"
Team:Rice University/Notebook/20 June 2008
From 2008.igem.org
(Difference between revisions)
StevensonT (Talk | contribs) (New page: =Friday, 20 June= *Taylor Stevenson: **VCS257 SupA+ cells were grown O/N @ 37*C in Lambda media. 4.5mL culture was infected with 4.5uL of phage packaging product from November, 2007 and a...) |
StevensonT (Talk | contribs) |
||
| Line 1: | Line 1: | ||
=Friday, 20 June= | =Friday, 20 June= | ||
*Taylor Stevenson: | *Taylor Stevenson: | ||
| - | **VCS257 SupA+ | + | **Lysis Assay of VCS257 SupA+ |
| + | *#Cells were grown O/N @ 37*C in Lambda media. | ||
| + | *#4.5mL culture was infected with 4.5uL of phage packaging product from November, 2007 and allowed to incubate for 20min @ 37*C shaking @ 250 rpm. Infected culture was heat shocked @ 42*C for 20min, inducing lysis by denaturing the CI857 repressor. | ||
| + | *#Cells were then grown and their optical density was measured at different time points after heat shock. | ||
| + | **Lysogeny Screen - Results | ||
| + | *#An infected VCS257 culture was streaked onto LB-agar. Isolated colonies were used to innoculate a 96 deep-well plate which was grown O/N @ 30*C shaking @ 300rpm. Using the well replicator, each of the wells was spotted onto two large petri dishes. One dish was grown @ 30*C and the other was grown @ 42*C O/N. Spots that grew on 30*C plates and not on 42*C plates are lysogens as the phage infected cells would lyse due to the temperature sensitive cI. The plates show that there is only one colony that could be a possible lysogen. | ||
| + | *# The possible lysogen colony was streaked onto LB plates to be grown O/N @ 30*C and 42*C to verify temperature screen. | ||
| + | *# A colony PCR was performed on the possible lysogen using the CroF and CroR primers. If a copy of the lambda genome is incorporated into the lysogen's, the PCR should result in amplification of the phage gene ''cro'' and produce a 400bp product. Additionally, three other PCR reactions were performed in parallel. | ||
| + | *## -negative control using water | ||
| + | *## -positive control using lambda DNA | ||
| + | *## -second sample using lambda particles from stocks | ||
Revision as of 18:04, 20 June 2008
Friday, 20 June
- Taylor Stevenson:
- Lysis Assay of VCS257 SupA+
- Cells were grown O/N @ 37*C in Lambda media.
- 4.5mL culture was infected with 4.5uL of phage packaging product from November, 2007 and allowed to incubate for 20min @ 37*C shaking @ 250 rpm. Infected culture was heat shocked @ 42*C for 20min, inducing lysis by denaturing the CI857 repressor.
- Cells were then grown and their optical density was measured at different time points after heat shock.
- Lysogeny Screen - Results
- An infected VCS257 culture was streaked onto LB-agar. Isolated colonies were used to innoculate a 96 deep-well plate which was grown O/N @ 30*C shaking @ 300rpm. Using the well replicator, each of the wells was spotted onto two large petri dishes. One dish was grown @ 30*C and the other was grown @ 42*C O/N. Spots that grew on 30*C plates and not on 42*C plates are lysogens as the phage infected cells would lyse due to the temperature sensitive cI. The plates show that there is only one colony that could be a possible lysogen.
- The possible lysogen colony was streaked onto LB plates to be grown O/N @ 30*C and 42*C to verify temperature screen.
- A colony PCR was performed on the possible lysogen using the CroF and CroR primers. If a copy of the lambda genome is incorporated into the lysogen's, the PCR should result in amplification of the phage gene cro and produce a 400bp product. Additionally, three other PCR reactions were performed in parallel.
- -negative control using water
- -positive control using lambda DNA
- -second sample using lambda particles from stocks
