Extensive but Coordinated Reorganization of the Membrane Skeleton in Myofibers of Dystrophic (mdx) Mice

McRae W. Williams, and Robert J. Bloch

Department of Physiology, School of Medicine, University of Maryland, Baltimore, Maryland 21201

    Abstract
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Abstract
Introduction
Materials & Methods
Results
Discussion
References

We used immunofluorescence techniques and confocal imaging to study the organization of the membrane skeleton of skeletal muscle fibers of mdx mice, which lack dystrophin. beta -Spectrin is normally found at the sarcolemma in costameres, a rectilinear array of longitudinal strands and elements overlying Z and M lines. However, in the skeletal muscle of mdx mice, beta -spectrin tends to be absent from the sarcolemma over M lines and the longitudinal strands may be disrupted or missing. Other proteins of the membrane and associated cytoskeleton, including syntrophin, beta -dystroglycan, vinculin, and Na,K-ATPase are also concentrated in costameres, in control myofibers, and mdx muscle. They also distribute into the same altered sarcolemmal arrays that contain beta -spectrin. Utrophin, which is expressed in mdx muscle, also codistributes with beta -spectrin at the mutant sarcolemma. By contrast, the distribution of structural and intracellular membrane proteins, including alpha -actinin, the Ca-ATPase and dihydropyridine receptors, is not affected, even at sites close to the sarcolemma. Our results suggest that in myofibers of the mdx mouse, the membrane- associated cytoskeleton, but not the nearby myoplasm, undergoes widespread coordinated changes in organization. These changes may contribute to the fragility of the sarcolemma of dystrophic muscle.

Key words: sarcolemma;  membrane skeleton;  muscular dystrophy;  spectrin;  dystrophin
    Introduction
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

DYSTROPHIN is the protein that is missing or mutated in patients with Duchenne or Becker muscular dystrophy (for review see 22, 23) and in the mdx mouse (6, 80). The absence of dystrophin is believed to weaken the sarcolemma, which becomes more susceptible to damage during the contractile cycle (22, 52, 74). How dystrophin stabilizes the sarcolemma of healthy muscle fibers and how its loss destabilizes the sarcolemma of dystrophic fibers are still poorly understood, despite the extensive molecular characterization of dystrophin and its ligands.

Molecular cloning and sequencing of dystrophin place it in the spectrin superfamily of cytoskeletal proteins (1, 15, 17, 40, 43). Like other members of this superfamily, including alpha -actinin and beta -spectrin, dystrophin has an NH2-terminal domain that binds actin and a central rod domain composed of a series of triple helical repeats. Like alpha -actinin and alpha -spectrin, dystrophin has a sequence in its COOH- terminal region containing EF hands. The COOH-terminal domain of dystrophin also binds a complex of integral membrane glycoproteins that includes dystroglycan and the sarcoglycans (8, 35, 57, 85). Analysis of the severity of the myopathies caused by different mutations of dystrophin in humans and in transgenic mdx mice suggests that changes limited to the central rod domain and the actin-binding domain have relatively modest effects. However, changes that inhibit binding to the glycoprotein complex are associated with the severest forms of dystrophy (10, 24, 65, 84).

Some of these changes associated with binding to the glycoprotein complex are likely to be related to extracellular structures, as dystroglycan (also known as cranin) binds laminin with high affinity (26, 35, 70). Thus, the dystrophin-glycoprotein complex has the potential of linking actin in the sarcomeres of superficial myofibrils through dystrophin and the trans-sarcolemmal glycoprotein complex, to laminin in the basal lamina of the muscle fiber. This role of the dystrophin-glycoprotein complex is consistent with the observation that dystrophin is concentrated at the sarcolemma of skeletal muscle fibers in costameres, regions of the sarcolemma that overlie Z and M lines, as well as in longitudinally oriented strands (47, 49, 62, 73). Costameres are believed to be involved in linking the contractile apparatus to the basal lamina (60, 69, 75). Thus, they may serve to transmit the force of contraction to extracellular elements (75). Mutations that alter this linkage would be expected to alter the stresses on the sarcolemma that occur during contraction, perhaps resulting in tears in the membrane that lead to the formation of delta lesions (52). This force transmission model for the damage caused in muscular dystrophy is consistent with nearly all the current structural and genetic evidence with one notable exception: it does not account for the mild effects of mutations affecting dystrophin-actin binding.

As an alternative to this model for the physiological role of dystrophin, we are examining the possibility that the fragility of the sarcolemma in dystrophic myofibers is linked to changes in the organization of the membrane-associated cytoskeleton. Dystrophin is only one of several structural proteins that underlie and support the sarcolemma. We hypothesize that, in the absence of dystrophin, changes in the organization of these other structural proteins may leave the sarcolemma vulnerable to damage. This idea is based on earlier observations that beta -spectrin and vinculin colocalize with dystrophin in the costameres of skeletal muscle fibers (62). Furthermore, our earlier results suggested that, although beta -spectrin remained associated with the sarcolemma in human and mouse muscle fibers that lacked dystrophin, its distribution at the membrane was abnormal (62; see also 20, 50). Here we provide morphological evidence that the membrane skeletal proteins of dystrophic, mdx mice codistribute in abnormal sarcolemmal structures. These morphological changes leave extensive regions of the membrane with little apparent support from the membrane skeleton and may contribute to the fragility of the sarcolemma of dystrophic muscle.

    Materials and Methods
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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animals

All mice (Jackson Laboratories) used were male C57-black-10smsc-DMD-mdx mice and control littermates aged 6 mo.

Tissue for Immunofluorescence

Animals were anesthetized by intraperitoneal injection of a combination of ketamine (80 mg/kg) and xylazine (7 mg/kg). Fixed tissue was obtained by perfusing the anesthetized animal through the left ventricle with a solution of 2% paraformaldehyde in PBS (10 mM NaP, 145 mM NaCl, pH 7.2). Fast twitch muscles, including the tibialis anterior, extensor digitorum longus, and quadriceps muscles, were dissected; the quadriceps muscle was incubated for an additional 5 min in 2% paraformaldehyde in PBS. Tissue was blotted dry and placed on a cryostat chuck in O.C.T. mounting medium (4583 tissue tek; Skura Finetek USA, Inc.). The chuck was plunged into a slush of liquid nitrogen, generated under vacuum. 20-µm-thick sections were cut on a cryostat (model 2800, Frigocut, Reichart-Jung, Cambridge Instruments), collected on glass slides coated with 0.5% gelatin and 0.05% chromium potassium sulfate, and stored desiccated at -70°C.

For the preparation of unfixed longitudinal sections, tissue was obtained without perfusion, mounted, frozen, and cryosectioned as above. To prevent contraction, the frozen sections were collected on the surface of an ice-cold bath of PBS containing 10 mM EGTA, pH 7.4. Sections were rapidly lifted from the surface of the bath directly onto gelatin-coated slides. Unfixed longitudinal sections were cut fresh for each experiment and used immediately.

Antibodies

Mouse mAbs (Novocastra Laboratories) to the COOH terminus (amino acids 3669-3685) of human dystrophin (Dys2; ref. 54), to the COOH terminus of human beta -dystroglycan (5), and to a fusion protein containing the NH2-terminal region of utrophin (NCL-DRP-2; ref. 4) were used at dilutions of 1:5, 1:10, and 1:5, respectively. An mAb against all known syntrophin isoforms, 1351, was provided by Dr. S. Froehner (University of North Carolina, Chapel Hill, NC), and was used at 16 µg/ml. Mouse mAbs (Affinity Bioreagents) against the alpha  subunit of the dihydropyridine receptor (DHPR1; clone 1A), and the sarcoplasmic/endoplasmic reticulum Ca-ATPase from rabbit skeletal muscle (SERCA 1) were used at dilutions of 1:200 and 1:100, respectively. Mouse mAbs against alpha -actinin from rabbit skeletal muscle (EA-53) and vinculin from chicken gizzard (VIN-11-5; both from Sigma Immuno Chemicals) were used at dilutions of 1:200 and 1:50, respectively.

The rabbit polyclonal antibody, 9050, was prepared against purified human erythrocyte beta -spectrin. It was affinity-purified over a column of erythrocyte beta -spectrin and cross-adsorbed against beta -fodrin and alpha -fodrin, purified from bovine brain as previously described (63, 87). Antibodies to erythrocyte beta -spectrin were also generated in chickens. IgY was purified from egg yolk using the EggStract kit (Promega Corp.) and anti-beta -spectrin antibodies were affinity-purified as described (63). Specificity for beta -spectrin was demonstrated by immunoblotting (Ursitti, J.A., L. Martin, W.G. Resneck, T. Chaney, C. Zielke, B.E. Alger, and R.J. Bloch, manuscript submitted for publication). Both affinity-purified antibodies to beta -spectrin were used at 3 µg/ml. Polyclonal rabbit antibodies to a fusion protein containing residues 335-519 of the alpha 1 subunit of the Na,K-ATPase and to a fusion protein containing residues 338-519 of the alpha 2 subunit of the Na,K-ATPase (Upstate Biotechnologies) were used at 3 µg/ml.

Nonimmune mouse mAbs, MOPC21, were obtained from Sigma Chemical Co. Nonimmune chicken IgY was purified from preimmune controls collected from the same chickens and used to generate the anti- beta -spectrin antibodies. Normal rabbit serum was purchased from Jackson ImmunoResearch Laboratories.

Secondary antibodies included goat anti-rabbit and goat anti-mouse IgGs, and donkey anti-chicken IgY. All secondary antibodies (Jackson ImmunoResearch) as fluorescein or tetramethylrhodamine conjugates were species-specific with minimal cross-reactivity and were used at a dilution of 1:100.

The specificities of all these antibodies have been established by immunoblotting or immunoprecipitation, as reported by the suppliers or in the relevant publications.

Fluorescent Immunolabeling

Sections were incubated in PBS/BSA (PBS containing 1 mg/ml BSA and 10 mM NaN3) for 15 min to reduce nonspecific binding and placed in primary antibody in PBS/BSA for 2 h at room temperature, or overnight at 4°C. Samples were washed with PBS/BSA and incubated for 1 h with fluorescein- or tetramethylrhodamine-conjugated secondary antibodies diluted in PBS/BSA. After additional washing, samples were mounted in a solution containing nine parts glycerol, one part 1 M Tris-HCl, pH 8.0, supplemented with 1 mg/ml p-phenylenediamine to reduce photobleaching (37). Slides were observed with a Zeiss 410 confocal laser scanning microscope (Carl Zeiss, Inc.) equipped with a 63× NA 1.4 plan-apochromatic objective. The pinholes for both fluorescein and tetramethylrhodamine fluorescence were set to 18. Images were collected and stored with software provided by Zeiss.

To generate figures, images were arranged into montages, labeled, and given scale bars with Corel Draw 6 (Corel Corporation Ltd.). Inset pictures were prepared with MetaMorph (Universal Imaging) and magnified twofold with Corel Draw 6. No other processing was used on any of the images.

For the quantitations shown in Fig. 3, images were prepared by one of the authors and scored double blind by the other. Images were taken of all sarcolemmal regions in controls and mdx myofibers that did not show obvious tears, holes, or other processing artifacts. Sampling was otherwise random. Images of control and mdx sarcolemma were coded and mixed randomly. Each image was then evaluated for the pattern of beta -spectrin distribution that was most common over the region of the sarcolemma in clear focus. Images were sorted into one of four categories: clear costameric distribution, including regular labeling over Z and M lines and in longitudinal domains; label present at Z lines, but absent over M lines or in longitudinal domains; label present at Z lines but absent both over M lines and in longitudinal domains; and label absent at Z lines, M lines, and longitudinal domains, but present in polygonal arrays or other irregular structures. We obtained consistent results when other naive observers scored the same or a similar set of images.


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Fig. 3.   Quantitation of beta -spectrin patterns in mdx fibers. Images of samples processed, as in Fig. 2, were evaluated double blind for the dominant patterns of beta -spectrin distribution. Afterwards they were sorted into four categories: A, clear costameric distribution, including regular labeling over Z lines and M lines, and in longitudinal domains; B, labeling absent over M lines or in longitudinal domains; C, labeling absent both over M lines and in longitudinal domains; and D, labeling of polygonal arrays or other structures that do not demonstrate regular labeling over Z lines. 108 mdx fibers and 72 control fibers were examined. Closed bars: controls; open bars: mdx.


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Fig. 2.   Altered distribution of beta -spectrin at the sarcolemma of mdx muscle fibers. Samples were processed as in Fig. 1 and labeled with 9050 rabbit anti-beta -spectrin antibodies. Control fibers show a clear costameric distribution for beta -spectrin (A). Fibers from the mdx mouse show a range of distributions of beta -spectrin (B-L), from normal (B) to highly altered (J-L). In most mdx fibers, beta -spectrin was depleted or missing at the sarcolemma in longitudinal domains (C and D), overlying M lines (E and F), or both (G and H). In some regions, beta -spectrin could not be detected at the sarcolemma overlying some Z lines (I-L), which led to the formation of zig-zag patterns (I and J) or polygonal arrays (K and L). Bars, 5 µm. Inserts show the regions enclosed by white boxes at twofold magnification.


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Fig. 1.   Immunolabeling of beta -spectrin and dystrophin in wild-type and mdx muscle. Perfusion-fixed quadriceps muscles from wild-type (A-C, G-J) and mdx mice (D-F, K-N) were snap frozen, and cryosectioned (see Materials and Methods). The sections were double-labeled with affinity-purified rabbit antibodies (9050) to beta -spectrin (A and D) and with the mouse mAb, Dys2, to dystrophin (B and E). Typical costameric structures overlying a Z line (thick arrow), an M line (thin arrow), and in a longitudinal strand (double arrowheads) are indicated in A. Color composite images were created to show beta -spectrin in green, dystrophin in red, and areas containing both proteins in yellow (C and F). These images show extensive overlap of labeling for beta -spectrin and dystrophin in costameres of wild-type (C) but not mdx (F) muscle. Controls were double-labeled with 9050 (G and K) and MOPC21, a nonimmune mouse mAb (H and L), or with a mouse mAb to alpha -actinin (I and M) and normal rabbit serum (J and N). Control samples, imaged under conditions identical to those used in A-F, showed little nonspecific labeling or bleedthrough of fluorescence. This was also true for the mdx sample shown in D-F. Bars, 5 µm.

Materials

Unless otherwise stated, all materials were purchased from Sigma Chemical Co. and were the highest grade available.

    Results
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Abstract
Introduction
Materials & Methods
Results
Discussion
References

We used immunofluorescence labeling and confocal microscopy to examine the distribution of several membrane skeletal proteins in longitudinal sections through the sarcolemma of fast twitch muscle fibers from the dystrophic mdx mouse. The use of confocal optics allowed us to isolate the fluorescence signal arising from proteins located within ~1.2 µm of the sarcolemmal bilayer (83), thereby reducing any fluorescence signals, specific or nonspecific, associated with structures lying deeper in the myoplasm. Each of the sarcolemmal proteins we examined has been shown to be concentrated in costameres, together with dystrophin and beta -spectrin (12, 32, 47, 49, 59, 62, 73; Williams, M.W., and R.J. Bloch, manuscript in preparation). We limited our observations to fast twitch fibers because the rectilinear pattern generated by immunolabeling of membrane skeletal elements at the sarcolemma, overlying Z and M lines and in longitudinally oriented strands, is much more clearly defined than in slow twitch fibers (Williams, M.W., and R.J. Bloch, manuscript in preparation). In addition, fast twitch fibers are more susceptible to damage associated with dystrophinopathies (82).

beta -Spectrin in mdx Muscle

Longitudinal cryosections were prepared from the quadriceps muscle of control and mdx mice. Sections from control and mdx samples were placed on the same slides and were treated simultaneously during all stages of our experiments. We first labeled sections with 9050, an affinity-purified polyclonal antibody against beta -spectrin, and Dys2, an mAb against dystrophin. Primary antibodies were visualized with species-specific secondary antibodies coupled to either fluorescein or tetramethylrhodamine. In controls, beta -spectrin was found in costameres, areas overlying the Z lines and M lines, and in longitudinally oriented strands (Fig. 1 A, arrows and arrowheads indicate examples of each of these structures), as we reported previously (62; see also 12). In our samples, costameres overlying Z and M lines could be distinguished under fluorescence illumination by the fact that structures over Z lines were usually wider than those over M lines (62). Labeling of all these structures was specific, as it was not obtained in either wild-type (Fig. 1, G and H) or mdx tissue (Fig. 1, K and L) with nonimmune rabbit antibodies or with a secondary antibody that failed to bind rabbit IgG. Dystrophin, recognized by labeling with Dys2, was also enriched in costameres (Fig. 1 B), as previously reported (47, 49, 62, 73).

The distribution of beta -spectrin in the quadriceps of the mdx mouse differed significantly from that in control muscles. Although in some cases the beta -spectrin distribution was very similar to that seen in the control tissue (Fig. 2, normal rectilinear distribution) such examples were rare in mdx muscle (<3% of 108 fibers scored double blind). Many of the samples (~36%) failed to show labeling for beta -spectrin either over M lines (Fig. 2, E and F) or in longitudinally oriented strands (Fig. 2, C and D). Approximately the same proportion of mdx fibers (~42%) failed to show labeling of both these structures (Fig. 2, G and H), and so retained organized domains of beta -spectrin only over Z lines. This pattern of labeling is similar to that reported by Porter et al. (62), Minetti et al. (50), and Ehmer et al. (20). The mdx muscle fibers that could not be placed into any of the above categories showed different morphologies, including small irregular boxes, zig-zag patterns, or polygonal arrays (Fig. 2, I-L). Some regions of the sarcolemma of mdx muscle lacking visible beta -spectrin extended over several sarcomeres (Fig. 2 J, inset) or encompassed large areas (>50 µm2) of the sarcolemma between Z lines (Fig. 2 H). The fact that all of these patterns were associated with muscle fibers that lacked dystrophin was confirmed by double immunofluorescence studies with anti- beta -spectrin and Dys2 anti-dystrophin. The latter antibody did not label any structures at the sarcolemma of the dystrophic muscle fibers studied here (not shown).

In contrast to our results with mdx muscle fibers, we found that >75% of control myofibers had regular rectilinear distributions of beta -spectrin at the sarcolemma (Figs. 1 A and 2 A), with prominent elements in longitudinal strands and overlying Z and M lines. Most of the remaining control fibers were not labeled at the sarcolemma either over M lines or in longitudinal domains. Only one control fiber out of the 72 that we scored did not show labeling of the sarcolemma over M lines or longitudinal domains. We found no control fibers with irregular boxes, polygonal arrays, or zig-zag patterns as seen in mdx. Typically, the regions of the control sarcolemma that failed to label with antibodies to beta -spectrin extended over areas of only 1-2 µm2 (the area enclosed by adjacent Z and M lines and a pair of well-spaced longitudinal strands) in control muscle fibers. In very few cases (<1% of all fibers in controls and mdx), we found regions of the sarcolemma of muscle fibers that showed little or no organization of the sarcolemma. These may represent regions that were poorly preserved or damaged during processing.

The altered arrangement of proteins at the sarcolemma of dystrophic muscle fibers was not due to differences in fixation or labeling of these fibers. We routinely examined samples that were fixed by perfusion in situ before the muscle was dissected and cryosectioned, as well as samples that were unfixed and collected under conditions that prevented contraction following cryosectioning (see Materials and Methods). To examine their possible effects, we also varied the perfusion and fixation regimens. We found no significant differences among these samples, suggesting that our results were independent of the methods we used. Furthermore, control and mdx samples were matched for age and sex, so these factors did not contribute to the differences in sarcolemmal organization. Finally, most control and mdx samples were also collected, frozen, sectioned, and stained together. Therefore, this ruled out the possibility that differences in handling could account for the morphological changes we observed. These results suggest that the organization of beta -spectrin at the sarcolemma of mdx is altered from the control. The differences between the mdx and control samples, summarized in Fig. 3, are highly significant (P < 0.0001 by chi 2 analysis).

Other Membrane-Skeletal Proteins

Unfixed longitudinal cryosections of quadriceps muscle from control and mdx animals were labeled in double immunofluorescence protocols for beta -spectrin, with either 9050 or chicken anti-beta -spectrin antibodies, and with antibodies to other integral membrane or cytoskeletal proteins, including syntrophin, beta -dystroglycan, vinculin, utrophin, and the alpha 1 and alpha 2 subunits of the Na,K-ATPase. Structures labeled by primary antibodies were visualized with species-specific secondary antibodies coupled to either fluorescein or tetramethylrhodamine.

The alpha 1 and alpha 2 subunits of the Na,K-ATPase form a complex with ankyrin and beta -spectrin at the sarcolemma of skeletal muscle fibers (Williams, M.W., and R.J. Bloch, manuscript in preparation). This results in the codistribution of the two subunits of the Na,K-ATPase with beta -spectrin in costameres (for a typical control, see Fig. 4, A-C). Therefore, we expected both subunits to redistribute with beta -spectrin at the sarcolemma of mdx muscle. This prediction was confirmed by double immunofluorescence experiments (alpha 1: Fig. 4, D-F; alpha 2: Fig. 4, G-I). We observed extensive overlap in the distributions of these proteins with beta -spectrin (Fig. 4, C and F; in the color overlays, red represents the Na,K-ATPase, green represents beta -spectrin and yellow represents regions containing both proteins). The absence of labeling at regions overlying M lines, the disruption of longitudinally oriented strands and structures overlying Z lines, and the presence of irregular polygonal structures were evident in the patterns of labeling of the alpha 1 and alpha 2 subunits of the Na,K-ATPase, as they were for beta -spectrin.


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Fig. 4.   Altered distribution of the Na,K-ATPase at the sarcolemma of mdx muscle. Unfixed quadriceps muscles of wild-type (A-C, J-M) and mdx (D-I, N-Q) mice were snap frozen and sectioned on a cryostat. Experimental samples (A-I) were double-labeled with affinity-purified chicken antibodies to beta -spectrin (B, E, and H) and polyclonal rabbit antibodies to the alpha 1 (A and D) or alpha 2 (G) subunits of the Na,K-ATPase. In color composite images, the alpha 1 or alpha 2 subunits are represented in red, beta -spectrin in green, and sites containing both proteins in yellow. (A-C) beta -Spectrin and the alpha 1 subunit of the Na,K-ATPase colocalize in costameres in control muscle fibers. Similar results were obtained with the alpha 2 subunit of the Na,K-ATPase (not shown). (D-I) The distribution of the alpha 1 (D) and alpha 2 (G) subunits of the Na,K-ATPase at the sarcolemma is altered, but these subunits still colocalize with the beta -spectrin (yellow structures in F and I). (J-Q) Controls were double-labeled either with nonimmune chicken IgY (K and O) and rabbit antibodies to the alpha 1 subunit of the Na,K-ATPase (J and N), or with normal rabbit serum (L and P) and chicken anti-beta -spectrin (M and Q). No nonspecific labeling or bleedthrough of fluorescence was observed. Bars, 5 µm.

beta -Dystroglycan is the transmembrane glycoprotein of the dystrophin-associated glycoprotein complex that binds dystrophin (39, 77). Syntrophin is a peripheral membrane protein that binds to dystrophin at sites COOH-terminal to those recognized by beta -dystroglycan (2, 9). In control muscle fibers, both syntrophin and beta -dystroglycan are enriched in costameres (Williams, M.W., and R.J. Bloch, manuscript in preparation), as previously reported for dystrophin itself (see above). In mdx tissue, the amounts of beta -dystroglycan and syntrophin decrease significantly, but low levels of both proteins can still be found at the sarcolemma (7, 56, 58). We used mAbs against beta -dystroglycan or syntrophin together with 9050 anti-beta -spectrin to label longitudinal sections of mdx muscle. Both syntrophin and beta -dystroglycan were enriched in costameric structures at the sarcolemma that lacked longitudinal strands and elements overlying M lines, as well as in regions of the sarcolemma that were more severely altered (Fig. 5, A and D). Comparison of beta -spectrin with either beta -dystroglycan or syntrophin demonstrated extensive colocalization (Fig. 5, C and F). Thus, the reduced amounts of syntrophin and beta -dystroglycan at the sarcolemma of mdx muscle codistributed in the membrane skeleton together with beta -spectrin.


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Fig. 5.   Altered distribution of syntrophin, beta -dystroglycan, utrophin, and vinculin at the sarcolemma of mdx muscle. Perfusion-fixed quadriceps muscles from mdx mice were processed as in Fig. 2 and double-labeled with affinity-purified rabbit antibodies to beta -spectrin (9050: B, E, H, and K) and mouse mAb to syntrophin (A), beta -dystroglycan (D), vinculin (G), or utrophin (J). In composite pictures (C, F, I, and L), beta -spectrin is shown in green, the other protein in red, and regions containing both proteins in yellow. The distribution of each of these proteins is altered in mdx muscle, but each continues to colocalize with beta -spectrin (yellow structures in C, F, I, and L). Bars, 5 µm.

Vinculin is a protein involved in the attachment of actin filaments to the membrane at focal adhesions (28) that is also found in costameres in skeletal muscle fibers (59, 69), where it codistributes with beta -spectrin and dystrophin (62). We labeled mdx tissue with anti-vinculin mAbs and with 9050 anti-beta -spectrin. We found that the distribution of vinculin was also altered at the sarcolemma of the mdx mouse. Like the proteins studied above, vinculin was much less regularly organized in mdx muscle than in control muscle, with gaps appearing because of the loss of longitudinal domains or domains overlying Z or M lines. Vinculin continued to colocalize with beta -spectrin in these altered structures (Fig. 5, G-I). This result contradicts a recent report (51) stating that the organization of dystrophin, but not vinculin, was altered at the sarcolemma of muscle fibers from patients with Becker muscular dystrophy.

We also examined the distribution of utrophin expressed in mdx muscle (42, 46, 48, 86). Recent results with muscles that lack both dystrophin and utrophin (16, 30) support the idea that the expression of low levels of utrophin in mdx muscle may protect it from the severe damage seen in Duchenne patients (79). Labeling of mdx muscle by anti-utrophin antibodies was apparent over wide areas of the sarcolemma in the same kinds of altered arrays as described above. When we compared the distribution of utrophin to that of beta -spectrin by double label immunofluorescence, utrophin codistributed with beta -spectrin at the sarcolemma (Fig. 5, J-L).

Control experiments ensured that our observations were not due to cross-reaction of the species-specific secondary antibodies with inappropriate primary antibodies, or to bleedthrough of the fluorescent label from one channel into another (Fig. 1, G-L; Fig. 4, J-M). Antibodies to beta -spectrin generated in chickens and used to label mdx and wild-type muscle, together with appropriate controls, gave the same results. Thus, it is unlikely that the coincident labeling for beta -spectrin and the other membrane skeletal proteins at the sarcolemma of wild-type or mdx muscle fibers was artifactual. Therefore, our results suggest that several proteins that codistribute with beta -spectrin in costameres at the sarcolemma of healthy muscle also codistribute with beta -spectrin in the irregularly organized membrane skeleton of mdx myofibers.

Intracellular Proteins

The changes we observed in the organization of the sarcolemma might simply reflect extensive changes in the cytoarchitecture of dystrophic myofibers (52). To assess the effects of the mdx phenotype on the organization of intracellular structures lying near the dystrophic sarcolemma, we used antibodies to alpha -actinin and to two integral membrane proteins of intracellular membranes, coupled with confocal laser scanning microscopy. alpha -Actinin is the main component of the Z disc and may be involved in anchoring the connections between the costamere and the contractile apparatus near the Z line (for review see 71, 76). Double labeling with mouse mAbs to the sarcomeric form of alpha -actinin and rabbit antibodies against beta -spectrin (9050) showed alpha -actinin distributed normally at Z lines (Fig. 6 J), even at sites near the sarcolemma that showed highly disrupted patterns of labeling for beta -spectrin (Fig. 6 K). Thus alpha -actinin does not become disorganized in mdx muscle, even at Z lines that are in close proximity to areas of the dystrophic sarcolemma with abnormal membrane skeletal arrays.


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Fig. 6.   Unaltered distribution of intracellular proteins near the sarcolemma of mdx muscle. Samples of wild-type (A-C) and mdx (D-L) muscle were labeled with rabbit anti- beta -spectrin 9050 (B, E, H, and K) and mouse mAb to SERCA (A and D), DHPR (G), or alpha -actinin (J). In composite images, beta -spectrin is shown in green, the other proteins in red, and regions in the confocal plain that contain both proteins in yellow. (A-C) Near the sarcolemma of wild-type mouse skeletal muscle, SERCA is concentrated around Z lines, with additional elements around M lines and in longitudinally oriented domains. Labeling for SERCA in the sarcoplasmic reticulum around the M and Z lines appears to coincide with beta -spectrin in the nearby sarcolemma (yellow structures in C), because of the ~1.2-µm depth of the confocal plane sampled. Labeling in longitudinally oriented structures in the sarcoplasmic reticulum containing SERCA and similar structures at the sarcolemma containing beta -spectrin are apparently not coordinated (red and green structures in C). (D-F) The concentration of SERCA in the sarcoplasmic reticulum at the levels of the Z and M lines, and in longitudinally oriented structures, does not change in the vicinity of the mdx sarcolemma, which shows an altered distribution of beta -spectrin. (G-I) DHPR is normally concentrated in the t-tubules that surround each sarcomere at the A-I junction (see text). This also holds for t-tubules surrounding the A-I junctions of the myofibrils that lie near the mdx sarcolemma, despite the fact that the distribution of beta -spectrin at the sarcolemma is changed. (J-L) alpha -Actinin is normally concentrated in the Z disk (see text; Fig. 1); its distribution at Z disks of myofibrils in the vicinity of the mdx sarcolemma is not changed. Bars, 5 µm.

The Ca-ATPase of the sarcoplasmic reticulum (SERCA) and DHPR of the transverse tubules are also readily studied in double label immunofluorescence protocols. SERCA is normally distributed in tubular elements surrounding the Z line and M lines, as well as in elements aligned with the longitudinal axis of the myofibers (Fig. 6, A-C). DHPR is easily visualized in mammalian muscle as a double line at the junctions of the A and I bands, where the transverse tubules surround each sarcomere, including those near the sarcolemma (38; for review see 25). The distributions of both these membrane proteins showed no evidence of an altered organization in mdx fibers, even when they were examined in the same confocal plane as the dystrophic sarcolemma, visualized with 9050 anti-beta -spectrin (SERCA: Fig. 6, D-F; DHPR, Fig. 6, G-I). These results suggest that the changes in the organization of muscle fibers in adult mdx mice are limited to the sarcolemma and closely associated proteins. This is consistent with ultrastructural studies that reveal little change in the sarcoplasm of adult mdx muscle (13, 80).

    Discussion
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Abstract
Introduction
Materials & Methods
Results
Discussion
References

We used immunofluorescence labeling and confocal microscopy to examine the distribution of membrane skeletal proteins in healthy and dystrophic (mdx) mouse muscle. Our experiments were designed to test the hypothesis that the absence of dystrophin is accompanied by extensive changes in the organization of the sarcolemma. Our results strongly support this hypothesis by demonstrating widespread and potentially significant changes in the distribution of several peripheral and integral membrane proteins at the sarcolemma. Surprisingly, all the proteins we examined continued to codistribute at the altered sarcolemma despite the absence of dystrophin.

Earlier studies from this laboratory indicated the presence of beta -spectrin in transverse structures overlying the Z lines and M lines, and in longitudinal strands (62). We noted that the beta -spectrin pattern in muscle from mdx mice and from patients with Duchenne muscular dystrophy "always appeared less ordered than in controls" (62). Here we confirm and extend these earlier observations and show further that the extent of damage sustained by dystrophic myofibers can vary widely. This variability probably occurs because of differences in contractile activity and the load experienced in the period before sampling (41, 45, 68, 74), and previous cycles of degeneration and regeneration (14, 19, 53; for review see 22). Therefore, sampling a large number of myofibers may be necessary to reach any conclusions about the extent of spectrin-based membrane skeleton reorganization in dystrophic muscle.

Although much of our research has focused on beta -spectrin, many other membrane-associated proteins codistribute with beta -spectrin in irregular cytoskeletal arrays found at the dystrophic sarcolemma. These include all of the following: Na,K-ATPase, present in a complex with spectrin in skeletal muscle (Williams, M.W., and R.J. Bloch, manuscript in preparation); utrophin, the dystrophin homologue; two dystrophin-associated proteins, syntrophin and beta -dystroglycan (for review see 9, 55); and vinculin, a protein normally found at focal adhesions and other plasmalemmal sites associated with organized bundles of actin microfilaments (for review see 11). The fact that all of these proteins are enriched in costameres of dystrophic and healthy skeletal muscle suggests that their organization is coordinated (however, see 51).

The identity of the protein (or proteins) responsible for coordinating the distribution of proteins at the sarcolemma is still unclear. The most likely candidate is actin because it binds to dystrophin, beta -spectrin, and vinculin, but the evidence that actin is enriched at costameres is minimal (12). Furthermore, mutations in dystrophin that eliminate its actin-binding activity produce mild phenotypes (9, 10, 84; however, see 3). If the extent of disorganization of the membrane-associated cytoskeleton is related to the severity of dystrophinopathy (see below), then the mild effects of these mutations would argue against a primary role for actin in coordinating the organization of dystrophin and its associated proteins with other membrane skeletal elements at the sarcolemma.

In contrast, loss of dystrophin's binding site for dystroglycan results in the severest dystrophinopathies (9, 65). This suggests that dystroglycan or other ligands (e.g., gamma -sarcoglycan; ref. 31) interacting with the COOH-terminal region of dystrophin may be the primary organizers. For example, syntrophin binds to the voltage-gated sodium channel (27) that also associates with spectrin through ankyrin (72), suggesting that it may link the spectrin-based membrane skeleton to dystrophin in healthy muscle. However, as deletion of the syntrophin binding site in the COOH-terminal region of dystrophin (2) is not associated with myopathy in mice (65), syntrophin-dystrophin interactions are probably not required to maintain the integrity of the sarcolemma.

Utrophin, expressed in mdx muscle (42, 46, 48, 86), may partially substitute for dystrophin at the sarcolemma (79). Although it concentrates at the sarcolemma and binds to many of the same ligands as dystrophin, utrophin is unlikely to organize sarcolemmal spectrin and vinculin. Utrophin is present in mdx muscle at levels significantly lower than the levels of dystrophin in wild-type muscle, but levels of spectrin and vinculin are not appreciably reduced in mdx muscle (our unpublished observations). Thus, if utrophin does help to link the dystrophin-associated cytoskeleton to spectrin and vinculin at the sarcolemma, the stoichiometry of this linkage must differ significantly from that present in normal muscle. Furthermore, although utrophin, dystrophin, and spectrin have been shown to codistribute in a membrane skeletal network in cultures of rat myotubes, this network does not contain vinculin (18, 64; Bloch et al., manuscript in preparation). These results suggest that utrophin is unlikely to coordinate the organization of the various membrane skeletal proteins in mdx muscle fibers.

Although the proteins that organize the membrane skeleton in dystrophic muscle must still be identified, dystrophin clearly plays an important role in maintaining the organization of the membrane skeleton in normal muscle. In dystrophinopathies, several of the structural domains at the sarcolemma of wild-type muscle tend to disappear. However, the nature of the relationship between this reorganization of the membrane skeleton and the absence of dystrophin in mdx muscle fibers is still not clear.

The reorganization of the membrane skeleton in mdx myofibers may be an indirect result of the absence of dystrophin, perhaps related to changes in Ca2+ homeostasis (21, 33, 36, 44, 66, 78). Ca2+-dependent proteases, such as calpain and caspases, activated by Ca2+ entering the myofiber through the dystrophic sarcolemma, are capable of cleaving spectrins (34, 61, 67, 81) and other structural proteins (29). The proteolysis of spectrin, coupled with the absence of dystrophin, might disrupt the membrane-associated cytoskeleton sufficiently to destabilize sarcolemmal organization. This model predicts an increase in mdx muscle of proteolytic fragments of spectrin, perhaps associated with the altered costameric structures described here.

Alternatively, the changes in sarcolemmal organization may not be directly linked to the absence of dystrophin at all. For example, they may be related to the stage of muscle regeneration reached by each dystrophic myofiber at the time of sampling. The polygonal arrays seen in a small percentage of mdx fibers also appear in myofibers developing in vivo (our unpublished results). However, myofibers in the mdx mouse tend to undergo only a single cycle of degeneration and regeneration occurring 3-5 wk after birth. Afterwards, only a small number of muscle fibers degenerate at any given time (13, 14, 53). As our current studies were limited to 6-mo-old animals, it is unlikely that this alone can account for our observation that the membrane skeleton is significantly altered in >90% of mdx muscle fibers (Fig. 3).

Our results may also be interpreted in terms of models that invoke a direct role for dystrophin in organizing the membrane skeleton in healthy muscle fibers. For example, dystrophin in healthy muscle may stabilize the costameric sites at which membrane skeletal proteins accumulate. Therefore, the absence of dystrophin in mdx muscles may render their membrane skeleton more susceptible to distortion and disruption by the forces exerted on the sarcolemma during muscle contraction and relaxation. This suggests that the membrane domains most easily disrupted at the sarcolemma are the longitudinal strands and the structures lying over M lines. These are more readily lost in mdx muscle, whereas sarcolemmal structures located over Z lines are more stable. Our previous studies of fast twitch rat muscle fibers have shown that the domains over Z lines contain beta -spectrin complexed with alpha -fodrin, whereas the longitudinal strands and domains over M lines contain beta -spectrin with little alpha -fodrin or any other alpha  subunit of the spectrin superfamily that we have been able to identify (63). Such differences in the structure of membrane-bound spectrin may account for the greater instability of longitudinal and M line domains in mdx muscle.

Structural differences may also explain why normal contractions lead to damage and degeneration of dystrophic muscle fibers. The altered organization of costameres suggests that the connections between the sarcolemma and the sarcomeres of superficial myofibrils are not as periodic in mdx muscle as they are in controls. In healthy myofibers, these connections mediate the transmission of force from the contractile apparatus to the sarcolemma and the extracellular matrix, while keeping the sarcolemma in close register with the underlying myoplasm during the contractile cycle (75). The reduced number and the abnormal arrangement of such connections are likely to render the dystrophic sarcolemma more fragile than controls.

Disruption of the membrane skeleton of mdx also generates regions of the sarcolemma that are devoid of costameres. These regions can cover relatively large areas (>50 µm2; e.g., Fig. 2 H, regions of the sarcolemma between neighboring Z lines). In normal fast twitch muscle fibers of the rat, where longitudinal strands and structures overlying M lines are normally present, the regions between costameres usually do not exceed 2 µm2 in area, and even these small regions are likely to be stabilized by low levels of dystrophin (Williams, M.W., and R.J. Bloch, manuscript in preparation). This protein is, of course, absent in mdx muscle. The gaps in the membrane skeleton of dystrophic myofibers are considerably smaller than the "delta lesions" documented in samples of Duchenne muscle (52), and unlike delta lesions they appear to be limited to structures at or immediately adjacent to the sarcolemma. Nevertheless, areas lacking a membrane skeleton may be especially susceptible to damage; indeed, they may even be the sites at which lesions are initiated. The reorganization of the sarcolemma and the appearance of gaps in the membrane skeleton may therefore lead directly to the damage sustained by dystrophic muscle fibers. It follows that measuring the reduction in the number and size of these gaps may provide a sensitive and quantitative way to test therapies now being developed to treat Duchenne muscular dystrophy.

    Footnotes

Address correspondence to Robert J. Bloch, 660 W. Redwood St., Baltimore, MD 21201. Tel. and Fax: (410) 706-8341. E-mail: rbloch{at}umaryland.edu

Received for publication 23 November 1998 and in revised form 9 February 1999.

   This paper is dedicated to Guido Guidotti on his 65th birthday.
   Our research has been supported by grants to R.J. Bloch from the National Institutes of Health (NS 17282) and from the Muscular Dystrophy Association.

We are grateful to Ms. W.G. Resneck and A. O'Neill for their assistance at different stages of this research, to Dr. S.C. Froehner (University of North Carolina, Chapel Hill, NC) for his gift of antibodies to syntrophin and to DHPR, to Drs. N.C. Porter, J. Ursitti, D.W. Pumplin, W.R. Randall, M.P. Blaustein, and M.F. Schneider (University of Maryland School of Medicine, Baltimore, MD) for useful discussions, and to the reviewers for their constructive criticism.

    Abbreviations used in this paper

DHPR, dihydropyridine receptor; SERCA, Ca-ATPase of the sarcoplasmic reticulum.

    References
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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