Richard Lab:Restriction Digest: Difference between revisions

Revision as of 10:36, 23 June 2009

This protocol is typically used to do bio-brick digests with the restriction sites consisting of the following configuration:

-----EcoRI--XbaI--Part--SpeI--PstI-----

Prepared DNA from miniprep, PCR, or Gel Extraction
Restriction Endonucleases
- With corresponding 10X buffer. NEBuffer 2 can be used for most applications but check this chart to be sure.
BSA (optional)
Phosphatase
Distilled water

Quickly vortex all ingredients (Buffer, BSA, DNA, Enzymes) before beginning
Add the following in a micro-centrifuge tube
1. 5μl of Buffer
2. 1μl of BSA
3. 40μl of DNA solution (Dilute PCR products 1:4)
Vortex Enzymes and add 20 units (1μl) of each to the tube
Incubate reaction in a 37°C water bath for at least one hour (I like 1:45).
Heat kill the digest for 15 minutes at 75°C.
If digesting a vector add 10 units (1µl) phosphatase) and 5µl Phosphatase Buffer and incubate an additional 45 minutes at then heat kill againat 75°C for 15 min.
Store digested DNA in the freezer (-20°C).

Please feel free to post comments, questions, or improvements to this protocol. Happy to have your input!

If you're not getting good digestion it might be because your enzyme is bad. Double the digestion time and see.
Longer digest gives more complete digestion, especially if you have >1µg of DNA, but can sometimes give nonspecific digestion

For more information you can check out the other restriction digest protocols.

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 ==Overview==
 This protocol is typically used to do bio-brick digests with the restriction sites consisting of the following configuration: