Talk:IGEM:MIT/2006/Communications

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Questions for Stephen

Do we have the regulated wintergreen GC data in a form that we could generate plots similar to the banana timecourse?
- Yes, we could. It would take some digging through old files and sorting out through each protocol we used on each day. I don't know if it's necessary to show though.
What did you use to shake the cultures? i.e. what incubator or shaker?
- 220 RPM- the shaker in 37 C room
- 110 RPM- the shaker by Samantha's/2007 iGEM team's bench
Are both J45200 and J45250 on pSB1AT3?

General outstanding issues

Funding sources for each person

See last email... all undergrads were funded in the summer of 2006 by the MIT UROP office

Protocol for transformation

See below

Transformation - André Transform competent cells
- Thaw ~50 μl cells (whichever you like) on ice. Do not use glass tubes, which adsorb DNA.
- Add 200 uL DNA to cells
- Incubate on ice for 30 minutes
- Incubate cells for 50-60 seconds at 42°C.
- Incubate cells on ice for 2 min.
- Add 200-300μL of room temperature SOC (not critical)
- Incubate for 1 hour at 37°C on shaker.
- Spread 200 μl onto plates made with appropriate antibiotic.
- Grow overnight at 37°C.

Describing figure 6
Update <bbpart>BBa_Q04401</bbpart>

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