Source 

Thermusaquaticus

Description

• Thermostableenzymeofapproximately94kDafrom Thermusaquaticus
• Ultrapure,Recombinantprotein

Applications

• RecommendedforuseinPCRandprimerextensionreactionsatelevatedtemperaturestoobtainawiderangeofDNAproducts upto10Kb
• TaqDNAPolymeraseenzymereplicatesDNAat74°Candexhibitsahalf-lifeof40minutesat95°C(1,2)
• TaqDNAPolymerasecatalyzesthepolymerizationofnucleotidesintoduplexDNAinthe5"→3"directioninthepresenceofmagnesiumions
• Maintainsthe5"→3"exonucleaseactivity
• Lacksthe3"→5"exonucleaseactivity

ReagentsSupplied

10XTaqBufferA
10XTaqBufferB
10XTaqBufferC 

UnitDefinition 

Oneunitisdefinedastheamountofenzymerequiredtocatalyzetheincorporationof10nmolesofdNTPintoacid-insolublematerialin30minutesat70°C

10XReactionBuffer

10XTaqBufferA(optimizationbufferwithoutMgCl₂):BufferallowstooptimizeMgCl₂ concentration
10XTaqBufferB(generalapplication,upto10kb):Buffercontains15mM MgCl₂ andis optimizedforusewith0.2 mMofeachdNTP
10XTaqBufferC(colored): 10XTaqBufferBEnrichedwithtwogeltrackingdyesandagelloADIngreagent;EnablesdirectloadingofPCRproductsontoanagarosegel

AssayConditions

25mMTris-HCl(pH9.5at25°C)
50mMKCl
10mMMgCl₂
1mMdithiothreitol
200μMeachofdCTP,dGTP,dTTP,anddATP(amixofunlabeledand[α-³²P]dATP)
10μgactivatedcalfthymusDNA 
1mg/mlbovineserumalbumin
15 µgactivatedcalfthymusDNA
Totalreactionvolumeis50 µl

QualityControl

Allpreparationsareassayedforcontaminatingendonuclease,3"-exonuclease,andnonspecificsingle-anddouble-strandedDNaseactivities
Typicalpreparationsaregreaterthan95%pure,asjudgedbySDSpolyacrylamidegelelectrophoresis

StorageConditions

Storeat-20°C
Shippedondryice 

Downloads

MSDSPDF

References

1.Chien,A.,Edgar,D.B.andTrela,J.M.(1976)J.Bacteriol.127,1550
2.Kaledin,A.S.,Sliusarenko,A.G.andGorodetskii,S.I.(1980)Biokhimiya45,644