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Preparation of Segmented and Polarity Marked Microtubules
Segmentedandpolarity-markedmicrotubulesareveryusefulformanydifferenttypesofinvitroassays.Segmentedmicrotubulesaremicrotubuleswithabrightseedanddimelongatedsegmentsonbothends.Polaritymarkedmicrotubulesaremicrotubuleswithabrightseedandadimelongatedsegmentonlyononeend--theplusend.SelectiveelongationofoneendisachievedbyinclusionofNEM-treatedtubulin,acompetitiveinhibitorofminusendpolymerization.MorecomplexmicrotubulesubstratessuchasGDPmicrotubulelatticescappedwithsegmentsofGMPCPPtubulincanalsobepreparedbyplayingaroundwithinvitropolymerizationconditions.Also,segmentedandpolaritymarkedmicrotubulescanbemadefromdifferentcolortubulinsinsteadofdifferentintensityofasinglecolortubulinasdescribedhere.
Notethatthepreciseratiosoflabeledtounlabeledtubulindescribedheremayneedtobeadjusteddependingonthelabeledtubulinprep.DescribedhereiswhathasworkedwellforususingtetramethylrhodamineNHSester-labeledtubulin(stoichiometryoflabeling~1.4).
- I.Solutions&Supplies
- II.SegmentedTaxolMicrotubules
- III.PolarityMarkedTaxolMicrotubules
- IV.SegmentedGMPCPPMicrotubules
- V.PolarityMarkedGMPCPPMicrotubules
Backtoprotocols
I.Solutions&Supplies
BRB80(1X):80mMPIPES,1mMMgCl2,1mMEGTA,pH6.8withKOH(generallymadeasa5Xstockandstoredat4¡C)
100mMGTP
100mMGMPCPP
Taxol:10mMstock;200µM,20µMand2µMdilutionallinanhydrousDMSO;soldundertradename"Paclitaxel"bySigma
BrightGMPCPPSeedMix(2mg/ml;1partrhodaminetubulinto2partsunlabeledtubulin;preparedandstoredat-80¡Casdescribedabove)
NEMGTP-Tubulin(preparedbytreatingrecycledtubulin(~5-15mg/ml)inBRB80+0.5mMGTPwith1mMNEM(N-ethylmaleimide;fromafresh50mMstockinwaterpreparedjustbeforeuse)for10"at0¡C,quenchingtheNEMwith8mMb-mercaptoethanolfor10"at0¡C,freezingaliquotsinliquidnitrogenandstoringat-80¡C.
NEMCPP-Tubulin(preparedbytreatingrecycledtubulin(~5-15mg/ml)inBRB80+0.5mMGMPCPPwith1mMNEM(freshlypreparedasa50mMstockinwater)for10"at0¡C,quenchingNEMwith8mMb-mercaptoethanolfor10"at0¡C,freezingaliquotsinliquidnitrogenandstoringat-80¡C.
II.SegmentedTaxolMicrotubules
1.PolymerizebrightGMPCPPseedmixat37¡Cfor15"-30".
2.Onicepreparethedimelongationmixconsistingof15µMtubulin(1partrhodaminetubulinto10partsunlabeledtubulin)in1XBRB80,1mMDTT,1mMGTP.Incubateat0¡Cfor5"and(optionally)clarifyat90Kfor5"at2¡CinaTLA100rotor.
3.Incubatedimelongationmixat37¡Cfor1".Add1/10-1/20volumeofGMPCPPseedsandmixgently.Incubateat37¡Cfor20".GMPCPPseedsarecold-lABIleandwilldepolymerizeonice.Therefore,onlyaddtheseedsaftertheelongationmixhaswarmedup.
4.Addtaxolstepwiseto20µM.
5.Thesegmentedtaxol-stabilizedmicrotubulescanbepelletedoveraglycerolcushionandresUSPended,oruseddirectlyafterdilution.Alldilutionsoftaxol-stabilizedMTsshouldbedoneintobufferscontaining10-20µMtaxol.
III.PolarityMarkedTaxolMicrotubules
1.PolymerizebrightGMPCPPseedmixat37¡Cfor15"-30".
2.Onicepreparethedimpolarelongationmixconsistingof15µMtubulin(1partrhodaminetubulinto10partsunlabeledtubulin)and12µMNEMGTP-tubulinin1XBRB80,1mMDTT,1mMGTP.Incubateat0¡Cfor5"and(optionally)clarifyat90Kfor5"at2¡CinaTLA100rotor.
3.Incubatedimpolarelongationmixat37¡Cfor1".Add1/10-1/20volumeofGMPCPPseedsandmixgently.Incubateat37¡Cfor20".
4.Addtaxolstepwiseto20µM.
5.Thepolarity-markedtaxol-stabilizedmicrotubulescanbepelletedoveraglycerolcushionandresuspended,oruseddirectlyafterdilution.Alldilutionsoftaxol-stabilizedMTsshouldbedoneintobufferscontaining10-20µMtaxol.
IV.SegmentedGMPCPPMicrotubules
1.PreparedimGMPCPPElongationMix:10µM(1mg/ml)1:9rhodaminelabeled:unlabeledtubulinin1XBRB80,1mMDTT,0.5mMGMPCPP.Incubateonicefor5"-10",spin90K5"inTLA100at2¡C,freezeinliquidnitrogenin10µlaliquots(orusefresh).
2.ThawGMPCPPbrightseedmixbyadding9volofwarm(37¡C)BRB80+1mMDTT(resultingin2µMtubulinfinal)andincubateat37¡Cfor30"-45".
3.ThawCPPelongationmixandstoreonice.Diluteasfollowsonice:17µlBRB80+1mMDTT3µlCPPelongationmix(Thisresultsinelongationof~1.5µMCPP-tubulin)
4.IncubatedilutedCPPelongationmixat37¡Cfor20secbeforeadding2µlofpolymerizedbrightCPPseeds.
5.Incubateat37¡Cfor1-2hours.Pelletandresuspendorusedirectly.
V.PolarityMarkedGMPCPPMicrotubules
1.PreparedimGMPCPPpolarelongationmix:10µM(1mg/ml)1:9rhodaminelabeled:unlabeledtubulinand8µMNEMCPP-Tubulinin1XBRB80,1mMDTT,0.5mMGMPCPP.Incubateonicefor5"-10",spin90K5"inTLA100at2¡C,freezeinliquidnitrogenin10µlaliquots(orusefresh).
2.ThawGMPCPPbrightseedmixbyadding9volofwarm(37¡C)BRB80+1mMDTT(2µMtubulinfinal)andincubateat37¡Cfor30"-45".
3.ThawCPPpolarelongationmixandstoreonice.Diluteasfollowsonice:17µlBRB80+1mMDTT3µlCPPPolarElongationMix(Thisresultsinelongationof~1.5µMCPP-tubulin)
4.IncubatedilutedCPPpolarelongationmixat37¡Cfor20secbeforeadding2µlofpolymerizedbrightCPPseeds.
5.Incubateat37¡Cfor1-2hours.Pelletandresuspendorusedirectly.
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