Influence of static magnetic fields on human myoblast/mesenchymal stem cell co‑cultures

Mol Med Rep. 2018 Mar;17(3):3813-3820. doi: 10.3892/mmr.2017.8334. Epub 2017 Dec 20.

Abstract

The results of surgical repair of extensive muscle tissue defects are still of primary concern, leaving patients with residual cosmetic and functional impairments. Therefore, skeletal muscle tissue engineering attempts to grow functional neo‑tissue from human stem cells to promote tissue regeneration and support defect closure. Despite intensive research efforts, the goal of stable induction of myogenic differentiation in expanded human stem cells by using clinically feasible stimuli, has not yet been reached to a sufficient extent. Therefore, the present study investigated the differentiation potential of static magnetic fields (SMFs), using co‑cultures of human satellite cells and human mesenchymal stem cells (MSCs). It has previously been demonstrated that SMFs may act as a promising myogenic stimulus. Tests were performed on co‑cultures with and without SMF exposure, using growth medium [high growth factor concentrations (GM)] and differentiation medium [low growth factors concentrations (DM)]. AlamarBlue® assay‑based cell proliferation analysis revealed no significant difference between co‑cultures with, vs. without SMF stimulation, regardless of growth factor concentrations in the cell culture medium. To determine the degree of differentiation in co‑cultures under stimulation with SMFs, semi‑quantitative gene expression measurements of the following marker genes were performed: Desmin, myogenic factor 5, myogenic differentiation antigen 1, myogenin, adult myosin heavy chain 1 and skeletal muscle α1 actin. In neither GM nor DM was a steady, significant increase in marker gene expression detected. Verifying the gene expression findings, immunohistochemical antibody staining against differentiation markers revealed that SMF exposure did not enhance myogenic maturation. Therefore, SMF treatment of human satellite cell/MSC co‑cultures did not result in the desired increase in myogenic differentiation. Further studies are required to identify a suitable stimulus for skeletal muscle tissue engineering.

Keywords: tissue engineering; myoblast; satellite cell; mesenchymal stem cell; static magnetic field; differentiation; co-cultures.

MeSH terms

  • Actins / genetics
  • Actins / metabolism
  • Biomarkers / metabolism
  • Cardiac Myosins / genetics
  • Cardiac Myosins / metabolism
  • Cell Differentiation / radiation effects
  • Cell Proliferation / radiation effects
  • Coculture Techniques
  • Culture Media / chemistry
  • Culture Media / pharmacology
  • Desmin / genetics
  • Desmin / metabolism
  • Gene Expression / radiation effects*
  • Humans
  • Intercellular Signaling Peptides and Proteins / pharmacology
  • Magnetic Fields*
  • Mesenchymal Stem Cells / cytology
  • Mesenchymal Stem Cells / metabolism
  • Mesenchymal Stem Cells / radiation effects*
  • Muscle, Skeletal / cytology
  • Muscle, Skeletal / metabolism
  • Muscle, Skeletal / radiation effects
  • MyoD Protein / genetics
  • MyoD Protein / metabolism
  • Myoblasts / cytology
  • Myoblasts / metabolism
  • Myoblasts / radiation effects*
  • Myogenic Regulatory Factor 5 / genetics
  • Myogenic Regulatory Factor 5 / metabolism
  • Myogenin / genetics
  • Myogenin / metabolism
  • Myosin Heavy Chains / genetics
  • Myosin Heavy Chains / metabolism
  • Primary Cell Culture
  • Tissue Engineering*

Substances

  • Actins
  • Biomarkers
  • Culture Media
  • Desmin
  • Intercellular Signaling Peptides and Proteins
  • MYF5 protein, human
  • MYH7 protein, human
  • MyoD Protein
  • MyoD1 myogenic differentiation protein
  • Myogenic Regulatory Factor 5
  • Myogenin
  • Cardiac Myosins
  • Myosin Heavy Chains