Development of the excitation-contraction coupling machinery and its relation to myofibrillogenesis in human iPSC-derived skeletal myocytes

Jeanne Lainé; Gunnar Skoglund; Emmanuel Fournier; Nacira Tabti

doi:10.1186/s13395-017-0147-5

Skeletal Muscle (Jan 2018)

Development of the excitation-contraction coupling machinery and its relation to myofibrillogenesis in human iPSC-derived skeletal myocytes

Jeanne Lainé,
Gunnar Skoglund,
Emmanuel Fournier,
Nacira Tabti

Affiliations

Jeanne Lainé: Département de Physiologie, Faculté de Médecine Pierre & Marie Curie site Pitié-Salpêtrière, UPMC
Gunnar Skoglund: Département de Physiologie, Faculté de Médecine Pierre & Marie Curie site Pitié-Salpêtrière, UPMC
Emmanuel Fournier: Département de Physiologie, Faculté de Médecine Pierre & Marie Curie site Pitié-Salpêtrière, UPMC
Nacira Tabti: Département de Physiologie, Faculté de Médecine Pierre & Marie Curie site Pitié-Salpêtrière, UPMC

DOI: https://doi.org/10.1186/s13395-017-0147-5
Journal volume & issue: Vol. 8, no. 1
pp. 1 – 13

Abstract

Read online

Abstract Background Human induced pluripotent stem cells-derived myogenic progenitors develop functional and ultrastructural features typical of skeletal muscle when differentiated in culture. Besides disease-modeling, such a system can be used to clarify basic aspects of human skeletal muscle development. In the present study, we focus on the development of the excitation-contraction (E-C) coupling, a process that is essential both in muscle physiology and as a tool to differentiate between the skeletal and cardiac muscle. The occurrence and maturation of E-C coupling structures (Sarcoplasmic Reticulum-Transverse Tubule (SR-TT) junctions), key molecular components, and Ca2+ signaling were examined, along with myofibrillogenesis. Methods Pax7+-myogenic progenitors were differentiated in culture, and developmental changes were examined from a few days up to several weeks. Ion channels directly involved in the skeletal muscle E-C coupling (RyR1 and Cav1.1 voltage-gated Ca2+ channels) were labeled using indirect immunofluorescence. Ultrastructural changes of differentiating cells were visualized by transmission electron microscopy. On the functional side, depolarization-induced intracellular Ca2+ transients mediating E-C coupling were recorded using Fura-2 ratiometric Ca2+ imaging, and myocyte contraction was captured by digital photomicrography. Results We show that the E-C coupling machinery occurs and operates within a few days post-differentiation, as soon as the myofilaments align. However, Ca2+ transients become effective in triggering myocyte contraction after 1 week of differentiation, when nascent myofibrils show alternate A-I bands. At later stages, myofibrils become fully organized into adult-like sarcomeres but SR-TT junctions do not reach their triadic structure and typical A-I location. This is mirrored by the absence of cross-striated distribution pattern of both RyR1 and Cav1.1 channels. Conclusions The E-C coupling machinery occurs and operates within the first week of muscle cells differentiation. However, while early development of SR-TT junctions is coordinated with that of nascent myofibrils, their respective maturation is not. Formation of typical triads requires other factors/conditions, and this should be taken into account when using in-vitro models to explore skeletal muscle diseases, especially those affecting E-C coupling.

Published in Skeletal Muscle

ISSN: 2044-5040 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine: Internal medicine: Specialties of internal medicine: Diseases of the musculoskeletal system
Website: https://skeletalmusclejournal.biomedcentral.com

About the journal

Abstract

Keywords