Team:Peking S/team/protocol
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Protocol
Double Digestion |Gel Extraction|Miniprep | Chemical Inducible Expression of GFP |DNA Purification |Ligation of Insert DNA | PCR |Preparation of Competent Cells| Site-directed Mutagenesis| Transformation|
DNA Double Digestion Protocol
Materials:
- DNA sample(s) in water or TE buffer
- 10x digestion buffer
- Restriction enzymes (EcoRI or SpeI or XbaI or PstI)
- DNA loading buffer (if electrophoresis is subsequent)
- Agarose gel 1.5% (or different depending on expected band sizes)
Procedure:
1. Test the concentration of the DNA sample(s).
2. Pipet the following into a microfuge tube:
20uL reaction system 50uL reaction system
DNA around 1ug around 2.5ug
10x Digestion buffer 2uL 5uL
1st Enzyme 1-1.5uL 2.5-4uL
2ndEnzyme 1-1.5uL 2.5-4uL
ddWater Rest of volume Rest of volume
3. Incubate at recommended temperature (37.0 degrees) for 2 or 4 hours (0.5~2hfor enzymes of NEB, 4h for enzymes of Takara).
4. Take 2 to 5 uLof the digested sample, add loading buffer, and run it on the agarose gel to check the result, or take the entire sample to run to extract a wanted fragment).
Tips:
1. DNA:
- For identification of DNA, use 0.4 ug/uL DNA; (or 2uL from a nice DNA mini prep)
- For cloning, 1ug/uL DNA is enough.
2. Buffer: we’d better use the buffer that comes with the enzyme, which means buffers from other company may cause some abnormal results.
3. Enzyme: the maximum volume that an enzyme can be used is 1/10 of the total reaction volume (example: 2 uL for 20 uL reaction system). If you want to do overnight digestion, add less enzyme (example: 1 uL for 20 uL reaction system). It is necessary to point that too many enzymes will reduce the efficiency of enzyme digestion with glycerol in it.
4. Gel: make sure to run the uncut DNA as a control along with the digested DNA sample(s). And, always run a DNA marker!
References:
- Current protocols in molecular biology (3.1.1-3.1.2)