Overview

PrinterFriendlyVersion

Warning:Donotaddadditionalprobenecid.ItisrecommendedtoincubatethedyeloADIngsolutionnolongerthan2hours.

1.Preparecells:

1.1   Foradherentcells:Platecellsovernightingrowthmediumat40,000to80,000cells/well/100µLfora96-wellplateor10,000to20,000cells/well/25µLfora384-wellplate.

1.2   Fornon-adherentcells:CentrifugethecellsfromtheculturemediumandthensUSPendthecellpelletinFluo-8NWdye-loadingsolution(seeStep2.4)at125,000to250,000cells/well/100µLfora96-wellpoly-Dlysineplateor30,000to60,000cells/well/25µLfora384-wellpoly-Dlysineplate.Centrifugetheplateat800rpmfor2minuteswithbrakeoffpriortotheexperiments.

Note:Eachcelllineshouldbeevaluatedonanindividualbasistodeterminetheoptimalcelldensityfortheintracellularcalciummobilization.

2.PrepareFluo-8NWdye-loadingsolution(foroneplate):

2.1   Thaw1vialofFluo-8NW(ComponentA),1bottleof10XPluronic^®F127Plus(ComponentB)andHHBS(ComponentC)atroomtemperaturebeforeuse.

2.2   MakeFluo-8NWstocksolution:Add10µL(forCat.#36307)or100µL(forCat.#36308and#36309)ofDMSOintoFluo-8NW(ComponentA),andmixthemwell.

Note:10µLofFluo-8NWstocksolutionisenoughfor1plate.UnusedFluo-8NWstocksolutioncanbealiquotedandstoredat<-20^oCformorethanonemonthifthetubesaresealedtightly.Protectfromlightandavoidrepeatedfreeze-thawcycles.

2.3   Make1Xassaybuffer:

a).ForCat.#36307(1platekit)and36308(10plateskit),make1Xassaybufferbyadding9mLofHHBS(ComponentC)into10XPluronic®F127Plus(1mL,ComponentB),andmixthemwell.

b).ForCat.#36309(100plateskit),make1Xassaybufferbyaddingthewholebottleof10XPluronic®F127Plus(10mL,ComponentB)into90mLofHHBSbuffer(notincludedinthekit),andmixthemwell.

Note:10mLof1Xassaybufferisenoughforoneplate.Aliquotandstoreunused1Xassaybufferat<‑20 ^oC.Protectfromlightandavoidrepeatedfreeze-thawcycles.

2.4   MakeFluo-8NWdye-loadingsolutionforonecellplate:Add10µLofFluo-8NWDMSOstocksolution(fromStep2.2)into10mLof1Xassaybuffer(fromStep2.3),andmixthemwell.Thisworkingsolutionisstableforatleast2hoursatroomtemperature.

3.Runcalciumassay:

3.1   Removethegrowthmediumfromthecellplate.

Note1:Itisimportanttoremovethegrowthmediuminordertominimizebackgroundfluorescence,andcompoundinterferencewithserumorculturemedia.

Note2:Alternatively,growthecellsingrowthmediumwith0.5-to1%FBStoavoidmediumremovalstep.Inthiscase,2XdyeloadingsolutioninHHBSbufferisneeded.[Weoffer2separatenowashcalciumassaykits(Cat.#36315andCat.#36316)forthosewhouse0.5-to1%FBSingrowthmediumtoavoidthemediumremovalstep].

3.2    Add100µL/well(96-wellplate)or25µL/well(384-wellplate)ofFluo-8NWdye-loadingsolution(fromStep2.4)intothecellplate(fromStep3.1).

3.3    Incubatethedye-loadingplateinacellincubatorfor30minutes,andthenincubatetheplateatroomtemperatureforanother30minutes.

Note1:Iftheassayrequires37^oC,performtheexperimentimmediatelywithoutfurtherroomtemperatureincubation.

Note2:Ifthecellscanfunctionwellatroomtemperatureforlongertime,incubatethecellplateatroomtemperaturefor1-2hours(Itisrecommendedthattheincubationtimebenolongerthan2hours.)

3.4    PreparethecompoundplateswithHHBSoryourdesiredbuffer.

3.5   RunthecalciumfluxassaybymonitoringthefluorescenceintensityatEx/Em=490/525nm.

Note:Itisimportanttorunthesignaltestbeforeyourexperiment.Differentinstrumentshavetheirownintensityrange.Adjustthesignaltestintensitytothelevelof10%to15%ofthemaximumintensitycounts.Forexample,themaximumfluorescenceintensitycountforFLIPR-384is65,000,sotheinstrumentsettingshouldbeadjustedtohaveitssignaltestintensityaround7,000to10,000.

References&Citations

CitationExplorer