Myostatin regulates fiber-type composition of skeletal muscle by regulating MEF2 and MyoD gene expression

被引:156
|
作者
Hennebry, Alex [2 ]
Berry, Carole [2 ]
Siriett, Victoria [2 ]
O'Callaghan, Paul [2 ]
Chau, Linda [2 ]
Watson, Trevor [2 ]
Sharma, Mridula [2 ,3 ]
Kambadur, Ravi [1 ,2 ]
机构
[1] Nanyang Technol Univ, Sch Biol Sci, Singapore 639798, Singapore
[2] AgResearch, Funct Muscle Gen, Hamilton, New Zealand
[3] Natl Univ Singapore, Dept Biochem, Singapore 117548, Singapore
来源
关键词
myocyte enhancer factor 2; myosin heavy chain; HEAVY-CHAIN ISOFORMS; TRANSCRIPTION FACTOR; TRANSGENIC MICE; DIFFERENTIATION; ACTIVATION; ENHANCER; PROLIFERATION; TRANSITIONS; MECHANISMS; PATHWAYS;
D O I
10.1152/ajpcell.00259.2007
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Hennebry A, Berry C, Siriett V, O'Callaghan P, Chau L, Watson T, Sharma M, Kambadur R. Myostatin regulates fiber-type composition of skeletal muscle by regulating MEF2 and MyoD gene expression. Am J Physiol Cell Physiol 296: C525-C534, 2009. First published January 7, 2008; doi:10.1152/ajpcell.00259.2007.-Myostatin (Mstn) is a secreted growth factor belonging to the tranforming growth factor (TGF)-beta superfamily. Inactivation of murine Mstn by gene targeting, or natural mutation of bovine or human Mstn, induces the double muscling (DM) phenotype. In DM cattle, Mstn deficiency increases fast glycolytic (type IIB) fiber formation in the biceps femoris (BF) muscle. Using Mstn null ((-/-)) mice, we suggest a possible mechanism behind Mstn-mediated fiber-type diversity. Histological analysis revealed increased type IIB fibers with a concomitant decrease in type IIA and type I fibers in the Mstn(-/-) tibialis anterior and BF muscle. Functional electrical stimulation of Mstn(-/-) BF revealed increased fatigue susceptibility, supporting increased type IIB fiber content. Given the role of myocyte enhancer factor 2 (MEF2) in oxidative type I fiber formation, MEF2 levels in Mstn(-/-) tissue were quantified. Results revealed reduced MEF2C protein in Mstn(-/-) muscle and myoblast nuclear extracts. Reduced MEF2-DNA complex was also observed in electrophoretic mobility-shift assay using Mstn(-/-) nuclear extracts. Furthermore, reduced expression of MEF2 downstream target genes MLC1F and calcineurin were found in Mstn(-/-) muscle. Conversely, Mstn addition was sufficient to directly upregulate MLC promoter-enhancer activity in cultured myoblasts. Since high MyoD levels are seen in fast fibers, we analyzed MyoD levels in the muscle. In contrast to MEF2C, MyoD levels were increased in Mstn(-/-) muscle. Together, these results suggest that while Mstn positively regulates MEF2C levels, it negatively regulates MyoD expression in muscle. We propose that Mstn could regulate fiber-type composition by regulating the expression of MEF2C and MyoD during myogenesis.
引用
收藏
页码:C525 / C534
页数:10
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