The elusive role of the SPRY2 domain in RyR1

dc.contributor.authorTae, HanShen
dc.contributor.authorWei, L
dc.contributor.authorWillemse, Hermia
dc.contributor.authorMirza, Shamaruh
dc.contributor.authorGallant, Esther
dc.contributor.authorBoard, Philip
dc.contributor.authorDirksen, Robert
dc.contributor.authorCasarotto, Marco
dc.contributor.authorDulhunty, Angela
dc.date.accessioned2015-12-10T23:35:20Z
dc.date.issued2011
dc.date.updated2016-02-24T08:22:22Z
dc.description.abstractThe second of three SPRY domains (SPRY2, S1085 -V1208) located in the skeletal muscle ryanodine receptor (RyR1) is contained within regions of RyR1 that influence EC coupling and bind to imperatoxin A, a toxin probe of RyR1 channel gating. We examined the binding of the F loop (P1107-A1121) in SPRY2 to the ASI/basic region in RyR1 (T3471-G3500, containing both alternatively spliced (ASI) residues and neighboring basic amino acids). We then investigated the possible influence of this interaction on excitation contraction (EC) coupling. A peptide with the F loop sequence and an antibody to the SPRY2 domain each enhanced RyR1 activity at low concentrations and inhibited at higher concentrations. A peptide containing the ASI/basic sequence bound to SPRY2 and binding decreased ~10-fold following mutation or structural disruption of the basic residues. Binding was abolished by mutation of three critical acidic F loop residues. Together these results suggest that the ASI/basic and SPRY2 domains interact in an F loop regulatory module. Although a region that includes the SPRY2 domain influences EC coupling, as does the ASI/basic region, Ca2+ release during ligand- and depolarization-induced RyR1 activation were not altered by mutation of the three critical F loop residues following expression of mutant RyR1 in RyR1-null myotubes. Therefore the electrostatic regulatory interaction between the SPRY2 F loop residues (that bind to imperatoxin A) and the ASI/basic residues of RyR1 does not influence bi-directional DHPR-RyR1 signaling during skeletal EC coupling, possibly because the interaction is interrupted by the influence of factors present in intact muscle cells.
dc.identifier.issn1933-6950
dc.identifier.urihttp://hdl.handle.net/1885/69814
dc.publisherLandes Bioscience
dc.sourceChannels
dc.subjectKeywords: dihydropteridine reductase; gamma glutamylcyclotransferase; ryanodine receptor; signal peptide; SPRY2 protein, human; alternative RNA splicing; animal; article; chemistry; cytoplasm; genetics; human; kinetics; metabolism; protein binding; protein tertiary
dc.titleThe elusive role of the SPRY2 domain in RyR1
dc.typeJournal article
local.bibliographicCitation.issue2
local.bibliographicCitation.lastpage160
local.bibliographicCitation.startpage148
local.contributor.affiliationTae, HanShen, University of Melbourne
local.contributor.affiliationWei, L, University of Rochester Medical Center
local.contributor.affiliationWillemse, Hermia, College of Medicine, Biology and Environment, ANU
local.contributor.affiliationMirza, Shamaruh, College of Medicine, Biology and Environment, ANU
local.contributor.affiliationGallant, Esther, College of Medicine, Biology and Environment, ANU
local.contributor.affiliationBoard, Philip, College of Medicine, Biology and Environment, ANU
local.contributor.affiliationDirksen, Robert, University of Rochester
local.contributor.affiliationCasarotto, Marco, College of Medicine, Biology and Environment, ANU
local.contributor.affiliationDulhunty, Angela, College of Medicine, Biology and Environment, ANU
local.contributor.authoruidWillemse, Hermia, u4617864
local.contributor.authoruidMirza, Shamaruh, u4284865
local.contributor.authoruidGallant, Esther, u4141180
local.contributor.authoruidBoard, Philip, u7701651
local.contributor.authoruidCasarotto, Marco, u9611346
local.contributor.authoruidDulhunty, Angela, u8404877
local.description.embargo2037-12-31
local.description.notesImported from ARIES
local.identifier.absfor060406 - Genetic Immunology
local.identifier.ariespublicationf2965xPUB2129
local.identifier.citationvolume5
local.identifier.doi10.4161/chan.5.2.14407
local.identifier.scopusID2-s2.0-79960634407
local.identifier.thomsonID000289404400009
local.type.statusPublished Version

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