Literature DB >> 23589853

Direct real-time detection of the actin-activated power stroke within the myosin catalytic domain.

Joseph M Muretta1, Karl J Petersen, David D Thomas.   

Abstract

We have used transient kinetics, nanosecond time-resolved fluorescence resonance energy transfer (FRET), and kinetics simulations to resolve a structural transition in the Dictyostelium myosin II relay helix during the actin-activated power stroke. The relay helix plays a critical role in force generation in myosin, coupling biochemical changes in the ATPase site with the force-transducing rotation of the myosin light-chain domain. Previous research in the absence of actin showed that ATP binding to myosin induces a dynamic equilibrium between a bent prepower stroke state of the relay helix and a straight postpower stroke state, which dominates in the absence of ATP or when ADP is bound. We now ask whether actin binding reverses this transition and if so, how this reversal is coordinated with actin-activated phosphate release. We labeled a Cys-lite Dictyostelium myosin II motor domain with donor and acceptor probes at two engineered Cys residues designed to detect relay helix bending. We then performed transient time-resolved FRET following stopped-flow mixing of actin with labeled myosin, preincubated with ATP. We determined the kinetics of actin-activated phosphate release, using fluorescent phosphate-binding protein. The results show that actin binding to the myosin.ADP.P complex straightens the relay helix before phosphate dissociation. This actin-activated relay helix straightening is reversible, but phosphate irreversibly dissociates from the postpower stroke state, preventing reversal of the power stroke. Thus, relay helix straightening gates phosphate dissociation, whereas phosphate dissociation provides the thermodynamic driving force underlying force production.

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Year:  2013        PMID: 23589853      PMCID: PMC3645529          DOI: 10.1073/pnas.1222257110

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  30 in total

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4.  Kinetics of nucleoside triphosphate cleavage and phosphate release steps by associated rabbit skeletal actomyosin, measured using a novel fluorescent probe for phosphate.

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8.  Direct, real-time measurement of rapid inorganic phosphate release using a novel fluorescent probe and its application to actomyosin subfragment 1 ATPase.

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  31 in total

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6.  A Cardiomyopathy Mutation in the Myosin Essential Light Chain Alters Actomyosin Structure.

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7.  Fluorescence lifetime plate reader: resolution and precision meet high-throughput.

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8.  Irrelevance of the power stroke for the directionality, stopping force, and optimal efficiency of chemically driven molecular machines.

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10.  Direct real-time detection of the structural and biochemical events in the myosin power stroke.

Authors:  Joseph M Muretta; John A Rohde; Daniel O Johnsrud; Sinziana Cornea; David D Thomas
Journal:  Proc Natl Acad Sci U S A       Date:  2015-11-02       Impact factor: 11.205

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