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© The Rockefeller University Press,
0021-9525/2000//1209 $5.00
The Journal of Cell Biology, Volume 150, Number 5,
, 2000 1209-1214
Report |
The Dystrophin Complex Forms a Mechanically Strong Link between the Sarcolemma and Costameric Actin
ervasti{at}physiology.wisc.edu
The absence of dystrophin complex leads to disorganization of the force-transmitting costameric cytoskeleton and disruption of sarcolemmal membrane integrity in skeletal muscle. However, it has not been determined whether the dystrophin complex can form a mechanically strong bond with any costameric protein. We performed confocal immunofluorescence analysis of isolated sarcolemma that were mechanically peeled from skeletal fibers of mouse hindlimb muscle. A population of
-actin filaments was stably associated with sarcolemma isolated from normal muscle and displayed a costameric pattern that precisely overlapped with dystrophin. However, costameric actin was absent from all sarcolemma isolated from dystrophin-deficient mdx mouse muscle even though it was localized to costameres in situ. Vinculin, 
-actinin, β-dystroglycan and utrophin were all retained on mdx sarcolemma, indicating that the loss of costameric actin was not due to generalized membrane instability. Our data demonstrate that the dystrophin complex forms a mechanically strong link between the sarcolemma and the costameric cytoskeleton through interaction with -actin filaments. Destabilization of costameric actin filaments may also be an important precursor to the costamere disarray observed in dystrophin-deficient muscle. Finally, these methods will be broadly useful in assessing the mechanical integrity of the membrane cytoskeleton in dystrophic animal models lacking other costameric proteins.
Key Words: dystrophin • actin • muscular dystrophy • membrane skeleton • costameres
© 2000 The Rockefeller University Press
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Introduction |
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 TopAbstract Introduction Materials and MethodsResults and DiscussionReferences |
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To address this question, we isolated inside-out sarcolemmal membranes by mechanically peeling the membranes from single myofibers teased from normal mouse hindlimb muscles. We used confocal immunofluorescence microscopy to visualize the cytoskeletal proteins retained on the sarcolemma without interference from sarcomeric proteins (Straub et al. 1992). In brief, we have obtained the first evidence demonstrating that the dystrophin complex is necessary for a mechanically strong physical linkage between the sarcolemmal membrane and -actin of the costameric cytoskeleton. Furthermore, our data point toward destabilization of -actin filaments as a possible intermediate between dystrophin deficiency and global disorganization of the costameric apparatus (Minetti et al. 1992, Minetti et al. 1994; Porter et al. 1992; Ehmer et al. 1997; Williams and Bloch 1999). Finally, our approach should be broadly applicable to assessing the contributions made by other costameric proteins toward the macromolecular organization and mechanical integrity of the membrane cytoskeleton in skeletal muscle.
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Materials and Methods |
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TopAbstractIntroductionMaterials and MethodsResults and DiscussionReferences |
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-actinin, -sarcomeric actin, β-actin, and vinculin were purchased from Sigma-Aldrich. The preparation and characterization of -actin polyclonal antibodies was previously described (Otey and Bulinski 1988). The β-dystroglycan monoclonal antibody was purchased from Vector Laboratories. FITC- and TRITC-conjugates of anti-rabbit IgG and anti-mouse IgG were purchased from Jackson ImmunoResearch Laboratories, Inc. Alexa488- and Alexa568-conjugates of phalloidin, anti-rabbit IgG and anti-mouse IgG were purchased from Molecular Probes.
Mechanical Isolation of Single Myofibers and Sarcolemma
Age matched, or littermate control, C57BL/10ScSn-DMDmdx/J, or C57BL/6J-Lama2dy mice were obtained from Jackson ImmunoResearch Laboratories. The vastus lateralis was dissected from tendon to tendon in ice-cold Ringers solution and transferred to a 0.5-ml drop of relaxing solution (100 mM BES, 15 mM creatine phosphate, 5 mM DTT, 4.74 mM ATP, 5.43 mM MgCl2, 7 mM EGTA, and 0.02 mM CaCl2 with the ionic strength adjusted to 180 mM with potassium proprionate, pH 7.0) surrounded by silicone oil. To isolate sarcolemma membranes, one end of a single myofiber was secured with a very fine forceps, the sarcolemma was hooked near the forceps with a stainless steel micro-needle (<100 µm diameter filed to a fine point) and rolled down and off the free end of the myofiber. Isolated sarcolemma and mechanically peeled or intact single myofibers were transferred with fine-tipped glass micropipets to a 0.02-ml drop of relaxing solution stationed on a gelatin-coated glass slide. Isolated sarcolemma and mechanically peeled myofibers were fixed for 5 min with 4% paraformaldehyde in PBS. To assess the location of -actin in situ, intact myofibers from the vastus lateralis were fixed and permeabilized for 5 min with 4% paraformaldehyde and 0.1% Triton X-100 in PBS.
Immunofluorescence Analysis
Isolated myofibers and sarcolemmal membranes were blocked for 30 min at room temperature with 5% goat serum in PBS and incubated with primary antibodies overnight at 4°C. The samples were washed with PBS, incubated with the appropriate fluorescently tagged secondary antibodies for 30 min at 37°C, rinsed, and sealed under coverslips in an anti-fade solution. Confocal microscopy was performed with a Bio-Rad MRC1000 scan head mounted transversely to an inverted Nikon Diaphot 200 microscope in the Keck Neural Imaging Lab at the University of Wisconsin. The krypton/argon mixed gas air–cooled laser was set to allow only the 488- and 568-nm excitation lines, while the green and red emission signals were directed to separate photomultiplier tubes. Images were collected during a sequential scan to reduce the possibility of fluorescence bleed-through. To further verify that bleed-through of the green signal was not contaminating the red signal, serial optical sections (z series) were collected in some experiments using both single channel and double channel modes. Digital images were cropped using Adobe Photoshop 5.0 and figure montages prepared with Adobe Illustrator 8.0.
Miscellanea
The dystrophin/utrophin-glycoprotein complexes were amplified for immunoblot analysis from control and mdx total skeletal muscle membranes (Ohlendieck and Campbell 1991) using digitonin extraction and WGA-Sepharose chromatography (Ervasti et al. 1990). Immunofluorescence analysis of frozen cryostat sections from control and mdx muscle was performed as previously described (Ervasti and Campbell 1991).
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Results and Discussion |
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TopAbstractIntroductionMaterials and MethodsResults and DiscussionReferences |
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-dystroglycan in the dystrophin-glycoprotein complex (Campbell 1995). In contrast to mdx muscle, the dystrophin-glycoprotein complex is normally expressed at the sarcolemma of dy/dy muscle (Ohlendieck and Campbell 1991) and shows little evidence of sarcolemmal membrane damage (Straub et al. 1997). Sarcolemma isolated from dy/dy muscle retained both dystrophin and actin in an overlapping pattern (Fig. 2, g–i) similar to the costameric distribution observed in non-dystrophic control sarcolemma (Fig. 2, a–c). These results suggest that in the absence of dystrophin, costameric actin is not stably associated with the sarcolemma membrane.
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-actinin (Fig. 4 e) were retained on sarcolemma isolated from mdx muscle. Recently, both residual β-dystroglycan and upregulated utrophin in mdx muscle were shown to exhibit a costameric staining pattern in situ (Williams and Bloch 1999). Consistent with this study, we observed that β-dystroglycan and utrophin were also retained on mdx sarcolemma and exhibited a costameric staining pattern (Fig. 3, b–d). Importantly, these data indicate that the loss of costameric actin was not due to generalized weakness of the sarcolemma membrane but is instead a specific consequence of dystrophin deficiency. Furthermore, our data suggest that utrophin either lacks the actin filament stabilizing activity of dystrophin (Amann et al. 1999), or that the amount of costameric utrophin in mdx muscle was not sufficient to retain costameric actin on mechanically isolated sarcolemma.
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-actin isoform was previously shown to colocalize with vinculin at costameres in chick skeletal muscle (Craig and Pardo 1983). However, the polyclonal antibody used in this study (Craig and Pardo 1983) did not significantly stain the sarcolemma of mouse diaphragm (Pardo et al. 1983b). Thus, it remained unclear which actin isoform(s) may populate costameres of mammalian muscle. Therefore, we stained normal sarcolemma with monoclonal antibodies specific for -sarcomeric actin, or β-actin, or a polyclonal antibody raised against a peptide corresponding to the unique amino-terminus of -actin (Otey and Bulinski 1988). Only the -isoform antibody yielded a bright, costameric pattern of staining while - and β-specific antibodies yielded only weak and diffuse background labeling (Fig. 4, a–c). As was found using monoclonal antibody C4 (Fig. 2), or phalloidin (Fig. 3), the -actin staining pattern evident on normal sarcolemma (Fig. 4c and Fig. d) was absent from dystrophin-deficient mdx sarcolemma (Fig. 4 e). These data indicate that costameric actin appears to be exclusively comprised of the -isoform.
It remained to be determined whether costameric actin was absent from mdx muscle before mechanical peeling, or was lost as a result of the peeling procedure. Therefore, we examined -actin staining in single fibers from control and mdx muscle that were fixed and permeabilized, but not mechanically peeled. Both control and mdx myofibers exhibited peripheral -actin staining patterns marked by regularly spaced transverse fluorescent bands of similar intensities (Fig. 4f and Fig. g). Finally, the -actin antibodies also labeled the periphery of Z-lines in mechanically peeled myofibers from both control and mdx muscle, however, the -actin signal appeared brighter on mdx myofibers compared with controls (not shown). Taken together, our results indicate that -actin is appropriately expressed and assembled into costameres in mdx muscle, but that its stable association with the sarcolemmal membrane is severely compromised.
Based on its structure, protein interactions, and membrane defects associated with its absence or abnormality in dystrophic muscle, the dystrophin complex has long been hypothesized to mechanically stabilize the sarcolemmal membrane against the stresses imposed during muscle contraction or stretch (Petrof et al. 1993; Campbell 1995). Whereas dystrophin is strongly anchored to the sarcolemmal membrane (Straub et al. 1992), no study has demonstrated a mechanically strong linkage between dystrophin and any component of the costameric cytoskeleton. Thus, ours are the first data demonstrating that the dystrophin complex is necessary for a mechanically strong physical linkage between the sarcolemmal membrane and costameric -actin. Furthermore, our data point toward destabilization of -actin filaments as a possible intermediate between dystrophin deficiency and global disorganization of the costameric apparatus (Porter et al. 1992; Minetti et al. 1992, Minetti et al. 1994; Ehmer et al. 1997; Williams and Bloch 1999). Complexes comprised of ankyrin/spectrin(Williams and Bloch 1999), vinculin/talin/-actinin (Williams and Bloch 1999) and intermediate filament/intermediate filament associated proteins (Milner et al. 1996; Andra et al. 1997; Dalpe et al. 1999) are also localized to costameres and are capable of binding actin (Fig. 5). Therefore, it is possible that multiple, distinct costameric protein complexes act synergistically to form a strong mechanical linkage between the sarcolemmal membrane and the force-generating sarcomeric apparatus. In support of this possibility, targeted inactivation of desmin (Milner et al. 1996), plectin (Andra et al. 1997), or BPAGn1/dystonin (Dalpe et al. 1999) also cause muscular dystrophy and sarcolemmal instability. Our methods should be valuable in further assessing the macromolecular organization and mechanical integrity of the membrane cytoskeleton in dystrophic animal models lacking other components of costameres.
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-syntrophin (Iwata et al. 1998). Analysis of sarcolemma from mdx mice transgenically expressing dystrophin constructs deleted in different domains (Chamberlain et al. 1997), or mice lacking -syntrophin (Kameya et al. 1999) will resolve which elements in the dystrophin complex are necessary for strong actin filament association with the sarcolemmal membrane. Finally, the methods used in this study will be valuable in assessing whether utrophin over-expression (Tinsley et al. 1998) can rescue the mechanically strong linkage between costameric actin and the sarcolemmal membrane observed in normal muscle.
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Acknowledgments |
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-actin. We are also grateful to Dr. Donata Oertel for providing access to her stereo dissecting microscope and Dr. Richard Moss for his expert advice and encouragement. This work was supported by grants from the National Institutes of Health to J.M. Ervasti (AR42423 and AR01985) and a Development Grant from the Muscular Dystrophy Association to I.N. Rybakova.
Submitted: 12 June 2000
Revised: 17 July 2000
Accepted: 17 July 2000
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