Team:Heidelberg/k4l1um

Revision as of 13:09, 19 June 2009 by Larsplus (Talk | contribs)

6-15-2009

Lab: LV, SH, CZ

SH:

LV:

Lab: LV, SH, CZ

=> Only bands at ca. 50 Bp => no successful amplification

Lab: LV, SH

No transformations could be observed
Replace Phsuion stocks to Phusion Master Mix from Nathan
Repeat DNA synthesis with a different protocol: 1:10 - 1:1000 dilution of Oligos, 95° 5', 7* [95° 45 58° 45 72° 1'], add 1:10 diluted primers, 95° 5' 25* same temperatures
Annealing successful for JeT and Min

Annealing might not have been successful with Fos beacuse it contains a very repetetive proximal promoter.

gel purfifcation of JeT and Min
Repeat PCR of pcDNA5/FRT and mcherry with lower annealing temperature (58°C) and fresh Polymerase: Follow PCR protcol from Strategene site directed mutagenesis kit.

mcherry PCR might not have been successful because we used a template we didn't make ourselves - does it contain TE?

Lab: LV, SH

DNA synthesis for Fos (proximal) and Fos (core)
Transformation of DH5a with pcDNA/FRT ΔPstI
HeLa cells, MCS7 and U20S were splitted 1:3. Therefore DEMED medium (containing additionally 10% FCS, PenStrap, glutamate and non-essential aminoacids) was removed. Cells were washed afterwards with HGSS and trypsinised with 1 ml of trypsin and incubated for 5 min. at 37°C 5% CO2. The used flasks were filled up to an endvolume of 7 ml with DMEM. 2 ml of the suspension was transfered to a new flask and incubated for another 3-4 days at 37°C and 5% CO2.