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Monoclonal Antibody Production

MouseImmunization

Order6sixweekoldBalb/CmiceandlettheARCknowtheyarecoming.Haveyourantigenreadyforwhentheyarrive.Oncetheygetthereearmarkthemiceandperformapre-bleedonthemtobeusedasanELISAcontrolformonitoringthetiterandscreeningofthehybridomas:

BleedingMice

  1. Placethemouseinamouserestrainer.
  2. Sterilizethetailwith70%ethanol.
  3. Witharazorblade,nipoffthelast2mmofthetipofthetail.
  4. Usingamilkingmotion,pullblooddownandletdripofftheendofthetailuntilyouhavecollected~200µL.(Youmayhavetopre-bleedtwice,withaweekorsobetweenbleeds).
  5. Takethecollectedbloodandplaceat37°Cfor30min.toremovecomplement.
  6. Placebloodat4°Covernighttoclot.
  7. Centrifugesamplesat10,000g10min.
  8. Pipetofftheserumsupernatant.Storeat-20°C.Thisisyourpre-bleedcontrol.

HybridomaFusion

Foronefusionyouwillneed:

  1. 8500mLbottlesofDMEMmedia
  2. 3500mLbottlesoffetalcalfserum(FCS)
  3. 250mLbottlesof100Xpenicillin-streptomycin
  4. 10mLof100XHATselectionsolution
  5. 10mLof100XHTsolution
  6. 10sterileflat-bottomed96-wellplates

AssayingforPositiveClones

RunanELISA.html">indirectELISAusingtheantigenyouwanttheMAbdirectedagainst.IfyouareraisingtheMAbsagainstasmallhaptenthatyoucoupledtoacarrierproteinforimmunizationofthemice,thenusethehaptencoupledtoadifferentcarrierproteinforthescreen.

ExpandingPositiveClones

  1. Thedaypriortoanyexpansion,obtainfeedercells.Forthisfirstexpansionfromthe200µLculturesin96-wellplatesto500µLculturesin24-wellplates,add200µLoffeedercells/wellinDMEM/20%FCSHTtothe24-wellplatesthedaybeforeexpansion.LetthefeedercellsgrowovernightintheCO2incubator.
  2. Fortheinitialexpansion,resUSPendthepositivetestinghybridomacellsandplaceallbutthelast10µL(200µL)inthewellofthe24-wellplatewiththefeedercells.Thenbringto500µLwithDMEM/20%FCSHT.
  3. Add200µLofDMEM/20%FCSHTtothelittlebitofcellsleftinthe96-wellplate.Thisservesasabackupforyourpositiveclones.
  4. PlaceallplatesintheCO2incubator.
  5. Whenthecellsarebeginningtoacidifythemedia(getsorange-yellow),changethemediaanddoubletheculturevolumebypipettingoff400µL,andreplacewith900µLfreshDMEM/20%FCSHT.
  6. Harvestmorefeedercellsforyournextexpansion.Put0.5mLffeedercellsinDMEM/20%FCS(notetheremovaloftheHT)inaT25flask(oneforeachpositiveclone)forlateruse
  7. Whenthecellsarereadyforexpansionoutofthe24-wellplate,resuspendthemandpipettotheT25flaskswithfeedercells.Againleavealittlebitinthe24-wellplateandrefillwithDMEM/20FCSasabackup.VolumetotheT25culture5mLwithDMEM/20%FCS(add3.5mL)Placeallculturesintheincubator.


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