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AAT Bioquest/Tide Fluor™ 2WS maleimide [TF2WS Maleimide] *Superior replacement for FITC*/2350/1 mg
Overview | PrinterFriendlyVersion |
Ex/Em(nm) | 495/518 |
MW | 871.89 |
CAS# | N/A |
Solvent | DMSO |
Storage | F/D/L |
Category | SuperiorLabelingDyes TideFluor™DyesandKits |
Related | PeptideLabelingReagents QuencherCPGs BiochemicalAssays |
Spectrum | AdvancedSpectrumViewer |
LabelThiol-ModifiedOligonucleotideswithTideFluor™Dyes
Thefollowingprotocolhasbeenoptimizedforlabeling200µg(~6A260nmunits)ofaproprietaryoligonucleotide.Youneedmodifytheprotocoltogetthebestresultsforyourparticularapplicationbymultipleexperimentations.YOURTHIOL-MODIFIEDOLIGOMUSTBETREATEDTOREMOVESMALLTHIOLCOMPOUNDS(SUCHASDTT)THATRAPIDLYREACTSANDCONSUMESDYEMALEIMIDES.
1. PrepareOligoSolution(SolutionA)
a. Dissolveyourthiol-modifiedoligo(~200µg)inaPBSbuffer(100µL,pH7.2).
b. Note1:Theoligonucleotidemustbesynthesizedwithathiolgrouponthe5’end.SeeAppenxidx1forthepurificationofthiolmodifiedoligos.
c. Note2:Avoidbuffersthatcontainthiolcompounds,suchasDTT,asthesecompeteforconjugationwiththethiol-reactivecompound.
2. PrepareDyeSolution(SolutionB)
a. Dissolve1mgdyemaleimidein100µLDMSO(>10mg/mLifpossible)bypipettingupanddown.Centrifugethesolutionstockonthesidesofthevialtothevialbottom.
b. Note:preparetheDMSOdyesolutionbeforestartingtheconjugation.Extendedstorageofthedyesolutionmayreducethedyeactivity.Anysolutionscontainingthedyeshouldbekeptfromlight.
3. RunConjugationReaction
a. Tothedyesolution(B,20-50µL)addtheoligosolution(A,100µL)withstirringorshaking(keepingthereactionmixturefromlight).
b. Rotateorshakethereactionmixturefor4-6hoursatroomtemperatureonarotatororshaker.
c. Note:Gentlyvortextapthevialevery10minutesforthefirsthourtoensurethatthereactionsolutionremainswellmixed.Donotmixviolently,asmaterialmaybeleftonthesidesofthevial.Aftersixhours,50–90%ofthethiol-modifiedoligonucleotidemoleculesshouldbelabeled.Thereactionmightbeincubatedovernightifitismoreconvenient.However,overnightincubationwillnotresultinagreaterlabelingefficiencyinmostcases.
4. PurifyDye-OligoConjugate
a. Preliminarypurificationbyethanolprecipitationoflabeledoligonucleotide
i. Add20µL(one-tenthreactionsolutionvolumeingeneral)of3MNaCland300µLcoldabsoluteethanol(twoandhalfreactionsolutionvolumevolumesingeneral)tothereactionvial.
ii. Mixthesolutionwellandplaceitat–20°Cfor30minutes.
iii. Centrifugethesolutioninamicrocentrifugeat10,000to15,000×gfor30minutes.
iv. Note:Lossofsamplemayoccurifthecentrifugationisnotlongenough.
v. Carefullyremovethesupernatant,rinsethepellet1-3timeswithcold70%ethanolanddrybriefly.
vi. Note:Someunreactedlabelingreagentmayhaveprecipitatedoverthecourseofthereactionormaybestuckonthewallsofthereactionvial.Thismaterialshouldbecompletelyredissolvedbyextensivevortexmixingbeforecentrifugation.Redissolvingthelabelingreagentensuresthattheprecipitatedoligonucleotidewillbeminimallycontaminatedwithunreactedlabel.
b. FinalPurificationbyHPLCorbygelelectrophoresis
i. SeeAppendixI
LabelPeptideswithTideFluor™Dyes
Thefollowingprotocolhasbeenoptimizedforlabeling10mgofaproprietarypeptide(MW~2000)thatcontainsonlyasinglefreethiolgroup.YOUNEEDMODIFYTHEPROTOCOLTOARCHIETHEBESTRESULTSFORYOURPARTICULARAPPLICATIONBYMULTIPLEEXPERIMENTATIONS.
1. PreparePeptideSolution(SolutionA)
a. Dissolvethepepetide(tobelabeled)inDMF,DMSOorwater(>10mg/mLifpossible).
b. Note:Foreffectivelabeling,higherpeptideconcentrationispreferable.
2. PrepareDyeSolution(SolutionB)
a. DissolvethedyemaleimideinDMForDMSO(>5mg/mLifpossible).
b. Note:Foreffectivelabeling,higherdyeconcentrationispreferable.
3. Mixthepeptideanddyesolutions(fromSteps1and2)inroughlyequalmolarratio.
a. Note:Eitherpeptideordyemaleimidecanbeusedinexcessdependingonthecostofpeptideanddye.Goodseparationoffreedye,freepeptideanddye-peptideconjugateisanotherimportantfactorthatneedbeconsideredaswelltodecidethateitherpeptideordyeneedbeusedinslightexcess.
4. Stirthereactionmixtureatroomtemperaturefor12-24hours.
a. Note:Thisreactionisquiteefficient.Itisgenerallycompletedwithinafewhours.Ifthereactiondoesnotgenerateaconsiderableamountofdesiredconjugatewithin2hours,youneedcheckthereactionpH,averycriticalfactor.TheoptimalpHis4-6.ToolowpHsignificantlydecreasesthereactionratewhileinhighpHsolutionspeptidestendtobeoxidizedtogivethedisulfides.PeptidesoftencontainTFA,thereforeitisimportanttocheckthereactionmixturepHandadjustittopH4-6usingNaHCO3ifnecessary.
5. PurifyDye-PeptideConjugate
a. ThereactionsolutionwasconcentratedandpurifiedonaC18columntoaffordthedesiredconjugate.ThefractionswereanalyzedbyHPLC,andthefractionsof>97%puritywerepooledandlyophilized.
b. Note1:HPLCPurificationConditions:TEABbuffer(triethylammoniumbicarbonate,0.25mmol,pH=7.0-8.0)wasusedasbufferAandacetonitrileasbufferB.TheHPLCwasrunfrom0%Bto30%Bin60min(flowrate:100mL/min).
c. Note2:Avoidstronglightduringtheoperation.
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