Literature DB >> 25992329

Barriers in contribution of human mesenchymal stem cells to murine muscle regeneration.

Anabel S de la Garza-Rodea1, Hester Boersma1, Cheryl Dambrot1, Antoine Af de Vries1, Dirk W van Bekkum1, Shoshan Knaän-Shanzer1.   

Abstract

AIM: To study regeneration of damaged human and murine muscle implants and the contribution of added xenogeneic mesenchymal stem cells (MSCs).
METHODS: Minced human or mouse skeletal muscle tissues were implanted together with human or mouse MSCs subcutaneously on the back of non-obese diabetic/severe combined immunodeficient mice. The muscle tissues (both human and murine) were minced with scalpels into small pieces (< 1 mm(3)) and aliquoted in portions of 200 mm(3). These portions were either cryopreserved in 10% dimethylsulfoxide or freshly implanted. Syngeneic or xenogeneic MSCs were added to the minced muscles directly before implantation. Implants were collected at 7, 14, 30 or 45 d after transplantation and processed for (immuno)histological analysis. The progression of muscle regeneration was assessed using a standard histological staining (hematoxylin-phloxin-saffron). Antibodies recognizing Pax7 and von Willebrand factor were used to detect the presence of satellite cells and blood vessels, respectively. To enable detection of the bone marrow-derived MSCs or their derivatives we used MSCs previously transduced with lentiviral vectors expressing a cytoplasmic LacZ gene. X-gal staining of the fixed tissues was used to detect β-galactosidase-positive cells and myofibers.
RESULTS: Myoregeneration in implants of fresh murine muscle was evident as early as day 7, and progressed with time to occupy 50% to 70% of the implants. Regeneration of fresh human muscle was slower. These observations of fresh muscle implants were in contrast to the regeneration of cryopreserved murine muscle that proceeded similarly to that of fresh tissue except for day 45 (P < 0.05). Cryopreserved human muscle showed minimal regeneration, suggesting that the freezing procedure was detrimental to human satellite cells. In fresh and cryopreserved mouse muscle supplemented with LacZ-tagged mouse MSCs, β-galactosidase-positive myofibers were identified early after grafting at the well-vascularized periphery of the implants. The contribution of human MSCs to murine myofiber formation was, however, restricted to the cryopreserved mouse muscle implants. This suggests that fresh murine muscle tissue provides a suboptimal environment for maintenance of human MSCs. A detailed analysis of the histological sections of the various muscle implants revealed the presence of cellular structures with a deviating morphology. Additional stainings with alizarin red and alcian blue showed myofiber calcification in 50 of 66 human muscle implants, and encapsulated cartilage in 10 of 81 of murine muscle implants, respectively.
CONCLUSION: In mouse models the engagement of human MSCs in myoregeneration might be underestimated. Furthermore, our model permits the dissection of species-specific factors in the microenvironment.

Entities:  

Keywords:  Mesenchymal stem cells; Muscle implants; Muscle regeneration; Satellite cells; Skeletal muscle

Year:  2015        PMID: 25992329      PMCID: PMC4436938          DOI: 10.5493/wjem.v5.i2.140

Source DB:  PubMed          Journal:  World J Exp Med        ISSN: 2220-315X


  25 in total

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Journal:  Hum Gene Ther       Date:  2010-09       Impact factor: 5.695

2.  Endowing human adenovirus serotype 5 vectors with fiber domains of species B greatly enhances gene transfer into human mesenchymal stem cells.

Authors:  Shoshan Knaän-Shanzer; Marloes J M van de Watering; Ietje van der Velde; Manuel A F V Gonçalves; Dinko Valerio; Antoine A F de Vries
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Journal:  J Biol Chem       Date:  2005-11-02       Impact factor: 5.157

4.  Exercise improves the success of myoblast transplantation in mdx mice.

Authors:  Manaf Bouchentouf; Basma F Benabdallah; Philippe Mills; Jacques P Tremblay
Journal:  Neuromuscul Disord       Date:  2006-08-21       Impact factor: 4.296

5.  Mesenchymal stem cells: revisiting history, concepts, and assays.

Authors:  Paolo Bianco; Pamela Gehron Robey; Paul J Simmons
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6.  Growth of skeletal muscle from patients with amyotrophic lateral sclerosis transplanted into nude mice.

Authors:  A K Gulati; M H Rivner; M Shamsnia; T R Swift; G S Sohal
Journal:  Muscle Nerve       Date:  1988-01       Impact factor: 3.217

7.  In vivo visualization of the origination of skin graft vasculature in a wild-type/GFP crossover model.

Authors:  Maurizio Calcagni; Martina K Althaus; Alicia D Knapik; Niels Hegland; Claudio Contaldo; Pietro Giovanoli; Nicole Lindenblatt
Journal:  Microvasc Res       Date:  2011-07-20       Impact factor: 3.514

8.  Isoenzyme studies of whole muscle grafts and movement of muscle precursor cells.

Authors:  M D Grounds; T A Partridge
Journal:  Cell Tissue Res       Date:  1983       Impact factor: 5.249

9.  Highly efficient, functional engraftment of skeletal muscle stem cells in dystrophic muscles.

Authors:  Massimiliano Cerletti; Sara Jurga; Carol A Witczak; Michael F Hirshman; Jennifer L Shadrach; Laurie J Goodyear; Amy J Wagers
Journal:  Cell       Date:  2008-07-11       Impact factor: 41.582

10.  Pericytes of human skeletal muscle are myogenic precursors distinct from satellite cells.

Authors:  Arianna Dellavalle; Maurilio Sampaolesi; Rossana Tonlorenzi; Enrico Tagliafico; Benedetto Sacchetti; Laura Perani; Anna Innocenzi; Beatriz G Galvez; Graziella Messina; Roberta Morosetti; Sheng Li; Marzia Belicchi; Giuseppe Peretti; Jeffrey S Chamberlain; Woodring E Wright; Yvan Torrente; Stefano Ferrari; Paolo Bianco; Giulio Cossu
Journal:  Nat Cell Biol       Date:  2007-02-11       Impact factor: 28.824

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1.  Effect of Stem Cells, Ascorbic Acid and SERCA1a Gene Transfected Stem Cells in Experimentally Induced Type I Diabetic Myopathy.

Authors:  Maha B Zickri; Eman M Sadek; Amal E Fares; Nehal G Heteba; Ahmed M Reda
Journal:  Int J Stem Cells       Date:  2020-03-30       Impact factor: 2.500

  1 in total

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