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Team:University of Lethbridge/Notebook/Project1July
From 2008.igem.org
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===July 9, 2008=== | ===July 9, 2008=== | ||
====Munima, Christa==== | ====Munima, Christa==== | ||
| - | Growth observed on amp plate that was plated with transformed competent RP1616 cells with pSB1A7. Approximately 10 colonies were observed. | + | Growth observed on amp plate that was plated with transformed competent RP1616 cells with pSB1A7. Approximately 10 colonies were observed, but they look strange. |
Subcultured one colony into 5mL LB + amp culture tube (50ug/mL ampicillin). Left overnight in shaker incubator at 37 C at 225 RPM. | Subcultured one colony into 5mL LB + amp culture tube (50ug/mL ampicillin). Left overnight in shaker incubator at 37 C at 225 RPM. | ||
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===July 10, 2008=== | ===July 10, 2008=== | ||
====Munima, Christa==== | ====Munima, Christa==== | ||
| - | Did plasmid mini prep on RP1616 competent cells with pSB1A7 from the culture tube left overnight. Eppendorf FastPlasmid mini kit was used and the tube was stored in the -20 C iGEM freezer labelled comp RP1616 + pSB1A7. | + | Did plasmid mini prep on RP1616 competent cells with pSB1A7 from the culture tube left overnight. Eppendorf FastPlasmid mini kit was used and the tube was stored in the -20 C iGEM freezer labelled "comp RP1616 + pSB1A7". |
Revision as of 22:29, 11 July 2008
Contents |
July 1, 2008
Nathan Puhl
Subcultured RP1616 into liquid LB and pTopp cells into liquid LB + amp
July 2, 2008
Nathan Puhl, Christa, Munima
Plasmid mini prepped pTopp cells.
Attempted to make RP1616 cells competent using the open wet ware [http://openwetware.org/wiki/Preparing_chemically_competent_cells protocol]. 100 uL aliquots of cells were frozen in liquid nitrogen and stored in the -80 freezer.
Ran CheZ in pUC19 plasmid and pUC19 plasmid from last year with high range ladder. The pUC19 plasmid seems weird, I don't think it should have two bands; I will have to ask someone about that. The CheZ plasmid appears to be the right size (2600 + 620 = 3220 bp)
July 3, 2008
Nathan Puhl, Munima, Christa
No colonies on either plate, but the max-efficiency DH5-alpha cells transformed with pSB1A7 were successfully transformed (~1500 cfu). There are two possibilities: 1. the cells are competent but are low efficiency and we did not add enough DNA, or 2. The cells are not competent. To assess possibility one we will try more DNA. If that does not work we will try a protocol using electroporation.
July 8, 2008
Munima, Christa
Objective: Attempt to transform pSB1A7 into RP1616 cells (made competent on July 2/08) again, but using more DNA and changes to June 16/08 transformation protocol
1. Thawed RP1616 cells and pSB1A7 on ice (obtained from Wieden -80 C freezer) 2. Added 50uL of RP1616 cells to a 15mL falcon tube (prechilled) 3. Left on ice for 10 minutes 4. Added 4uL of pSB1A7 to falcon tube 5. Incubated on ice for 30 minutes 6. Heat shocked without shaking for 45 seconds at 42 C 7. Placed on ice for 2 minutes 8. Added 1mL of SOC media preheated to 42 C. Incubated for 1 hour at 37 C in shaker incubator 9. Put a 400uL aliquot of mixture from incubator into a centrifuge tube 10. Centrifuged for 1 minute on max speed 11. Poured off supernatant and resuspended in 100uL of SOC media 12. Plated 100uL on LB + amp plate. Left overnight in incubator.
July 9, 2008
Munima, Christa
Growth observed on amp plate that was plated with transformed competent RP1616 cells with pSB1A7. Approximately 10 colonies were observed, but they look strange.
Subcultured one colony into 5mL LB + amp culture tube (50ug/mL ampicillin). Left overnight in shaker incubator at 37 C at 225 RPM.
July 10, 2008
Munima, Christa
Did plasmid mini prep on RP1616 competent cells with pSB1A7 from the culture tube left overnight. Eppendorf FastPlasmid mini kit was used and the tube was stored in the -20 C iGEM freezer labelled "comp RP1616 + pSB1A7".
