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J. Biol. Chem., Vol. 256, Issue 10, 4741-4746, May, 1981
A Bennick, AC McLaughlin, AA Grey and G Madapallimattam
The location of the calcium-binding sites in the human acidic proline- rich
proteins, salivary proteins A and C, were determined by equilibrium
dialysis of the tryptic peptides with buffers containing 45Ca. All the
calcium-binding sites are located in the NH2-terminal tryptic peptide (TX
peptide). The nature of the calcium binding sites in the TX peptide and
native salivary proteins A and C, as well as dephosphorylated proteins were
compared. Two types of sites can be distinguished in peptide TX. Type I
sites have an apparent dissociation constant (K) of 38 microM and are
responsible for the binding of 2.6 mol of Ca/mol of peptide. The
corresponding figures for Type II sites are 780 microM and 5.3 mol of
Ca/mol of peptide. In the native proteins, the amount of calcium bound at
the type II sites decreases to 3.9 mol of Ca/mol of proteins A and C and K
increases to 1100 microM. The amount of calcium bound at type I sites
decreases to 1.5 mol/mol of protein A and 0.6 mol/mol of protein C, but
there is no change in K. Dephosphorylation affects the calcium binding at
both types of sites. The experiments indicate that the COOH-terminal parts
of the native proteins affect the number and the nature of the protein
calcium- binding sites. Proton and phosphorous NMR data demonstrate that
beta- COOH in aspartic acid, as well as phosphoserine, are part of the
calcium-binding sites. The difference in calcium binding to salivary
proteins A and C may be due at least partially to differences in the
environment of one or more aspartic acids.
The location and nature of calcium-binding sites in salivary acidic proline-rich phosphoproteins
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