Pfu/Psp red DNA Polymerase RTL
Pfu DNA polymerase (RTU=READY-TO-LOAD) is a convenient Mixture of proof-reading Enzyme, red dye and loading buffer. It generated PCR fragments exhibits the lowest error rate of any thermostable DNA polymerases. The fragements are blunt-ended for direct ligation
| Cat.-no | Description | Amount | Price € | Shop |
| S127 | Pfu/Psp RTL DNA Polymerase | 1x250 units | 65.00 | add |
| S119 | Pfu/Psp RTL DNA Polymerase | 2x250 units | 125.00 | add |
| S120 | Pfu/Psp RTL DNA Polymerase | 10x250 units | 570.00 | add |
Pfu/Psp red (RTL) DNA Polymerase: Order/request by E-mail:
Pfu/Psp red (RTL) DNA Polymerase: Datasheet RTL = ready-to-load
Pfu/Psp red (RTL) DNA Polymerase: Deutsche Beschreibung
Features:
Pfu/Psp DNA polymerase replicates DNA at 75°C catalyzing the polymerization of nucleotides into duplex DNA in the 5´→3´ direction in the presence of Mg+. Pfu DNA polymerase possesses 3' to 5' exonuclease proof reading activity that enables the polymerase to correct nucleotide-misincorporation errors. For visual control and for fast loading on the gel the enzyme contains a red dye and loading buffer for agarose electrophoresis.
Applications:
- blunt end PCR cloning
- PCR and primer extension where "high fidelity" is required
- Site-directed mutagenesis
- PCR where visual control is needed
Description:
Pfu/Psp DNA polymerase ready-to-load is isolated from the archae bacteria Pyrococcus f-species is a thermostable Polymerase of approximately 90000 daltons. Base misinsertions that may occur during polymerization are rapidly excised by the proofreading activity of the polymerase. The Pfu/Psp DNA Polymerase has no detectable reverse transcriptase activity.
Concentration: (1 u/µl)
Unit definition:
One unit is defined as the amount of enzyme required to catalyze the incorporation of 10 nM of dNTPs into acid insoluble material in 30 minutes at 75°C.
Storage Buffer:
50 mM Tris-HCl, pH 8.2, 0.1 mM EDTA, 0.1% Tween 20, 0.1% Nonident P40, 1 mM DTT, 50% Glycerol and red dye
Reaction Buffer 10 X:
100 mM KCl, 160 mM (NH4)2SO4, 20 mM MgSO4, 200 mM Tris-HCl, pH8.8, 1% Triton X-100, 1 mg/ml BSA
Quality control:
- Tested for the DNA amplification of 2,2 kb from lambda DNA
- Contamination level check of bacterial DNA
- Purity by SDS-Page > 90 %
Usage:
Standard protocol:
- Do not use dUTP or dITP or primers containing these nucleotides
| Components | Volume per reaction | end conc. |
| 10X reaction buffer with MgSO4 | 5 µl | 1X |
| dNTP-Mix (40mM = 10mM each) | 1.0 µl | 200 µM each |
| Up-stream primer (e.g. 20 µM) | 0,5 µl | 0.1-1.0 µM |
| Down-stream primer (e.g. 20 µM) | 0.5 µl | 0.1-1.0 µM |
| Template DNA (10 ng/µl) | 1.0 µl | <= 0,5 µg |
| Pfu/Psp DNA Polymerase (1 u/µl) | 1 - 2 µl | 1-2 units |
| Sterile dest. Water (molecular grade) | up to 50 µl |
Note:
- vortex all solutions carefully before using
- dispense all reagents on ice to avoid degradation of primers and dNTP's
- add the enzyme after Template DNA
- may you have to optimize the MgSO4 concentration for best result
General Thermo-Cycler protocol:
| Step | Time | Temperature |
| Initial denaturation | 1-3 min | 95°C |
| 25-35 Cycles: Denaturation Annealing Extension |
30-100 sec 30-65 sec 1-2 min (per 1 kb) |
95°C 37-69°C 72-75°C |
| Final extension | 5 min | 72-75°C |
Loading on the gel:
Recommended volume is 10 µl of reaction mixture
Storage: at -20°C for 24 months
Transportation: on blue ice
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