Calmodulin (CaM) is a 148-residue regulatory calcium-binding
protein that activates a wide range of target proteins
and enzymes. Calcium-saturated CaM has a bilobal structure,
and each domain has an exposed hydrophobic surface region
where target proteins are bound. These two “active
sites” of calmodulin are remarkably rich in Met residues.
Here we have biosynthetically substituted (up to 90% incorporation)
the unnatural amino acids ethionine (Eth) and norleucine
(Nle) for the nine Met residues of CaM. The substituted
proteins bind in a calcium-dependent manner to hydrophobic
matrices and a synthetic peptide, encompassing the CaM-binding
domain of myosin light-chain kinase (MLCK). Infrared and
circular dichroism spectroscopy show that there are essentially
no changes in the secondary structure of these proteins
compared to wild-type CaM (WT-CaM). One- and two-dimensional
NMR studies of the Eth-CaM and Nle-CaM proteins reveal
that, while the core of the proteins is relatively unaffected
by the substitutions, the two hydrophobic interaction surfaces
adjust to accommodate the Eth and Nle residues. Enzyme
activation studies with MLCK show that Eth-CaM and Nle-CaM
activate the enzyme to 90% of its maximal activity, with
little changes in dissociation constant. For calcineurin
only 50% activation was obtained, and the KD
for Nle-CaM also increased 3.5-fold compared with WT-CaM.
These data show that the “active site” Met
residues of CaM play a distinct role in the activation
of different target enzymes, in agreement with site-directed
mutagenesis studies of the Met residues of CaM.
