Myosin Motors Drive Long Range Alignment of Actin Filaments
The bulk alignment of actin filament sliding movement, powered by randomly oriented myosin molecules, has been observed and studied using an in vitro motility assay. The well established, actin filament gliding assay is a minimal experimental system for studying actomyosin motility. Here, we show th...
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Veröffentlicht in: | The Journal of biological chemistry 2010-02, Vol.285 (7), p.4964-4974 |
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Sprache: | eng |
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Zusammenfassung: | The bulk alignment of actin filament sliding movement, powered by randomly oriented myosin molecules, has been observed and
studied using an in vitro motility assay. The well established, actin filament gliding assay is a minimal experimental system for studying actomyosin
motility. Here, we show that when the assay is performed at densities of actin filaments approaching those found in living
cells, filament gliding takes up a preferred orientation. The oriented patterns of movement that we have observed extend over
a length scale of 10â100 μm, similar to the size of a mammalian cell. We studied the process of filament alignment and found
that it depends critically upon filament length and density. We developed a simple quantitative measure of filament sliding
orientation and this enabled us to follow the time course of alignment and the formation and disappearance of oriented domains.
Domains of oriented filaments formed spontaneously and were separated by distinct boundaries. The pattern of the domain structures
changed on the time scale of several seconds and the collision of neighboring domains led to emergence of new patterns. Our
results indicate that actin filament crowding may play an important role in structuring the leading edge of migrating cells.
Filament alignment due to near-neighbor mechanical interactions can propagate over a length scale of several microns; much
greater than the size of individual filaments and analogous to a log drive. Self-alignment of actin filaments may make an
important contribution to cell polarity and provide a mechanism by which cell migration direction responds to chemical cues. |
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ISSN: | 0021-9258 1083-351X |
DOI: | 10.1074/jbc.M109.044792 |