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- A Model of Cross-Bridge Attachment to Actin in the A·M·ATP S...A Model of Cross-Bridge Attachment to Actin in the A·M·ATP State Based on X-Ray Diffraction from Permeabilized Rabbit Psoas Muscle
Biophysical Journal, Volume 82, Issue 4, 1 April 2002, Pages 2123-2133
Jin Gu, Sengen Xu and Leepo C. Yu
AbstractA model of cross-bridges binding to actin in the weak binding A·M·ATP state is presented. The modeling was based on the x-ray diffraction patterns from the relaxed skinned rabbit psoas muscle fibers where ATP hydrolysis was inhibited by N-phenylmaleimide treatment (S. Xu, J. Gu, G. Melvin, L. C. Yu. 2002. 82:2111–2122). Calculations included both the myosin filaments and the actin filaments of the muscle cells, and the binding to actin was assumed to be single headed. To achieve a good fit, considerable flexibility in the orientation of the myosin head and the position of the S1-S2 junction is necessary, such that the myosin head can bind to a nearby actin whereas the tail end was kept in the proximity of the helical track of the myosin filament. Hence, the best-fit model shows that the head binds to actin in a wide range of orientations, and the tail end deviates substantially from its lattice position in the radial direction (∼60Å). Surprisingly, the best fit model reveals that the detached head, whose location thus far has remained undetected, seems to be located close to the surface of the myosin filament. Another significant requirement of the best-fit model is that the binding site on actin is near the N terminus of the actin subunit, a position distinct from the putative rigor-binding site. The results support the idea that the essential role played by the weak binding states M·ATP ↔ A·M·ATP for force generation lies in its flexibility, because the probability of attachment is greatly increased, compared with the weak binding M·ADP·P ↔ A·M·ADP·P states.
Abstract | Full Text | PDF (455 kb) - Three-Dimensional Reconstruction of Thin Filaments Containin...Three-Dimensional Reconstruction of Thin Filaments Containing Mutant Tropomyosin
Biophysical Journal, Volume 78, Issue 2, 1 February 2000, Pages 908-917
M. Rosol, W. Lehman, R. Craig, C. Landis, C. Butters and L.S. Tobacman
AbstractInteractions of the components of reconstituted thin filaments were investigated using a tropomyosin internal deletion mutant, D234, in which actin-binding pseudo-repeats 2, 3, and 4 are missing. D234 retains regions of tropomyosin that bind troponin and form end-to-end tropomyosin bonds, but has a length to span only four instead of seven actin monomers. It inhibits acto-myosin subfragment 1 ATPase (acto-S-1 ATPase) and filament sliding in vitro in both the presence and absence of Ca (Landis et al., 1997, 272:14051–14056) and lowers the affinity of S-1·ADP for actin while increasing its cooperative binding. Electron microscopy and three-dimensional reconstruction of reconstituted thin filaments containing actin, troponin, and wild-type or D234 tropomyosin were carried out to determine if Ca-induced movement of D234 occurred in the filaments. In the presence and absence of Ca, the D234 position was indistinguishable from that of the wild-type tropomyosin, demonstrating that the mutation did not affect normal tropomyosin movement induced by Ca and troponin. These results suggested that, in the presence of Ca and troponin, D234 tropomyosin was trapped on filaments in the Ca-induced position and was unable to undergo a transition to a completely activated position. By adding small amounts of rigor-bonded -ethyl-maleimide-treated S-1 to mutant thin filaments, thus mimicking the myosin-induced “open” state, inhibition could be overcome and full activation restored. This myosin requirement for full activation provides support for the existence of three functionally distinct thin filament states (off, Ca-induced, myosin-induced; cf. Landis et al., 1997; Vibert et al., 1997, 266:8–14). We propose a further refinement of the three-state model in which the binding of myosin to actin causes allosteric changes in actin that promote the binding of tropomyosin in an otherwise energetically unfavorable “open” state.
Abstract | Full Text | PDF (487 kb) - Fluorescence Depolarization of Actin Filaments in Reconstruc...Fluorescence Depolarization of Actin Filaments in Reconstructed Myofibers: The Effect of S1 or pPDM-S1 on Movements of Distinct Areas of Actin
Biophysical Journal, Volume 86, Issue 5, 1 May 2004, Pages 3020-3029
Yu.S. Borovikov, I.V. Dedova, C.G. dos Remedios, N.N. Vikhoreva, P.G. Vikhorev, S.V. Avrova, T.L. Hazlett and B.W. Van Der Meer
AbstractFluorescence polarization measurements were used to study changes in the orientation and order of different sites on actin monomers within muscle thin filaments during weak or strong binding states with myosin subfragment-1. Ghost muscle fibers were supplemented with actin monomers specifically labeled with different fluorescent probes at Cys-10, Gln-41, Lys-61, Lys-373, Cys-374, and the nucleotide binding site. We also used fluorescent phalloidin as a probe near the filament axis. Changes in the orientation of the fluorophores depend not only on the state of acto-myosin binding but also on the location of the fluorescent probes. We observed changes in polarization (i.e., orientation) for those fluorophores attached at the sites directly involved in myosin binding (and located at high radii from the filament axis) that were contrary to the fluorophores located at the sites close to the axis of thin filament. These altered probe orientations suggest that myosin binding alters the conformation of F-actin. Strong binding by myosin heads produces changes in probe orientation that are opposite to those observed during weak binding.
Abstract | Full Text | PDF (143 kb) - …more
Copyright © 1980 The Biophysical Society. All rights reserved.
Biophysical Journal, Volume 30, Issue 1, 69-77, 1 April 1980
doi:10.1016/S0006-3495(80)85077-6
Research Article
Geometrical factors influencing muscle force development. II. Radial forces
M. Schoenberg
Abstract
If the subfragment-2 (S2) portion of the myosin cross-bridge to actin does not lie parallel to the myofilament axes then when a muscle fiber contracts, there will be a radial component to the cross-bridge force. When the subfragment-1 (S1) portion of the cross-bridge attaches to actin with its long axis projecting through the filament axis, the magnitude of the radial force depends upon the azimuthal location of the actin site, but when the attachment of the S1 to actin is slewed, as in the reconstruction of Moore et al. (J. Mol. Biol., 1970, 50:279–294), then for a single cross-bridge the radial component of the cross-bridge force is not quite so sensitive to actin site location and is approximately 0.1 the axial component. In both cases, the ratio of the radial to axial force decreases with decreasing filament separation. If the radial-axial force ratio for each cross-bridge is approximately 0.1, then at full overlap in a frog skeletal muscle fiber the radial component of the cross-bridge force accompanying full activation will exert a compressive pressure of approximately 5 X 10(-3) atm. This would have little effect upon an intact muscle fiber where the volume constraints are likely osmotic, but it might produce a 1–2% change in filament spacing in a "skinned" muscle fiber from which the sarcolemma had been removed. These computations assume that the S2 link between the S1 head and the myosin filament does not support a bending moment of shear. If it does, then the radial component of the cross-bridge will be either greater or less, depending on the specific cross-bridge geometry.
