Plasmid DNA | 5 μl (500ng) | |
MQ | 3 μl | |
CutSmart Buffer | 1 μl | |
Enzyme | 0.5 μl each | |
10 μl total |
Note: check that you use enzymes that work at the same temperature as the incubating temperature (on snapgene)!
To find out if DigLig worked and the inserts are in plasmids correctly, we choose restriction enzymes for the plasmids so that one of the restriction sites lies on the insert and the other one accordingly on the backbone to produce unequal cuts. It is of course also possible to generate more than two fragments. That way, if the insert was inserted correctly, the digestion should produce distinguishable bands at different positions relative to the ladder.
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