Time-lapse imaging of In Vitro myogenesis using atomic force microscopy |
| |
| Authors: | B STÄDLER† T M BLÄTTLER‡ & A FRANCO-OBREGÓN |
| |
| Affiliation: | Laboratory of Biosensors and Bioelectronics, Mechanobiology Laboratory, Institute for Biomedical Engineering, ETH Zurich, Switzerland;Centre for Nanoscience and Nanotechnology, Department of Chemical &Biomolecular Engineering, The University of Melbourne, Australia;Laboratory for Surface Science and Technology, Department of Materials, ETH Zurich, Switzerland |
| |
| Abstract: | Myoblast therapy relies on the integration of skeletal muscle stem cells into distinct muscular compartments for the prevention of clinical conditions such as heart failure, or bladder dysfunction. Understanding the fundamentals of myogenesis is hence crucial for the success of these potential medical therapies. In this report, we followed the rearrangement of the surface membrane structure and the actin cytoskeletal organization in C2C12 myoblasts at different stages of myogenesis using atomic force microscopy (AFM) and confocal laser scanning microscopy (CLSM). AFM imaging of living myoblasts undergoing fusion unveiled that within minutes of making cell–cell contact, membrane tubules appear that unite the myoblasts and increase in girth as fusion proceeds. CLSM identified these membrane tubules as built on scaffolds of actin filaments that nucleate at points of contact between fusing myoblasts. In contrast, similarly behaving membrane tubules are absent during cytokinesis. The results from our study in combination with recent findings in literature further expand the understanding of the biochemical and membrane structural rearrangements involved in the two fundamental cellular processes of division and fusion. |
| |
| Keywords: | Atomic force microscopy actin cell fusion confocal laser scanning microscopy myogenesis |
|
|
