Pathways of Ca²⁺ entry and cytoskeletal damage following eccentric contractions in mouse skeletal muscle

Muscles that are stretched during contraction (eccentric contractions) show deficits in force production and a variety of structural changes, including loss of antibody staining of cytoskeletal proteins. Extracellular Ca(2+) entry and activation of calpains have been proposed as mechanisms involved...

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Bibliographic Details
Published in:Journal of applied physiology (1985) 2012-06, Vol.112 (12), p.2077-2086
Main Authors: Zhang, Bao-Ting, Whitehead, Nicholas P, Gervasio, Othon L, Reardon, Trent F, Vale, Molly, Fatkin, Diane, Dietrich, Alexander, Yeung, Ella W, Allen, David G
Format: Article
Language:English
Subjects:
Animals
Calcium - metabolism
Calpain - metabolism
Connectin
Cytoskeletal Proteins - metabolism
Cytoskeleton - metabolism
Cytoskeleton - physiology
Male
Mice
Mice, Inbred BALB C
Mice, Inbred C57BL
Mice, Knockout
Muscle Contraction - physiology
Muscle Proteins - metabolism
Muscle, Skeletal - metabolism
Muscle, Skeletal - physiology
Protein Kinases - metabolism
Proteolysis
TRPC Cation Channels - metabolism
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Summary:Muscles that are stretched during contraction (eccentric contractions) show deficits in force production and a variety of structural changes, including loss of antibody staining of cytoskeletal proteins. Extracellular Ca(2+) entry and activation of calpains have been proposed as mechanisms involved in these changes. The present study used isolated mouse extensor digitorum longus (EDL) muscles subjected to 10 eccentric contractions and monitored force production, immunostaining of cytoskeletal proteins, and resting stiffness. Possible pathways for Ca(2+) entry were tested with streptomycin (200 μM), a blocker of stretch-activated channels, and with muscles from mice deficient in the transient receptor potential canonical 1 gene (TRPC1 KO), a candidate gene for stretch-activated channels. At 30 min after the eccentric contractions, the isometric force was decreased to 75 ± 3% of initial control and this force loss was reduced by streptomycin but not in the TRPC1 KO. Desmin, titin, and dystrophin all showed patchy loss of immunostaining 30 min after the eccentric contractions, which was substantially reduced by streptomycin and in the TRPC1 KO muscles. Muscles showed a reduction of resting stiffness following eccentric contractions, and this reduction was eliminated by streptomycin and absent in the TRPC1 KO muscles. Calpain activation was determined by the appearance of a lower molecular weight autolysis product and μ-calpain was activated at 30 min, whereas the muscle-specific calpain-3 was not. To test whether the loss of stiffness was caused by titin cleavage, protein gels were used but no significant titin cleavage was detected. These results suggest that Ca(2+) entry following eccentric contractions is through a stretch-activated channel that is blocked by streptomycin and encoded or modulated by TRPC1.
ISSN:8750-7587
1522-1601
DOI:10.1152/japplphysiol.00770.2011