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2Belozersky Institute of Physico-Chemical Biology, Lomonosov Moscow State University, Moscow, 119899 Russia; fax: (095) 939-3181
* To whom correspondence should be addressed.
Received October 20, 1998; Revision received December 8, 1998
It is known that ternary complexes of myosin subfragment 1 (S1) with ADP and the Pi analogs beryllium fluoride (BeFx) and aluminum fluoride (AlF4-) are stable analogs of the myosin ATPase intermediates M*·ATP and M**·ADP·Pi, respectively. Using kinetic approaches, we compared the rate of formation of the complexes S1·ADP·BeFx and S1·ADP·AlF4- in the absence and in the presence of F-actin, as well as of the interaction of these complexes with F-actin. We show that in the absence of F-actin the formation of S1·ADP·BeFx occurs much faster (3-4 min) than that of S1·ADP·AlF4- (hours). The formation of these complexes in the presence of F-actin led to dissociation of S1 from F-actin, this process being monitored by a decrease in light scattering. The light scattering decrease of the acto-S1 complex occurred much faster after addition of BeFx (during 1 min) than after addition of AlF4- (more than 20 min). In both cases the light scattering of the acto-S1 complex decreased by 40-50%, but it remained much higher than that of F-actin measured in the absence of S1. The interaction of the S1·ADP·BeFx and S1·ADP·AlF4- complexes with F-actin was studied by the stopped-flow technique with high time resolution (no more than 0.6 sec after mixing of S1 with F-actin). We found that the binding of S1·ADP·BeFx or S1·ADP·AlF4- to F-actin is accompanied by a fast increase in light scattering, but it does not affect the fluorescence of a pyrene label specifically attached to F-actin. We conclude from these data that within this time range a “weak” binding of the S1·ADP·BeFx and S1·ADP·AlF4- complexes to F-actin occurs without the subsequent transition of the “weak” binding state to the “strong” binding state. Comparison of the light scattering kinetic curves shows that S1·ADP·AlF4- binds to F-actin faster than S1·ADP·BeFx does: the second-order rate constants for the “weak” binding to F-actin are (62.8 ± 1.8)·106 M-1·sec-1 in the case of S1·ADP·AlF4- and (22.6 ± 0.4)·106 M-1·sec-1 in the case of S1·ADP·BeFx. We conclude that the stable ternary complexes S1·ADP·BeFx and S1·ADP·AlF4- can be successfully used for kinetic studies of the “weak” binding of the myosin heads to F-actin.
KEY WORDS: myosin subfragment 1, F-actin, “weak” binding of myosin to actin, kinetics, skeletal muscle
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