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Analysis of flexural rigidity of actin filaments propelled by surface adsorbed myosin motors
Author(s) -
Bengtsson Elina,
Persson Malin,
Månsson Alf
Publication year - 2013
Publication title -
cytoskeleton
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.95
H-Index - 86
eISSN - 1949-3592
pISSN - 1949-3584
DOI - 10.1002/cm.21138
Subject(s) - heavy meromyosin , myosin , protein filament , motility , actin , biophysics , biology , rigidity (electromagnetism) , flexural rigidity , persistence length , cytoskeleton , motor protein , molecular motor , meromyosin , microtubule , anatomy , microbiology and biotechnology , myosin head , materials science , myosin light chain kinase , biochemistry , composite material , polymer , cell
Actin filaments are central components of the cytoskeleton and the contractile machinery of muscle. The filaments are known to exist in a range of conformational states presumably with different flexural rigidity and thereby different persistence lengths. Our results analyze the approaches proposed previously to measure the persistence length from the statistics of the winding paths of actin filaments that are propelled by surface‐adsorbed myosin motor fragments in the in vitro motility assay. Our results suggest that the persistence length of heavy meromyosin propelled actin filaments can be estimated with high accuracy and reproducibility using this approach provided that: (1) the in vitro motility assay experiments are designed to prevent bias in filament sliding directions, (2) at least 200 independent filament paths are studied, (3) the ratio between the sliding distance between measurements and the camera pixel‐size is between 4 and 12, (4) the sliding distances between measurements is less than 50% of the expected persistence length, and (5) an appropriate cut‐off value is chosen to exclude abrupt large angular changes in sliding direction that are complications, e.g., due to the presence of rigor heads. If the above precautions are taken the described method should be a useful routine part of in vitro motility assays thus expanding the amount of information to be gained from these. © 2013 Wiley Periodicals, Inc.

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