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小片段RNA抽提纯化试剂盒(HybridR miRNA)
来自 : mayitao
货号:325-106;325-150
英文名:Hybrid-RmiRNA
保存条件:Roomtemperature(15~25℃)/4℃(RiboEx)
Cat.No. ProductDescriptionSize
325-106Hybrid-RTM miRNA6
325-150Hybrid-RTM miRNA50
 



Description
 
Inrecentyears,interestinsmallRNA,suchassiRNAandmiRNAwhicharerelatedtoresearchofgeneregulation,hasexpanded.TherearemanycommercialkitsfortotalRNApreparation,butmostofthesearefocusedonpreparationoflargeRNAlongerthan200nucleotides.BecausebothsiRNAandmiRNAarebetween15~30nucleotidesinlength,theneedofspeciallyoptimizedkitforsmallRNA(<200nucleotides)isgrowingrapidly.Hybrid-RTM miRNAisdesignedforpurificationoflargeandsmallRNAseparatelyfromculturecellsoranimaltissuesandco-purificationinasingletubeisalsoavailablebymodifiedprotocol.ThiskitutilizesthelysismethodofRiboExTM whichhasapowerfulabilityoflysisandthepurificationmethodbasedonglassfibermembranetechnology.SamplesarehomogenizedinRiboExTM,amonophasicsolutioncontainingphenolandguanidiumsalt,whichrapidlylysecellsandinactivatesnucleases.Additionofchloroformbringsaboutaseparationofthelysateintoaqueousandorganicphases.TotalRNAlocatesintheaqueousphasewhileDNAandproteinremainintheinterphaseandorganicphase.LargeandsmallRNAintheaqueousphaseisselectivelyboundtocolumntypeBandtypeWrespectively.ThecolumntypeBselectivelyadsorbstheRNAlargerthan200nucleotidesinlength,whilethecolumntypeWspecificallyholdstheRNAsmallerthan200nucleotidesinlength.TopurifylargeRNA,theaqueousphaseismixedwithethanolandthemixtureisappliedtoacolumntypeB.Aftercentrifugation,largeRNAisboundtomembraneandthemixturecontainingsmallRNAgoesintocollectiontubethroughthemembrane.Themembraneiswashedawaybytwowashbuffer(SW1andRNW)andpurifiedlargeRNAiselutedfromthemembranebyRNase-freewater.TopurifysmallRNA,thepass-throughcomefromthebindingoflargeRNAismixedwithethanolandthenappliedtoacolumntypeW.AfterwashingwithbufferRBWandRNW,smallRNAiselutedbyRNase-freewater.TheprocedureofHybrid-RTM miRNAtakesonly30minutesforcompletepreparationsofpureRNA.ThepurifiedRNAissuitablefortheisolationofPolyA+RNA,northernblotting,dotblotting,invitrotranslation,cloning,RT-PCR,RPAandotheranalyticalprocedures.
 



FeaturesandBenefits
 
■Preparationtime:~30minutes
■Stableandconsistentyield
■Highpurityandyield
■PerfectseparationofsmallRNAfragment
■Samplesize:Upto50mgtissueorupto1x107 culturedcells
■Recoveryrange:LargeRNA:>200nucleotides
          SmallRNA:<200nucleotides
■Instantuse:Noneedofadditionalmaterials
■Noethanolprecipitation
■NoGenomicDNAcontamination
■Readyforuseinnorthernblotting,dotblotting,invitrotranslation,cloning,RT-PCR,RPAandother analyticalprocedures
 


Procedure


 
温馨提示:不可用于临床治疗。
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