1 Muscle Mechanics Laboratory, Institute of Gerontology, University of Michigan, Ann Arbor 48109-2007; and 2 Gilbert Engineering, Inc., Ann Arbor, Michigan 48103-9005
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ABSTRACT |
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The purpose of this study was to compare the excitability and contractility of three-dimensional skeletal muscle constructs, termed myooids, engineered from C2C12 myoblast and 10T1/2 fibroblast cell lines, primary muscle cultures from adult C3H mice, and neonatal and adult Sprague-Dawley rats. Myooids were 12 mm long, with diameters of 0.1-1 mm, were excitable by transverse electrical stimulation, and contracted to produce force. After ~30 days in culture, myooid cross-sectional area, rheobase, chronaxie, resting baseline force, twitch force, time to peak tension, one-half relaxation time, and peak isometric force were measured. Specific force was calculated by dividing peak isometric force by cross-sectional area. The specific force generated by the myooids was 2-8% of that generated by skeletal muscles of control adult rodents. Myooids engineered from C2C12-10T1/2 cells exhibited greater rheobase, time to peak tension, and one-half relaxation time than myooids engineered from adult rodent cultures, and myooids from C2C12-10T1/2 and neonatal rat cells had greater resting baseline forces than myooids from adult rodent cultures.
tissue engineering; myooid; myogenesis; isometric force; rodent tissue culture
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INTRODUCTION |
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IN VITRO SKELETAL MUSCLE TISSUE engineering involves culturing isolated myoblasts and fibroblasts in an environment conducive to the formation of a three-dimensional tissue construct. Cell sources employed to engineer such constructs include the C2C12 mouse muscle sarcoma cell line (15, 26, 29), embryonic avian muscles (1, 21-23, 25, 28), and skeletal muscles of neonatal (21) and adult (5, 17, 27) mammals. To promote formation of a three-dimensional structure, cells have been cultured in collagen gels (1, 15, 21, 26, 27, 30), on an elastic membrane (1, 21, 28), or between two stationary anchor points to which the cell monolayer remains attached (5, 21, 23). Collagen gels provide a scaffold for the cells and define the size and shape of the construct but may interfere with the force and power production of the myotubes. In the absence of an artificial scaffold, embryonic avian cells were developed into cylindrical organoids when subjected to uniaxial mechanical strain (28) or when cultured on prestrained elastic substrates (21). In one report, the isometric force of organoids was measured by lateral displacement of the organoids with a calibrated microneedle after elevation of the extracellular K+ concentration (28).
Cylindrical musclelike structures, termed myooids, were engineered from cocultures of primary mammalian myoblasts and fibroblasts (5), without a preexisting scaffold, the application of uniaxial mechanical strain, or prestressed substrates. Myooids were supported under tension between artificial tendons of laminin-coated silk suture; organoids were attached to stainless steel screens. In the case of myooids, the laminin-coated silk suture segments served as flexurally compliant artificial tendons, permitting easy attachment to a force transducer for functional evaluation. The excitability and contractility of myooids were measured with a force transducer by transverse electrical stimulation between parallel electrodes and measurement of axial force development (5). When normalized for cross-sectional area (CSA), the specific force (sPo) generated by myooids was not different from that of organoids, both being equivalent to ~1% of the sPo of adult rodent skeletal muscle (5).
The purpose of this study was to compare the CSA, excitability, and contractility of myooids engineered from cocultures of C2C12 myoblast and 10T1/2 fibroblast cell lines and primary cultures from the skeletal muscles of adult mice and neonatal and adult rats. For simplicity in terminology, myooids engineered from C2C12-10T1/2 cells, adult mouse, neonatal rat, and adult rat are referred to as C2C12-10T1/2 myooids, adult mouse myooids, neonatal rat myooids, and adult rat myooids, respectively. On the basis of preliminary data and observations, our working hypothesis is that the excitability and contractility of myooids engineered from primary cell sources do not differ, while the excitability and contractility of C2C12-10T1/2 myooids are lower than those of myooids engineered from primary cells. Our specific hypotheses are that 1) the measures of excitability and contractility do not differ among myooids engineered from primary cell sources and 2) C2C12-10T1/2 myooids have greater rheobase, chronaxie, time to peak tension, and one-half relaxation time and lower twitch force and peak isometric force than primary rodent myooids.
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MATERIALS AND METHODS |
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The methods for engineering myooids from primary cultures of rat soleus (SOL) muscles and the methods and instrumentation for measuring the excitability and contractility of myooids have been described in detail (5). For the formation of neonatal rat myooids, modifications were made in the surgical techniques for the removal of muscle tissue and in the composition of the cell culture and tissue dissociation media. The formation of myooids from established cell lines was accomplished only with the coculture of C2C12 myoblasts with 10T1/2 fibroblasts and the use of a reduced-serum culture medium (CM).
Media and solutions. The CM were growth medium (GM) and differentiation medium (DM), which have been described previously (5). For the culture of C2C12 cells, a CM was prepared [465 ml of DMEM (catalog no. 11995-065, GIBCO BRL), 35 ml of fetal bovine serum (FBS; catalog no. 10437-036, GIBCO BRL), and 100 U/ml penicillin G]. For storing neonatal muscle during harvesting, mincing solution (4) was prepared, brought to pH 7.4, and sterilized through 0.22-µm filters. Preincubation medium (PIM) was prepared as described previously (5). The CM and PIM were stored at 4°C until use. Tissues from adult animals were dissociated in an "adult" dispase-and-collagenase (D & C) solution [4 U/ml dispase (catalog no. 17105-041, GIBCO BRL) and 100 U/ml type IV collagenase (CLS 4, Worthington) in DMEM]. The neonatal muscle tissue was dissociated using "neonatal" D & C (ND & C) solution [4 U/ml dispase (catalog no. 17105-041, GIBCO BRL) and 100 U/ml type IV collagenase (CLS 4, Worthington) in mincing solution]. D & C and ND & C solutions were prepared immediately before use and sterilized through 0.22-µm filters.
Isolation and culture of primary cells. All animals were handled in accordance with the Guide for the Care and Use of Laboratory Animals. Neonatal Sprague-Dawley rats were delivered in litters of 11-14 within 1 day of birth from Charles River (Wilmington, MA), and muscle tissue was harvested from all the pups in the litter. On arrival, neonates were placed in 15-cm glass petri dishes on ice for 0.75-1.5 h as a general anesthesia. In a biological safety cabinet, the anesthetized pups were completely immersed in 70% ethanol before surgical removal of the muscle tissue. The muscles from the fore- and hindlimbs were removed and placed in 8 ml of mincing solution. ND & C solution (12 ml) was added, and the tissue was dissociated by magnetic stirring at room temperature for 1.5 h. The magnetic stir bar was removed, and the slurry was centrifuged for 15 min at 1,000 g. The pellet was resuspended in 20 ml of 0.1% (wt/vol) collagenase type IV (Worthington) in Ham's F-12 nutrient medium (GIBCO BRL) and placed in a shaker bath at 37°C for 1.5 h. The pellet was then centrifuged for 15 min at 1,000 g and resuspended in GM. Cells were counted with a hemocytometer, and the solution was adjusted to achieve the desired cell plating density (1 × 106, 1 × 105, 1 × 104, 1 × 103, 1 × 102, or 10 cells/cm2). Two milliliters of the cell suspension were plated onto each 35-mm culture dish with anchors in place, and the culture dishes were placed in a water-saturated incubator with 5% CO2 at 37°C.
For the harvesting of satellite cells and fibroblasts from adult (5- to 6-mo-old) Sprague-Dawley rats and C3H mice, animals were anesthetized with an intraperitoneal injection of pentobarbital sodium and the whole SOL or extensor digitorum longus (EDL) muscles were surgically removed. Each rat SOL muscle was sliced into six strips longitudinally from tendon to tendon; the mouse SOL and EDL muscles were left whole. The muscles and muscle strips were pinned at slack length in 35-mm culture dishes with Sylgard (Dow Corning, Midland, MI), preincubated for 50 h in PIM in a water-saturated incubator with 5% CO2 at 37°C, and then dissociated in 7.5 ml of D & C solution per strip or whole muscle for 3-4 h at 37°C. To achieve the greatest possible yield of satellite cells, the dissociated tissue was plated directly into the prepared culture dishes with laminin-coated suture anchors in place, without an attempt to filter the dissociated cells from the tissue debris. The plating density was therefore expressed as the amount of muscle tissue dissociated for each myooid in each 35-mm culture plate. Optimal plating densities for primary cells from rat and mouse muscle had been determined previously, with myooid size and contractility as the parameters to be optimized. The rat SOL muscle was plated at 13 g of tissue per plate, and the adult mouse SOL and EDL muscles were plated at 10 and 13 g of dissociated tissue per plate, respectively. For primary cultures, beginning at 48 h after cell plating, the GM was replaced every 48 h until the cells became confluent, which typically required 3-8 days. One day after the cells reached confluence, the medium was replaced with DM, and the cells were fed three times per week thereafter. Shortly after they were switched to DM, the myocytes fused to form multinucleated myotubes that began to contract spontaneously.Culture of cells from established lines. Myoblasts of the C2C12 cell line (CRL-1772; American Type Culture Collection, Rockville, MD) formed myooids only when cultured with 10T1/2 fibroblasts (provided by Dr. G. Salvatori). In preliminary experiments, plating densities of 1 × 106, 1 × 105, 1 × 104, 1 × 103, and 1 × 102 cells/cm2 were used for cocultured cells and for monocultured C2C12 cells. On the basis of the results from the preliminary experiments, for the cocultures of C2C12 and 10T1/2 cells the plating density was fixed at 1 × 105 cells/cm2. The myoblasts and fibroblasts were combined to produce cocultures with 30-80% C2C12 cells in increments of 10%. The C2C12 and 10T1/2 cells were mixed in CM, plated, and allowed to remain in culture for 48 h before the first media change. Until the myooids were evaluated, regular media changes were carried out every 48-72 h. There were no differences in the excitability or contractility of the myooids formed from different initial ratios of cell types. Consequently, these groups, termed C2C12-10T1/2 myooids, were pooled for subsequent analysis.
Myooid formation.
For all cell sources, myooids formed by delamination of the monolayer
of cultured cells from the Sylgard substrate. Artificial tendons of
silk suture with one end frayed and coated with natural mouse laminin
were employed, and the Sylgard substrate in each dish was coated with
laminin at a density of 1.0 µg/cm2. The failure rate due
to contamination of the culture plates was <5% for each experiment.
Contaminated plates were discarded immediately and not included in
subsequent analysis. The C2C12-10T1/2 myooids frequently did not detach completely from the Sylgard substrate. To aid detachment, the closed tips of a pair of sterile no.
5 forceps (Fine Science Tools) were used to gently tease the myooid
from the substrate. The myooids were then allowed to remodel for 72 h
before evaluation.
Experimental groups. The five experimental groups, based on the source of the cells for the myooids, were C2C12 and 10T1/2 cells, adult mouse SOL muscle, adult mouse EDL muscle, neonatal rat limb muscle, and adult rat SOL muscle. The values of 13 experimental variables were determined for each of the 5 experimental groups. Nine variables were measured directly: morphology (diameter), excitability [rheobase (R50) and chronaxie (C50)], isometric force measurements [passive baseline (Pb), peak twitch (Pt), and peak isometric force (Po)], and the time-dependent variables [time to peak twitch force (TPT), rate of force development (dP/dt), and one-half relaxation time (RT1/2)]. Four additional parameters were calculated from the measured variables: CSA of the myooid from the diameter, sPo by dividing Po by the CSA, and the ratios of peak twitch to peak isometric force (Pt/Po) and passive baseline to peak isometric force (Pb/Po). Since CSA was calculated directly from diameter, the diameter was not included in the statistical analysis, leaving 12 experimental variables.
Histology. After contractile properties were measured, myooids were pinned at the length at which they were cultured (Lc) and fixed for 4 h at 4°C in Karnovsky's solution (0.1 M sodium cacodylate buffer with 3% formaldehyde and 3% glutaraldehyde at pH 7.4). Myooids were rinsed three times (30 min, 30 min, and 4 h) with cacodylate buffer (pH 7.4) with 7.5% sucrose. Myooids were postfixed in 1% osmium tetroxide for 2 h at room temperature, dehydrated in graded concentrations of ethanol and propylene oxide, and embedded in Epon (Eponate 12 resin; Ted Pella, Redding, CA) for light microscopy. Cross sections were cut 600 nm thick for light microscopy and stained with 1% toluidine blue.
Data collection and analysis.
The methods for measuring the excitability and contractility of myooids
have been described in detail previously (5). Culture times were defined from the time of cell plating, rather than from the
time of myooid formation. The myooid diameter was defined as the
minimum diameter of each myooid along the length between the anchors.
Myooid diameter was measured using a calibrated eyepiece reticle while
each myooid was viewed through a ×10 objective lens on an inverted
microscope (Zeiss Axiovert 25, Thornwood, NY). CSA was calculated from
the measured diameter, assuming a circular cross section. All
contractile properties were measured 32 ± 4 days after the cells
were plated and 72 h after formation of each myooid. Myooid
temperature was maintained at 37 ± 1°C during the measurement
of contractile properties by use of a heated aluminum platform.
Myooid life span. Myooids from three of the experimental groups (adult mouse SOL and neonatal and adult rat SOL) were maintained in culture beyond 30 days to determine the time over which they remained viable. Myooids continue to contract spontaneously and may be functionally evaluated until the point at which they mechanically fail, typically by breaking at some point between the suture anchors. We define the time from cell plating until the myooid breaks as the "life span" of the myooid. Life spans were not observed for adult mouse EDL myooids, because a culture contamination at the preincubation stage left only enough tissue for the formation of four myooids, all of which were used for measurement of excitability and contractility. C2C12-10T1/2 myooids were not included in the life span study, because excitability and contractility were so variable for this group that a large "n" was required to achieve statistical significance for comparisons. No contractile function tests were performed on any myooids used for the life span study. Myooids were fed and monitored three times each week until they failed by mechanical breakage between the suture anchors.
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RESULTS |
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Spontaneous activity of myotubes and myooids in culture. When the spontaneous contractile activity of the myotubes before delamination of the monolayer was compared, qualitative and quantitative differences were evident. The C2C12 myotubes contracted singly and sporadically and at a frequency of 3-5 Hz, whereas the sheet of myotubes from the primary explants contracted regularly and vigorously as a syncytium, with a frequency of 0.5-1.5 Hz. Under low-power magnification, spontaneous contractions were observed in all the myooids from primary cells. In contrast, C2C12-10T[1/2] myooids often appeared inactive until electrically excited. Occasionally, large-amplitude spontaneous contractions occurred after electrical stimulation of the C2C12-10T1/2 myooids.
Myooid formation. Monocultured C2C12 cells never formed a myooid regardless of the plating density, although in all cases they formed a monolayer of myoblasts and myotubes on the substrate. After ~3-10 days in culture, the monolayer of monocultured C2C12 cells delaminated in small (1- to 2-mm-diameter) irregular patches, resulting ultimately in disintegration of the monolayer. In contrast, the cocultures of C2C12 cells and the 10T1/2 fibroblasts formed myooids ~50% of the time, independent of the mixing ratio of the cells, in the range of 30-80% C2C12 cells. The inability of the monocultured C2C12 cells to form myooids appeared to be attributable to the absence of fibroblasts. The fibroblasts likely function to provide an extracellular matrix that strengthens the monolayer before delamination, as reported earlier by Vandenburgh et al. (28).
Since no differences were observed between groups of myooids engineered from different proportions of C2C12 cells and fibroblasts, these data were pooled for subsequent analysis. The larger diameters of the C2C12-10T1/2 myooids (Table 1) suggest incomplete remodeling of the monolayer of cells into a cylindrical myooid within the allotted 72 h. The success rate for myooid formation using neonatal cells was >95% at plating densities of 1 × 106 cells/cm2, ~50% at 1 × 105 cells/cm2, and 0% for lower plating densities. In contrast, the cells from adult rat cultures formed myooids ~95% of the time when plated on 1.0 µg/cm2 laminin at 13 mg of dissociated tissue per plate.
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Excitability and contractility.
The mean values for each of the 12 experimental variables in each of
the 5 experimental groups are summarized in Tables 1 and
2. Table 1 shows mean values for CSA,
excitability (R50 and C50), and the
time-dependent isometric twitch parameters (TPT, dP/dt, and
RT1/2) of myooids. The mean values for the isometric contractility measures (Pb, Pt, Po,
sPo, Pb/Po, and
Pt/Po) are summarized in Table 2. The results
of the Tukey-Kramer method for all 120 pairwise comparisons of
variables between groups are summarized in Fig.
1 for the five original experimental
groups.
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Life span of myooids in culture.
Myooids spontaneously contracted throughout their life span. Typically,
the diameter decreased steadily until the myooid broke, usually during
a media change after the diameter had decreased to <50 µm. The
average and maximum life spans for adult mouse SOL and neonatal and
adult rat SOL myooids are presented in Fig. 3. Adult mouse SOL myooids, plated at 10 mg of dissociated tissue per plate, remained viable in culture for an
average of 101 ± 12 (SE) days (n = 8), with a
maximum observed life span of 168 days. Neonatal rat myooids plated at
1 × 106 cells/cm2 were viable for an
average of 52 ± 2.5 days (n = 25), with a maximum
observed life span of 69 days. Adult rat SOL myooids, plated at 13 mg
of dissociated tissue per plate, remained viable for an average of
74 ± 6 days (n = 11), with a maximum observed life span of 127 days.
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DISCUSSION |
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The sPo for whole muscles from adult rats is ~250 kN/m2 (3). Few reports exist of the sPo of mammalian skeletal muscle at early stages of development, but the sPo for SOL and EDL muscles of newborn Wistar rats were 44 and 74 kN/m2, respectively (2). The low values of sPo of skeletal muscles from newborn rats, only 18 and 30% of values for adult rats, have been attributed to the presence of embryonic and neonatal isoforms of myosin heavy chain (MHC) present in neonatal (11) and developing muscles (18). For each of the five groups of myooids, sPo of 4-19 kN/m2 are 5-43% of the values for muscles of newborn rats and 2-8% of the values for muscles of adult rats. Of the myooids, the C2C12-10T1/2, neonatal rat and adult rat myooids had the lowest values for sPo, ~4 kN/m2, whereas the adult mouse myooids had the highest values, 16 kN/m2. On the basis of the sPo, myooids in each of five groups appear to have poorly developed contractile apparatus, in addition to the possibility of the expression of predominantly developmental isoforms of MHC (18).
Although direct measurements of the MHC isoform composition of myooids have not been made, the time-dependent characteristics of the twitch, TPT, RT1/2, and dP/dt, as well as Pt/Po, are consistent with the hypothesis that the predominant myosin isoforms in myooids are developmental, not adult, isoforms. For myooids from each of the primary cultures of muscles from mice or rats, TPT was 50-65 ms, values within the range reported for SOL and EDL muscles of newborn rats (2, 6). Even for the newborn rats, RT1/2 varies more widely than the TPT, with a value of 70 ms for the SOL muscles and 50 ms for the EDL muscles. Only the pooled mouse myooid experimental group had an RT1/2 in this range, 62 ms, and in the remainder of the myooids from primary cultures RT1/2 ranged from 81 to 100 ms. The TPT and RT1/2 of the C2C12-10T1/2 myooids were considerably more prolonged than the values for other myooids. The time-dependent characteristics of the myooid twitches appear to be dependent on the same mechanisms that impose the differences in the force-velocity relationships of neonatal and adult muscles, namely, the rate of Ca2+ release and reuptake in muscle as a function of age from birth (2, 6). The similarity of the TPT and RT1/2 of the mouse and rat myooids, regardless of age of the donor, to those of the newborn rats is in contrast to the widely divergent values for the C2C12-10T1/2 myooids. The magnitude of the differences for the C2C12-10T1/2 myooids suggests major impairments in development of this cell line in culture.
The maximum rate of rise of force has been used to study the developmental changes in skeletal muscles of neonatal and young rats (2, 6). When normalized as a percentage of the rise in Po, the maximum rate of rise of force correlates strongly with the maximum velocity of shortening (2). The maximum rate of rise of force in skeletal muscles is low at birth, largely because of the low actomyosin ATPase activity (6), but increases rapidly to achieve adult values after the first month. During this period, the maximum rate of rise of force increases fivefold (6) and the maximum velocity of unloaded shortening of the EDL muscles doubles (2). The dP/dt values of the myooids, expressed in absolute terms of micronewtons per millisecond, were at least four to five orders of magnitude slower than values of 45 and 120 mN/ms reported for SOL and EDL muscles of adult rats (6, 20) and were still two orders of magnitude slower when expressed as a percentage of the Po. These data suggest that the capacity of the myooids to develop force rapidly and to shorten at high velocity is even more impaired than their ability to generate sPo.
The Pt/Po of the four groups of primary rodent myooids ranged from 0.43 to 0.60. These values for Pt/Po compare favorably with 0.60 ± 0.05 (SD) and 0.53 ± 0.08 reported for SOL and EDL muscles of newborn rats, respectively (2). The ratio decreases rapidly and stabilizes within the 1st mo of life at the adult values of 0.25 for SOL muscles and 0.19 for EDL muscles. As with the other variables, the Pt/Po of the C2C12-10T1/2 myooids was outside the range of the other groups. The similarity of the Pt/Po data for rodent myooids to that of neonatal and newborn rodents, as well as the time-dependent properties of the twitch, support the conclusion that the myooids are arrested in the state wherein they express predominantly, if not exclusively, embryonic and neonatal isoforms of myosin (2, 11, 18).
The absence of any differences in the excitability or contractility for adult mouse myooids, whether engineered from SOL or EDL muscles, indicates that myooids can be developed from muscles expressing exclusively either slow and intermediate or fast isoforms of MHC (16). Unexpectedly, a fourfold greater sPo was observed for pooled adult mouse myooids than for adult rat SOL myooids. We have no explanation for such a large difference in such a critical measure of function, particularly in the absence of any other difference between these two groups.
The lower excitability and contractility of C2C12-10T1/2 myooids than of the primary cultures of rodent myooids may be attributable to the lack of normal metabolism, phenotype, or growth regulation of C2C12 myoblasts (8, 13, 24). Even when cultured with 10T1/2 fibroblasts, C2C12 myoblasts formed myooids only one-half as reliably as the 95% success rate for the formation of myooids from primary cultures of skeletal muscles from neonatal and adult rodents. The differences between the C2C12-10T1/2 myooids and the primary culture myooids were spread over more than one-half of the 12 variables. Interestingly, one variable that did not differ among the groups was C50, which ranged from 416 to 603 µs. In contrast, R50 for the C2C12-10T1/2 myooids was two- to fourfold greater than that of any other group. Despite the lack of an explanation for the reduced excitability of the C2C12-10T1/2 myooids, the functional data taken as a whole suggest important differences in the cellular organization and chemomechanical coupling of C2C12-derived myotubes compared with primary myotubes.
Fibroblasts assist in extracellular matrix formation during myogenesis in vitro (7, 12, 19, 21, 22, 28). C2C12 myoblasts did not form myooids when monocultured, yet they formed myooids with some success when cocultured with fibroblasts, substantiating the critical role of fibroblasts in the formation of myooids. As reported earlier (5), fibroblasts generally oriented around the periphery and along the total length of the myooid. Apparently, in primary cultures of skeletal muscles of mice and rats, the simple dissociation of muscle tissue used for this study provided an adequate source of myoblasts and fibroblasts for the formation of the myooids. The Pb of myooids may be generated by the fibroblasts within the myooid, because fibroblasts generate tensile forces in culture in the presence of serum (9, 10). Since larger baseline forces also correlate with shorter myooid life span in culture, further studies should consider the influence of fibroblasts in myooid function and longevity.
The primary limitation with the myooid model as presented is the failure of the myotubes in the myooid to express a fully adult phenotype, in terms of sarcomere structure, excitability, and contractility. We hypothesize that the arrested developmental state of the myotubes involves the expression of chiefly embryonic and neonatal isoforms of myosin, resulting from the culture conditions we imposed, in which there was no application of mechanical strain, either active or passive, no electrical stimulation, and no innervation. As such, the data presented form the basis for future experiments in which experimental interventions can be applied to study the effect of controlled mechanical strain, electrical stimulation, nerve-muscle coculture, and addition of growth factors and trophic agents on muscle development, contractility, and excitability in culture. Thus myooids could prove to be useful in the study of skeletal muscle organogenesis, synaptogenesis, and chemomechanical transduction. The presence of the suture anchors allows the attachment of force transducers and servo motors, so that controlled mechanical strain may be applied while forces are monitored. The three-dimensional, cylindrical structure permits electrical fields to be generated across the tissue more easily and accurately than is possible with a cell monolayer, facilitating chronic exposure of the tissue to electrical fields to influence development as well as activation of the tissue for functional evaluation.
Myooids may also be used for studying the physiology of muscle engineered from cells from animals with neonatal-lethal mutations affecting skeletal muscle, stem cell incorporation into muscle tissue, and plasticity and function of skeletal muscle engineered from the satellite cells of aged mammals. If the myooid model is adapted for use with human tissue, it could be used to test the effectiveness of specific gene therapy approaches to correct such disorders as malignant hyperthermia or muscular dystrophy. Tissue samples or tissue from human fetal tissue banks could be employed, thus eliminating the risks inherent to the introduction of genetic material into living humans until the effectiveness of the therapy in human muscle tissue can be established.
In summary, functional three-dimensional skeletal muscle constructs may be engineered from primary cultures of cells from fast and slow muscles of neonatal and adult rodents. The muscle constructs develop without the use of synthetic scaffolds to support the contractile section of the muscle and can be maintained in culture for several months. The excitability and contractility of myooids is similar to that which would be expected from embryonic or neonatal muscle tissue under conditions of chronic denervation. On the basis of the consistency, diversity, and magnitude of the differences between the C2C12-10T1/2 myooids and primary adult rodent myooids, the C2C12 cells appear to be less suitable than adult rodent primary cultures for engineering functional muscle constructs.
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ACKNOWLEDGEMENTS |
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The authors thank Cheryl Hassett for assistance in the development of the surgical techniques used for the neonatal rat dissections and histology, Dr. Krystyna Pasyk for assistance with histological sections for this research, Dr. Giovanni Salvatori for providing the 10T1/2 fibroblasts, and Dr. Joseph Chromiak (Brown University) for invaluable assistance and advice on the details of neonatal skeletal muscle primary culture.
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FOOTNOTES |
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This work was supported by a pilot grant from the University of Michigan Center for Biomedical Engineering Research, by National Institute on Aging Grant RO1-AG-06157, and by access to space and resources in the Contractility Core of the Nathan Shock Center in the Institute of Gerontology at the University of Michigan.
Address for reprint requests and other correspondence: R. G. Dennis, 300 N. Ingalls, Rm. 956, Ann Arbor, MI 48109-2007 (E-mail: bobden{at}umich.edu and bdennis{at}ai.mit.edu).
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Received 19 May 2000; accepted in final form 1 September 2000.
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