IGEM06 DNA Distribution Issues
From 2006.igem.org
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|iGEM06 DNA-1 | |iGEM06 DNA-1 | ||
|we tried 10 times!! | |we tried 10 times!! | ||
- | |||
- | |||
- | |||
- | |||
- | |||
|- | |- | ||
|PennState | |PennState | ||
|BBa_R0051 | |BBa_R0051 | ||
|pSB1A2, pSB2K3 | |pSB1A2, pSB2K3 | ||
- | | | + | |DH5a |
|iGEM06/05 DNA-1 | |iGEM06/05 DNA-1 | ||
|neither amp plate seems to work | |neither amp plate seems to work | ||
+ | |- | ||
+ | |Davidson | ||
+ | |BBa_B0015 | ||
+ | |pSB1AK3 | ||
+ | |JM109 | ||
+ | |iGEM06 DNA-1 | ||
+ | |no insert at all; had to use stocks from last year; pSB1A2 | ||
+ | |- | ||
+ | |Berkeley | ||
+ | |BBa_P1000 (CmR) | ||
+ | |pSB1AC3 | ||
+ | |TG1 | ||
+ | |iGEM06 DNA-2 | ||
+ | |Austin says it should be a pSB2K* plasmid; no CmR colonies generated upon transformation | ||
+ | |- | ||
+ | |Berkeley | ||
+ | |BBa_P1001 (tet) | ||
+ | |pSB1AT3 | ||
+ | |TG1 | ||
+ | |iGEM06 DNA-2 | ||
+ | |Austin says it should be a pSB2K* plasmid; no tetR colonies generated upon transformation | ||
+ | |- | ||
+ | |Ljubljana, Slovenia | ||
+ | |BBa_P1010 (tet) | ||
+ | |pSB1AT3 | ||
+ | |DB3.1 | ||
+ | |iGEM06 DNA-2 (23P) | ||
+ | |Plasmid pSB1AT3 should have tet resistance, but instead it has Kan resistance (so it should be labeled pSB1AK3). | ||
+ | |- | ||
+ | |Cambridge | ||
+ | |BBa_J04430 | ||
+ | |pSB1A2 | ||
+ | |DH5-a; XL-1 Blue; MG-1655; MC1000 | ||
+ | |iGEM06 DNA-2 (1L) | ||
+ | |On transforming, this biobrick persistently results in segregated colonies, some show the expected green fluorescence but others show surprisingly red fluorescence. IPTG does not have an effect. This has been our experience | ||
+ | |- | ||
+ | |||
+ | |||
|} | |} | ||
Latest revision as of 13:37, 21 October 2006
This page is to keep a record of any troubles that you have when trying to successfully transform parts from either of the two iGEM 2006 DNA Distribution plates (See Biobrick Delivery page for delivery details)
Please include:
- Biobrick part number
- Plasmid
- Cell strain used
- Plate (iGEM 2006 DNA-1 or DNA-2) and well number
Team | Part number | Plasmid | Cell strain | Distribution plate | Comments |
---|---|---|---|---|---|
Example | BBa_xxxx | pSB1A2 | TOP10 | iGEM06 DNA-1 | we tried 10 times!! |
PennState | BBa_R0051 | pSB1A2, pSB2K3 | DH5a | iGEM06/05 DNA-1 | neither amp plate seems to work |
Davidson | BBa_B0015 | pSB1AK3 | JM109 | iGEM06 DNA-1 | no insert at all; had to use stocks from last year; pSB1A2 |
Berkeley | BBa_P1000 (CmR) | pSB1AC3 | TG1 | iGEM06 DNA-2 | Austin says it should be a pSB2K* plasmid; no CmR colonies generated upon transformation |
Berkeley | BBa_P1001 (tet) | pSB1AT3 | TG1 | iGEM06 DNA-2 | Austin says it should be a pSB2K* plasmid; no tetR colonies generated upon transformation |
Ljubljana, Slovenia | BBa_P1010 (tet) | pSB1AT3 | DB3.1 | iGEM06 DNA-2 (23P) | Plasmid pSB1AT3 should have tet resistance, but instead it has Kan resistance (so it should be labeled pSB1AK3). |
Cambridge | BBa_J04430 | pSB1A2 | DH5-a; XL-1 Blue; MG-1655; MC1000 | iGEM06 DNA-2 (1L) | On transforming, this biobrick persistently results in segregated colonies, some show the expected green fluorescence but others show surprisingly red fluorescence. IPTG does not have an effect. This has been our experience |
If we see the same Biobrick parts giving multiple teams trouble it will give us a better sense of what we need to fix.
Note: Please take a look and see if your team has been able to successfully transform any of the parts on this list. You might want to contact the team that was having trouble and let them know that you were able to successfully transform that particular part. All of the distribution plates were done in the same method at the same time so they should be the same, but that isn't always the case.