoscreen (Pelech et al., 2003
). The immunoblots were then subjected to enhanced chemiluminescence, and were identified based upon human protein sequences. Finally, the bands were detected with a Bio-Rad FluorS Max Multi-imager (Bio-Rad Laboratories, Hercules, CA) and the relative intensities were quantified with Quantity One software (Bio-Rad) and reported as arbitrary units (a.u.), normalized to correct for differences in protein concentration. The results are accurate to within 25%.
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Results |
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NIglass/NIAclar was determined for C57 and SG/ cells at both 2 and 7 days after plating (Fig. 1). In comparing day 7 to day 2, we found a 17-fold increase in the NIglass/NI for Aclar
SG/ cells. The ratios for C57 cells at both days were not significantly different, and also compared well with the NIglass/NIAclar for
SG/ cells at day 2. Thus, we concluded that within 7 days,
SG/ cells cultured on glass apoptosed to a far greater extent than either C57 cells or nascent
SG/ myotubes.
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SG/cells striate more than controls
Representative proteins expressed by C57 and SG/ cells on day 6 in culture were quantified as the average fluorescence intensity after immunostaining of parallel cultures. Intensities were measured for cells growing both on top of other cells (upper layer) and also directly on the IPN-patterned glass (lower layer). The cells-on-cells accounted for approximately 60% of the patterned cells and occurred as cells crawled onto other cells, without any outside impetus. Intensities were normalized by dividing by the average intensity of cells stained only with secondary, and not primary, antibody. The resulting values were defined as the relative intensities and converted to simpler `+' and `' notation in Table 1 (see Materials and Methods).
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Table 1 confirms that the SG/ cells did not express
SG and also lost
SG (Hack et al., 1998
). We also saw that both cell types growing directly on the IPN-patterned glass expressed significantly less myosin than cells growing on top of other cells at day 6. At day 6, utrophin followed a similar trend;
SG/ cells showed less utrophin than normal cells and C57 cells-on-cells expressed slightly more utrophin than cells-on-glass. As it has been documented that utrophin expression in muscle culture increases and then decreases with differentiation (Radojevic et al., 2000
), the reduced utrophin levels implied that
SG/ cells were either less differentiated or more differentiated than normal cells. Results below show that the latter appeared to be the case.
In addition to measuring the fluorescence intensity, cells immunostained for myosin were scored based on the amount of structured or striated myosin present (Fig. 2). Structured myosin was identified as fibrous and non-diffuse, but without any striations. Although a small percentage of cells growing directly on the glass formed myosin fibers instead of exhibiting only diffuse myosin (Fig. 2B), completely striated myosin formed only in cells-on-cells (Fig. 2C), consistent with results previously reported by our laboratory (Engler et al., 2004a; Engler et al., 2004b
; Griffin et al., 2004b
). Striated myosin was seen in almost 50% of
SG/ cells-on-cells, whereas in normal, C57 cells, less than half that amount of striation was observed (Fig. 2D).
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Although the upper layer of C57 cells seemed to express more myosin than the upper layer of SG/ cells (Table 1), the myosin in
SG/ cells showed more structure and striation overall. It could be that the tighter organization made immunostaining less efficient, reducing the intensity. Regardless, the data in Table 1 indicated differences between upper and lower cells.
SG/ cells relax more than controls
By detaching the end of an adherent myotube from its substrate, the relative length of the myotube was seen to decrease as the cell relaxed from its adhesive constraints (Fig. 3A). The decay was exponential over time (Fig. 3B). Myotube relaxation can be modeled simply as a Voigt solid (Griffin et al., 2004a), and the relative length fits very well to the equation,
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Although SG/ cells exhibited more heterogeneity during relaxation, there was a clear difference in relaxation dynamics compared with normal C57 cells. The average shortening amplitude of
SG/ cells was twice as large as that of C57 cells. This difference applied regardless of whether A was calculated from a fit of the data compiled from multiple cells as in Fig. 3B, or by averaging A from fits of individual cells. There was no significant difference in time constants between the cell types. Because
is indicative of the adhesive drag, whereas A represents the cellular prestress, the stronger dependence on A suggested that a contractile prestress, rather than adhesion, caused the difference in relaxation dynamics.
When observing fixed cells that have not been mechanically disturbed, we also saw that a fraction of isolated myotubes growing on IPN-patterned glass appeared very wide in the center compared with the ends (Fig. 4A). This shape was reminiscent of a cell mechanically induced to relax by micropipette perturbation: in either case the cell is tethered at one end, but it shortens and widens as it pulls back. It appeared that cells with this wider shape were `self-relaxing' or relaxing without mechanical end-detachment. The percentage of cells undergoing self-relaxation was quantified by determining the ratio of cell widths at the middle (Wmid) compared with the width at the end (Wend) (Fig. 4B). Based on these data, we concluded that more SG/ cells than C57 cells were sufficiently stressed to self-relax. Cells of a rectangular shape were studied further in their adhesion to determine whether adhesion of
SG/ cells was reduced or intracellular stresses were higher compared with normal cells.
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SG/cells and controls show similar adhesion Two parameters control the relaxation process: cellular prestress, which drives cell relaxation, and drag, which slows relaxation dynamics. C57 cells therefore either have less initial prestress than
SG/ cells, or more drag, or a combination of both. In order to further separate the effects of prestress from the effects of adhesive drag, especially relevant because
SG is a membrane-localized protein, cells were forcibly peeled from the substrate using the micropipette technique described in the Materials and Methods and depicted in Fig. 5A. This technique quantified the adhesion strength of cells, and isolated the adhesive effect from the prestress. Peeling, like relaxation, was conducted on 6-day-old cells.
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A typical example of the peeling velocity (Vpeel) versus imposed tension (Tpeel) for a single peeling run is plotted in Fig. 5B. The velocity of a peeling primary cell fluctuated during the course of the peel owing to strongly adherent points along the cell length. Such strongly adherent points were seen in previous studies and defined as physical focal adhesions (PFAs) (Griffin et al., 2004a) (Fig. 5B, squares). For both normal C57 and
SG/ cells, peak velocities, Vpeel_pk versus Tpeel were binned according to the tension and averaged (Fig. 5C), and the results were then fitted to the equation,
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As is clear from Fig. 5C, there was no significant difference between the peeling fits for the two cell types. The intercept To = e (b/a) represents the minimum tension required to detach a cell from the substrate. Recent studies of myotubes adhering to different substrates have demonstrated considerable differences in To and so the method appears sufficiently sensitive (Engler et al., 2004b). Here, however, for both normal C57 and
SG/ myotubes, this peeling tension is To =6 nN/µm. This result was obtained regardless of whether To was calculated by averaging the individual intercepts for the separate fits, or determined directly from fitting both sets of data at once.
ERK-1, MAPKAPK2 and MYPT1/2 hyperactivation in SG/ cells
Apoptosis seen here and in vivo (Hack et al., 1999) in
SG/ myocytes as well as the hypercontractility described above suggest possible changes in signaling pathways. Our initial phosphoscreens here are focused on activators, especially the MAP kinases ERK and p38-MAPK, which are midstream in signaling pathways. More than a dozen phosphoproteins in
SG/and normal TA muscle were quantified (Fig. 6 and Table 2). Although a screen of the cultured myotubes would also have been desirable, protein yields from the micropatterns were far too limited.
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At least four phosphoproteins appear hyperactivated in SG/ muscle relative to constitutive levels in normal muscle: (P)-ERK1, (P)-MAPKAPK2, (P)-MYPT1/2, and (P)-FAK. ERK1 showed the greatest hyperactivation (+126%), at more than twofold above normal (Table 2). As discussed below, hyperactivation of ERK in these non-proliferating, terminally differentiated cells appears consistent with apoptotic mechanisms.
(P)-hsp27 appeared weakly activated in SG/ muscle but not detectably phosphorylated in normal muscle (data not shown). Eight other proteins examined showed no significant difference between normal and
SG/ tissue. This included the focal adhesion protein paxillin and the most strongly reactive phospho-species detected, (P)-cofilin, which is involved in actin cytoskeleton reorganization in crawling cells. Table 2 indicates that at least six phosphoproteins showed decreased activation in
SG/ muscle: (P)-adducin-
, (P)-MAPKAP2 (at T334), (P)-p38MAPK, (P)-SMAD-1, (P)-adducin-
and (P)-AcCoA-Carb. Note that the adducins are also involved in actin cytoskeleton reorganization and showed highly significant changes relative to normal tissue whereas (P)-cofilin did not. Also, the midstream signaling molecules like p38 MAPK and MAPKAP2 showed significantly lower phosphorylation indicating phospho-site-specific functions. These differences between muscle samples, with both up- and downactivation, are discussed later.
Hyperphosphorylation in stretched TA muscles
Given the in vitro and in vivo stress/apoptosis demonstrations of SG/ tissue, we focused here more on the upstream or midstream effectors rather than on downstream markers of mechanotransduction. A select set of 18 selected phosphoproteins were compared for stretch activation in normal and
SG/ muscle. As shown in Fig. 6 and Table 3 hyperactivation of ERK1/2 was more than several-fold above basal levels in both normal and
SG/ stretched muscles. P38 MAPK and MAPKAPK2 activation exhibited the most striking changes in stretched muscles, indicating a p38 MAPK pathway in stretch-induced mechanotransduction. Importantly, the focal adhesion phosphoproteins paxillin and FAK did not show any significant change between stretched and unstretched tissue, however, and the activation of the regulatory factor Smad1 was only slightly higher in
SG/ stretched muscle. Smad1 is known to mediate extracellular signaling, transferring mechanical strains into transcriptional events (Scherer and Graff, 2000
).
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Apoptosis/survival phosphoproteins in muscle tissues of normal and SG/
Based on our in vitro studies of apoptosis, we also included upstream `apoptotic' proteins in the initial phosphoscreen. As shown, in Table 2, (P)-ERK, and (P)-FAK were activated and have been shown to be regulators of cell apoptosis/survival. FAK activation at two different tyrosine residues Y577 and Y397 proves to be similarly hyperactivated (+114 and +38%) giving values above the accepted limits of significance (>25%). PKC-, PKC-
the signaling molecules and CREB, a transcriptional regulatory protein, showed no significant change in 8-week
SG/ muscle tissue compared with controls. However, in older mice, more profound apoptotic events may lead to significant activation of these proteins (Jung et al., 2004
; Matassa et al., 2003
; Trevisan et al., 2004
).
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Discussion |
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Structural and functional differences suggest hypercontractility in SG/ cells
Immunofluorescence shows here that acto-myosin striations are almost twofold more frequent in SG/ myotubes than in normal myotubes (Fig. 2D). From this finding alone, these cells would be expected to be more contractile and stiffer than normal myocytes. Cells treated with contractile agonists become stiffer whereas cells in which the acto-myosin contractile apparatus is inhibited become less stiff (Hubmayr et al., 1996
; Lee et al., 1998
). Moreover, cell stiffness increases linearly with prestress (Wang et al., 2002
).
Immunofluorescence also reveals that acto-myosin striations form only in cells-on-cells, and not in cells growing directly on the glass substrate. However, in both C57 and SG/ cells stained for actin and myosin, a majority of the collagen-coated strips contained cells-on-cells and both upper and lower cells generally relaxed together. It is therefore safe to correlate the results of the immunofluorescent studies with the relaxing and peeling cells, noting that the overall cytoskeletal organization in
SG/ cells was greater than that in C57 cells. In other words, the highly organized cytoskeleton of the upper cells drives relaxation.
This increase in cytoskeletal structure further suggests that increased prestress causes SG/ cells to relax to a greater extent than C57 cells. This is supported by the forced peeling data, which showed no difference between the two cell types, leading to the conclusion that the adhesive drag is not changed in the knockout cells. The higher prestress is also evident in the increased frequency of `self-relaxation' with the
SG/ cells. Acto-myosin contractility thus appears strong enough to break adhesive attachments of the patterned myotubes to the surface in the absence of mechanical stimulation, as evident in the high incidence of `self-relaxation' in the
SG/ cells.
Signaling possibilities for SG
We have shown here that SG does not factor into muscle adhesion strength; hence,
SG and the SG complex must contribute to cell function and contractility in some other way. In addition to providing a structural link between the cytoskeleton and ECM, the DGC is increasingly understood to contribute to signaling pathways (Rando, 2001
). Filamin is one actin-binding protein that is widely implicated in signaling cascades that influence motility and mechanotransduction (Bellanger et al., 2000
; Kainulainen et al., 2002
; Leonardi et al., 2000
). This is suggestive, because although muscle-specific filamin-C binds
SG and has been reported to have a much higher level of membrane localization in
SG/ tissue (Fig. 7A) (Thompson et al., 2000
), overexpression of filamin-B in C2C12 cells was also recently reported to accelerate, by up to twofold, the fusion and differentiation into thin myotubes (van der Flier et al., 2002
). Filamins may thus be key to the increased myotube differentiation seen here in
SG/ cells. Along with the increased rate of apoptosis in
SG/ myotubes found both here and by others (Hack et al., 1998
), the results implicate
SG in moderating signals of differentiation and contractility that also influence viability.
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Entire studies are devoted to the complex signaling cascades in muscle, and the SG-complex may be just a small, if important, component of multiple pathways. Our initial screen for possible components of relevant signaling pathways is a useful starting point, with a number of hyper- and hypophosphorylated proteins detected in C57 and SG/ muscle tissue. Combined with published results from other groups, these data lead us to propose a potential signaling pathway (Fig. 7) that would result in increased apoptosis in
SG/ tissue. Thick lines indicate stretch-activated signals and dashed lines indicate likely signaling connections that have not yet been firmly documented.
First, although a signaling pathway to (P)-cJun has been connected to the DGC in rabbit skeletal muscle microsomes (Oak et al., 2003), no differences in (P)-cJun were detected here between normal C57 and
SG/ tissue preparations. Of the many phosphoproteins studied, the clearest link between hypercontractility and increased apoptosis in
SG/ tissue seems to be provided by the hyperactivation of ERK 1/2. In unstretched tissue, ERK1/2 was the most hyperactivated, with expression in
SG/ tissue 126% greater than that in normal tissue (Table 2). This is particularly interesting given the role of (P)-ERK in mechanotransduction, sarcomeric reorganization, and as a regulator of apoptosis (Hornberger et al., 2005
; Kumar et al., 2004
; Loth et al., 2003
; Ryder et al., 2000
; Zechner et al., 1997
). Moreover, Kumar and colleagues recently demonstrated with ex vivo muscle fibers that ERK1/2 is activated by externally imposed stretch (Kumar et al., 2002
), data confirmed by our phosphoscreens (Table 3). Importantly, ERK 1/2 phosphorylation increased by more than 800% in stretched
SG/ tissue compared with unstretched, but activity in stretched normal tissue increased by only 200%. ERK 1/2 activation has previously been linked to increased apoptosis (Cheung et al., 2004
; Subramaniam et al., 2004
), so the overstretched or hypercontractile character of adherent
SG/ cells in vitro (Figs 3, 4) may provide the extra stimulus towards apoptosis via a (P)-ERK 1/2 pathway (Fig. 7), which may translate to
SG/ tissue in vivo.
MAPKAPK2 is also hyperactivated, with 114% activation in SG/ muscle tissue compared with normal muscle (Table 2). MAPKAPK2 has been shown to stimulate muscle contractility via (P)-hsp27 (Ibitayo et al., 1999
), which also appears to be activated in
SG/ tissue but not in C57 tissue. Because (P)-MAPKAPK2 is a target for (P)-ERK and is itself stretch-activated (Ibitayo et al., 1999
; Krook et al., 2000
; Mizutani et al., 2004
; Ryder et al., 2000
), these proteins may be part of a hypercontractile signaling loop (Fig. 7) that couples to externally imposed (stretch) as well as internally generated mechanical stress (prestress). However, the function may depend on site-specific phosphorylation. Consistent with hypercontractility, the myosin phosphatase MYPT1/2 also appeared more phosphorylated in
SG/ tissue than in C57 tissue. It has recently been shown that phosphorylation of MYPT inhibits myosin light chain phosphatase activity, leading to increased myosin phosphorylation and higher force (Sward et al., 2000
). MYPT1/2 probably sits in a parallel signaling pathway coupled to intracellular calcium levels, which are altered in dystrophin-depleted murine tissue (Fong et al., 1990
).
Another link between hypercontractility and increased apoptosis in SG/ tissue is provided by increased activation in stretched
SG/ tissue of p38 MAPK and MAPKAP2 in addition to ERK. P38 MAPK is known to be stretch- and stress-activated (Azuma et al., 2001
; Martineau and Gardiner, 2001
; Mizutani et al., 2004
), and increased phosphorylation of p38 MAPK has been linked to increased apoptosis (Deschesnes et al., 2001
). Thus, although we found that p38 MAPK exhibits decreased activation in unstretched
SG/ tissue (Table 2), the 900% increase of p38 MAPK phosphorylation in stretched
SG/ tissue (compared with a 500% increase in stretched normal cells) (Table 3) reveals its sensitivity to mechanotransduction. It should be noted that while overall phosphoprotein levels after 20 minutes at
10% stretch happen to be similar to normal C57 tissue after similar length change and time, MAPK activation is known to be a quantitative reflection of the magnitude of mechanical stress applied to muscle (Martineau and Gardiner, 2001
), and so longer times and larger stretches are likely to be different, especially given the large changes here. More thorough investigations are certainly needed. In light of the sensitive response of p38 MAPK to stretching in both normal and
SG/ tissue, we suggest that the hypercontractility of the
SG/ cells in vitro may also trigger a p38 MAPK apoptotic signaling cascade (Fig. 7),
We have further investigated a possible cross-talk between p38 MAPK and MAPKAP2 and a role for heat shock protein 27 (hsp27) in mediating this interaction under externally imposed stress (stretch) in normal and SG/ muscle (Fig. 7). In parallel, these midstream mediators can interact with molecules of other signaling pathways. Here we suggest that ERK1/2 and FAK signal the survival/apoptotic pathway (Cheung and Slack, 2004
; Frisch et al., 1996
). (P)-ERK has been shown to phosphorylate FAK (Carragher et al., 2003
), and we found (P)-FAK/Y397 and Y577 are hyperactivated in
SG/ tissue. FAK is believed to associate with the DGC through the signaling protein Grb2 (Cavaldesi et al., 1999
). Both (P)-FAK and (P)-ERK have also been associated with myocyte apoptosis (Cheung and Slack, 2004
; Kurenova et al., 2004
; Lin et al., 2004
; Liu and Hofmann, 2004
; Subramaniam et al., 2004
). The balance between ERK and JNK/p38 MAPK is critical in signaling apoptosis or viability (Xia et al., 1995
). A recent study has revealed that ERK is a key apoptotic factor in potassium deprivation-induced neuronal cell death by showing that ERK inhibitors protect neurons from low potassium conditions, whereas constitutively activated ERK activates cell death. Most importantly, this study shows how ERK can promote neuronal cell death by causing plasma membrane and DNA damage that is independent of caspase-3 activity (Subramaniam et al., 2004
). Further studies on the mechanism of ERK in neuronal cell death may shed light on the possibility of using ERK as a therapeutic target in treating neurodegeneration.
Structural targets also showed differential phosphorylation: adducin was found to be less phosphorylated in SG/ muscle and is well known to associate with actin and thus influence cytoskeletal organization (Matsuoka et al., 2000
). Coupled to the hypercontractile state of
SG/ cells, a different cytoskeletal organization in these cells is consistent with our findings (Fig. 2). (P)-adducin-
has also been linked to apoptosis in epithelial cells (Imamdi et al., 2004
; van de Water et al., 2000
), and has been suggested as a monitor of ERK1/2 activity (Je et al., 2004
). Downregulation of activated adducin could thus play a part in the runaway activation of ERK1/2 in
SG/ tissue.
Beyond the scope of this initial phosphoscreen where we have primarily focused on the upstream and midstream mediators of apoptosis and myocyte mechanics, further studies would help clarify the signaling cascade that has gone awry in SG/ cells. Several, sensible candidates like p38 MAPK, MAPKAP2 and Smad1 for deeper examination of protein interactions have been identified in stretch-induced mechanotransduction. The phosphoscreen results corroborate our in vitro studies as well as the data of other groups on increased apoptosis in
SG/ cells. Activation of the MAPK pathways in
SG/ cells begins to establish a signaling link to apoptosis (Cheung and Slack, 2004
; Lesay et al., 2001
; Xia et al., 1995
). Given the lack of adhesive defect in these cells, as some of the adhesion proteins like paxillin remain unchanged, it is becoming increasingly clear that molecular signaling is critical in the progression of limb girdle muscular dystrophy (LGMD2C). Future studies might not only clarify the coupled signaling circuits but also eventually lead to pharmacological interventions.
In summary, we have shown that myotubes lacking SG have an acto-myosin cytoskeleton that is more organized than that of normal myotubes, at least when growing on top of other compliant cells. This organization increases the overall cellular prestress. Future studies involving contractile agonists and/or antagonists could serve to elucidate the contribution of the acto-myosin network to the prestress of skeletal myotubes. In addition, apoptosis is increased in
SG/ cells in vitro, corroborating previous tissue-level studies by another group (Hack et al., 1998
). We propose that
SG is part of a signaling cascade, which controls the rate of sarcomerogenesis and/or apoptosis. Specifically, activation of ERK, p38 MAPK and MAPKAP2 as well as FAK phosphoproteins indicates that distinct MAPK signaling pathways contribute to contractile stress and high occurrence of apoptosis in the muscular dystrophy phenotype expressed by mice and humans lacking the gene for
SG.
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Acknowledgments |
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