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SERCA-1 conformational change exerted by the Ca-channel blocker diltiazem affects mammalian skeletal muscle function.

作者信息

Jiménez-Garduño Aura, Ramirez-Soto Ibrahim, Miranda-Rodríguez Ileana, Gitler Sofía, Ortega Alicia

机构信息

Department of Biochemistry, Facultad de Medicina, School of Medicine, Universidad Nacional Autónoma de México, México City, Mexico; Department of Health Sciences, Universidad de las Américas Puebla, San Andrés Cholula, Puebla, Mexico.

Department of Biochemistry, Facultad de Medicina, School of Medicine, Universidad Nacional Autónoma de México, México City, Mexico; Department of Kinesiology and Health Sciences, University of Waterloo, Ontario, Canada.

出版信息

Cell Calcium. 2024 May;119:102852. doi: 10.1016/j.ceca.2024.102852. Epub 2024 Feb 8.

DOI:10.1016/j.ceca.2024.102852
PMID:38412581
Abstract

In skeletal muscle (SM), inward Ca-currents have no apparent role in excitation-contraction coupling (e-c coupling), however the Ca-channel blocker can affect twitch and tetanic muscle in mammalian SM. Experiments were conducted to study how diltiazem (DLZ) facilitates e-c coupling and inhibits contraction. 1) In complete Extensor Digitorum Longus (EDL) muscle and single intact fibres, 0.03 mM DLZ causes twitch potentiation and decreases force during tetanic activity, with increased fatigue. 2) In split open fibres isolated from EDL fibres, DLZ inhibits sarcoplasmic reticulum (SR) Ca-loading in a dose-dependent manner and has a potentiating effect on caffeine-induced SR Ca-release. 3) In isolated light SR (LSR) vesicles, SERCA1 hydrolytic activity is not affected by DLZ up to 0.2 mM. However, ATP-dependent Ca-uptake was inhibited in a dose-dependent manner at a concentration where e-c coupling is changed. 4) The passive Ca-efflux from LSR was reduced by half with 0.03 mM diltiazem, indicating that SR leaking does not account for the decreased Ca-uptake. 5) The denaturation profile of the SERCA Ca-binding domain has lower thermal stability in the presence of DLZ in a concentration-dependent manner, having no effect on the nucleotide-binding domain. We conclude that the effect of DLZ on SM is exerted by crossing the sarcolemma and interacting directly with the SERCA Ca-binding domain, affecting SR Ca-loading during relaxation, which has a consequence on SM contractility. Diltiazem effect on SM could be utilized as a tool to understand SM e-c coupling and muscle fatigue.

摘要

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