In this study, we define calmodulin binding sites of skeletal, cardiac, and brain ryanodine receptor (RYR) Ca2+ channels. Cardiac and brain RYR peptides corresponding to the calmodulin binding sites present in the skeletal RYR [Menegazzi, P., et al. (1994) Biochemistry 33, 9078-90841 were synthesized, and their interaction with calmodulin was monitored by fluorescent techniques. The central portions of the skeletal, cardiac, and brain RYR protomers display one high (CaM1; Kd ranging between 2.7 and 10.2 nM) and one low affinity (CaM2; Kd ranging between 116 and 142 nM) calmodulin binding site. Depending on the RYR model having 4 or 12 transmembrane segments, a third calmodulin binding site (CaM3) was identified a few residues upstream from the putative transmembrane segment M1 or M5. Its affinity for calmodulin varied between the RYR isoforms: the cardiac RYR CaM3 displays a high affinity (9.09 f 1.0 nM, n = 3, while the skeletal and brain RYR CaM3 have low affinity, the lowest affinity being displayed by the brain isoform (234 f 39 nM, n = 3). The RYRs calmodulin binding site CaMl encompasses the sequence Arg-His-Arg-Val(I1e)-Ser-Lewu,h ich is phosphorylated in vitro by the catalytic subunit of the CAMP-dependent protein kinase. Phosphorylation of RYR PM1 peptides occurs on the Ser, corresponding to amino acid number 2919, 3020, and 3055 of the brain, cardiac, and skeletal RYR protomers, respectively. We found that phosphorylation of the RYR PM1 peptides was inhibited by calmodulin binding and that the formation of the PM 1 peptide-calmodulin complex was inhibited by peptide phosphorylation. These data indicate that the effect of calmodulin binding to RYR CaMl may be regulated by the phosphorylation state of the Ser residue localized within the sequence Arg-His-Arg-Val(I1e)-Ser-Le
Calmodulin Binding Sites of the Skeletal, Cardiac, and Brain Ryanodine Receptor Ca2+ Channels: Modulation by the Catalytic Subunit of cAMP-Dependent Protein Kinase?
GUERRINI, RemoPrimo
;MARASTONI, Mauro;ZORZATO, FrancescoPenultimo
;TREVES, Susan Nella
Ultimo
1995
Abstract
In this study, we define calmodulin binding sites of skeletal, cardiac, and brain ryanodine receptor (RYR) Ca2+ channels. Cardiac and brain RYR peptides corresponding to the calmodulin binding sites present in the skeletal RYR [Menegazzi, P., et al. (1994) Biochemistry 33, 9078-90841 were synthesized, and their interaction with calmodulin was monitored by fluorescent techniques. The central portions of the skeletal, cardiac, and brain RYR protomers display one high (CaM1; Kd ranging between 2.7 and 10.2 nM) and one low affinity (CaM2; Kd ranging between 116 and 142 nM) calmodulin binding site. Depending on the RYR model having 4 or 12 transmembrane segments, a third calmodulin binding site (CaM3) was identified a few residues upstream from the putative transmembrane segment M1 or M5. Its affinity for calmodulin varied between the RYR isoforms: the cardiac RYR CaM3 displays a high affinity (9.09 f 1.0 nM, n = 3, while the skeletal and brain RYR CaM3 have low affinity, the lowest affinity being displayed by the brain isoform (234 f 39 nM, n = 3). The RYRs calmodulin binding site CaMl encompasses the sequence Arg-His-Arg-Val(I1e)-Ser-Lewu,h ich is phosphorylated in vitro by the catalytic subunit of the CAMP-dependent protein kinase. Phosphorylation of RYR PM1 peptides occurs on the Ser, corresponding to amino acid number 2919, 3020, and 3055 of the brain, cardiac, and skeletal RYR protomers, respectively. We found that phosphorylation of the RYR PM1 peptides was inhibited by calmodulin binding and that the formation of the PM 1 peptide-calmodulin complex was inhibited by peptide phosphorylation. These data indicate that the effect of calmodulin binding to RYR CaMl may be regulated by the phosphorylation state of the Ser residue localized within the sequence Arg-His-Arg-Val(I1e)-Ser-LeI documenti in SFERA sono protetti da copyright e tutti i diritti sono riservati, salvo diversa indicazione.