Abstract
Monoclonal antibodies binding to distinct epitopes on the tail of brush border myosin were used to modulate the conformation and state of assembly of this myosin. BM1 binds 1:3 of the distance from the tip of the tail to the head and prevents the extended-tail (6S) monomer from folding into the assembly-incompetent folded-tail (10S) state, whereas BM4 binds to the tip of the myosin tail, and induces the myosin to fold into the 10S state. Thus, at physiological ionic strength BM1 promotes and BM4 blocks the assembly of the myosin into filaments. Using BM1 and BM4 together, we were able to prevent both folding and filament assembly, thus locking myosin molecules in the extended-tail 6S monomer conformation at low ionic strength where they normally assemble into filaments. Using these myosin-antibody complexes, we were able to investigate independently the effects of folding of the myosin tail and assembly into filaments on the myosin MgATPase. The enzymatic activities were measured from the fluorescent profiles during the turnover of the ATP analogue formycin triphosphate (FTP). Extended-tail (6S) myosin molecules had an FTPase activity of 1-5 X 10(-3) s-1, either at high ionic strength as a monomer alone or when complexed with antibody, or at low ionic strength as filaments or when maintained as extended-tail monomers by the binding of BM1 and BM4. Folding of the molecules into the 10S state reduced this rate by an order of magnitude, effectively trapping the products of FTP hydrolysis in the active sites.
Highlights
Using these myosin-antibody complexes, we were able to investigate independently the effects of folding of the myosin tail and assembly into filaments on the myosin MgATPase
This was in agreement with our previous observations, showing that at physiological ionic strength, MgATP disassembles brush border myosin filaments (Citi and Kendrick-Jones, 1986; Kendrick-Jones et al, 1987)
We have described a novel approach to investigate the influence of myosin conformation on its enzymatic activity, using specific monoclonal antibodies
Summary
Using these myosin-antibody complexes, we were able to investigate independently the effects of folding of the myosin tail and assembly into filaments on the myosin MgATPase. Since filamentous myosin released the products of hydrolysis at a rate comparable to that of extended monomer, it was suggested that the folding of the myosin tail was involved in nucleotide trapping (Cross et al, 1988). To test this hypothesis and investigate the role of the myosin tail in the conformational changes that the myosin molecule can undergo (e.g., in folding, unfolding, and filament assembly), we have used two anti-(brush border myosin) monoclonal antibodies. Measuring the enzymatic activities of these antibody-myosin complexes using formycin triphosphate (Jackson and Bagshaw, 1988a) demonstrated that the trapped state is a property exclusively of folded molecules, and that assembly into filaments per se does not greatly affect the enzymatic activity of the extended myosin molecules
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