Myogenesis in Adult Mammalian Skeletal Muscle in Vitro

Overview

Journal J Anat

Specialty Anatomy & Histology

Date 1981 Jan 1

PMID 7275784

Citations 8

Authors

A C Nag

J D Foster

Affiliations

Soon will be listed here.

Abstract

An injury to adult mammalian skeletal muscle is followed by regeneration, which involves a process believed to be similar to the differentiation of muscle fibres in the embryo. The origin of these differentiating myogenic cells is conjectural. The aim of the present study was to examine the source of myogenic cells and the process of myogenesis in adult skeletal muscle. Mononucleated cells were released from adult rat leg muscle mince after incubation with 0.1% pronase for 50-60 minutes at 37 degrees C. The ultrastructural studies revealed that the freshly dissociated mononucleated cells consisted of at least two populations of cells: myogenic satellite cells and non-myogenic fibroblastic cells. These cells were plated in growth media at various densities in cell culture dishes and incubated for 3 weeks in a balanced air atmosphere at 37 degrees C. The culture was routinely examined with a phase contrasted microscope for evidence of myogenic activities of the plated cells. At selected time intervals, the cell cultures were processed for autoradiography and scanning and transmission electron microscopy (SEM and TEM). Attachment of cells to the dish began soon after plating, with flattening of some non-muscle cells. The round- to spindle-shaped cells, indicative of myoblasts, began to appear within 24 hours. DNA synthesis and cell proliferation were observed in myogenic and non-myogenic cells within 24 hours of culture. SEM revealed that at 72 hours some myoblasts aligned and fused with one another, forming myotubes. Quantitation of autoradiographs indicated that the maximum number of labelled myotubes were present in the 3 days old culture, and thereafter, the labelled myotubes decreased in number and were absent in the 7 days old culture. Within 5-7 days the myotubes became larger and showed contractility. TEM of 6 to 21 day culture revealed that the myotubes contained well differentiated myofibrils, T-tubules and sarcoplasmic reticulum. It was evident from our studies that the mononucleated cells, having satellite cell morphology, were capable of differentiating into fully formed muscle fibres. This study lends support to the satellite cell hypothesis for regeneration of the skeletal muscle.

Citing Articles

3D Bioprinting and Differentiation of Primary Skeletal Muscle Progenitor Cells.

Ngan C, Quigley A, OConnell C, Kita M, Bourke J, Wallace G Methods Mol Biol. 2020; 2140:229-242.

PMID: 32207116 DOI: 10.1007/978-1-0716-0520-2_15.

Long-Term High-Density Extracellular Recordings Enable Studies of Muscle Cell Physiology.

Lewandowska M, Bogatikov E, Hierlemann A, Punga A Front Physiol. 2018; 9:1424.

PMID: 30356837 PMC: 6190753. DOI: 10.3389/fphys.2018.01424.

On-chip, multisite extracellular and intracellular recordings from primary cultured skeletal myotubes.

Rabieh N, Ojovan S, Shmoel N, Erez H, Maydan E, Spira M Sci Rep. 2016; 6:36498.

PMID: 27812002 PMC: 5095645. DOI: 10.1038/srep36498.

Identification and Characterization of the Dermal Panniculus Carnosus Muscle Stem Cells.

Naldaiz-Gastesi N, Goicoechea M, Alonso-Martin S, Aiastui A, Lopez-Mayorga M, Garcia-Belda P Stem Cell Reports. 2016; 7(3):411-424.

PMID: 27594590 PMC: 5032673. DOI: 10.1016/j.stemcr.2016.08.002.

Muscle fibers from senescent mice retain excitation-contraction coupling properties in culture.

Wang Z, Zheng Z, Messi M, Delbono O In Vitro Cell Dev Biol Anim. 2007; 43(7):222-34.

PMID: 17712595 DOI: 10.1007/s11626-007-9047-z.

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