Inhibition of Acto-Myosin Subfragment-1 ATPase Activity by Peptides Corresponding to Various Segments of the 20-kDa Domain of Myosin Heavy Chain

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As reported previously, the synthetic heptapeptide having the amino acid sequence around the reactive Cys (SH1) of myosin heavy chain, IRICRKG-NH₂, inhibited acto-myosin subfragment-1 (S-1) ATPase activity and half inhibition (K_1/2) was observed at a peptide concentration of 0.06mM. The inhibitory ability of the peptide was found to be decreased to one-fifth by acetylation of its N-terminal α-amino group. A similar effect of N-acetylation was observed with a nonapeptide, EGIRICRKG-NH₂, and an undecapeptide, VLEG-IRICRKG-NH₂. These results indicate that N-terminal-free synthetic peptides do not act as proper analogs of the corresponding segment of S-1 heavy chain against F-actin. We isolated a longer peptide extending from Thr⁶⁸² to Lys⁷⁰⁹ in S-1 heavy chain, with two Cys residues corresponding to SH1 and SH2. This peptide, having 28 residues (28peptide), inhibited acto-S-1 ATPase activity with a K_1/2 of 0.23mM. A cosedimentation binding assay indicated that the 28peptide completely dissociated acto-S-1 in the presence of ATP. This behavior is different from that observed with the N-terminal-free synthetic heptapeptide, and thus the 28peptide might be an analog of the corresponding segment. There is a possibility that the region corresponding to the 28peptide in S-1 heavy chain may bind directly with F-actin and may be involved in determining the acto-S-1 link during the steady state of the acto-S-1 ATPase reaction.