TheEpiQuik™m6ARNAMethylationQuantificationKit(Colorimetric)isacompletesetofoptimizedbuffersandreagentstocolorimetricallyquantifyN6-methyladenosine(m6Aor6mA)inRNA.Itissuitableforadirectdetectionofm6ARNAmethylationstatususingtotalRNAisolatedfromanyspeciessuchasmammals,plants,fungi,bacteria,andviruses.Thekithasthefollowingadvantagesandfeatures:

• ColorimetricELISA-likeassayusinganm6Aantibodywitheasy-to-followstepsforconvenienceandspeed.Theentireprocedurecanbecompletedwithin3hoursand45minutes.
• Highsensitivity,ofwhichthedetectionlimitcanbeaslowas10pgofm6A.
• UniquebindingsolutionallowsRNA>70ntstobetightlyboundtothewells,whichenablesquantificationofm6AfrombothmRNAandncRNAsuchastRNA,rRNA,andsnRNA.
• Optimizedantibodyandenhancersolutionsallowhighspecificitytom6A,withnocross-reactivitytounmethylatedadenosinewithintheindicatedconcentrationrangeofthesampleRNA.
• Universalpositiveandnegativecontrolsareincluded,whicharesuitableforquantifyingm6Afromanyspecies.
• Strip-wellmicroplateformatmakestheassayflexIBLeformanualorhighthroughputanalysis.
• Simple,reliable,andconsistentassayconditions.

BackgroundInformation 
N6-methyladenosine(m6A)isthemostcommonandabundantmodificationinRNAmoleculespresentineukaryotes.Them6AmodificationiscatalyzedbyamethyltransferasecomplexMETTL3andremovedbytherecentlydiscoveredm6ARNAdemethylasesFTOandALKBH5,whichcatalyzem6Ademethylationinanα-ketoglutarate(α-KG)-andFe2+-dependentmanner.ItwasshownthatMETTL3,FTO,andALKBH5playimportantrolesinmanyBIOLOGicalprocesses,rangingfromdevelopmentandmetabolismtofertility.m6Aaccountsformorethan80%ofallRNAbasemethylationsandexistsinvariousspecies.m6AismainlydistributedinmRNAandalsooccursinnon-codingRNAsuchastRNA,rRNA,andsnRNA.Therelativeabundanceofm6AinmRNAtranscriptshasbeenshowntoaffectRNAmetabolismprocessessuchassplicing,nuclearexport,translationABIlityandstability,andRNAtranscription.Abnormalm6Amethylationlevelsinducedbydefectsinm6ARNAmethylaseanddemethylasecouldleadtodysfunctionofRNAanddiseases.Forexample,abnormallylowlevelsofm6AintargetmRNAsduetoincreasedFTOactivityinpatientswithFTOmutations,throughanas-yetundefinedpathway,contributestotheonsetofobesityandrelateddiseases.Thedynamicandreversiblechemicalm6AmodificationinRNAmayalsoserveasanovelepigeneticMarkerofprofoundbiologicalsignificance.Therefore,moreusefulinformationforabetterunderstandingofm6ARNAmethylationlevelsanddistributiononRNAtranscriptscouldbenefitdiagnosticsandtherapeuticsofdisease.

Principle&Procedure
Inthisassay,totalRNAisboundtostripwellsusingaRNAhighbindingsolution.N6-methyladenosine(m6A)isdetectedusingaspecificcaptureN6-methyladenosineantibodyanddetectionantibody.ThedetectedsignalisenhancedandthenquantifiedcolorimetricallybyreADIngtheabsorbanceinamicroplatespectrophotometeratawavelengthof450nm.Theamountofm6AisproportionaltotheODintensitymeasured. BothnegativeandpositiveRNAcontrolsareprovidedinthiskit.Astandardcurvecanbeperformed(range:0.02to1ngofm6A)orasinglequantityofm6Acanbeusedasapositivecontrol.Becausem6Acontentcanvaryfromtissuetotissue,andfromnormalanddiseasedstates,orvaryundertreatedanduntreatedconditions,itisadvisedtorunreplicatesamplestoensurethatthesignalgeneratedisvalidated.Thiskitwillallowtheusertoquantifyanabsoluteamountofm6Aanddeterminetherelativem6ARNAmethylationstatesoftwodifferentRNAsamples.

StartingMaterials
Startingmaterialscanincludevarioustissueorcellsamplessuchascellsfromflaskormicroplateculturedcells,freshandfrozentissues,paraffin-embeddedtissues,blood,bodyfluidsamples,etc.

Fig.1. SchematicprocedureoftheEpiQuik™m6ARNAMethylationQuantificationKit(Colorimetric).

Fig.2. m6AstandardcontrolwasaddedintotheassaywellsatdifferentconcentrationsandthenmeasuredwiththeEpiQuik™m6ARNAMethylationQuantification Kit(Colorimetric).

Fig.3.  Quantificationofm6ARNAmethylationindifferentsamples. 200ngofRNAisolatedfromdifferenttissuesorcellswereaddedintotheassaywellsandthem6AcontainedinRNAwasmeasuredusingtheEpiQuik™m6ARNAMethylationQuantificationKit.