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JBC, Vol. 250, Issue 14, 5481-5486, Jul, 1975
P. Sherline, J. T. Leung and D. M. Kipnis
The binding of colchicine to tubulin, purified by two cycles of
assembly-disassembly, has been studied. Equilibrium studies indicated a
dissociation constant which declined during incubation approaching a
minimum value of approximately 0.30 times 10- minus 6 M after 13 hours of
incubation. Because tubulin is unstable during prolonged incubation (t1/2
of 5.2 hours for free tubulin, t1/2 of 12.5 hours for tubulin bound to
colchicine), the equilibrium Kd was felt to be an overestimation of the
true Kd. The rate constant of dissociation (k-1 equal to 0.009 hour- minus
1 hour- minus 1) and the rate constant of association (k1 equal to 0.37
times 10-6 M-minus 1) were measured under conditions designed to circumvent
or correct for tubulin instability. The dissociation constant determined by
the ratio k-1/k1 was 0.024 times -minus 6 M. To determine whether the
discrepancy between the "equilibrium" and "kinetic" determined dissociation
constants could be accounted for on the basis of tubulin instability, the
binding reaction was computer-simulated using the measured association and
dissociation rate constants and the rate constants for decay of bound and
free tubulin. Computer simulation was in close agreement with the
experimentally determined behavior of the reaction during a 13-hour
incubation. It is concluded that the Kd determined by equilibrium
methodology results in a considerable overestimation due to the instability
of tubulin, and that the best estimate for the Kd of the colchicine-tubulin
equilibrium is the value determined by the ratio of the rate constants.
Binding of colchicine to purified microtubule protein
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