©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
The Association of Cardiac Dystrophin with Myofibrils/Z-disc Regions in Cardiac Muscle Suggests a Novel Role in the Contractile Apparatus (*)

(Received for publication, November 20, 1995; and in revised form, February 23, 1996)

Heping Meng (1)(§) John J. Leddy (1)(¶) Joy Frank (2) Paul Holland (3) Balwant S. Tuana (1)(**)

From the  (1)Department of Pharmacology, University of Ottawa, Ottawa, Ontario K1H 8M5, Canada, the (2)Department of Medicine and Physiology, School of Medicine, University of California, Los Angeles, California 90024-1760, and (3)The Montreal Neurological Institute, McGill University, Montreal, Quebec H3A 2B4, Canada

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Dystrophin serves a variety of roles at the cell membrane through its associations, and defects in the dystrophin gene can give rise to muscular dystrophy and genetic cardiomyopathy. We investigated localization of cardiac dystrophin to determine potential intracellular sites of association. Subcellular fractionation revealed that while the majority of dystrophin was associated with the sarcolemma, about 35% of the 427-kDa form of dystrophin was present in the myofibrils. The dystrophin homolog utrophin was detectable only in the sarcolemmal membrane and was absent from the myofibrils as were other sarcolemmal glycoproteins such as adhalin and the sodium-calcium exchanger. Extraction of myofibrils with KCl and detergents could not solubilize dystrophin. Dystrophin could only be dissociated from the myofibrillar protein complex in 5 M urea followed by sucrose density gradient centrifugation where it co-fractionated with one of two distinctly sedimenting peaks of actin. Immunoelectron microscopy of intracellular regions of cardiac muscle revealed a selective labeling of Z-discs by dystrophin antibodies. In the genetically determined cardiomyopathic hamster, strain CHF 147, the time course of development of cardiac insufficiency correlated with an overall 75% loss of myofibrillar dystrophin. These findings collectively show that a significant pool of the 427-kDa form of cardiac dystrophin was specifically associated with the contractile apparatus at the Z-discs, and its loss correlated with progression to cardiac insufficiency in genetic cardiomyopathy. The loss of distinct cellular pools of dystrophin may contribute to the tissue-specific pathophysiology in muscular dystrophy.


INTRODUCTION

The dystrophin gene encodes a 427-kDa protein in muscle and brain tissues. Absence of this full-length form of dystrophin causes severe, progressive muscle weakness in patients with Duchenne's or Becker's muscular dystrophies(1, 2, 3) . These patients may also experience dilated cardiomyopathy, which in some cases may be much more severe than the myopathy(37, 38, 39) . The precise physiological role of dystrophin is not fully known although, due to its subsarcolemmal localization, it has been proposed to serve a variety of functions such as providing stability to the membrane and signal transduction(4, 9, 10, 14) . Dystrophin forms a tight association with a glycoprotein complex embedded in the plasma membrane(5, 6, 7) . One of these glycoproteins, alpha-dystroglycan, has been shown to bind to the G-domains of laminin (8) and agrin to mediate clustering of acetylcholine receptors(9, 10) . The association of a pool of subsarcolemmal dystrophin with laminin in the extracellular matrix via the membrane glycoproteins may be vital for linking the cytoskeleton to the extracellular matrix, and the disruption of this complex leads to increased membrane fragility(4, 9, 10) . Alterations in components of the dystrophin-glycoprotein-laminin complex, such as the laminin- alpha2 gene product, and a 50-kDa dystrophin-associated glycoprotein, adhalin, are associated with muscle membrane instability and muscular dystrophy(11, 12, 13) . A deficiency in adhalin and disruption of the membrane dystrophin-glycoprotein complex has also been reported in the cardiomyopathic hamster that experiences both hereditary cardiomyopathy and myopathy(14) .

In addition to its role in membrane stability and receptor clustering, recent studies imply that dystrophin serves a unique role in signal transduction by localizing nitric-oxide synthase to the sarcolemma (15) . In order to elucidate the cellular roles of dystrophin, it is paramount to precisely define its associations. Although it is well documented that dystrophin localizes at the plasma membrane in a variety of cells(16, 17, 18, 19) , studies indicate that there may be tissue- and cell-specific differences in dystrophin localization. For example, recent studies using confocal imaging (20, 21, 22, 23) and immunogold labeling (23) have shown that in addition to the sarcolemma, a substantial pool of dystrophin also localizes at the transverse tubules in cardiac muscle. Furthermore, cardiac dystrophin was found to be distributed in three distinct subcellular pools, a cytoplasmic pool, a membrane-bound pool not associated with WGA(^1)-binding glycoproteins, and a membrane-bound pool associated with WGA-binding glycoproteins(20, 22) . In view of the notion that dystrophin may serve diverse roles through its associations, here we demonstrate a selective pool of dystrophin molecules that associate with the myofibrils and localize to the Z-discs in cardiac muscle. Furthermore, the specific loss of myofibrillar dystrophin during progression to cardiac insufficiency in the cardiomyopathic hamster CHF 147 suggests that dystrophin may serve a unique role at the level of the sarcomere in addition to its recently described membrane functions. The distinct pools of dystrophin and their selective loss may be of significance in explaining the tissue-specific pathophysiological responses in muscular dystrophy(24) .


EXPERIMENTAL PROCEDURES

General Conditions

All muscle preparations were performed at 4 °C, and all buffers contained the following protease inhibitors, 1 mM benzamidine, 1 mM iodoacetamide, 1 µg/ml trypsin inhibitor, 2 µg/ml leupeptin, 1 µg/ml pepstatin A, and 0.2 mM phenylmethanesulfonyl fluoride.

Isolation of Myofibrils from Cardiac and Skeletal Muscle

Myofibrils were prepared as described(25) . Ventricular muscle of rabbit heart or fast-twitch skeletal muscle (4-5 g) from rabbits was homogenized in 20 volumes of buffer I (39 mM sodium borate, 25 mM KCl, 5 mM EGTA, and 1 mM dithiothreitol (DTT), pH 7.1) with the Brinkman polytron (PT-20) for 15 s, twice. The homogenate was centrifuged at 1,500 times g for 12 min and the pellet was re-extracted. The pellet was resuspended in 20 volumes of buffer II (39 mM sodium borate, 25 mM KCl, and 1 mM DTT, pH 7.1) and centrifuged at 1,500 times g for 12 min. This step was repeated and the pellet further extracted for 30 min with Triton X-100 buffer (39 mM sodium borate, 25 mM KCl, 1 mM DTT, and 1% Triton X-100, pH 7.1). The material was filtered and centrifuged at 1,500 times g for 12 min and the pellet re-extracted once more. The pellet was then washed twice with suspension buffer (10 mM Tris, 100 mM KCl, and 1 mM DTT, pH 7.1). The final pellet (myofibrils) was resuspended in low-salt buffer (10 mM Tris, 100 mM KCl, 1 mM DTT, and 20% glycerol, pH 7.1) at 2-3 mg/ml and stored at -78 °C for further analysis.

Purification of Sarcolemmal Membrane

Cardiac sarcolemmal membranes from rabbit hearts were prepared by differential and discontinuous sucrose density gradient as described previously(26) . The isolation of crude sarcolemmal membranes from rabbit skeletal muscle was as described by Seiler and Fleischer(27) .

Separation of Myofibrillar Proteins

Approximately 2.5 mg of isolated myofibrils were solubilized in 4 ml of urea buffer (0.5 M KCl, 50 mM Tris, 5 M urea, 1 mM EGTA, 10 mM ATP, 1 mM DTT, and protease inhibitors, pH 8.0) and centrifuged at 100,000 times g for 1 h at 4 °C. The supernatant was loaded on a 5-30% continuous sucrose density gradient and centrifuged at 200,000 times g for 24 h at 4 °C. The sucrose gradient fractions were collected and concentrated using Centricon-30 tubes (Amicon) and protein composition analyzed by 7.5% SDS-PAGE.

Cardiomyopathic Animals

Cardiomyopathic hamsters of the CHF 147 line (derived from the UM-X 7.1 line) were obtained from Canadian Hybrid Farms (Nova Scotia, Canada). Hearts from cardiomyopathic and normal hamsters at various ages (30, 60, 120, and 180 days) were obtained and the homogenate, membrane, and myofibrillar fractions isolated as described above.

Antibodies and Western Blotting

Polyclonal antibody against dystrophin was raised in rabbits by injecting synthesized antigenic peptide corresponding to the C-terminal amino acid sequence (SSRGRNTPGKPMREDTM) of the human dystrophin, conjugated to keyhole limpet hemocyanin as described(22) . Monoclonal antibody Mancho-7 against utrophin was a gift from Dr. Glen Morris and has been previously characterized(28, 29) . The monoclonal antibody against cardiac Na-Ca exchanger was a gift from Dr. K. D. Philipson, University of California Los Angeles. The monoclonal antibody against alpha-actinin and alkaline phosphatase conjugated anti-mouse IgG antibody were purchased from Sigma. The monoclonal antibody against desmin was a gift from Dr. D. Parry, University of Ottawa, and anti-adhalin was provided by Dr. S. Carbonetto, McGill University. Protein samples were separated by SDS-PAGE in the presence of dithiothreitol and transferred to nitrocellulose. The nitrocellulose was blocked with 5% Blotto in Tris-buffered saline and incubated with primary antibody for 1 h. The membranes were washed three times with Tris-buffered saline-Tween (0.05%) solution and incubated with alkaline phosphatase-conjugated second antibody for 1 h. Color was developed with the mixture of nitro blue tetrazolium and 5-bromo-4-chloro-3-indolyl phosphate. For WGA overlay nitrocellulose was blocked with 5% bovine serum albumin for 1 h and then incubated with horseradish peroxidase-conjugated WGA for 1 h. Color was developed with a mixture of 4-chloro-1-naphthol and hydrogen peroxide.

Immunolabeling at the Electron Microscopic Level

Adult rabbit hearts were rapidly excised and placed in oxygenated Tyrode's solution as described previously(23) . Fresh solution was added containing 2% formaldehyde, 0.01% glutaraldehyde for 20 min. Papillary muscles were removed, minced into small pieces, and fixed for an additional 40 min. Samples of papillary muscles were immersed in 2.3 M sucrose for 4 h and then rapidly frozen by immersion in liquid propane as described previously(30) . The sections (70-100 µm) were mounted on Formvar-coated grids, incubated with blocking solution, followed by incubation with antibody at room temperature. After washing, the sections were incubated in goat-anti-rabbit IgG-5m gold conjugate (Amersham Corp.). The sections were post-fixed in 2% glutaraldehyde in phosphate-buffered saline, rinsed, counterstained, coated with a thin layer of 1.5% methylcellulose, and allowed to air-dry. In order to quantitate the number of gold particles over the Z-disc versus gold distributed in other areas of the myofibrils, we examined 50 micrographs from 4 papillary muscles. In total, we examined 63 µm of Z-discs and 63 µm of A band region of the contractile proteins. All electron microscopic observations were with a JEOL 100CX.


RESULTS

Subcellular Fractionation Reveals Dystrophin Is Associated with the Myofibrillar Fraction

We raised antibodies to the C-terminal 17 amino acids of the skeletal dystrophin sequence. This sequence is exclusive to the 427-kDa form of dystrophin and is not present in any other protein including alpha-actinin(31) . The antibodies were affinity purified on the peptide and specifically recognized dystrophin from skeletal muscle, heart, and brain as we described previously(20, 22, 23) . We used the purified antibodies to investigate the localization of dystrophin.

Subcellular fractions from fresh rabbit hearts were isolated as described under ``Experimental Procedures.'' SDS-PAGE analysis of the protein composition of the different fractions obtained during myofibril isolation is shown in Fig. 1A. The cardiac homogenate (lane H) was centrifuged to obtain a supernatant fraction (lane S1) and a pellet fraction (lane P1). The pellet was washed extensively with buffer II to obtain supernatant (lane S2) and pellet (lane P2). Fraction P2 was further extracted with Triton X-100 to obtain supernatant (lane S3) and pellet (lane P3). The final product represented isolated myofibrils (MF). The MF fraction consisted predominantly of myosin (200 kDa) and actin (42 kDa). Other cytoskeletal proteins, such as alpha-actinin (105 kDa) and desmin (55 kDa) were also present in this fraction.


Figure 1: Presence of dystrophin in cardiac myofibrils. A, Coomassie Blue staining of SDS gels representing cardiac fractions obtained during isolation of myofibrils. Each lane was loaded with 60 µg of proteins, and the proteins were separated on a 6.25% SDS-polyacrylamide gel. H, homogenate; S1, supernatant fraction of the homogenate (buffer I wash); P1, pellet of the homogenate; S2, supernatant of the buffer II wash; P2, pellet of the buffer II wash; S3, supernatant of the Triton X-100 (buffer III) wash; P3, pellet of the Triton X-100 wash; MF, the isolated myofibrils washed with the suspension buffer. Standard protein markers (bands from the top to the bottom represent 211, 117, 81, 49, and 31 kDa, respectively). B, immunoblots of cardiac fractions obtained from A. Panel a, anti-alpha-actinin antibody (1:20,000) and anti-desmin ab (1:1,000); Panel b, anti-Na-Ca exchanger antibody (1:1000); Panel c, anti-dystrophin antibody (1:1000). The mobility of myosin (My), alpha-actinin (alpha-A), actin (Ac), desmin (Des), Na-Ca exchanger (Na-Ca) and dystrophin (Dys) is indicated.



The protein composition of the myofibril preparation was further examined by immunoblotting with various antibodies directed against known myofibrillar proteins and dystrophin. Gels with identical sample loading to that shown in Fig. 1A were electroblotted onto nitrocellulose and immunostained with the various antibodies (Fig. 1B). Anti-desmin and anti-alpha-actinin staining indicated that these proteins co-fractionated in a similar manner. The pellets of the washes and the isolated myofibrils stained strongly for desmin and alpha-actinin (Fig. 1B, panel a, lanes P1, P2, P3, and MF), whereas the supernatant fractions had no detectable desmin signal and stained only faintly for alpha-actinin (Fig. 1B, lanes S1, S2, and S3). Staining with anti-dystrophin antibodies was readily detectable in the cardiac homogenate, and it became stronger in the myofibrillar pellets obtained after extraction with buffer I and buffer II (Fig. 1B, panel c, lanes P1 and P2). In contrast to this, there was little dystrophin staining found in the corresponding supernatant fractions (Fig. 1B, lanes S1 and S2). Furthermore, the nonionic detergent, Triton X-100, failed to extract a significant amount of dystrophin from the pellet fraction (Fig. 1B, lane S3). After the Triton X-100 extractions the isolated myofibrils still contained a significant amount of dystrophin staining (Fig. 1B, lane MF).

To identify any cross-contamination of the myofibril fractions with the sarcolemmal membrane, we investigated the presence of the Na-Ca exchanger which is a transmembrane glycoprotein. Immunostaining with cardiac Na-Ca exchanger antibody revealed that some of this plasma membrane marker remained in the myofibril pellet during the first two washes of the isolation procedure (Fig. 1B, panel b, lanes P1 and P2). However, this residual membrane glycoprotein was completely removed from the pellet fraction by extraction with Triton X-100 (Fig. 1B, lanes S3 and P3). This immunostaining pattern for the various polypeptides was consistent in all 18 different myofibril preparations examined.

Proportion of Total Cardiac Dystrophin Associated with the Myofibrillar Fraction

To determine the relative amount of dystrophin present in the sarcolemmal membrane and myofibrillar fractions, the myofibril isolation protocols were modified to prepare both of these fractions from the same rabbit heart. A Coomassie Blue-stained SDS gel containing these fractions is shown in (Fig. 2A). The cardiac muscle was first used to purify a crude sarcolemmal fraction, which was then subjected to discontinuous sucrose density gradient centrifugation to obtain a purified sarcolemmal fraction. The pellet obtained from the cardiac homogenate (Fig. 2A, lane P1) was used to isolate myofibrils (lane MF), whereas the supernatant was used to prepare crude sarcolemmal membranes (lane C) which were then subjected to discontinuous sucrose gradient to purify the sarcolemma (lane SL). The myofibril fraction contained mainly myosin, alpha-actinin, and actin (Fig. 2A, lane MF) similar to the protein composition of the myofibrillar fraction shown in Fig. 1. The crude sarcolemmal fraction contained substantially less of these myofibrillar proteins (Fig. 2A, lane C), and they were further diminished in the purified sarcolemmal fraction as judged by protein staining (Fig. 2A, lane SL).


Figure 2: Presence of dystrophin in cardiac sarcolemmal and myofibrillar fractions. A, Coomassie Blue staining of the myofibrillar and sarcolemmal fractions obtained from the same rabbit heart. Each lane was loaded with 5 µg of proteins, and samples were separated on a 6.25% SDS-polyacrylamide gel. H, homogenate; S1, supernatant fraction of the homogenate (buffer I) wash; P1, pellet of the homogenate; MF, the isolated myofibrils; C, crude cardiac sarcolemma; SL, purified cardiac sarcolemma. Standard protein markers (bands from the top to the bottom represent 211, 117, 81, 49, and 31 kDa, respectively). B, immunoblots of cardiac myofibrillar and sarcolemmal fractions. Each lane was loaded with 60 µg of protein, and samples were separated on a 6.25% SDS-polyacrylamide gel and transferred to nitrocellulose for Western blotting. Panel a, anti-alpha-actinin antibody (1:5000); Panel b, anti-desmin antibody (1:1000); Panel c, anti-Na-Ca exchanger antibody (1:1,000); anti-dystrophin antibody (1:1000). Dys, dystrophin; NaCa, Na-Ca exchanger; Des, desmin; alpha-A, alpha-actinin; My, myosin. The data are typical of four independent experiments.



As observed with the previous fractionation procedure, desmin and alpha-actinin staining was intense in the myofibrillar fraction (Fig. 2B, lane MF) when compared with the homogenate or sarcolemmal fractions. Immunostaining for the Na-Ca exchanger revealed a 120-kDa band in the crude sarcolemmal fraction (Fig. 2B, lane C) that was significantly stronger in the purified sarcolemmal fraction (Fig. 2B, lane SL). A 70-kDa band also present with the 120-kDa band in the SL fraction was most likely a degradation product of the Na-Ca exchanger(32) . Na-Ca exchanger staining was undetectable in the myofibrillar fraction (Fig. 2B, lane MF). These findings indicate that the modified protocol worked well and gave a clear separation of the sarcolemmal and myofibrillar fractions.

Immunoblotting of the various fractions obtained using the modified protocols revealed the presence of the 427-kDa form of dystrophin in the purified sarcolemma (Fig. 2B, lane SL) and in the myofibrillar fraction (Fig. 2B, lane MF). Although the intensity of dystrophin staining was slightly lower in the myofibrillar fraction than in the purified sarcolemma, we reasoned that quantitatively it may represent a substantial fraction of the total dystrophin content of cardiac muscle. Western blots of the fractions shown in Fig. 2B were therefore digitally scanned to quantitate the signal intensity of the immunostaining per lane, and this was normalized to the microgram of protein loaded per lane. These values were then multiplied by the total amount of protein present in each fraction to determine the relative amount of dystrophin, Na-Ca exchanger, desmin, and alpha-actinin present in the homogenate and the various fractions prepared from it. The percent of dystrophin present in the membrane and myofibrillar fractions was compared with the various markers. The results show that approximately 35% ± 5 of the total dystrophin present in the homogenate was recovered in association with the myofibrillar fraction, whereas the recovery of desmin and alpha-actinin in this fraction was calculated to be 88% ± 17 and 80% ± 18, respectively (n = 4). The total amount of homogenate dystrophin that was recovered in the sarcolemmal fraction was approximately 55%, compared with a 90% recovery of the Na -Ca exchanger.

Dystrophin is known to localize at the sarcolemma in association with membrane glycoproteins. We examined the glycoprotein composition of the MF and SL fractions in a WGA overlay reaction (Fig. 3a). WGA staining of glycoproteins of various molecular mass was detected in the homogenate (lane H) and crude membranes (lane C), and this intensified in the purified sarcolemmal membranes (lane SL). There was weak WGA staining detected in the pellet (lane P1) of the homogenate of glycoproteins of 160, 220, and 300 kDa, and these were seen to enrich in the myofibrils (lane MF) purified from this pellet. These glycoproteins did not appear in the soluble fraction (lane S) or the crude (lane C) and purified membranes (lane SL). Immunoblotting with an antibody against adhalin, a 50-kDa dystrophin-associated sarcolemmal glycoprotein (Fig. 3b), revealed that while this glycoprotein was detectable in the homogenate (lane H) and enriched in the sarcolemmal membrane (lane SL), it was absent from the myofibrils (lane MF).


Figure 3: Distribution of glycoproteins in cardiac fractions. Panel a, WGA overlay and panel b, Western blotting with adhalin (Ad) antibodies of cardiac myofibrils (MF), sarcolemma (SL), crude membranes (C), and supernatant (S1) and pellet (P1) isolated from the same heart homogenate (H). Arrowheads indicate glycoproteins of 160, 220, and 300 kDa enriched in MF. The data are typical of two independent experiments.



Dystrophin Is Tightly Associated with the Myofibrillar Fraction

To determine how tightly dystrophin was associated with proteins of the myofibrillar fraction, we examined the conditions required to dissociate dystrophin from other components of this fraction. We first examined the effect of high-salt extraction. The isolated myofibrils were extracted with 0.7 M KCl for 60 min at 4 °C, and the soluble proteins were separated from the insoluble material by centrifugation. The KCl wash solubilized approximately 30% of the myofibrillar proteins, and the protein composition of the soluble versus the insoluble fractions was examined in SDS gels and Western blots (Fig. 4). The polypeptide patterns of the myofibrils, supernatant, and pellet were quite similar as seen by Coomassie Blue staining (Fig. 4a, lanes MF, S, and P). However, immunoblotting with dystrophin antibodies detected the polypeptide only in the myofibrils and the insoluble pellet and not the soluble material (Fig. 4b). Similar results were seen when detergents, such as Triton X-100, Nonidet P-40, deoxycholate, and digitonin, were used to extract the myofibrils together with KCl (data not shown).


Figure 4: Effect of salt extraction on myofibrillar dystrophin. Protein patterns (panel a) and immunoblots (panel b) of the fractions obtained from the isolation of myofibrils with or without a KCl wash. Isolated myofibrils (MF) without KCl extraction; supernatant (S) and pellet (P) obtained after KCl extraction of MF. Dys, dystrophin. Dystrophin antibody was applied at a dilution of 1:500. The data are typical of three independent experiments. My, myosin; alpha-A, alpha-actinin; Ac, actin.



The dissociation of dystrophin from myofibrils was further examined by solubilizing the myofibrillar fraction in 5 M urea, followed by separating the proteins in a 5-30% continuous sucrose density gradient. Protein assay indicated that more than 85% of total myofibrillar protein remained soluble in the urea buffer after centrifugation at 100,000 times g for 1 h. Western blot analysis confirmed that the dystrophin was in the soluble fraction (data not shown). The protein patterns of the various fractions obtained from the sucrose gradient fractionation are shown in Fig. 5a. Myosin, alpha-actinin, and actin were the major components in the sucrose gradient fractions. A single myosin peak was clearly separated from a single alpha-actinin peak. Actin appeared in two distinct peaks in the gradient. The first actin peak (Fig. 5a, Fractions 14-19) was located near the top of the sucrose gradient. This represented most of the actin present in the myofibrillar fraction. A second smaller peak was localized near the bottom of the sucrose gradient (Fig. 5a, Fractions 6-8). This peak did not precisely correspond to the myosin peak, although it substantially overlapped it. The lower actin peak did, however, precisely correspond to a single dystrophin peak in the gradient (Fig. 5, a and b, Fractions 6-8).


Figure 5: Sedimentation of myofibrillar dystrophin in a sucrose density gradient. Isolated myofibrils were solubilized in urea and separated in a 5-30% sucrose density gradient. Numbers at the bottom of the figure indicate the fractions collected from the bottom (lane 1) to the top (lane 23) of the sucrose gradient. Coomassie Blue staining (a) and immunoblotting (b) of proteins in the various fractions was examined. Dystrophin antibody was applied at a dilution of 1:500. My, myosin; alpha-A, alpha-actinin; Ac, actin; Dys, dystrophin. The data are a typical of four independent experiments.



Comparison with Skeletal Muscle

To determine whether some cofractionation of dystrophin with the myofibrillar fraction may also occur in skeletal muscle, various subcellular fractions were prepared from rabbit fast twitch skeletal muscle. The protein patterns of the skeletal muscle fractions are shown in Fig. 6a. Skeletal myofibrils (lane MF(s)) contained mostly myosin, alpha-actinin, and actin, similar to cardiac myofibrils (lane MF(c)). In the skeletal muscle sarcolemma (SL(s)) and cardiac sarcolemma (SL(c)) there was much less myosin, actin, and alpha-actinin compared with the myofibrils. Immunoblotting with anti-dystrophin antibodies indicated dystrophin staining was significantly enriched in skeletal muscle sarcolemma, but in contrast to cardiac myofibrils (Fig. 6b, lane MF(c)) no dystrophin was detected in the myofibrils from skeletal muscle (Fig. 6b, lane MF(s)). Dystrophin staining was evident in the homogenates from both types of muscle (lanes H(c) and H(s)).


Figure 6: Dystrophin in skeletal and cardiac muscle. Coomassie Blue staining of SDS gels (a) and immunoblotting (b) of cardiac (c) and skeletal (s) muscle homogenate (H), myofibrils (MF), and sarcolemma (SL). Dystrophin antibody was applied at a dilution of 1:500. Dys, dystrophin; My, myosin; alpha-A, alpha-actinin; Ac, actin. The data are typical of three independent experiments.



Utrophin Is Present Exclusively in the Sarcolemmal Fraction of Cardiac Muscle

The distribution of the dystrophin homolog utrophin in cardiac fractions was compared with that of dystrophin. Western blot analyses with utrophin antibodies revealed that utrophin staining was present exclusively in the purified sarcolemmal fraction (Fig. 7, lane SL) and was notably absent from the cardiac myofibril fraction (Fig. 7, lane MF), whereas dystrophin staining was readily detectable in the myofibrils, sarcolemma, homogenate (H), and crude membranes (C). It should be noted that overdevelopment of the reaction resulted in minor labeling of utrophin in the homogenate and crude membranes, but no utrophin was detected in myofibrils.


Figure 7: Distribution of utrophin and dystrophin in the heart. All fractions were from the same rabbit heart. Each lane was loaded with 60 µg of proteins, and samples were separated on a 6.25% SDS-polyacrylamide gel. H, homogenate; S3, supernatant fraction of the Triton X-100 wash; MF, isolated myofibrils; C, crude cardiac sarcolemma; SL, purified cardiac sarcolemma. Dystrophin (Dys) antibody was applied at a dilution of 1:500. Monoclonal antibody against utrophin (Utr) was applied at a dilution of 1:500. The data are typical of three independent experiments.



Immunogold Labeling Shows Dystrophin Localizes to Z-discs

To determine whether dystrophin was localized preferentially to one region within myofibrils, we examined the localization of dystrophin in intracellular regions of cardiac muscle using immunogold-labeled antibodies directed against dystrophin. Fig. 8is a typical electron micrograph that illustrates the distribution of gold over the contractile proteins. Immunogold labeling was clearly more abundant over the Z-disc than in any other region of the myofibrils. In 50 micrographs (4 hearts, 4 sections per heart for a total of 63 µm counted), we found a total of 373 gold particles over the Z-discs and 104 particles over other areas of the contractile proteins. We have previously documented the localization of dystrophin at the sarcolemma and transverse tubules using electron microscopy(23) .


Figure 8: Localization of dystrophin at the sarcomere monitored with immunogold 5-µm labeling on ultrathin cryosections. A typical of 50 micrographs generated from four different hearts is shown. Gold label (black dots) is seen along the Z line with some labeling present at the sarcolemma. 58,750 times.



Myofibrillar Dystrophin and Cardiac Derangement in Genetic Cardiomyopathy

In order to determine a potential role for myofibrillar dystrophin in cardiac derangement, we examined the expression of dystrophin in the genetically determined cardiomyopathic hamster which experiences severe cardiac insufficiency. The time-dependent developments in cardiac derangements in the CHF 147 line (descendents of the UM-X7 line) of cardiomyopathic hamsters has been well documented(33, 34, 35, 36) . The CHF 147 strain of hamsters is particularly relevant here because these animals experience dilated cardiomyopathy as well as muscular dystrophy symptoms similar to that seen in some human cases of muscular dystrophy(37, 38, 39) . This strain of hamsters exhibits the following chronology of events in the myocardium, cardiac myolysis at 60 days followed by cardiac dilation at 80-120 days and cardiac insufficiency at 150 days and in older animals. Previous studies have documented a number of ultrastructural alterations at the cardiac insufficiency stage including disorganization of the myofibrillar arrangement where the Z-discs were noted to be irregular(33, 34, 35) . We examined the expression of dystrophin which may account for some of these changes in the cardiomyopathic hamster heart. Western blot analysis (Fig. 9) shows that at day 180 there was a marked decrease in the dystrophin staining in the homogenate (lane H) from cardiomyopathic hamsters (M) compared with their age-matched control (C). The membranes (lane S) isolated from the homogenates of these animals also indicated a difference in dystrophin staining between the myopathic and normal animals, although the decrease in staining intensity was not as marked as that noted in the homogenates. Dystrophin staining in the myofibrillar fraction (MF) indicated that there was a marked decrease in the myofibrillar dystrophin in the cardiomyopathic hamster heart. Quantification of the data using densitometry indicated that the total dystrophin content in the cardiomyopathic hamster heart was reduced by 63% (average n = 2) which was reflected as a drop in membrane dystrophin of 28% (average n = 2) while myofibrillar dystrophin decreased by 75% (average n = 2). We further examined the time course of dystrophin loss from the myofibrillar fraction as these animals develop cardiac insufficiency. Fig. 10A shows dystrophin staining in myofibrils isolated from cardiomyopathic hamsters (M) and age-matched controls (C) at day 30, 60, 120, and 180. The data were quantified (Fig. 10B), and it can be seen that at day 30 the dystrophin content in the myofibrils from cardiomyopathic and normal hearts was similar, and thereafter there was a progressive time-dependent decrease in dystrophin with a 75% ± 7 (n = 3) drop at day 180. The expression of desmin was noted to be similar in the two groups of animals (Fig. 10B). The time course of myofibrillar dystrophin loss closely paralleled the decrease in contractile function reported for the CHF 147 hamster heart muscle (36) while the time-dependent accumulation of myofibrillar dystrophin in the normal hamster (Fig. 10) correlated with the age-dependent increase in contractile performance documented previously(36) .


Figure 9: Immunoblot analysis of dystrophin expression in normal and cardiomyopathic hamster heart. Subcellular fractions were isolated from cardiomyopathic CHF 147 strain (M) and normal hamster hearts (C) and separated in SDS-PAGE and analyzed in Western blots with affinity purified dystrophin antibodies. Lane S, sarcolemma; lane H, heart homogenate; lanes MF, myofibrils. Identical amounts of protein (40 µg) per lane were loaded between the myopathic and control groups. The results shown are typical of two to three independent experiments from groups of animals at day 180.




Figure 10: Evidence for myofibrillar dystrophin loss in the development of cardiomyopathy. A, myofibrils were prepared from hearts of cardiomyopathic hamsters (M) and normal control (C) hearts at ages 30, 60, 120, and 180 days and analyzed in Western blots with affinity purified dystrophin antibodies. B, Western blots were quantified by densitometry, and dystrophin content was plotted as a function of age in the normal (C dys) and cardiomyopathic (M dys) hamster. The desmin content in normal (C des) and cardiomyopathic (M des) hamsters on the same blot was also quantified by Western blotting and densitometry at the various ages shown. The results are typical of two to three independent experiments performed on two to three different groups of animals.




DISCUSSION

The present results demonstrate that a distinct pool of dystrophin molecules associated with the myofibrillar fraction and localized to the Z-discs in cardiac muscle. Whereas a majority of the dystrophin is localized at the surface membrane in association with glycoproteins, our results show that dystrophin at the Z-discs exists in the absence of any of these glycoproteins. Myofibrillar localization of dystrophin was exclusive to cardiac muscle, and its loss correlated with the development of cardiac insufficiency in the genetically determined cardiomyopathic hamster.

Dystrophin was tightly associated with the cardiac myofibrillar fraction that was enriched in cytoskeletal proteins such as alpha-actinin and desmin. While dystrophin associated with the sarcolemmal membrane was soluble in detergents such as digitonin, Nonidet P-40, Triton X-100, and deoxycholate as previously reported(22, 40, 41, 42) , these treatments failed to extract dystrophin from cardiac myofibrils. High concentrations of KCl solubilized approximately 30% of the protein content of isolated cardiac myofibrils, but dystrophin was not present in the soluble fraction. Dissociation of dystrophin from other proteins in the myofibrillar fraction could only be achieved by solubilization of myofibrils in buffer containing 5 M urea followed by separation of dissolved proteins on a sucrose density gradient. On the sucrose gradient, the peak of myofibrillar dystrophin followed a pattern different from the myosin and alpha-actinin peaks, but it coincided with one of two distinct actin peaks, suggesting that myofibrillar dystrophin may be associated with actin. Dystrophin is known to bind actin via its N-terminal domain(43, 44, 45) . Various isoforms of actin are expressed by mature striated muscle. In addition to muscle-specific actin present in the thin filaments, actin is also present in the Z-disc and in the cytoskeletal scaffold surrounding myofibrillar bundles(46) . Further work is therefore required to determine the significance of the existence of two distinct pools of actin in the myofibrillar fraction and the selective association of dystrophin with one of these pools. Given our present observation of immunogold labeling of Z-discs with dystrophin antibody in cardiac muscle, the pool of actin cofractionating with dystrophin on the sucrose gradient may represent Z-disc actin.

The tight association of cardiac dystrophin with the myofibrillar fraction suggests that dystrophin may play a unique role in the structure or function of the cardiac myofibril and that this pool of dystrophin may associate with proteins that are distinct from those of the sarcolemmal membrane dystroglycan complex. Accordingly, we found that adhalin, the 50-kDa dystrophin-associated glycoprotein, was present only in the sarcolemmal and not the myofibrillar fractions. The pool of myofibrillar dystrophin cannot therefore be associated with any of the glycoproteins found in the dystroglycan complex as is the case for a sarcolemmal pool of dystrophin. The model for the structure of the dystrophin-containing membrane cytoskeletal complex suggests that dystrophin is anchored in this complex via actin at its N-terminal domain and to one or more components of the membrane glycoprotein complex via its C-terminal domain. It will therefore be of interest to determine whether actin alone anchors dystrophin so tightly to the cardiac myofibrils or whether an additional dystrophin-binding protein is present in the Z-discs. In this regard dystrophin has been shown to localize nitric-oxide synthase to the sarcolemmal membrane and proposed to serve a role in nitric oxide signaling(15) . Whether dystrophin at the Z-disc can anchor such signaling molecules at the sarcomere is now under investigation. The origin and the nature of glycoproteins of 160, 220, and 300 kDa in the myofibrillar fraction are intriguing. These glycoproteins could not be extracted with detergents and high salt. Whether dystrophin can associate with any of these glycoproteins to anchor them at the Z-disc remains to be investigated. The dystrophin-related protein, utrophin, was exclusively distributed in the sarcolemmal membrane fraction of cardiac muscle and was absent from the myofibrillar fraction. This is consistent with the immunohistochemical localization of utrophin in heart sarcolemma(47) . The fact that utrophin was absent from the cardiac myofibrillar fraction argues against artificial redistribution of dystrophin during the subcellular fractionation procedure. The expression of substantial amounts of utrophin in normal adult cardiac muscle is another noteworthy difference between cardiac and skeletal muscle(29) .

Our finding that about 35% of the total cardiac muscle content of the 427-kDa form of dystrophin is associated with myofibrils points to a unique role for dystrophin in the structure/function of the cardiac myofibril. It is evident that dystrophin is a component not only of the membrane cytoskeleton but also of the intracellular cytoskeletal network that organizes myofibrils at the level of the Z-disc. It is of interest that the most frequent cardiac abnormality observed in dystrophin deficiency is dilated cardiomyopathy(37, 38, 39) , a condition associated with cytoskeletal disorganization as well as irregular sarcomeric and Z-disc structures(48) . The cardiomyopathic hamster that exhibits autosomal recessive cardiomyopathy and experiences muscular dystrophy has been widely used as a model system. While the precise genetic defects remain to be defined, several biochemical abnormalities associated with Ca overload have been noted(49) . The CHF 147 strain of hamsters experience dilated cardiomyopathy and have been shown to exhibit age-dependent morphological alterations in the sarcomeric and Z-disc arrangements that correlate with the decrease in contractile function and progression to cardiac insufficiency (33, 34, 35, 36) . Our results indicating the loss of myofibrillar dystrophin during the time course of these cardiac derangements suggest that dystrophin at the Z-disc may play an essential role in maintaining structural integrity, and its loss may contribute to the more severe cardiomyopathy compared with the milder muscular dystrophy experienced by these animals. Furthermore, the time-dependent increase in myofibrillar dystrophin paralleled the enhanced contractile performance documented for the normal hamster heart(36) , implying that dystrophin serves an important role in the contractile apparatus. It should be noted that the expression of desmin was essentially unaltered during the progression of cardiac insufficiency in the CHF 147 hamster heart, and this is consistent with results obtained in human-dilated cardiomyopathy(48) . The CHF 147 hamster is related to the BIO 14.6 cardiomyopathic strain that has been reported to completely lack adhalin expression in both cardiac and skeletal muscle with either no change or only a slight decrease in membrane dystrophin levels(14, 50) . The lack of adhalin has been suggested to result in disruption of the membrane dystrophin-glycoprotein complex in the cardiomyopathic hamster BIO 14.6 strain(14, 50) . We also noted the absence of adhalin in the CHF 147 hamster heart as early as day 30, prior to the onset of any symptoms (data not shown), while the membrane pool of dystrophin was reduced by only 28% at much later stages (i.e. day 180) of the disease. The expression of another membrane cytoskeletal protein, spectrin, was also unaltered in the cardiomyopathic hamster heart(50, 51) . While the absence of adhalin may contribute to cardiomyopathy and myopathy in these animals, our studies show that it is the loss of dystrophin from the cardiac myofibrils that correlates with progression to cardiac insufficiency. We suggest that alterations in unique cellular pools of dystrophin in cardiac muscle may underlie some of the differential pathophysiological responses of cardiac and skeletal muscle observed in muscular dystrophy.


FOOTNOTES

*
This work was supported by grants from the Heart and Stroke Foundation of Ontario and the Medical Research Council of Canada (to B. S. T.), a grant from the National Institutes of Health (to J. F.), and a grant from the Muscular Dystrophy Association of Canada (to P. H.). The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

§
Postdoctoral fellow of the Medical Research Council of Canada.

Studentship recipient from the Medical Research Council of Canada.

**
Career Investigator of the Heart and Stroke Foundation of Ontario, Canada. To whom correspondence should be addressed: Dept. of Pharmacology, University of Ottawa, 451 Smyth Rd., Ottawa, Ontario K1H 8M5, Canada. Tel.: 613-562-5800 (ext. 8355); Fax: 613-562-5456.

(^1)
The abbreviations used are: WGA, wheat germ agglutinin; MF, myofibril; SL, sarcolemma; PAGE, polyacrylamide gel electrophoresis; DTT, dithiothreitol.


REFERENCES

  1. Hoffman, E. P., Brown, J., and Kunkel, L. M. (1987) Cell 51, 919-928 [Medline] [Order article via Infotrieve]
  2. Hoffman, E. P., Knudson, C. M., Campbell, K. P., and Kunkel, L. M. (1987) Nature 330, 754-758 [CrossRef][Medline] [Order article via Infotrieve]
  3. Ahn, A. H., and Kunkel, L. M. (1993) Nat. Genet. 3, 283-291 [Medline] [Order article via Infotrieve]
  4. Menke, A., and Jokusch, H. (1991) Nature 349, 69-71 [CrossRef][Medline] [Order article via Infotrieve]
  5. Campbell, K., and Kahl, S. (1989) Nature 338, 259-262 [CrossRef][Medline] [Order article via Infotrieve]
  6. Yoshida, M., and Ozawa, E. (1990) J. Biochem. (Tokyo) 108, 748-752
  7. Ohlendieck, K., Ervasti, J. M., Snook, J. B., and Campbell, K. P. (1991) J. Cell Biol. 112, 135-148 [Abstract]
  8. Ibraghimov-Beskrovnaya, O., Ervasti, J. M., Leveille, C. J., Slaughter, C. A., Sernett, S. W., and Campbell, K. P. (1992) Nature 355, 696-702 [CrossRef][Medline] [Order article via Infotrieve]
  9. Gee, S. H., Montanaro, F., Lindenbaum, M. H., and Carbonetto, S. (1994) Cell 77, 675-686 [Medline] [Order article via Infotrieve]
  10. Campanelli, J. T., Roberds, S. L., Campbell, K. P., and Scheller, R. H. (1994) Cell 77, 663-674 [Medline] [Order article via Infotrieve]
  11. Xu, H., Wu, X. R., Wewer, U. M., and Engvall, E. (1994b) Nat. Genet. 8, 297-302 [Medline] [Order article via Infotrieve]
  12. Matsumura, K., Tomé, F. M. S., Collin, H., Azibi, K., Chaouch, M., Kaplan, J. C., Fardeau, M., and Campbell, K. P. (1992b) Nature 359, 320-322 [CrossRef][Medline] [Order article via Infotrieve]
  13. Roberds, S. L., Leturcq, F., Allamand, V., Piccolo, F., Jeanpierre, M., Anderson, R. D., Lim, L. E., Lee, J. C., Tome, F. M. S., Romero, N. B., Fardeau, M., Beckmann, J. C., Kaplan, J.-C., and Campbell, K. P. (1994) Cell 78, 625-633 [Medline] [Order article via Infotrieve]
  14. Roberds, S. L., Ervasti, J. M., Anderson, R. D., Ohlendieck, K., Kahl, S. D., Zoloto, D., and Campbell, K. P. (1993) J. Biol. Chem. 268, 11496-11499 [Abstract/Free Full Text]
  15. Brenman, J. E., Chao, D. S., Xia, H., Aldape, K., and Bredt, D. S. (1995) Cell 82, 743-752 [Medline] [Order article via Infotrieve]
  16. Arahata, K., Ishiura, S., Ishigura, T., Tsukahara, T., Suhara, Y., Eguchi, C., Ishihara, T., Nonaka, I., Ozawa, E., and Sugita, H. (1988) Nature 333, 861-863 [CrossRef][Medline] [Order article via Infotrieve]
  17. Bonilla, E., Samitt, C. E., Miranda, A. F., Hays, A. P., Salviati, G., DiMauro, L. M., Kunkel, E., Hoffman, P., and Rowland, L. P. (1988) Cell 54, 447-452 [Medline] [Order article via Infotrieve]
  18. Zubrzycka-Gaarn, E., Bulman, D., Karpati, G., Burghes, A., Belfall, B., Klamut, H., Talbot, J., Hodges, R., Ray, P., and Worton, R. (1988) Nature 333, 466-469 [CrossRef][Medline] [Order article via Infotrieve]
  19. Watkins, S. C., Hoffman, E. P., Slayter, H. S., and Kunkel, L. M. (1988) Nature 333, 863-866 [CrossRef][Medline] [Order article via Infotrieve]
  20. Peri, V. (1992) Characterization of a 360-kDa Protein and Dystrophin from the Myocardium . M.Sc. thesis, University of Ottawa
  21. Klietsch, R., Ervasti, J. M., Arnold, W., Campbell, K. P., and Jorgensen, A. O. (1993) Circ. Res. 72, 349-360 [Abstract]
  22. Peri, V., Ajdukovic, B., Holland, P., and Tuana, B. S. (1994) Mol. Cell. Biochem. 130, 57-65 [Medline] [Order article via Infotrieve]
  23. Frank, J. S., Mottino, G., Chen, F., Peri, V., Holland, P., and Tuana, B. S. (1994) Am. J. Physiol. 36, C1707-C1717
  24. Nigro, G., Politano, L., Nigro, V., Petretta, V. R., and Comi, L. I. (1994) Neuromuscular Disorders 4, 371-379 [CrossRef][Medline] [Order article via Infotrieve]
  25. Belcastro, A. N., Scrubb, J., and Gilchrist, J. S. (1991) Mol. Cell. Biochem. 103, 113-120 [Medline] [Order article via Infotrieve]
  26. Tuana, B. S., Murphy, B. J., and Yi, G. (1987) Mol. Cell. Biochem. 76, 173-184 [Medline] [Order article via Infotrieve]
  27. Seiler, S., and Fleischer, S. (1988) Methods Enzymol. 157, 26-36 [Medline] [Order article via Infotrieve]
  28. thi Man, N., Ellis, J. M., Love, D. R., Davies, K. E., Gatter, K. C., Dickson, G., and Morris, G. E. (1991) J. Cell Biol. 115, 1695-1700 [Abstract]
  29. Karpati, G., Carpenter, S., Morris, G. E., Davies, K. E., Guerin, C., and Holland, P. (1993) J. Neuropathol. Exp. Neurol. 52, 119-128 [Medline] [Order article via Infotrieve]
  30. Frank J. S., Mottino, G., Reid, D., Molday, R. S., and Philipson, K. D. (1992) J. Cell Biol. 117, 337-345 [Abstract]
  31. Koenig, M., Monaco, A. P., and Kunkel, L. M. (1988) Cell 53, 219-228 [Medline] [Order article via Infotrieve]
  32. Philipson, K. D., Longoni, S., and Ward, R. (1988) Biochim. Biophys. Acta 945, 298-306 [Medline] [Order article via Infotrieve]
  33. Hunter, E. G., Hughes, V., and White, J. (1984) Can. J. Physiol. Pharmacol. 62, 1423-1428 [Medline] [Order article via Infotrieve]
  34. Jasmin, G., and Proschek, L. (1982) Muscle & Nerve 5, 20-25
  35. Perennec, J., Willemin, M., Pocholle, P., Hatt, P. Y., and Crozatier, B. (1992) Basic Res. Cardiol. 87, 54-64 [Medline] [Order article via Infotrieve]
  36. Li, K., and Rouleau, J. L. (1993) Cardiovas. Res. 27, 968-973 [Medline] [Order article via Infotrieve]
  37. Muntoni, F., Cau, M., Ganau, A., Congiu, R., Arvedi, G., Mateddu, A., Marrosu, M. G., Cianchetti, C., Realdi, G., Cao, A., and Melis, M. A. (1993) New Engl. J. Med. 329, 921-925 [Free Full Text]
  38. Nigro, G., Comi, L. I., Politano, L., and Bain, R. J. I. (1990) Int. J. Cardiol. 26, 271-277 [Medline] [Order article via Infotrieve]
  39. Yoshida, K., Ikeda, S., Nakamura, A., Kagoshima, M., Takeda, S., Shoji, S., and Yanagisawa, N. (1993) Muscle & Nerve 16, 1161-1166
  40. Ervasti, J. M., Kahl, S. D., and Campbell, K. P. (1991) J. Biol. Chem. 266, 9161-9165
  41. Sato, O., Nonomura, Y., Kimura, S., and Maruyama, K. (1992) J. Biochem. (Tokyo) 112, 631-636
  42. Salviati, G., Betto, R., Ceoldo, S., Biasia, E., Bonilla, E., and Dimauro, S. (1989) Biochem. J. 258, 837-841 [Medline] [Order article via Infotrieve]
  43. Hemmings, L., Kuhlman, P. A., and Critchley, D. R. (1992) J. Cell Biol. 116, 1369-1380 [Abstract]
  44. Levine, B. A., Moir, A. J. G., Patchell, V. B., and Perry, S. V. (1990) FEBS Lett. 263, 159-162 [CrossRef][Medline] [Order article via Infotrieve]
  45. Way, M., Pope, B., Cross, R. A., Kendrick-Jones, J., and Weeds, A. G. (1992) FEBS Lett. 301, 243-245 [CrossRef][Medline] [Order article via Infotrieve]
  46. Herman, I. M. (1993) Curr. Opin. Cell Biol. 5, 48-55 [Medline] [Order article via Infotrieve]
  47. Pons, F., Robert, A., Fabrizzio, E., Hugon, G., Califano, J.-C., Fehrentz, J. A., Martinez, J., and Mornet, D. (1994) Circulation 90, 369-374 [Abstract]
  48. Schaper, J., Froede, R., Hein, S., Buck, A., Hashizume, H., Speiser, B., Friedl, A., and Bleese, N. (1991) Circulation 83, 504-514 [Abstract]
  49. Sole, M. J., and Liew, C. C. (1988) Am. J. Cardiol. 62, 20G-24G [Medline] [Order article via Infotrieve]
  50. Iwata, Y., Nakamura, H., Fujiwara, K., and Shigekawa, M. (1993) Biochem. Biophys. Res. Commun. 190, 589-595 [CrossRef][Medline] [Order article via Infotrieve]
  51. Messina, D. A., and Lemanski, L. F. (1994) J. Mol. Cell. Cardiol. 26, 937-941 [CrossRef][Medline] [Order article via Infotrieve]

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