"
Team:Stockholm/13 September 2010
From 2010.igem.org
(→Cloning of N-CPPs into pSB1C3) |
|||
| Line 17: | Line 17: | ||
Blastn alignments against [[media:Blastn_N-Tra10_pSB1C3.nCPP_11sep.txt|N-Tra10]], [[media:Blastn_N-TAT_pSB1C3.nCPP_11sep.txt|N-TAT]] and [[media:Blastn_N-LMWP_pSB1C3.nCPP_11sep.txt|N-LMWP]] indicated successful cloning of N-Tra10 (clone 7) and N-TAT (clone 4). | Blastn alignments against [[media:Blastn_N-Tra10_pSB1C3.nCPP_11sep.txt|N-Tra10]], [[media:Blastn_N-TAT_pSB1C3.nCPP_11sep.txt|N-TAT]] and [[media:Blastn_N-LMWP_pSB1C3.nCPP_11sep.txt|N-LMWP]] indicated successful cloning of N-Tra10 (clone 7) and N-TAT (clone 4). | ||
| + | |||
| + | ====Transformations==== | ||
| + | Since pSB1C3.N-TAT and pSB1C3.N-Tra10 colony samples were accidentally discarded, prepared plasmids were used to transform new cells in order to prepare glycerol stocks. | ||
| + | |||
| + | Standard transformation with 1 μl plasmid DNA. | ||
| + | *pSB1C3.N-TAT | ||
| + | *pSB1C3.N-Tra10 | ||
| + | |||
| + | ====Sequencing==== | ||
| + | DNA concentrations of 11/9 plasmid preps were measured by Mimmi and samples were sent for sequencing for isolation of N-LMWP. | ||
| + | *'''pSB1C3.nCCP 2''': ABS0045 B92 | ||
| + | *'''pSB1C3.nCCP 3''': ABS0045 B93 | ||
| + | *'''pSB1C3.nCCP 5''': ABS0045 B94 | ||
| + | *'''pSB1C3.nCCP 8''': ABS0045 B95 | ||
| + | *'''pSB1C3.nCCP 9''': ABS0045 B96 | ||
| + | *'''pSB1C3.nCCP 10''': ABS0045 B97 | ||
| + | *'''pSB1C3.nCCP 11''': ABS0045 B98 | ||
| + | *'''pSB1C3.nCCP 12''': ABS0045 B99 | ||
Revision as of 18:02, 14 September 2010
| Home | Project Idea | Lab Work | Results | Modelling | Team | Follow us on  and 
| 2010.igem.org 
|
Contents |
Andreas
Preparation of Top10 chemically competent cells
None of the clones streaked onto the Amp 100 plate (11/9) grew, indicating no AmpR contamination in cells. One of the ON cultures were therefore selected for preparation of competent cells.
Procedures according to protocol. Growth conditions changed to 25 °C, 220 rpm (OD600 reached after ≈6 h).
A 100 μl aliquot was divided and spread onto Amp 100, Cm 25 and Km 50 plates to verify that they were not contaminated.
Cloning of N-CPPs into pSB1C3
Sequencing results from 8/9 returned.
- pSB1C3.nCPP 3 (failed)
- pSB1C3.nCPP 4 (fasta)
- pSB1C3.nCPP 6 (fasta)
- pSB1C3.nCPP 7 (fasta)
- pSB1C3.nCPP 8 (fasta)
Blastn alignments against N-Tra10, N-TAT and N-LMWP indicated successful cloning of N-Tra10 (clone 7) and N-TAT (clone 4).
Transformations
Since pSB1C3.N-TAT and pSB1C3.N-Tra10 colony samples were accidentally discarded, prepared plasmids were used to transform new cells in order to prepare glycerol stocks.
Standard transformation with 1 μl plasmid DNA.
- pSB1C3.N-TAT
- pSB1C3.N-Tra10
Sequencing
DNA concentrations of 11/9 plasmid preps were measured by Mimmi and samples were sent for sequencing for isolation of N-LMWP.
- pSB1C3.nCCP 2: ABS0045 B92
- pSB1C3.nCCP 3: ABS0045 B93
- pSB1C3.nCCP 5: ABS0045 B94
- pSB1C3.nCCP 8: ABS0045 B95
- pSB1C3.nCCP 9: ABS0045 B96
- pSB1C3.nCCP 10: ABS0045 B97
- pSB1C3.nCCP 11: ABS0045 B98
- pSB1C3.nCCP 12: ABS0045 B99
