Abstract
Both apocalmodulin (Ca(2+)-free calmodulin) and Ca(2+)-calmodulin bind to and regulate the activity of skeletal muscle Ca(2+) release channel (ryanodine receptor, RYR1). Both forms of calmodulin protect sites after amino acids 3630 and 3637 on RYR1 from trypsin cleavage. Only apocalmodulin protects sites after amino acids 1982 and 1999 from trypsin cleavage. Ca(2+)-calmodulin and apocalmodulin both bind to two different synthetic peptides representing amino acids 3614-3643 and 1975-1999 of RYR1, but Ca(2+)-calmodulin has a higher affinity than apocalmodulin for both peptides. Cysteine 3635, within the 3614-3643 sequence of RYR1, can form a disulfide bond with a cysteine on an adjacent subunit within the RYR1 tetramer. The second cysteine is now shown to be between amino acids 2000 and 2401. The close proximity of the cysteines forming the intersubunit disulfide to the two sites that bind calmodulin suggests that calmodulin is binding at a site of intersubunit contact, perhaps with one lobe bound between amino acids 3614 and 3643 on one subunit and the second lobe bound between amino acids 1975 and 1999 on an adjacent subunit. This model is consistent with the finding that Ca(2+)-calmodulin and apocalmodulin each bind to a single site per RYR1 subunit (Rodney, G. G., Williams, B. Y., Strasburg, G. M., Beckingham, K., and Hamilton, S. L. (2000) Biochemistry 39, 7807-7812).
Highlights
Ca2ϩ-calmodulin (Ca2ϩCaM) is an inhibitor of RyR1 (1)
Ca2؉-calmodulin and apocalmodulin both bind to two different synthetic peptides representing amino acids 3614 –3643 and 1975– 1999 of RYR1, but Ca2؉-calmodulin has a higher affinity than apocalmodulin for both peptides
The close proximity of the cysteines forming the intersubunit disulfide to the two sites that bind calmodulin suggests that calmodulin is binding at a site of intersubunit contact, perhaps with one lobe bound between amino acids 3614 and 3643 on one subunit and the second lobe bound between amino acids 1975 and 1999 on an adjacent subunit
Summary
Ca2ϩ-calmodulin (Ca2ϩCaM) is an inhibitor of RyR1 (1). CaM in both its Ca2ϩ-bound and Ca2ϩ-free forms binds to one site per RYR1 subunit (2). An intersubunit disulfide bond can be formed by treating RYR1 with oxidizing agents (7–9), and the formation of this cross-link is blocked by bound Ca2ϩCaM or apoCaM (7) These data suggest that the CaM binding site may be localized to a site of intersubunit contact. Consistent with this, one of the cysteines involved in this cross-link is found within the amino acid 3614 –3643 binding site for the C-lobe of CaM (10) These findings raise the possibility that the CaM could be interacting simultaneously with two subunits in the RYR1 tetramer. We identify a new sequence that could be the binding site for the N-lobe of CaM on an adjacent subunit in the RYR1 tetramer
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