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CHO Centrosome Prep
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ArshadDesai

4/94


Cells:

WegrowourCHOswithMEM[[alpha]](withoutnucleosides)+10%BovineCalfSerumandpenn/strep/glutamine.Foraprepitisbesttogrowtwentylargeplates(150mM)andthecellsshouldbegrowntooverconfluence-tilltheystartpilinguponeachother(youwillneedtofeedthemfrequentlytokeepthemhappy)

ProtocolRationale:

TheprotocolisidenticaltoTim"spublishedinVol134ofMethodsinEnzymology.ThekeystepisthelysiswhichsolubilizescentrosomesawayfromnucleibyverylowionicstrengthlysisaftertreatmentofcellswithnocodazoleandcytochalasinB.ThereleasedcentrosomesarethencentrifugedontoaFicollcushion(toavoidpelleting)andtheinterfacebetweenthelysateandtheFicolliscollectedandthecentrosomesareconcentratedonasucrosegrADIent.FractionsareassayedbyspindownanddoubleIFwith5051serumandanti-tubulinandthepooledfractionsarefrozeninliqN2.


Whatyouneed:

Equipment:

  • refractometer
  • SorvallwithcoldHB-4
  • UltrawithcoldSW27
  • Somesortofgradientfractionatorwithafractioncollector
  • 1630mlcorextubes(cold)

Solutions:

Alotofthesesolutionsarew/w;Timsaysthattomaketheseweighoutsucroseandthenaddbuffertillweightis100g.

Wash&Lysis:

PE:10mMPIPES,1mMEDTA,8mMBME
Makea50XstockandpHto7.2withKOH
LB:1mMTris-HCl,8mMBME
MakeTrisas2MstockandpHto8.0withHCl
LB+0.5%NP-40:
(warmfor30"to37deg.CtoensureNP-40hasdissolved)
PBS:130mMNaCl,2mMKCl.8mMNa2HPO4,2mMKH2PO4
Makea10Xstock

Nightbefore:

Make600mlof

  • 1XPBS
  • 0.1XPBS
  • 0.1XPBS,8%(w/w)ultrapuresucrose
  • 8%(w/w)ultrapuresucrose
  • LB(w/oBME):add280ulBMEbeforeuse
  • LB+0.5%NP-40(w/oBME):add280ulBMEbeforeuse

andputallthesebuffersincoldroom

SucroseGradients:

Useultrapuresucrose

20%(w/w)and62.5%(w/w)sucrosein1xPE+0.1%TX-100.Make100gramsofeachasfollows:
Weighoutsucroseandthenonthebalanceadd1XPE+0.1%TX-100tillweightis100grams.

Justbeforepouringgradientsadd28ulBME/50g

Pourgradientsnightbeforeorduringdrugtreatment(seelater).Ifinditeasiesttopournightbeforeandstoreincold.

Topourgradients-firstputa5mlheavysucrosepadandthenpourgradientontopofthat.FortheprepoutlinedbelowIpour2gradientsinSW27tubes:
4mlheavysucrosepad(use62.5%orhigher).
16mlgradient.

Thecentrosomesareveryclosetothebottomofthisgradient.Thepadeliminatesthemfromenteringthecurveofthetubeandalsogivesalittleleewayinsettingupthefractionation.

Ficollcushion:

20%(w/w)Ficoll(MW400,000)in1XPE+0.1%NP-40

  1. MakeupPE+0.1%NP-40(noBME).
  2. Weighout10gFicoll.
  3. AddPE+0.1%NP-40tilltotalweight=50grams.
  4. StiratRTforseveralhourstodissolveandstorecold.
  5. Beforeuse,add28ulBME

Protocol:

  1. Warmup300mlofCHOmediumto37deg.CandaddcytochalasinB(150ulof10mg/ml)andnocodazole(300ulof10mg/ml)
  2. Makesureallbuffersareincoldroom,thereisrockerinthecoldroomandthereisagoodaspiratorinthecoldroom.HookupasawedoffpipettotheaspiratorandmakesurethereisaLARGEtrap(atleast4L)
  3. Addmediumwithdrugsto10platesofcells.Addmediumwithdrugstotheother10plates45"later.
  4. After90"indrugmediumprocessfirst10plates:bringtocoldroomandwashwiththefollowingbuffers:
    1XPBS
    0.1XPBS,8%(w/w)sucrose
    8%(w/w)sucrose
    LB
    andthenpipeton
    LB+0.5%NP-40(10mls/plate)

    (Thesewashesmustbedonerapidly-allwashesshouldbeunder1"perplate.ThewayIdothemistopouronthewashbufferfromabeakerorgradcylinder(~30mls),immediatelyrockbackandforthandaspirateASAPbeforepouringonthenextwash.Itiscriticaltodothisquicklytogetgoodlysisoryouwilllosemostofthecentrosomesinthenuclearpellet).AfteraddingtheLB+0.5%NP-40transfertheplateontoarockerinthecoldroom.

  5. After10"pipetoffthelysateintoa30mlcorextube.Add1/50volof50XPE(0.5mlfor25mls;withBME)
  6. SpintubesinHB-4for3"at3000rpmat4deg.C
  7. Transfersupetoafreshcorextubeandunderlaywith2mlofFicollcushion(Iusea6ccsyringewith16gaugeneedlewithathinpieceoftygontubingwhichIcanslidetothebottomofthetube).
  8. Spinat12,700rpmfor15at4deg.Cfor15".Assoonasspinisstarted,processthenextsetofplatesthroughsteps4-7.
  9. Aspiratesupetillapprox.2mlabovecushionandthencollectinterfacewithapasteur-seeTim"sprotocol.Collect~2ml/tubeandpool.CheckFicollconcentrationbyrefractometryanddiluteto10%(w/w)orlower-necessarytomakesureitlayersontothesucrosegradientanddoesn"tsink.
  10. Finishcollectinginterfacesfromsecondsetofplatesandthenpoolallcollectedinterfaces,ensureFicollis<10%(w/w)andloadonto1gradient.Spin1hr-1hr30",SW27at2deg.C.
  11. Fractionategradientfrombottom-0.3-0.5mlfractionsandreadsucroseconcentrationbyrefractometry.Assayfractionsbetween48and60%(w/w)sucrose.5uloffraction+5mlPE-mixwellandpelletontocoverslips:12,500rpmfor15"at4deg.CinHB-4.Postfixinmethanol(-20deg.C)for5"andrehydrateanddo5051+antitubulinfollowedbyanti-mouse,anti-humansecondaries.Assesspeakbyconcentrationofdoublestainingdots,poolandfreezeinliqN2in10ulaliquots.

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