IGEM:Cambridge/2008/Notebook/Turing Pattern Formation/2008/08/20: Difference between revisions

Check Lux components

- Single colony PCR for :

• R0040 (MIT stuff)

• R0062 (MIT stuff)

• 4 different colonies of S0168 (from a transformation plate from 12/08)

• 4 different colonies of J04630 (from a transformation plate from 12/08)

- Protocol : add 1μL of cells (diluted in water), 10μL of Master Mis, 7μL of SDW, 1μL of VF primer and 1μL of VR primer

- Gel PCR products

- Results

• R0040 and R0062 : one big band of about 300b (expected size 293), OK!

• S0168 : one band of about 400b for the 4 different colonies (expected size 1234!), bad! This plate does not contain S0168

• J04630 (colonies 2 and 4) : one band of about 1100b (expected size 1173), OK!

• J04630 (colony 1) : one good band plus another band...

• J04630 (colony 3) : one band of about 600b, bad!

Check vector ECE190

- Plasmid miniprep

- Nanodrop

- Double digest : 6μL of SDW, 8μL of DNA, 1μL of buffer, 1μL of XbaI and 1μL of PstI

- Run on a gel

- Result : 2 bands (a little bit more than 3000b and a little bit more than 5000b) :ok!

Ligation

- Materials :

• AgrA
• AgrB
• AgrC
• AgrD
• Pupp
• Pspac
• Ppac
• Pxyl
• RBS S
• RBS W
• psB4C5

- Double digest of PCR products

- Run vector, AgrA and AgrD on a gel

- DNA clean and concentrator for AgrA, B,C and D, promoters

- Microclean for both RBS

- Nanodrop

- Extract plasmid annd Agr from gel and clean

- Ligation