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Signosis/AP1 Luciferase Reporter Hela Stable Cell Line/SL0019NP/1 Ea

Description:

AP-1ResponsiveLuciferaseReporterHelaStableCellLineisderivedfromhumancervicalcancer,andstablyexpressfireflyluciferasereportergeneunderthecontrolofAP-1responseelement. Thiscelllineisanidealcellularmodelformonitoringtheactivation ofJNK,ERK,MAPKSignalingReceptorSignalingPathwaytriggeredbystimulitreatment,enforcedgeneexpressionandgeneknockdown.

Principle:

AP-1playsakeyroleinthecontrolofcellproliferation,differentiation,transformation,survivalandapoptosis. cJunandFosdimerizetoformAP-1andthisproteincomplexselectivelybindstoDNAsequencescontainingtheTPA-responsiveelements(TREs)toregulategeneexpression. Manystimuli,bothphysiologicalandpathological,canregulateAP-1activity,includingTPA,serum,growthfactors,cytokines,stresssignals,infections,andoncoproteins,TNFandIL-1. AP-1activitycanbeusedasreadoutforJNK,ERK,orMAPKkinasesignalingpathway.  

SignosishasdevelopedAP-1luciferasereporterstablecelllinebytransducingcellswithbaculoviruscontainingbothAP-1luciferasereporterandhygromycinexpressioncassette. ThehygromycinresistantclonesweresubsequentlyscreenedforPMA-inducedluciferaseactivity.  ThecelllinecanbeusedasareportersystemformonitoringtheactivityofAP-1triggeredbystimulitreatment,suchasTNFa,IL-1,geneoverexpressionandgeneknockdown. Thecellscontainnoviralparticlesandrequirehandlingatbiosafetylevel1protocol. 

 

PrinciplebehindTFluciferasereporter. TFluciferasereporterstablecelllineutilizesartificialpromoterconstructstodriveluciferaseexpression. Thepromoterregioncanconsistsofmultiplerepeatsofacis-elementTFbindingsite,aDNAfragmentfromthepromoterregionofaknownTFdownstreamgene,oraDNAfragmentcontainingputative/knownTFbindingsites. ThereareseveralwaysthataTFcanbeactivated,suchasthroughextracellularstimuliorthroughintracellularsignalingpathways. Onceactivated,theTFtranslocatestothenucleusandofteninteractswithrelevantco-factorstodrivegeneexpression. Onceluciferaseisexpressed,itcangeneratelightinanenzymaticassayandtheamountoflightmeasuredispositivelycorrelatedwiththelevelofTFactivation.

 

Data:

 AnalysisofAP-1LuciferaseReporterHelaStableCellLine.  Thecellswereseededona96-wellplateforovernightwithDMEMincluding10%FBS.Thecellsthenweretreatedwithorwithout10ng/mlPMAinDMEMand0.1%FBSfor6hours. Morethan50foldincreaseinluciferaseactivitywasdetectedwhencomparedtountreatedcells.


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