Product Overview
PCR amplification of DNA fragments, DNA labeling, primer extension, sequence determination, blunt end addition of A, TA vector cloning
Product Information | |
---|---|
Molecular Weight | 94 KD |
Polymerase Activity | 5′-3′ DNA polymerase, 5′-3′ exonuclease (no 3′-5′ exonuclease) |
PCR Buffer | 10 X PCR Buffer for direct loading |
Experimental Efficiency | The PCR reaction can be directly detected by electrophoresis |
Extension Speed | 1-2 kb/min |
Terminal Base | Product has A at the 3′ end, facilitating TA vector cloning |
Reaction System (20μl) | Addition Amount | Remarks |
---|---|---|
Pure DNA Polymerase | 0.8μl | Adjust for amplification needs |
10x PCR Buffer | 2μl | |
dNTP (2.5mM) | 2μl | |
PrimerF | 0.1-1μl | 10-50pmol used |
PrimerR | 0.1-1μl | 10-50pmol used |
Template | <1μg | |
ddH2O | Up to 20μl |
Cycle Program | Temperature (°C) | Time | Remarks |
---|---|---|---|
Initial Denaturation | 94 | 3min | |
Denaturation | 94 | 30s (30-40 ciklusi) | |
Annealing | 45-60 | 30s | |
Extension | 72 | 30s-2min | Extension time varies with fragment |
Final Extension | 72 | 10min |
Procedure
Can be directly detected without adding a Loading Buffer
Result Detection
Nakon PCR-a, take 5 μl of product for agarose gel electrophoresis
Recenzije
Još nema recenzija.