Interaction Between PEVK-Titin and Actin Filaments: Origin of a Viscous Force Component in Cardiac Myofibrils

Interaction Between PEVK-Titin and Actin Filaments: Origin of a Viscous Force Component in Cardiac Myofibrils

The giant muscle protein titin contains a unique sequence, the PEVK domain, the elastic properties of which contribute to the mechanical behavior of relaxed cardiomyocytes. Here, human N2-B–cardiac PEVK was expressed in Escherichia coli and tested—along with recombinant cardiac titin constructs cont...

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Veröffentlicht in:Circulation research 2001-11, Vol.89 (10), p.874-881
Hauptverfasser: Kulke, M, Fujita-Becker, S, Rostkova, E, Neagoe, C, Labeit, D, Manstein, D J, Gautel, M, Linke, W A
Format: Artikel
Sprache:eng
Schlagworte:
Actin Cytoskeleton - metabolism
Amino Acid Motifs - physiology
Animals
Binding, Competitive - physiology
Biological and medical sciences
Biological Assay
Chickens
Connectin
Fundamental and applied biological sciences. Psychology
Heart
Humans
In Vitro Techniques
Macromolecular Substances
Muscle Proteins - genetics
Muscle Proteins - metabolism
Myocardial Contraction - physiology
Myocardium - metabolism
Myofibrils - metabolism
Protein Binding - physiology
Protein Kinases - genetics
Protein Kinases - metabolism
Protein Structure, Tertiary - physiology
Rabbits
Recombinant Proteins - genetics
Recombinant Proteins - metabolism
Sarcomeres - physiology
Stress, Mechanical
Temperature
Vertebrates: cardiovascular system
Viscosity
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Zusammenfassung:The giant muscle protein titin contains a unique sequence, the PEVK domain, the elastic properties of which contribute to the mechanical behavior of relaxed cardiomyocytes. Here, human N2-B–cardiac PEVK was expressed in Escherichia coli and tested—along with recombinant cardiac titin constructs containing immunoglobulin-like or fibronectin-like domains—for a possible interaction with actin filaments. In the actomyosin in vitro motility assay, only the PEVK construct inhibited actin filament sliding over myosin. The slowdown occurred in a concentration-dependent manner and was accompanied by an increase in the number of stationary actin filaments. High [Ca] reversed the PEVK effect. PEVK concentrations ≥10 μg/mL caused actin bundling. Actin-PEVK association was found also in actin fluorescence binding assays without myosin at physiological ionic strength. In cosedimentation assays, PEVK-titin interacted weakly with actin at 0°C, but more strongly at 30°C, suggesting involvement of hydrophobic interactions. To probe the interaction in a more physiological environment, nonactivated cardiac myofibrils were stretched quickly, and force was measured during the subsequent hold period. The observed force decline could be fit with a three-order exponential-decay function, which revealed an initial rapid-decay component (time constant, 4 to 5 ms) making up 30% to 50% of the whole decay amplitude. The rapid, viscous decay component, but not the slower decay components, decreased greatly and immediately on actin extraction with Ca-independent gelsolin fragment, both at physiological sarcomere lengths and beyond actin-myosin overlap. Steady-state passive force dropped only after longer exposure to gelsolin. We conclude that interaction between PEVK-titin and actin occurs in the sarcomere and may cause viscous drag during diastolic stretch of cardiac myofibrils. The interaction could also oppose shortening during contraction.
ISSN:0009-7330
1524-4571
DOI:10.1161/hh2201.099453