Article |
Address correspondence to Jennifer E. Morgan, Muscle Cell Biology Group, Medical Research Council Clinical Sciences Centre, Faculty of Medicine, Imperial College School of Technology and Medicine, Hammersmith Hospital Campus, Du Cane Road, London W12 ONN, UK. Tel.: 02-08-383-8262. Fax: 02-08-383-8264. E-mail: jmorgan{at}csc.mrc.ac.uk
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Abstract |
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Key Words: radiation; neoplasia; skeletal muscle; cell transplantation; muscle precursor cell
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Introduction |
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Skeletal muscle regeneration is a well-studied model that superficially closely recapitulates embryonic myogenesis in which activation, proliferation, and subsequent differentiation of muscle precursor cells (MPC)* to form new muscle tissue has been well described both in tissue culture and in vivo. We have attempted to bridge the gap between in vivo and in vitro models by transplantation of myoblasts, using the immunodeficient, dystrophin-deficient mdx nu/nu mouse host. A major goal in this work is to identify environmental factors that optimize muscle formation from implanted cells. Thus far, the most effective procedure is preirradiation of host mouse muscle with 18 Gy. This causes the implanted cells to proliferate (Beauchamp et al., 1999), form more muscle, and migrate to contiguous muscles more frequently than in the nonirradiated leg (Morgan et al., 1993). The irradiated muscle environment is thus clearly beneficial for myoblast transplantation. However, the dose is too high to be considered as a therapeutic option and we need, therefore, to understand its mechanism of action in the hope of reproducing it by less extreme means.
To this end, we have established a simple assay for the effect of preirradiation of the host muscle on implanted MPC, using the myogenic cell line C2 C12 (Yaffe and Saxel, 1977; Blau et al., 1983). These cells form muscle upon implantation into mouse muscle, but eventually form tumors (Wernig et al., 1991; Morgan et al., 1992). Such tumors formed far more rapidly in irradiated than in nonirradiated mdx nu/nu mouse muscles (Pagel et al., 2000), thus constituting a rapid and sensitive assay for the growth promoting effects of irradiation. Here, we have used C2 C12derived tumor formation as a measure of radiation-induced stimulation of muscle cell proliferation, showing that this effect is persistent and that switching of the C2 C12 cell phenotype from myogenic differentiation to aggressive neoplastic behavior is reversible. We have also identified individual retrovirally marked subclones of C2 C12 cells that do or do not show this capacity for conversion between neoplasia and differentiation.
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Results |
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Our results show that radiation delivered to one leg does not have a growth-promoting effect on cells implanted into the contra-lateral leg. There was no significant difference in the number of donor muscle fibers between the nonirradiated muscles of mice that had their right leg irradiated (Table I, experiments A2, E, and G) and mice of the same strain that had neither leg irradiated (Table I, experiments B, F, and H).
Preirradiation of host muscle augments C2 C12derived tumor formation
In both mdx and nonmyopathic immunodeficient host strains, implantation of 5 x 105 C2 C12 cells leads to the formation of macroscopically visible tumors in all of the irradiated muscles, but in none of the nonirradiated muscles (Fig. 2). Histologically, irradiated mdx nu/nu TA muscles that had been injected with C2 C12 cells contained large numbers of dystrophin-positive fibers, but also conspicuous areas of undifferentiated interstitial cells, which we presume to be tumor cells (Fig. 3 A). Similar undifferentiated cells were seen in irradiated, C2 C12 cellinjected beige/nu/Xid muscles (unpublished data). Nonirradiated muscles contained smaller numbers of undifferentiated cells, interspersed diffusely between donor muscle fibers (Fig. 3 B). In both host strains, significantly more nondifferentiated interstitial cells were found in the irradiated right TA than in the nonirradiated left TA (Table II, experiments A1, A2, and F). Thus, 18 Gy of gamma radiation, delivered to the host muscle 3 d before cell implantation, augments tumor formation from implanted C2 C12 cells in both myopathic and normal mouse muscles.
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Preirradiation of host skeletal muscle leads to a persistent enhancement of tumorogenesis
Visible tumors were found in all of the irradiated muscles that had been injected with C2 C12 cells at all three time points after irradiation (Table II, experiments AC). They were also seen in 2/7 of the nonirradiated muscles that were contralateral to muscles irradiated 28 d before cell implantation. Histologically, significantly more interstitial cells were found in the irradiated right TA muscles than in the nonirradiated, contralateral muscle at all three time points. Most undifferentiated tissue was found when the cells were injected 28 d after irradiation. However, noticeably less undifferentiated tissue was found in muscles injected 100 d after irradiation (Table II). This may reflect the loss of muscle mass 100 d after irradiation, leaving fewer irradiated host fibers than at earlier times to influence the implanted C2 C12 cells. Nonetheless, enhancement of C2 C12derived tumor formation clearly persists for at least 100 d after 18 Gy of irradiation. Moreover, significantly more muscle fibers of donor origin were also found in the muscles injected with C2 C12 cells at this time point than in the contralateral, nonirradiated legs (Table II).
C2 C12 tumorogenicity in vivo is dependent on the dose of preirradiation
Tumors were seen in 4/5 of the muscles irradiated with 9 Gy and in only 4/11 of the muscles irradiated with 4.5 Gy (Table II). The amount of nondifferentiated interstitial cells was far less in the muscles preirradiated with either 9 Gy or 4.5 Gy than in the muscles preirradiated with 18 Gy (Table II). These results show that the radiation dose required to elicit rapid tumor formation is critical; 18 Gy is effective, but 9 and 4.5 Gy are both suboptimal to induce C2 C12 cells to rapidly form tumors.
Although there were variations in the amount of tumor and extent of muscle formation between experiments, the results presented in Table II show no significant dose-dependent change in the number of donor muscle fibers in irradiated muscles. There does appear to be more donor muscle in muscles irradiated with 18 Gy compared with contralateral muscles, but this was not always significant. (Table II, experiments A1 and A2).
The finding that the amount of donor muscle and undifferentiated interstitial cells formed in nonirradiated muscles varies from group to group (Table II) seems likely to be due to interexperimental variation, rather than the irradiation of one leg having a systemic or contralateral effect on the opposite, nonirradiated leg. To confirm this, we injected C2 C12 cells from a single batch into both legs of mdx nu/nu hosts that either had their right legs irradiated with 4.5 or 18 Gy or had neither leg irradiated. We found no significant difference in the amount of donor muscle or the amount of nondifferentiated tissue in nonirradiated muscles, whether they were from mice in which the right leg had been irradiated with 4.5 or 18 Gy, or from mice which had neither leg irradiated (Table III, experiments A2, E2, and H).
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Subclones of C2 C12 cells form tumors
The ability of C2 C12 cells to form tumors and muscle in vivo was further examined using subclones derived from a population of C2 C12 cells retrovirally infected with a marker gene and an antibiotic resistance gene. Clones of retrovirally infected C2 C12 cells that were ß-gal positive and gave rise to myotubes in vitro were isolated and either pooled and analyzed as an oligoclonal population or analyzed as separate clones.
For the oligoclonal analysis, seven clones were coinjected into the irradiated right legs and nonirradiated left legs of 11 mice. Muscles from six of these mice were removed for analysis 21 d after cell injection. No tumors were visible in any of the injected muscles, and sections of these muscles contained very few, if any, undifferentiated cells. The remaining five mice were left until 90 d after grafting; only one of these irradiated muscles contained a small, macroscopically visible tumor. All muscles contained conspicious amounts of donor muscle (Fig. 5, A and B).
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These data show that some subclones of C2 C12 cells form tumors and some do not, indicating a heterogeneity in the original C2 C12 cell line in response to an irradiated muscle environment.
Candidate myoblast proliferation or migration factors are not augmented in mouse skeletal muscle by radiation
To investigate whether factors that have been implicated in the proliferation or migration of MPCs were altered in irradiated skeletal muscle (Bischoff, 1997; El Fahime et al., 2000; Kastner et al., 2000),we examined the expression of four growth factors (ß-fibroblast growth factor [FGF], FGF-4, FGF-6, and hepatocyte growth factor) and two matrix metalloproteinases (MMP-2 and MMP-9) in mdx and C57 Bl/10 muscles 3 d after 18 Gy of irradiation. There were no significant differences in expression of these proteins in irradiated and nonirradiated mdx and C57Bl/10 muscles (Fig. 6). Although the amounts of ß-FGF, FGF-4, and FGF-6 were slightly reduced in irradiated C57Bl/10 muscles and slightly elevated in irradiated mdx muscles, these differences were not significant. MMP-2 was slightly elevated in irradiated C57Bl/10 muscles and slightly reduced in irradiated mdx muscles, but there was no change in MMP-9 expression in irradiated muscles.
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Discussion |
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The immortal C2 C12 myogenic cell line forms skeletal muscle in greater amounts than do conditionally immortal H2K18.30 MPCs, but also gives rise to tumors after several weeks in vivo (Wernig et al., 1991; Morgan et al., 1992; Pagel et al., 2000). Previous experiments have shown that expansion of engrafted C2 C12 cells in muscle is not constrained by normal myoblasts (Morgan et al., 1992), implying that the irradiation-induced proliferation is not simply a response to the creation of a vacant niche by ablation of endogenous satellite cells. Formation of C2 C12derived neoplasms was considerably accelerated by preirradiation of the graft site. C2 C12 cells invariably gave rise to visible tumors within 3 wk in irradiated legs, but rarely in the nonirradiated, contralateral legs. This is reflected in the histology of the graft sites, which contained significantly larger undifferentiated interstitial cell areas in irradiated than in nonirradiated muscles in both mdx nu/nu and beige/nu/Xid hosts. The tumor-enhancing effect of radiation persists for at least 100 d and is dose dependent.
Our data imply that the effect of irradiation on enhancement of cell proliferation is restricted to the site of irradiation, for there is no systemic or contralateral effect, as has been observed, for instance, in increased proliferation of proximal tubule cells in mouse kidneys contralateral to an irradiated kidney (Otsuka and Meistrich, 1993).
The mechanism by which irradiated tissue influences the proliferation of grafted cells is not clear. Ionizing radiation causes DNA damage, which, if not effectively repaired, causes cell death after the first or second postirradiation mitosis. Therefore, rapidly dividing cells, such as satellite cells in growing skeletal muscle, are more sensitive to irradiation than nondividing cells. Apart from preventing growth and regeneration of dystrophic muscle (Wakeford et al., 1991; Weller et al., 1991; Quinlan et al., 1995, 1997; Heslop et al., 2000), the effects of high doses of radiation delivered to mainly postmitotic skeletal muscle have scarcely been documented. Some increase in muscle fiber permeability in vitro has been reported (Canaday et al., 1994), but does not seem to occur in vivo (Pagel and Partridge, 1999). It has also been reported that the structural proteins titin and nebulin are degraded immediately after irradiation (Horowits et al., 1986) and that microvascular networks within skeletal muscle are damaged by 10 Gy, causing a reduction of blood supply to the muscle 30 d later (Roth et al., 1999).
It is quite possible that radiation induces either muscle or nonmuscle cells within the graft site to produce growth factors that enhance donor cell proliferation. Indeed, radiation has been reported to raise levels of growth factors in various cells or tissues for up to 6 wk after irradiation (Peter et al., 1993; Yi et al., 1996; Gorski et al., 1999; Kruse et al., 1999; Mori et al., 2000; Wang et al., 2000). A survey of substances that may affect growth or migration of MPCs detected no elevation of ß-FGF, FGF-4, FGF-6, MMP-2, MMP-9, or scatter factor (hepatocyte growth factor) in irradiated muscles. However, the crucial determinant may be the availability or efficiency of presentation, rather than the actual amount, of growth factor. This explanation is consonant with the long-lasting effect of irradiation, because a persistent change in the composition of proteoglycans in the interstitium of muscle might affect the presentation of growth factors by connective tissue elements and augment muscle cell proliferation (Desgranges et al., 1999; Stockholm et al., 1999).
Alternatively, radiation might ablate an inhibitory agent. Skeletal muscle is rarely the site of tumor formation (Hundt et al., 1999), and it contains a substance(s) that inhibits tumor proliferation (Bar-Yehuda et al., 1999). The notion of inhibitory control of cell proliferation is also in accordance with the fact that the muscle satellite cells are deeply quiescent in normal, mature, undamaged muscle, but are capable of rapid proliferation in response to injury. Moreover, simple removal from the muscle environment evokes extremely rapid activation of satellite cells (Beauchamp et al., 2000).
Effects of irradiated cells on the proliferation of nonirradiated cells in vivo have been noted previously. For example, nonirradiated mouse tumor cells mixed with irradiated cells and implanted subcutaneously into host mice grew more rapidly than the nonirradiated cells alone (Revesz, 1956, 1958). Similarly, tumor formation from mouse mammary epithelial cells was enhanced by irradiation (4 Gy) of the host mouse mammary glands before cell implantation (Barcellos-Hoff and Ravani, 2000), and survival, migration, and proliferation of implanted O2-A progenitor cells were enhanced by preirradiation (40 Gy) of the rat spinal cord graft site (Franklin et al., 1996). The proliferative effects of irradiation that we have shown here appear, from previous work on conditionally immortal myoblasts, to be restricted to a small subpopulation of cells that shows characteristics of early precursors (Beauchamp et al., 1999), perhaps corresponding to the "reserve" satellite cells described by Schultz (1996). It remains to be determined whether the C2 C12 cells that respond to the preirradiated graft site fall into the analogous nondifferentiating reserve cells that have been described in this line (Yoshida et al., 1998) and characterized by expression of CD34 (Beauchamp et al., 2000). In the context of current interest in circulating multipotential stem cells (Ferrari et al., 1998; Gussoni et al. 1999; Lagasse et al., 2000; Krause et al., 2001; Orlic et al., 2001), such a specific stimulatory effect may be important, because these cells have not been observed, so far, to make more than a rare and trivial contribution to myogenesis, even when directly injected into the muscle.
To our surprise, the switch to tumor formation in C2 C12 cells implanted into an irradiated environment was not irrevocable, because fragments of C2 C12derived tumor produced very large amounts of muscle in a second host. Curiously, even in preirradiated sites in a second host, they produced more muscle than had been present in the original tumor, implying that they had been in some way altered by this first exposure to an irradiated environment. Thus, C2 C12 cells behave in an analogous way to primary (Yao and Kurachi, 1993) and conditionally immortal muscle cells (Morgan et al., 1994; Gross and Morgan, 1999) in that they function as MPCs after their implantation.
Our cloning experiments demonstrate that C2 C12 cells comprise a bimodal population in their propensity to form tumors in vivo. Initially, we implanted a mixture of retrovirally marked clones into irradiated mdx nu/nu mouse muscles and found a tumor in only one out of five muscles, examined 90 d later. This lack of tumorogenicity may have been due to the insertion of the retrovirus or the expression of ß-gal, or again, exposure to geneticin rather than to the clonal selection itself. Immune rejection of cells marked with ß-galexpressing retroviruses (Abina et al., 1996; Visted et al., 2000) is unlikely in our immunodeficient mice, where we always find ß-galexpressing muscle fibers. Moreover, upon analysis of single clones, we found one retrovirally infected C2 C12 subclone that produced only muscle and gave rise neither to tumors nor to the excess of interstitial cells that are normally associated with grafts of C2 C12 cells. Other subclones gave rise to both muscle and tumor in irradiated legs. Of practical interest, the clone that gave rise to no undifferentiated tumor tissue provides an excellent model of muscle regeneration. The existence of nontumor-forming clones may explain the lack of tumors in previous experiments where C2 cells had been transfected in vitro and selected or cloned before their transplantation (Hamamori et al., 1994, 1995; Dhawan et al., 1996; Bohl and Heard, 1997). We have yet to determine whether the tumor-forming clone contains subclones that can still form muscle in a second host mouse.
The interaction between a cell and its environment in postnatal tissue is crucial to the fate of the cell. Environmental changes occur during differentiation, growth, and disease processes and after external damage to the tissue. We have shown that modulating the host environment by gamma irradiation before cell implantation augments muscle formation from MPCs by driving them into proliferation. Similarly, it drives proliferation of C2 C12 cells, but, additionally, it generates an accelerated neoplastic transformation that is reversible upon return of the cells to a nonirradiated environment. This demonstrates a profound phenotypic modulation by purely environmental factors. It may be akin to the changes from neoplastic behavior of teratoma cells and their normal integration into developing embryos (Mintz and Illmensee, 1975; Illmensee and Mintz, 1976) and the effect of the environment on the transformation of a normal cell into a malignant cell (for review see Park et al., 2000). Identification of the factor(s) within irradiated muscle that effects the proliferation of implanted cells would be important for the development of new strategies both for preventing tumor formation and improving myoblast transfer to treat myopathies such as Duchenne muscular dystrophy.
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Materials and methods |
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To assay the growth promoting effects of irradiation, we used C2 C12 donor cells (Yaffe and Saxel, 1977; Blau et al., 1983). C2 C12 cells were cultured in flasks, coated with 0.01% gelatin, in DME containing 10% FCS. In some experiments, C2 C12 cells were infected with the retrovirus coding for cytoplasmic LacZ and cloned in G418 to obtain clones that were 100% ß-gal positive.
The above cell lines were kept as replicate vials frozen in liquid nitrogen. For each experiment, a single vial was thawed and cultured for 3 or 4 d before implantation. Pellets containing 5 x 105 cells were prepared for implantation.
Cell implantation
Dystrophin-deficient mdx mouse muscle undergoes extensive spontaneous degeneration and regeneration accompanied by infiltration of cells such as macrophages. To determine how the growth-promoting effect of irradiation is occurring, it is important to establish whether radiation has a similar effect on muscles that are not already undergoing these dynamic processes. We therefore compared two strains of nonmyopathic, immunodeficient mice to the mdx nu/nu host mouse as hosts for myoblast transplantation. The right legs of 3-wk-old mdx nu/nu (Partridge et al., 1989), beige/nu/Xid (Zietman et al., 1991), or C5-/ chaindeficient/Rag2- (Goldman et al., 1998; Mazurier et al., 1999; Cooper et al., 2001) mice were irradiated with either 18, 9, or 4.5 Gy at a dose rate of 0.7 Gy/min (Gross et al., 1999). Control host mice had neither leg irradiated. 3, 28, or 100 d after irradiation, mice were anaesthetized either as before or with isofluorane, and cell pellets were injected with a Hamilton syringe, via a small skin incision, into the TA muscles of the left and right legs (Partridge et al., 1989).
For serial transplant of C2 C12derived tumors, 5 x 105 C2 C12 cells were implanted into TA muscles of two mdx nu/nu hosts that had been preirradiated with 18 Gy. 3 wk later, the mice were killed and equal-sized pieces of tumor were excised from the TA muscles. These were implanted into a slit made in TA muscles of both legs of a fresh set of mdx nu/nu mice whose right legs had been irradiated with 18 Gy 3 d earlier.
Analysis of muscles
In mdx host mice, dystrophin may be used as a marker for muscle of donor origin. To enable us to identify muscle of donor origin in normal hosts, we marked the donor cells with a retrovirus expressing cytoplasmic-localizing LacZ. To validate this marker, we had to establish whether dystrophin and ß-gal expression concurred in mdx nu/nu host muscles that had been injected with retrovirally marked donor cells.
Muscles injected with H2K 18.30 cells were removed for analysis 5 wk after cell implantation. Muscles injected with C2 C12 cells were removed for analysis 3 wk after cell implantation. This earlier time point was chosen for the latter experiment because tumors had formed in the irradiated legs by this time. Where myogenic cells had been injected into mdx hosts, the number of dystrophin-positive fibers in a representative cryostat section was counted (Morgan et al., 1993). Where donor cells were expressing LacZ, the number of fibers expressing LacZ was counted (Gross and Morgan, 1999).
The amount of tumor was calculated by estimating (from a random spot sample) the percentage of a representative cross section that was occupied by undifferentiated interstitial cells (Curtis, 1960).
To determine whether estimates of donor muscle achieved by counting the number of donor muscle fibers in a representative cross section tallied with measurements of the amount of donor DNA and ß-gal activity present in a sample of a homogenate of the entire muscle, TA muscles from six female mice that had been injected with H2K 18.30 cells were removed and homogenized in 2 ml of DME. DNA was prepared from the entire muscle and the amount of male DNA was quantified by slot blotting (Beauchamp et al., 1999). In another experiment, TA muscles from seven female mice that had been injected with H2K 18.30 cells were removed, homogenized in DME, and an aliquot was taken for ß-gal assay (Guerette et al., 1997). Mean values were compared by the Mann-Whitney test.
Growth factor and MMP expression in irradiated and nonirradiated muscle
A number of candidate factors involved in myoblast proliferation and/or migration were compared between irradiated and nonirradiated muscle by Western blot analysis. Both legs of 3-wk-old mdx and wild-type C57Bl/10 mice were irradiated with 18 Gy. Nonirradiated littermate mdx and C57Bl/10 mice were used as controls. 3 d after irradiation, muscles were removed, snap frozen in liquid nitrogen, and prepared for SDS-PAGE and Western blotting. In brief, muscles from four to five mice were pooled, homogenized in 650 µl of 250 mM Tris HCl, 10 mM EDTA, pH 7.4, and fractionated (210 µg of protein per lane) on 412% Tris-glycine SDS-PAGE gels (Invitrogen). Separated proteins were electroblotted onto Hybond C+ extra nitrocellulose membranes (Amersham Pharmacia Biotech), and the membranes were stained with Ponceau red (Sigma-Aldrich) before blocking by incubation in 5.0% nonfat milk in PBS. After blocking, antibodies (15 µg per ml) against the following proteins were used to detect expression: hepatocyte growth factor (Cambio); ß-FGF, FGF-4, and FGF-6 (R&D Systems); and MMP-2 and MMP-9 (Oncogene Research Products). Primary antibodies were detected using biotinylated species-specific secondary antibodies followed by the ABC system (Vector Laboratories). Protein components were visualized using the ECL system (Amersham Pharmacia Biotech) followed by exposure of the stained membrane to X-ray film (Eastman Kodak Co.). Protein levels were determined by scanning densitometry using the Grab-it software (UVP). Values presented are representative of three experiments and the expression levels are given relative to that of ß-actin (Sigma-Aldrich) as loading control.
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Footnotes |
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Acknowledgments |
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This work was supported by the Medical Research Council, the Arthritis Research Campaign (D.J. Abraham), the Raynaud's and Scleroderma Association (X. Shiwen), the Duchenne Parents Group (The Netherlands) (I.B. Fisher), and EC Framework 5 (grants QL K3-CT-1999-00020 and QL K6-CT-1999-02034.
Submitted: 9 August 2001
Revised: 28 March 2002
Accepted: 2 April 2002
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References |
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Adam, M.A., N. Ramesh, A.D. Miller, and W.A. Osborne. 1991. Internal initiation of translation in retroviral vectors carrying picornavirus 5' non-translated regions. J. Virol. 65:49854990.[Medline]
Barcellos-Hoff, M.H., and S.A. Ravani. 2000. Irradiated mammary gland stroma promotes the expression of tumorigenic potential by unirradiated epithelial cells. Cancer Res. 60:12541260.
Beauchamp, J.R., J.E. Morgan, C.N. Pagel, and T.A. Partridge. 1999. Dynamics of myoblast transplantation reveal a discrete minority of precursors with stem celllike properties as the myogenic source. J. Cell Biol. 144:1131121.
Beauchamp, J.R., L. Heslop, D.S.W. Yu, S. Tajbakhsh, R.G. Kelly, A. Wernig, M.E. Buckingham, T.A. Partridge, and P.S. Zammit. 2000. Expression of CD34 and Myf5 defines the majority of quiescent adult skeletal muscle satellite cells. J. Cell Biol. 151:12211233.
Blau, H.M., C.P. Chiu, and C. Webster. 1983. Cytoplasmic activation of human nuclear genes in stable heterocaryons. Cell. 32:11711180.[Medline]
Canaday, D., P. Li, R. Weichselbaum, R.D. Astumian, and R.C. Lee. 1994. Membrane permeability changes in gamma-irradiated muscle cells. Ann. NY Acad. Sci. 720:153159.[Medline]
Curtis, A.S.G. 1960. Area and volume measurements by random sampling methods. Med. Biol. Illustr. 10:261266.
Desgranges, P., C. Barbaud, J.-P. Caruelle, D. Barritault, and J. Gautron. 1999. A substituted dextran enhances muscle fiber survival and regeneration in ischemic and denervated rat EDL muscle. FASEB J. 13:761766.
El Fahime, E., Y. Torrente, N.J. Carron, M.D. Bresolin, and J.P. Tremblay. 2000. In vivo migration of transplanted myoblasts requires matrix metalloproteinase activity. Exp. Cell Res. 258:279287.[CrossRef][Medline]
Ferrari, G., G. Cusella-De Angelis, M. Coletta, E. Paolucci, A. Stornaiuolo, G. Cossu, and F. Mavilio. 1998. Muscle regeneration by bone marrow-derived myogenic progenitors. Science. 279:15281530.
Goldman, J.P., M.P. Blundell, L. Lopes, C. Kinnon, J.P. Di Santo, and A.J. Thrasher. 1998. Enhanced human cell engraftment in mice deficient in RAG2 and the common cytokine receptor gamma chain. Br. J. Haematol. 103:335342.[CrossRef][Medline]
Gorski, D.H., M.A. Beckett, N.T. Jaskowiak, D.P. Calvin, H.J. Mauceri, R.M. Salloum, S. Seetharam, A. Koons, D.M. Hari, D.W. Kufe, and R.R. Weichselbaum. 1999. Blockage of the vascular endothelial growth factor stress response increases the antitumor effects of ionizing radiation. Cancer Res. 59:33743378.
Gross, J.G., G. Bou-Gharios, and J.E. Morgan. 1999. Potentiation of myoblast transplantation by host muscle irradiation is dependent on the rate of radiation delivery. Cell Tissue Res. 298:371375.[CrossRef][Medline]
Gussoni, E., Y. Soneoka, C.D. Strickland, E.A. Buzney, M.K. Khan, A.F. Flint, L.M. Kunkel, and R.C. Mulligan. 1999. Dystrophin expression in the mdx mouse restored by stem cell transplantation. Nature. 401:390394.[CrossRef][Medline]
Hamamori, Y., B. Samal, J. Tian, and L. Kedes. 1995. Myoblast transfer of human erythropoietin gene in a mouse model of renal failure. J. Clin. Invest. 95:18081813.[Medline]
Heslop, L., J.E. Morgan, and T.A. Partridge. 2000. Evidence for a myogenic stem cell that is exhausted in dystrophic muscle. J. Cell Sci. 113:22992308.
Hundt, W., R. Braunschweig, and M. Reiser. 1999. Diffuse metastatic infiltration of a carcinoma into skeletal muscle. Eur. Radiol. 9:208210.[CrossRef][Medline]
Illmensee, K., and B. Mintz. 1976. Totipotency and normal differentiation of single teratocarcinoma cells cloned by injection into blastocysts. Proc. Natl. Acad. Sci. USA. 73:549593.[Abstract]
Jat, P.S., M.D. Noble, P. Ataliotis, Y. Tanaka, N. Yannoutsos, L. Larsen, and D. Kioussis. 1991. Direct derivation of conditionally immortal cell lines from an H-2Kb-tsA58 transgenic mouse. Proc. Natl. Acad. Sci. USA. 85:50965100.
Kastner, S., M.C. Elias, A.J. Rivera, and Z. Yablonka-Reuveni. 2000. Gene expression patterns of the fibroblast growth factors and their receptors during myogenesis of rat satellite cells. J. Histochem. Cytochem. 48:10791096.
Kruse, J.J., C.I. Bart, A. Visser, and J. Wondergem. 1999. Changes in transforming growth factor-beta (TGF-beta 1), procollagen types I and II mRNA in the rat heart after irradiation. Int. J. Radiat. Biol. 75:14291436.[CrossRef][Medline]
Mazurier, F., A. Fontanellas, S. Salesse, L. Taine, S. Landriau, F. Moreau-Gaudry, J. Reiffers, B. Peault, J.P. Di Santo, and H. de Verneuil. 1999. A novel immunodeficient mouse modelRAG2 x common cytokine receptor gamma chain double mutantsrequiring exogenous cytokine administration for human hematopoietic stem cell engraftment. J. Interferon Cytokine Res. 19:533541.[CrossRef][Medline]
Mintz, B., and K. Illmensee. 1975. Normal genetically mosaic mice produced from malignant teratocarcinoma cells. Proc. Natl. Acad. Sci. USA. 72:35853589.[Abstract]
Morgan, J.E., S.E. Moore, F.S. Walsh, and T.A. Partridge. 1992. Formation of skeletal muscle in vivo from the mouse C2 cell line. J. Cell Sci. 102:779787.[Abstract]
Morgan, J.E., J.R. Beauchamp, C.N. Pagel, M. Peckham, P. Ataliotis, P.S. Jat, M.D. Noble, K. Farmer, and T.A. Partridge. 1994. Myogenic cell-lines derived from transgenic mice carrying a thermolabile T-antigen: a model system for the derivation of tissue-specific and mutation-specific cell-lines. Dev. Biol. 162:486498.[CrossRef][Medline]
Orlic, D., J. Kajstura, S. Chimenti, I. Jakoniuk, S.M. Anderson, B. Li, J. Pickel, R. McKay, B. Nadal-Ginard, D.M. Bodine, et al. 2001. Bone marrow cells regenerate infarcted myocardium. Nature. 410:701705.[CrossRef][Medline]
Pagel, C.N., and T.A. Partridge. 1999. Covert persistence of mdx mouse myopathy is revealed by acute and chronic effects of irradiation. J. Neurol. Sci. 164:103116.[CrossRef][Medline]
Park, C.C., M.J. Bissell, and M.H. Barcellos-Hoff. 2000. The influence of the microenvironment on the malignant phenotyope. Mol. Med. Today. 6:324329.[CrossRef][Medline]
Peter, R.U., A. Beetz, C. Ried, G. Michel, D. van Beuningen, and T. Ruzicka. 1993. Increased expression of the epidermal growth factor receptor in human epidermal keratinocytes after exposure to ionizing radiation. Radiat. Res. 136:6570.[Medline]
Quinlan, J.G., D. Cambier, S. Lyden, A. Dalvi, R.K. Upputure, P. Gartside, S.E. Michaels, and D. Denman. 1997. Regeneration-blocked mdx muscle: in vivo model for testing treatments. Muscle Nerve. 20:10161023.[CrossRef][Medline]
Revesz, L. 1958. Effect of lethally damaged tumor cells upon the development of ad-mixed viable cells. J. Natl. Cancer Inst. 20:11571186.[Medline]
Schultz, E. 1996. Satellite cell proliferative compartments in growing skeletal muscles. Dev. Biol. 175:8494.[CrossRef][Medline]
Visted, T., J. Thorsen, F. Thorsen, T.A. Read, E. Ulvestad, O. Engebraaten, D. Sorensen, S. Yla-Herttuala, K. Tyynela, G. Rucklidge, et al. 2000. LacZ-neoR transfected glioma cells in syngeneic rats: growth pattern and characterization of the host immune response against cells transplanted inside and outside the CNS. Int. J. Cancer. 85:228235.[CrossRef][Medline]
Wang, J.L., Y. Sun, and S. Wu. 2000. Gamma-irradiation induces matrix metalloproteinase II expression in a p53-dependent manner. Mol. Carcinog. 27:252258.[CrossRef][Medline]
Weller, B., G. Karpati, S. Lehnert, S. Carpenter, B. Ajdukovic, and P. Holland. 1991. Inhibition of myosatellite cell proliferation by gamma irradiation does not prevent the age-related increase of the number of dystrophin-positive fibers in soleus muscles of mdx female heterozygote mice. Am. J. Pathol. 138:14971502.[Abstract]
Yaffe, D., and O. Saxel. 1977. Serial passaging and differentiation of myogenic cells isolated from dystrophic mouse muscle. Nature. 270:725727.[Medline]
Yao, S.N., and K. Kurachi. 1993. Implanted myoblasts not only fuse with myofibers but also survive as muscle precursor cells. J. Cell Sci. 105:957963.
Yoshida, N., S. Yoshida, K. Koishi, K. Masuda, and Y. Nabeshima. 1998. Cell heterogeneity upon myogenic differentiation: down-regulation of MyoD and Myf-5 generates reserve cells. J. Cell Sci. 111:769779.