Murine muscle engineered from dermal precursors: an in vitro model for skeletal muscle generation, degeneration and fatty infiltration.

6533b7dbfe1ef96bd1270b9b

RESEARCH PRODUCT

Murine muscle engineered from dermal precursors: an in vitro model for skeletal muscle generation, degeneration and fatty infiltration.

José-carlos Fernández-morales Marcos Maroto Adolfo López De Munain Ana Aiastui Juan Fernando Padín M. Goicoechea José Iñaki ÁLava J. Lacalle José Manuel García-verdugo Patricia García-parra Paula García-belda Ander Izeta Neia Naldaiz-gastesi Antonio G. García

subject

Cellular differentiation Sarcoplasm Muscle Fibers Skeletal Biomedical Engineering Medicine (miscellaneous)Bioengineering Biology Muscle Development Models Biological Article Extracellular matrix Mice Tissue engineering Spheroids Cellular medicine Myocyte Animals Cell Proliferation Tissue Engineering Myogenesis Cell growth Muscles Skeletal muscle Cell Differentiation Dermis Lipids Acetylcholine Biologia experimental Cell biology Extracellular Matrix medicine.anatomical_structure Biochemistry Gene Expression Regulation Female Enginyeria biomèdica Ion Channel Gating Biomarkers

description

Skeletal muscle can be engineered by converting dermal precursors into muscle progenitors and differentiated myocytes. However, the efficiency of muscle development remains relatively low and it is currently unclear if this is due to poor characterization of the myogenic precursors, the protocols used for cell differentiation, or a combination of both. In this study, we characterized myogenic precursors present in murine dermospheres, and evaluated mature myotubes grown in a novel three-dimensional culture system. After 5-7 days of differentiation, we observed isolated, twitching myotubes followed by spontaneous contractions of the entire tissue-engineered muscle construct on an extracellular matrix (ECM). In vitro engineered myofibers expressed canonical muscle markers and exhibited a skeletal (not cardiac) muscle ultrastructure, with numerous striations and the presence of aligned, enlarged mitochondria, intertwined with sarcoplasmic reticula (SR). Engineered myofibers exhibited Na(+)- and Ca(2+)-dependent inward currents upon acetylcholine (ACh) stimulation and tetrodotoxin-sensitive spontaneous action potentials. Moreover, ACh, nicotine, and caffeine elicited cytosolic Ca(2+) transients; fiber contractions coupled to these Ca(2+) transients suggest that Ca(2+) entry is activating calcium-induced calcium release from the SR. Blockade by d-tubocurarine of ACh-elicited inward currents and Ca(2+) transients suggests nicotinic receptor involvement. Interestingly, after 1 month, engineered muscle constructs showed progressive degradation of the myofibers concomitant with fatty infiltration, paralleling the natural course of muscular degeneration. We conclude that mature myofibers may be differentiated on the ECM from myogenic precursor cells present in murine dermospheres, in an in vitro system that mimics some characteristics found in aging and muscular degeneration.

year	journal	country	edition	language
2013-01-01

http://hdl.handle.net/10550/33057