IGEM:UC Berkeley/2006/Analitic digestion: Difference between revisions
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#***.25 uL enzyme 1 | #***.25 uL enzyme 1 | ||
#***.25 uL enzyme 2 | #***.25 uL enzyme 2 | ||
#*** | #***1 uL BSA | ||
#***5.5 uL water | |||
#*If DNA product is low copy then use 4uL of product and 1uL of NEB2 adjusting the H2O and enzyme accordingly: | #*If DNA product is low copy then use 4uL of product and 1uL of NEB2 adjusting the H2O and enzyme accordingly: | ||
#***4 uL miniprep/DNA product | #***4 uL miniprep/DNA product | ||
Latest revision as of 11:20, 29 September 2006
- Use Ape to determine which enzymes to cut product with. Cuts should yield bands that are easily distinguishable on a gel.
- To digest make a cocktail of NEB2, Enzyme, H2O, and DNA product for a total volume of 10uL.
- If DNA product is high copy then use only 2uL of product 1uL of NEB2 and adjust the H2O and enzyme accordingly to make 10uL total:
- 2 uL miniprep/DNA product
- 1 uL NEB2
- .25 uL enzyme 1
- .25 uL enzyme 2
- 1 uL BSA
- 5.5 uL water
- If DNA product is low copy then use 4uL of product and 1uL of NEB2 adjusting the H2O and enzyme accordingly:
- 4 uL miniprep/DNA product
- 1 uL NEB2
- .25 uL enzyme 1
- .25 uL enzyme 2
- 4.5 uL water
- If DNA product is high copy then use only 2uL of product 1uL of NEB2 and adjust the H2O and enzyme accordingly to make 10uL total:
- Incubate for ~30min. and then run on gel.
