The Cauliflower mosaic virus (CaMV) open reading frame VI product (P6) is essential for the viral infection cycle. It controls translation reinitiation of the viral polycistronic RNAs and forms cytoplasmic inclusion bodies (viroplasms) where virus replicat
CaMVP6IsaNucleocytoplasmicProtein931
Figure2.SubcellularLocalizationAnalysisofP6FusedtoEGFPinTobaccoBY-2CellsandofP6inProtoplastsfromCaMV-InfectedTurnipPlantsbyCLSM.
(A)Green uorescentimagesofEGFP:P6(images1and4)weretaken20haftertransfectionoftobaccocellsbybombardmentwithpCK-EGFP:P6plasmid.A0.45-mm-thickopticalsectionwassampledusingasingletrackconfocalmicroscopeandappropriate lters.Image3correspondstoanenlargementofaggregatessimilartothoseobservedinimage1.Images2and5correspondtothesuperpositionofthe uorescentimageandthecorrespondingdifferentialinterferencecontrastimage.Bars¼10mm.N,nucleus;Nu,nucleolus.
(B)ProtoplastspreparedfromCaMV-infectedturnipleaveswere xedandimmunolabeledwithrabbitanti-P6antibodiesandmouseanti-rabbitIgGcoupledtoAlexa568assecondaryantibody.Shownisthered uorescentimageofatypicalprotoplast.Theconfocalimageswerecollectedwithafocaldepthof0.45mm.Bar¼10mm.
MutationsintheN-Terminala-HelixofP6AffecttheFormationofViroplasms
InviewofthefactthatsubdomainA1istotallyconservedamongCaMVstrainsandispartoftheputativeLeuzipper–containinga-helix,additionalexperimentswereperformedtofurtherin-vestigateitsroleinviroplasmformation.Weremovedboththei1andI1sequences(aminoacidsfrompositions5to20)fromP6(Figure5A)toseeifthereductionofthesizeofthea-heliximpairstheformationofviroplasms.The uorescenceofthecorrespond-ingEGFP:P6Di1-I1mutantwasveryabundantanddiffuseinthenucleus,whereasonlylowlevelswerefoundinthecytoplasm(Figure5B,panels1and2).SimilarbehaviorwasobservedwithmutantEGFP:P6DI1,inwhichwedeletedonlytheI1sequence(Figure5B,panels3and4).TheseP6mutantsdidnotformaggregates,thusreinforcingthehypothesisthattheN-terminala-helixisrequiredforP6self-assembly.Moreover,theseresultsstronglysuggestthatthea-helixand/orspeci cresiduesofI1arealsoimplicatedinthecytoplasmiclocalizationofP6becausebothconstructions,EGFP:P6Di1-I1andEGFP:P6DI1,localizedalmosttotallyinthenucleus,incontrastwithEGFP:P6(Fig-ure2A).
Insummary,theforegoingresultsstronglysuggestthattheN-terminala-helixhasstructuralfeaturesimportantforboththeaggregationofP6anditslocalizationinthecytoplasm.Todemonstrateitsroleintheformationofviroplasm,wemutatedthreeLeuresiduesoftheI1sequenceofP6(seealsobelow).TheLeuresiduesatpositions14and16weresubstitutedbyGlnresiduesandtheLeuatposition18byaHis(Figure4B,top).Aminoacidresidues14and18correspondtoposition‘‘d’’ofthesecondheptadandtoposition‘‘a’’inthethirdheptadoftheLeuzipper.Theyarepredictedtolieonthesurfaceofthea-helixandtobeinvolvedinhydrophobicinteractionsbetweenP6mole-culesinthecoiled-coilstructure(Figure4B).Leu16,ontheotherhand,isnotpredictedtobesurface-located.
First,wetestedthecapacityofthismutant,namedP6m1,tointeractwiththewild-typeP6byfarproteingelblotassay.
The