Team:Goettingen/week10-3

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Revision as of 13:21, 22 September 2012


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Startpoint of Saturated mutagenesis experiment!

Observations and results:
According to the agarose gel the PCR worked well. A band of the expected size of 3769 bp was observed for both reactions.

1^st round of mutagenesis PCR (mutation of aa residues 149, 150 and 159)

Experiment:
The saturated mutagenesis PCR was set up in a 50 µL batch according to the established protocol V07_02).

Observations and results:
The corresponding gel showed bands of the expected size.

V07_04_01 1^st round: PCR clean-up

Experiment:
The clean-up was performed using peqGOLD Cycle-Pure Kit (PeqLab) following the user manual. We modified the protocol by using columns from the peqGOLD Plasmid Miniprep Kit (PeqLab) because these can bind a higher amount of DNA (30 µg/column). Thus, we lose fewer DNA material in the cleaning steps. 50 µL of elution buffer was used.

Observations and results:
The corresponding gel showed a band of the expected size.

V07_04_02 1^st round: DpnI/BsaI digestion

Experiment:
The digestion was performed with a total volume of 50 µL according to protocol.

V07_04_03 1^st round: Digestion clean-up

Experiment:
The clean-up was performed using peqGOLD Cycle-Pure Kit (PeqLab) modified by using columns from the peqGOLD Plasmid Miniprep Kit (PeqLab) with an EB volume of 50 µL.

Observations and results:
The corresponding gel showed a band of the expected size.

V07_04_04 1^st round: Ligation

Experiment:
The ligation was set up in a 100 µL batch according to protocol. Incubation over night at 16 °C.

V07_05_01 1^st round: Ethanol precipitation of mutated plasmids

Observations and results:
Unfortunately we used the wrong amount of ethanol, so that the subsequent transformation did not work successfully!

V07_05_02 1^st round: Transforamtion of electrocompetent cells wir the mutant plasmid mixture

Experiment:
Electrocompetent cells were prepared according to protocol. We transformed 200 µL of cells with 10 µL of DNA. A detailed protocol for the electroporation can be found here. The transformed cells were transferred to 100 mL liquid LB medium and incubated over night at 37 °C, 180 rpm. We prepared three dilution plates LB+CM (10⁴, 10⁵, 10⁶) for counting colonies to verify whether the desired library diversity is reached. Plates were incubated over night at 37 °C aswell.

V07_06_01 1^st round: Analysis of transformation V07_05

Experiment:
Plates and liquid culture were checked for successful transformation.

Observations and results:
No bacterial growth on neither plates nor in liquid culture. Continuous bug see V07_05_01!

V07_06_02 1^st round: Restart of saturated mutagenesis PCR

Experiment:
The PCR V07_03 was set up again + 1 backup. The clean-up was performed with the peqGOLD Cycle-Pure Kit (PeqLab). Elution in 50 µL EB.

Observations and results:
The corresponding gel showed bands of the expected size.

@@ Line 138: / Line 138: @@
 <b>V07_06_02 1<sup>st</sup> round: Restart of saturated mutagenesis PCR</b><br>
 <ul>
-<li>Experiment: <br>The PCR V07_03 was set up again + 1 backup.
+<li>Experiment: <br>The PCR V07_03 was set up again + 1 backup. The clean-up was performed with the peqGOLD Cycle-Pure Kit (PeqLab). Elution in 50 µL EB.
 </li>
 </ul>