Literature DB >> 1534696

Velocity of movement of actin filaments in in vitro motility assay. Measured by fluorescence correlation spectroscopy.

J Borejdo1, S Burlacu.   

Abstract

We have measured the velocity of actin filaments in in vitro motility assay by fluorescence correlation spectroscopy. In this method, one measures fluctuations in the number of filaments in an open sample volume. The number of filaments was calculated from measurements of fluorescence of rhodamine-phalloidin bound to F-actin. Sample volume was defined by a diaphragm placed in front of the photomultiplier. Fluctuations arise when actin filaments enter and leave the sample volume due to translations driven by mechanochemical interactions with myosin heads which are immobilized on a glass surface. The average velocity of the translation of filaments determined by the correlation method, (Vc), was equal to the diameter of the diaphragm divided by the half-time of the relaxation of fluctuations. The average number of moving filaments determined by correlation method, (Nc), was inversely proportional to the relative fluctuations. By the fluctuation method it was possible to determine the average velocity of over 800 moving filaments in less than 4 min. There was good agreement between (Vc) and (Nc) and the average velocity and the average number of moving filaments determined manually. To be able to apply correlation measurements to an experimental problem, neither (Vc) nor (Nc) must depend on the position of observation of filaments. We first confirmed that this was indeed the case. We then applied the method to investigate the dependence of motility on the ATPase activity of myosin heads. ATPase activity was varied by mixing intact heads with heads which were labeled with different thiol reagents. It was found that the motion was drastically influenced by the reagent used for modification. When the reagent was N-ethyl-maleimide, 1.5% modification was sufficient to completely inhibit the motion. When the reagent was 5-iodoacetamidofluorescein, motion declined hyperbolically with the fraction of modified heads.

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Year:  1992        PMID: 1534696      PMCID: PMC1260390          DOI: 10.1016/S0006-3495(92)81935-5

Source DB:  PubMed          Journal:  Biophys J        ISSN: 0006-3495            Impact factor:   4.033


  28 in total

1.  Real-time imaging of single DNA molecules with fluorescence microscopy.

Authors:  T W Houseal; C Bustamante; R F Stump; M F Maestre
Journal:  Biophys J       Date:  1989-09       Impact factor: 4.033

2.  Direct observation of molecular motility by light microscopy.

Authors:  Y Harada; T Yanagida
Journal:  Cell Motil Cytoskeleton       Date:  1988

3.  Fluorescent actin filaments move on myosin fixed to a glass surface.

Authors:  S J Kron; J A Spudich
Journal:  Proc Natl Acad Sci U S A       Date:  1986-09       Impact factor: 11.205

4.  The regulation of rabbit skeletal muscle contraction. I. Biochemical studies of the interaction of the tropomyosin-troponin complex with actin and the proteolytic fragments of myosin.

Authors:  J A Spudich; S Watt
Journal:  J Biol Chem       Date:  1971-08-10       Impact factor: 5.157

5.  Fluorescence correlation spectroscopy. II. An experimental realization.

Authors:  D Magde; E L Elson; W W Webb
Journal:  Biopolymers       Date:  1974-01       Impact factor: 2.505

6.  Biochemistry without oxygen.

Authors:  S W Englander; D B Calhoun; J J Englander
Journal:  Anal Biochem       Date:  1987-03       Impact factor: 3.365

7.  Myosin movement in vitro: a quantitative assay using oriented actin cables from Nitella.

Authors:  M P Sheetz; S M Block; J A Spudich
Journal:  Methods Enzymol       Date:  1986       Impact factor: 1.600

8.  Fluorescence of fluorescein attached to myosin SH1 distinguishes the rigor state from the actin-myosin-nucleotide state.

Authors:  T Ando
Journal:  Biochemistry       Date:  1984-01-17       Impact factor: 3.162

9.  Dynamic study of F-actin by quasielastic scattering of laser light.

Authors:  S Fujime; S Ishiwata
Journal:  J Mol Biol       Date:  1971-11-28       Impact factor: 5.469

10.  Sliding distance of actin filament induced by a myosin crossbridge during one ATP hydrolysis cycle.

Authors:  T Yanagida; T Arata; F Oosawa
Journal:  Nature       Date:  1985 Jul 25-31       Impact factor: 49.962
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  6 in total

1.  Motion of actin filaments in the presence of myosin heads and ATP.

Authors:  S Burlacu; J Borejdo
Journal:  Biophys J       Date:  1992-12       Impact factor: 4.033

2.  Myosin II Activity Softens Cells in Suspension.

Authors:  Chii J Chan; Andrew E Ekpenyong; Stefan Golfier; Wenhong Li; Kevin J Chalut; Oliver Otto; Jens Elgeti; Jochen Guck; Franziska Lautenschläger
Journal:  Biophys J       Date:  2015-04-21       Impact factor: 4.033

3.  Buckling instabilities and spatio-temporal dynamics of active elastic filaments.

Authors:  Yaouen Fily; Priya Subramanian; Tobias M Schneider; Raghunath Chelakkot; Arvind Gopinath
Journal:  J R Soc Interface       Date:  2020-04-22       Impact factor: 4.118

4.  Differential scanning calorimetric study of the complexes of modified myosin subfragment 1 with ADP and vanadate or beryllium fluoride.

Authors:  N L Golitsina; A A Bobkov; I V Dedova; D A Pavlov; O P Nikolaeva; V N Orlov; D I Levitsky
Journal:  J Muscle Res Cell Motil       Date:  1996-08       Impact factor: 2.698

5.  Fluorescence polarization study of the rigor complexes formed at different degrees of saturation of actin filaments with myosin subfragment-1.

Authors:  O A Andreev; R Takashi; J Borejdo
Journal:  J Muscle Res Cell Motil       Date:  1995-08       Impact factor: 2.698

6.  ATPase activity of myosin in hair bundles of the bullfrog's sacculus.

Authors:  S Burlacu; W D Tap; E A Lumpkin; A J Hudspeth
Journal:  Biophys J       Date:  1997-01       Impact factor: 4.033
  6 in total

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