Abstract

Muscle satellite cells are the most studied cells in skeletal muscle. They fulfill many of the requirements of tissue-specific stem cells, including the ability to self-renew and to differentiate into multiple cell types. In addition to satellite cells, other myogenic progenitors have been isolated from both human and mouse skeletal muscle. These 'alternative'myogenic progenitors are distinct from satellite cells and many appear associated to the microvasculature or in the interstitial spaces between myofibers. One of these 'alternative'myogenic cell populations is the so-called 'side population'(SP). Our studies in human muscle have proposed that SP cells secrete factors (such as BMP4) that induce the proliferation of myogenic progenitors expressing receptors for these factors (BMP-receptor 1a, BMPR1a). In the current application, we will elucidate the ties between human muscle SP cells and BMPR1a+ progenitors, study whether forced expression of BMPR1a in muscle SP cells leads to their activation and commitment to the myogenic lineage, investigate if loss of BMPR1a+ expression in skeletal muscle progenitors expressing Myf5 or Pax3 will lead to muscle pathology, and determine in a mouse model whether muscle SP cells or BMPR1a+ progenitors are 'stem'-like cells with intrinsic high-replicative capacity.
The Specific Aims of these studies, which involve both human and mouse cells, are:
Aim 1 : Determine if human muscle SP cells are 'ancestors'of BMPR1a+ myogenic progenitors;
Aim 2 : Assess if forced expression of BMPR1a in human muscle SP cells is necessary and sufficient to induce their proliferation and specification towards the myogenic lineage;
Aim 3 : Investigate if BMPR1a+Myf5+ or BMPR1a+Pax3+ progenitors are important for muscle development and participate in muscle regeneration in post-natal life;
Aim 4 : Use the m-TERT GFP model to identify telomerase-expressing cells in skeletal muscle and determine their relationship to muscle SP, BMPR1a+ cells or other muscle 'stem'cells. These studies will unveil the function of BMPR1a expression in muscle progenitors and unravel the relationship between human muscle SP and BMPR1a-expressing cells. Mouse and human studies will synergize with one another, to define the significance and importance of each myogenic cell population in both species.

Public Health Relevance

Skeletal muscle is a tissue composed of large mature muscle cells that are non-dividing (myofibers) and of mononuclear cells, which have the ability to divide and form new muscle. In recent years, it has become clear that the mononuclear cells in muscle are not homogeneous. These heterogeneous mononuclear cells may also communicate with one another by using special signals that trigger their ability to divide or to become mature muscle. In the present application we will study the ties between stem-like cells and other myogenic progenitors in human muscle. We will define whether some of these mononuclear cells are ancestors of others, and determine if cells that have long-replicative capacity can be isolated prospectively from human and mouse muscles. The broad objective of these studies is to be able to identify and select 'stem'cells in human muscle that may be useful for therapy of muscle disorders.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
5R01NS047727-07
Application #
8044803
Study Section
Special Emphasis Panel (ZRG1-MOSS-H (04))
Program Officer
Porter, John D
Project Start
2003-12-01
Project End
2014-04-30
Budget Start
2011-05-01
Budget End
2012-04-30
Support Year
7
Fiscal Year
2011
Total Cost
$371,226
Indirect Cost

  Institution

Name
Children's Hospital Boston
Department
Type
DUNS #
076593722
City
Boston
State
MA
Country
United States
Zip Code
02115

  Publications

Robin, Jerome D; Wright, Woody E; Zou, Yaqun et al. (2015) Isolation and immortalization of patient-derived cell lines from muscle biopsy for disease modeling. J Vis Exp :52307
Huang, Ping; Schulz, Tim J; Beauvais, Ariane et al. (2014) Intramuscular adipogenesis is inhibited by myo-endothelial progenitors with functioning Bmpr1a signalling. Nat Commun 5:4063
Rozkalne, Anete; Adkin, Carl; Meng, Jinhong et al. (2014) Mouse regenerating myofibers detected as false-positive donor myofibers with anti-human spectrin. Hum Gene Ther 25:73-81
Wu, Melissa P; Doyle, Jamie R; Barry, Brenda et al. (2013) G-protein coupled receptor 56 promotes myoblast fusion through serum response factor- and nuclear factor of activated T-cell-mediated signalling but is not essential for muscle development in vivo. FEBS J 280:6097-113
Schulz, Tim J; Huang, Ping; Huang, Tian Lian et al. (2013) Brown-fat paucity due to impaired BMP signalling induces compensatory browning of white fat. Nature 495:379-83
Liadaki, Kalliopi; Casar, Juan Carlos; Wessen, McKenzie et al. (2012) ?4 integrin marks interstitial myogenic progenitor cells in adult murine skeletal muscle. J Histochem Cytochem 60:31-44
Lapan, Ariya D; Gussoni, Emanuela (2012) Isolation and characterization of human fetal myoblasts. Methods Mol Biol 798:3-19
Lapan, Ariya D; Rozkalne, Anete; Gussoni, Emanuela (2012) Human fetal skeletal muscle contains a myogenic side population that expresses the melanoma cell-adhesion molecule. Hum Mol Genet 21:3668-80
Lawlor, Michael W; Alexander, Matthew S; Viola, Marissa G et al. (2012) Myotubularin-deficient myoblasts display increased apoptosis, delayed proliferation, and poor cell engraftment. Am J Pathol 181:961-8
Wu, Melissa P; Gussoni, Emanuela (2011) Carbamylated erythropoietin does not alleviate signs of dystrophy in mdx mice. Muscle Nerve 43:88-93

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