Biochemistry. In the article “The putative actin-binding role of hydrophobic residues Trp546 and Phe547 in chicken gizzard heavy meromyosin” by Hirofumi Onishi, Manuel F. Morales, Kazuo Katoh, and Keigi Fujiwara, which appeared in number 26, December 19, 1995 of Proc. Natl. Acad. Sci. USA (92, 11965–11969), the authors request that the following be noted. In the Results section under “Enzymatic Properties,” 104 and 19 μM−1 should be 1.04 × 104 and 1.9 × 103 M−1, respectively. In the last column of Table 1, 22, 104, 27, and 19 μM−1 should be 2.2 × 103, 1.04 × 104, 2.7 × 103, and 1.9 × 103 M−1, respectively. The correct table is shown below.
Table 1.
ATPase activities of wild-type and mutant HMMs
| HMM | MgATPase, nmol of
Pi per min per mg of protein
|
Actin-activated
MgATPase
|
||
|---|---|---|---|---|
| High salt | Low salt | Vmax, nmol of Pi per min per mg | Ka, M−1 × 10−3 | |
| Wild-type | ||||
| −kinase | 3.7 | 1.3 | 76 | 2.2 |
| +kinase | — | 3.2 | 637 | 10.4 |
| Mutant | ||||
| −kinase | 4.4 | 2.7 | 49 | 2.7 |
| +kinase | — | 5.8 | 65 | 1.9 |
Vmax is the maximum actin-activated ATPase activity of HMM and Ka is the apparent binding constant for HMM to actin, which is defined to be the reciprocal of the apparent Km from the double reciprocal plots (Fig. 4). To phosphorylate the regulatory light chain of HMM, myosin light chain kinase, calmodulin, and Ca2+ were added to the ATPase assay medium. —, Not measured.