Acute and chronic effects of bupivacaine on muscle energetics during contraction in vivo: a modular metabolic control analysis

Author:

Arsac Laurent M.12,Nouette-Gaulain Karine34,Miraux Sylvain12,Deschodt-Arsac Veronique56,Rossignol Rodrigue3,Thiaudiere Eric12,Diolez Philippe56

Affiliation:

1. Centre de Résonance Magnétique des Systèmes Biologiques, Université Bordeaux, UMR 5536, F-33000 Bordeaux, France

2. Centre de Résonance Magnétique des Systèmes Biologiques, Centre National de la Recherche Scientifique, UMR 5536, F-33000 Bordeaux, France

3. Maladies Rares: Génétique et Métabolisme (MRGM), Université Bordeaux, EA 4576, F-33000 Bordeaux, France

4. Service Anesthésie Réanimation, Centre Hospitalier Universitaire de Bordeaux, F-33404 Bordeaux, France

5. Centre de Recherche Cardio-Thoracique de Bordeaux, Université Bordeaux, U1045, F-33000 Bordeaux, France

6. INSERM, Centre de Recherche Cardio-Thoracique de Bordeaux, U1045, F-33000 Bordeaux, France

Abstract

Bupivacaine is a widely used anaesthetic injected locally in clinical practice for short-term neurotransmission blockade. However, persistent side effects on mitochondrial integrity have been demonstrated in muscle parts surrounding the injection site. We use the precise language of metabolic control analysis in the present study to describe in vivo consequences of bupivacaine injection on muscle energetics during contraction. We define a model system of muscle energy metabolism in rats with a sciatic nerve catheter that consists of two modules of reactions, ATP/PCr (phosphocreatine) supply and ATP/PCr demand, linked by the common intermediate PCr detected in vivo by 31P-MRS (magnetic resonance spectroscopy). Measured system variables were [PCr] (intermediate) and contraction (flux). We first applied regulation analysis to quantify acute effects of bupivacaine. After bupivacaine injection, contraction decreased by 15.7% and, concomitantly, [PCr] increased by 11.2%. The regulation analysis quantified that demand was in fact directly inhibited by bupivacaine (−21.3%), causing an increase in PCr. This increase in PCr indirectly reduced mitochondrial activity (−22.4%). Globally, the decrease in contractions was almost fully explained by inhibition of demand (−17.0%) without significant effect through energy supply. Finally we applied elasticity analysis to quantify chronic effects of bupivacaine iterative injections. The absence of a difference in elasticities obtained in treated rats when compared with healthy control rats clearly shows the absence of dysfunction in energetic control of muscle contraction energetics. The present study constitutes the first and direct evidence that bupivacaine myotoxicity is compromised by other factors during contraction in vivo, and illustrates the interest of modular approaches to appreciate simple rules governing bioenergetic systems when affected by drugs.

Publisher

Portland Press Ltd.

Subject

Cell Biology,Molecular Biology,Biochemistry

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