IDENTIFICATION OF THE DOMAIN RECOGNIZED BY ANTI-(RYANODINE RECEPTOR) ANTIBODIES WHICH AFFECT CA2+-INDUCED CA2+ RELEASE

In the present paper we have defined putative functional domains of the ryanodine receptor Ca2+ channel. cDNA fragments of the skeletal muscle ryanodine receptor were fused in-frame with the Escherichia coli trpe protein and the resulting fusion proteins were evaluated for their ability to react with anti-(ryanodine receptor) antibodies, which are known to block Ca2+-dependent activation of the Ca2+-release channel. Anti-(ryanodine receptor) antibodies react with epitopes lying within a 245-amino-acid-long polypeptide which is located in a region (residues 4380-4625) encompassing most of myoplasmic loop 2, the predicted transmembrane segment M5 and part of the next lumenal loop (45 residues). Purification of the anti-(ryanodine receptor) antibodies by affinity chromatography led to the isolation of a population of antibodies which was capable of decreasing (by > 30 %) the doxorubicin-induced Ca2+ release from isolated terminal cisternae. Polyclonal antibodies raised against a ryanodine receptor fusion encompassing part (198 out of 245 residues) of the immunopositive polypeptide decreased by 2-fold the first-order rate constant of Ca2+-induced Ca-45(2+) efflux from isolated terminal cisternae. These results suggest strongly that the Ca2+-activating domain of the skeletal muscle Ca2+-release channel is close to, or associated with, myoplasmic loop 2.