Team:Freiburg/Notebook/15 July

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Meeting

attendants: Tobi, Theo, Julia, Rüdiger, Jakob, Sandra

blue light receptor

already done:

1. Transformation of Lov-Tap in cells.

To-do:

1. Cloning of promotor (medium) in Lov-Tap part and perform a transformation. Plating out of the cells on trypthophan-free medium.

Quick change

Investigators: Theo

already done:

1. repressor part (BBa_K098995) has no bases between RBS (B0034) and start codon (K098997), resulting in no translation.
   • quickchange of the repressor part to insert 6bp between RBS and start codon

To-do:

1. DpnI digestion to digest the DNA template (methylated DNA) of the PCR to have only the new synthesized DNA strand.
2. After digestion with DpnI, transformation of cells with the corrected part (BBa_K08995)

Lysis cassette

Digestion of Quickchange

35 μl total volume

Incubate for about 1h at 37°C + Heat inactivation at 80°C for 20min.

Precipitator

PCR

PCR-Mixture for one Reaction:

For a 50 µl reaction use

What program do you use?

10x (95C-41/52C-72C) + 25x ((95C-60C-72C)

How did you label the PCR-Product, where is it stored and what do you do next?

Reactions:

lane 1

quick load braod range marker

lane 2

empty

lane 3

P28+P18+M14.1

lane 4

P28+P19+M14.1

lane 5

P28+P20+M14.1

Results:

did not work well.

Strange band size in lane 3. 4 and 5 did not work.