Difference between revisions of "Team:Freiburg/Protocols/Restriction"

 
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Latest revision as of 07:05, 20 November 2015

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Restriction digest

Restriction enzymes are a basic component of classical cloning methods. They have the ability to induce DNA double strand breaks at specific sites leaving a characteristic overhang. By cutting two sequences with the same enzyme and thus producing compatible overhangs, these can be assembled in an easy way. DNA ligases can then be used to covalently link the fragments.
Restriciton digests are commonly used for two purposes. One is extract a desired fragment out of a whole plasmid to further use it for subcloning purposes (preparative digest). Another possibility to make use of a restriction digest is to verify successful insertion of a fragment by comparing the resulting fragments to theoretical expectations (analytical digest).

DNA Restriction Digest

Material: restriction endonucleases (store on ice), buffer, dH2O, heat block or incubator (37°C)
Duration: 2.5 h

The amount of DNA that is used for a reaction is dependent on the purpose. For an analytical digest, about 500 ng of DNA are sufficient to visualize the result on an agarose gel. If you aim to extract the DNA after agarose gel analysis, 2 - 3 µg of DNA can be used to obtain high yields.

Mix

Ingredient
Volume / Mass
DNA
2 - 3 µg
Restriction enzyme
1 µl each
BSA 100x (optional)
0.5 µl
NEB buffer 10x
5 µl
dH2O
ad 50 µl
Incubate at 37 °C for at least 2 h. If there are more than 2 recognition sites per enzyme, incubate for more than 2 h!