T4DNALigasecatalyzestheformationofaphosphodiesterbondbetweentheterminal5′phosphateand3′hydroxylgroupsofduplexDNAorRNA.TheenzymeefficientlyjoinsbluntandcohesiveendsandrepairssinglestrandednicksinduplexDNA,RNAorDNA/RNAhybrids.

10XT4DNALigaseBufferiscomposedof500mMTris-HCI,100mMMgCl₂,50mMdithiothreitol,10mMATP,pH7.6@25°C.

2XRapidLigationBufferiscomposedof132mMTris-HCI,20mMMgCl₂,2mMdithiothreitol,2mMATP,15%PEG,pH7.6@25°C.

Figure1: Purity ThepurityoftheT4DNAligaseisequalorgreaterthan95%asjudgedbySDS-polyacrylamidegelelectrophoresiswithCoomassiebluestaining. MolecularweightMarkersareinLane1. T4DNAligasewasloadedat5units(Lane2)and10units(Lane3).

Figure2: ExonucleaseandEndonucleaseActivityAssay TheT4DNAligaseisfreeofdetectableofexo-andendonucleaseactivities,asjudgedbyagarosegelelectrophoresisfollowingincubationof10unitsofenzymefor16hoursat37°Cwith1µgofHindIII-digestedλDNA(Lanes3and4)andsupercoiledpUC19DNA(Lanes5and6). MolecularweightmarkersareinLanes1and2.

UnitDefinition:OneWeissUnitisdefinedastheamountofenzymerequiredtoconvert1nmolof³²P-labeledinorganicpyrophosphateintoNoritadsorbablematerialin20minutesat37°C,usingspecifiedreactionconditions.Note:1WeissUnitisapproximately67cohesiveendunits.

Source:ArecombinantE.colistraincarryingtheclonedT4DNALigasegene.

ORDERINFORMATION

Storagebuffer:T4DNALigaseissuppliedin10mMTris-HCl,50mMKCl,1mMdithiothreitol,0.1mMEDTA,0.1%TritonX-100,50%glycerol,pH7.5@25°C.