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Daniel Zicha,1Ian M. Dobbie,2Mark R. Holt,3James Monypenny,1Daniel Y. H. Soong,3Colin Gray,1Graham A. Dunn3*
Transformed rat fibroblasts expressing two variants of green
fluorescent protein, each fused to -actin, were used to studyactin
dynamics during cell protrusion. The recently developedFLAP
(fluorescence localization after photobleaching) method permitsthe
tracking of one fluorophore after localized photobleachingby using the
other as a colocalized reference. Here, by visualizingthe ratio of
bleached to total molecules, we found that actinwas delivered to
protruding zones of the leading edge of the cellat speeds that
exceeded 5 micrometers per second. Monte Carlomodeling confirmed that
this flow cannot be explained by diffusionand may involve active
transport.
1 Light Microscopy, Cancer Research UK,
Lincoln's Inn Fields Laboratories, London WC2A 3PX, UK.
2 Genome Stability Laboratory, Department of
Biochemistry, National University of Ireland, Galway, Ireland.
3 The Randall Centre, New Hunt's House, Guy's
Campus, King's College London, London SE1 1UL, UK.
*
To whom correspondence should be addressed. E-mail:
graham.a.dunn{at}kcl.ac.uk
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