Team:Stockholm/23 July 2010
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JohanNordholm (Talk | contribs)
(New page: {{Stockholm/Top2}} ==Johan== ===Colony PCR=== *Another colony PCR on the second transformation of TAT CCP as the first one didn't show many colonies and none of the colonies showed any ...)
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(New page: {{Stockholm/Top2}} ==Johan== ===Colony PCR=== *Another colony PCR on the second transformation of TAT CCP as the first one didn't show many colonies and none of the colonies showed any ...)
Newer edit →
Revision as of 23:00, 25 July 2010
Johan
Colony PCR
- Another colony PCR on the second transformation of TAT CCP as the first one didn't show many colonies and none of the colonies showed any insert in the vector.
- Colony #1-36 +insert, colony #42-43 -insert.
- PCR reaction mix
- 0,5 µl Pfu polymerase
- 0,5 µl 10 mM dNTPs
- 2 µl 10 µm f.primer (VF2)
- 2 µl 10 µm r.primer (VR)
- 2,5 µl Pfu buffer 10x
- 17,5 µl H2O
- PCR program
- 98 °C - 2 min
- 35 cycles of
- 98 °C - 10 sec
- 55 °C - 15 sec
- 72 °C - 45 sec
- 72 °C - 5 min
- 4°C - ∞
Gel electrophoresis
A gel electrophoresis was performed on the PCR products.
Lane 1 & 40: FastRuler DNA Ladder low range, lane 2-37: +insert, lane 38-39: -insert.
The gel didn't turn out good, probably I used too much DNA template.