The endogenous calmodulin-protein kinase system of sarcoplasmic reticulum terminal cisternae of rabbit fast-twitch muscle was studied. Investigation of a single Ca2+-channel in terminal cisternae fused to planar lipid bilayers demonstrated that the endogenous kinase inhibits the channel, although it remained unclear whether the phosphorylation sites are on the channel protein or on other junctional sarcoplasmic reticulum specific proteins [Hain et al., (1994) Biophys. J. 67, 1823-1833]. Our results, which show that two junctional sarcoplasmic reticulum specific proteins,i.e., triadin and histidine-rich, Ca2+-binding protein, but not the ryanodine receptor/Ca2+-channel protein, are phosphorylated by membrane-bound 60 kDa protein kinase, seem to be able to resolve this ambiguity. Furthermore,such aprobably specific protein isoform of calmodulin-protein kinase, by its substrate specificity and exposure to the cytoplasmic side of terminal cisternae at the junctional membrane domain and based on protease sensitivity, also seems to possess some of the potential requirements for a regulatory role in the functional state of the Ca2+-channel.

IDENTIFICATION OF TRIADIN AND OF HISTIDINE-RICH CA2+-BINDING PROTEIN AS SUBSTRATES OF 60-KDA CALMODULIN-DEPENDENT PROTEIN- KINASE IN JUNCTIONAL TERMINAL CISTERNAE OF SARCOPLASMIC- RETICULUM OF RABBIT FAST MUSCLE

DAMIANI, ERNESTO;SAGGIN, LEOPOLDO;MARGRETH, ALFREDO
1995

Abstract

The endogenous calmodulin-protein kinase system of sarcoplasmic reticulum terminal cisternae of rabbit fast-twitch muscle was studied. Investigation of a single Ca2+-channel in terminal cisternae fused to planar lipid bilayers demonstrated that the endogenous kinase inhibits the channel, although it remained unclear whether the phosphorylation sites are on the channel protein or on other junctional sarcoplasmic reticulum specific proteins [Hain et al., (1994) Biophys. J. 67, 1823-1833]. Our results, which show that two junctional sarcoplasmic reticulum specific proteins,i.e., triadin and histidine-rich, Ca2+-binding protein, but not the ryanodine receptor/Ca2+-channel protein, are phosphorylated by membrane-bound 60 kDa protein kinase, seem to be able to resolve this ambiguity. Furthermore,such aprobably specific protein isoform of calmodulin-protein kinase, by its substrate specificity and exposure to the cytoplasmic side of terminal cisternae at the junctional membrane domain and based on protease sensitivity, also seems to possess some of the potential requirements for a regulatory role in the functional state of the Ca2+-channel.
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11577/132741
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