Team:Stockholm/23 June 2010
From 2010.igem.org
(Difference between revisions)
(→Andreas) |
(→Andreas) |
||
Line 32: | Line 32: | ||
'' '''Note:''' The transformed pEX vector was thought to carry a Cm resistance cassette insert. This was, however, discovered to be wrong.'' | '' '''Note:''' The transformed pEX vector was thought to carry a Cm resistance cassette insert. This was, however, discovered to be wrong.'' | ||
- | |||
===Plasmid preparation of pEX vector=== | ===Plasmid preparation of pEX vector=== | ||
Two clones picked and each inoculated in 5 ml LB with Amp and grown ON in 37°C, 250 rpm. | Two clones picked and each inoculated in 5 ml LB with Amp and grown ON in 37°C, 250 rpm. | ||
- | |||
===Transformation with pMA vector=== | ===Transformation with pMA vector=== |
Revision as of 09:28, 6 July 2010
Contents |
Andreas
Testing Top10 competent cells and antibiotic agar plates
Results from 22/6
Transformed plasmid | Plate | Growth |
pEX | 100 ug/ml Amp | Yes |
None | 100 ug/ml Amp | No |
pEX | 25 ug/ml Cm | No |
None | 25 ug/ml Cm | No |
Growth on Amp plate indicated transformation competence. No growth on other plates indicated good antibiotic selection.
Note: The transformed pEX vector was thought to carry a Cm resistance cassette insert. This was, however, discovered to be wrong.
Plasmid preparation of pEX vector
Two clones picked and each inoculated in 5 ml LB with Amp and grown ON in 37°C, 250 rpm.
Transformation with pMA vector
The pMA (BBa_K157000) vector could become useful for cloning and construction of our parts, as it carries the complete Freiburg prefix and suffix sequences (in contrast to the standard BioBrick vectors pSB1x3).
- Top10 cells was transformed with the pMA vector carrying a Freiburg fusion His tag (BBa_K157011) insert. Cells grown on 100 ug/ml Amp plates.
Hassan
Started to use softwares for making 3D animations and/or movies, started by making protein A and IgG Protease.
softwares used:
- Molecular Maya
- Chimera