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Vol. 11, Issue 1, 161-169, January 2000
Department of Anatomy and Structural Biology, Albert Einstein
College of Medicine, Bronx, New York 10461
In microtubule (MT) translocation assays, using colloidal gold
particles coupled to monoclonal tubulin antibodies to mark positions
along MTs, we found that relative motion is possible between the gold
particle and an MT, gliding on dynein or kinesin. Such motion evidently
occurred by an affinity release and rebinding mechanism that did not
require motor activity on the particle. As the MTs moved, particles
drifted to the trailing edge of the MT and then were released.
Sometimes the particles transferred from one MT to another, moving
orthogonally. Although motion of the particles was uniformly rearward,
movement was toward the (
) or (+) end of the MT, depending on whether
dynein or kinesin, respectively, was used in the assay. These results
open possibilities for physiological mechanisms of organelle and other
movement that, although dependent on motor-driven microtubule
transport, do not require direct motor attachment between the organelle
and the microtubule. Our observations on the direction of particle
drift and time of release may also provide confirmation in a dynamic system for the conclusion that
tubulin is exposed at the (+) end of
the MT.
Online version of this article contains video
material for Figures 2, 3, and 7. Online version available at
www.molbiolcell.org.
*
Corresponding author. E-mail address:
satir{at}aecom.yu.edu.
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