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Single actomyosin motor interactions in skeletal muscle
Authors:Zeno Földes-Papp  Shih-Chu Jeff LiaoBen Barbieri  Karol Gryczynski Jr  Rafal LuchowskiZygmunt Gryczynski  Ignacy GryczynskiJulian Borejdo  Tiefeng You
Institution:
  • a Department of Molecular Biology and Immunology, University of North Texas Health Science Center, 3500 Camp Bowie Boulevard, Fort Worth, TX 76107, USA
  • b ISS, 1602 Newton Drive, Champaign, IL 61822, USA
  • c Medical University of Graz, Department of Internal Medicine, Division of Clinical Angiology, A-8036 Graz, Austria
  • d Department of Physics, University of North Texas, Denton, TX, USA
  • Abstract:We present a study of intramuscular motion during contraction of skeletal muscle myofibrils. Myofibrillar actin was labeled with fluorescent dye so that the ratio of fluorescently labeled to unlabeled protein was 1:105. Such sparse labeling assured that there was on average only one actin-marker present in the focus at a given time. From the intensity signal in the two orthogonal detection channels, significant fluctuations, similar to fluorescent burst in diffusion-based single-molecule detection schemes, were identified via a threshold algorithm and analyzed with respect to their intensity and polarization. When only rigor complexes were formed, the fluctuations of polarized intensity were characterized by unimodal Gaussian photon distributions. During contraction, in contrast, bimodal Gaussian photon distributions were observed above the rigor background threshold. This suggests that the bimodal Gaussian photon distributions represent pre- and post-power stroke conformations. Clusters of polarized photons indicated an anisotropy decay of single actomyosin motors of ~ 9 s during muscle contraction.
    Keywords:Single actomyosin  Live skeletal muscle cell  Polarization dependent fluorescence fluctuations  Time-dependent photon distributions  Molecular orientations
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