Team:Wageningen UR/Notebook/Proj1/May
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and -I0460 (marker: Kan). | and -I0460 (marker: Kan). | ||
- | By colony PCR some of colonies were screened. The Invitrogen protocol was used. The PCR | + | By colony PCR some of colonies were screened. The Invitrogen protocol was used. The PCR thermocycler, of Biorad, was set to the following values for 30 cycles: 94°C at the denaturation, 50°C at the annealing and 72°C at the elongation step. Of the following transformants 4 colonies were taken: BBa_F2621, -32519, -32510, -E0422 and -I0462. |
The 4 colonies BBa_E0422 transformants and 3 colonies of the BBa_I0462 transformants were confirmed. For the rest of the samples the electrophoresis gel was not clear. | The 4 colonies BBa_E0422 transformants and 3 colonies of the BBa_I0462 transformants were confirmed. For the rest of the samples the electrophoresis gel was not clear. | ||
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The liquid cultures were made successfully on May 24 - unlike the other incubations, the negative control showed no growth. | The liquid cultures were made successfully on May 24 - unlike the other incubations, the negative control showed no growth. | ||
+ | With colony PCR the cultures were screened. The Biorad PCR thermocycler was set up in the following way: 30 cycles of 94°C at the denaturation, 50°C at the annealing and 72°C at the elongation step (duration of it was 2.5 min. because the length the luciferase gene is around 2600 bp). | ||
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+ | '''May 30''' | ||
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+ | PCRs were perfomed on BBa_I0462 transformants in liquid culture and colonies, a BBa_I0462 plasmid and a control. | ||
[https://2011.igem.org/Team:Wageningen_UR/Notebook/Proj1/April Previous Month] | [https://2011.igem.org/Team:Wageningen_UR/Notebook/Proj1/April Previous Month] |
Revision as of 13:27, 30 July 2011
Building a Synchronized Oscillatory System
May - Synchronized Oscillatory System