Team:Paris/September 11
From 2008.igem.org
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*ligase 2: our 50 µL (400 000 U/mL) tube | *ligase 2: our 50 µL (400 000 U/mL) tube | ||
*ligase 3: 2nd floor 50 µL (400 000 U/mL) tube | *ligase 3: 2nd floor 50 µL (400 000 U/mL) tube | ||
+ | The ligase 1 and 2 were used with our buffer tube, whereas the ligase 3 was used with the buffer tube from the 2nd floor lab. | ||
'''Reaction mixture''' | '''Reaction mixture''' | ||
*8 µL of purified digestion products | *8 µL of purified digestion products |
Revision as of 13:35, 12 September 2008
Checking our ligasesBecause we couldn't be sure of the results of yesterday experiment, we decided to carry it out one more time. DigestionDNA used for digestion: MP101
Reaction mixture
2h30 at 37°C and then 20 min at 65°C
PurificationD202 (EcoRI digestion) was purified in 2 ways:
D203 (BspHI digestion) was purified:
Elution in 30 µL of EB buffer Ligation3 ligases tested
The ligase 1 and 2 were used with our buffer tube, whereas the ligase 3 was used with the buffer tube from the 2nd floor lab. Reaction mixture
For the samples for which the digestion products have not been purified, 1 µL of ligase and 1 µL of ATP (1 mM final concentration) have been added directly in the digestion products (in the digestion buffer 2).
All the ligation were carried out overnight at 4°C.
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