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1.      Culturecellstoadensityoptimalforapoptosisinductionaccordingtoyourspecificinductionprotocol,butnottoexceed2x10⁶cells/mL.Atthesametime,cultureanon-inducednegativecontrolcellpopulationatthesamedensityastheinducedpopulationforeverylabelingcondition. Hereareafewexamplesfor inducingapoptosisinsUSPensionculture:

1)TreatingJurkatcellswith2μg/mlcamptothecinfor3hours.

2)TreatingJurkatcellswith1μMstaurosporinefor3hours.

3)TreatingHL-60cellswith4μg/mlcamptothecinfor4hours.

4)TreatingHL-60cellswith1μMstaurosporinefor4hours.

Note:Eachcelllineshouldbeevaluatedonanindividualbasistodeterminetheoptimalcelldensityforapoptosisinduction.

2.      Make150XFAM-LEHD-FMKDMSOstocksolutionbyadding50μLofDMSOtothevialofFAM-LEHD-FMK(ComponentA). 

3.      Add150XFAM-LEHD-FMKintothecellsolutionata1:150ratio,andincubatethecellsina37°C,5%CO₂incubatorfor1hour.

Note1:Thecellscanbeconcentratedupto~5X10⁶cells/mLforFAM-LEHD-FMKlabeling.Theunused150XFAM-LEHD-FMKDMSOstocksolutionshouldbedividedassingleusealiquotandstoredat-20°C.

Note2:Foradherentcells,gentlyliftthecellswith0.5mMEDTAtokeepthecellsintact,andwashthecellsoncewithserum-containingmediapriortoincubationwithFAM-LEHD-FMK.

Note3:Theappropriateincubationtimedependsontheindividualcelltypeandcellconcentrationused.Optimizetheincubationtimeforeachexperiment.

4.      Spindownthecellsat~200gfor5minutes,andwashcellswith1mLwashbuffer(ComponentB)twice.Resuspendthecellsindesiredamountofwashingbuffer.

Note1:FAM-LEHD-FMKisfluorescent,thusitisimportanttowashoutanyunboundreagenttoeliminatethebackground.

Note2:Fordetachedcells,theconcentrationofcellsshouldbeadjustedto2-5X10⁵cells/100μLaliquotpermicrotiterplatewellforuseinstep6.

5.      Ifdesired,labelthecellswithaDNAstain(suchaspropidiumiodidefordeadcells,orHoechstforwholepopulationofthecellnucleusstain).

6.      Monitorthefluorescenceintensitybyfluorescencemicroscopy,flowcytometer,orfluorescentmicroplatereaderatEx/Em=490/525nm(forpropidiumiodide,Ex/Em=535/635nm;forHoechstdyes,Ex/Em=350/461nm).

6.1   Forflowcytometry,monitorthefluorescenceintensityusingtheFL1channel(FL2channelforpropidiumiodidestaining).Gateonthecellsofinterest,excludingdebris.

6.2   Forfluorescencemicroscopyandfluorescentmicroplatereader.Place100μLofthecellsuspensionsintoeachofwellsofa96-wellblackmicrotiterplate. 

Note: Ifitisnecessarytoequilibratethecellconcentrations,adjustthesuspensionvolumefortheinducedcellstoapproximatethecelldensityofthenon-inducedpopulation. Thisadjustmentstepisoptionalifyourcelltreatmentdoesnotresultinadramaticlossinstimulatedcellpopulationnumbers.

6.3   ObservecellsunderafluorescencemicroscopeusingFITCchannel(TRITCchannelforpropidiumiodidestaining,DAPIchannelforHoechststaining). 

6.4   MonitorthefluorescenceintensityusingEx/Em=490/525nm(cutoffat515nm)bottomreadmodeusingafluorescentmicroplatereader.

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