Analysis of the transformant of FlhDC+promotor

• Analysis of the plasmids MP160.1 and MP160.2 (FlhDC+promotor in pSB1A2)
• Control: MP143 (GFP generator in pSB1A2)

PCR

PCR screening programm
elongation time: 1 min 30
total volume reaction (25 µL)

• 12,5 µL Quick load PCR Mix 2X
• 0,5 µL O18
• 0,5 µL O19
• 1 µL DNA
• 10,5 µL water

Digestion

total volume reaction (30 µL)

• 2 µL DNA
• 3 µL buffer 2 10X
• 0,3 µL BSA 100X
• 1 µL XbaI
• 1 µL SpeI
• 22,7 µL water

Incubation 2h55 at 37°C and then 20 min at 65°C.

Electrophoresis

• 1% agarose gel
• for PCR products: 10 µL loaded
• for digestion products (30 µL): adding of 7 µL of loading blue and then 20 µL loaded on gel

Results: The clones tested didn't have the insert.

Construction of pFlgA - GFP Generator

Aim : Construction of "pFlgA-RBS-GFP-dbl ter" (pFlgA-E0240)

Digestion

Digestion

Protocol Digestion

Gel Extraction

Protocol

Gel Extraction of D168

Measurement of the concentration of D168 purified

Protocol (it's same that for Miniprep)

Ligation

Protocol

Construction for FIFO

Aim : Construction of pFlgA - YFP tripart (+/- LVA) "pFlgA-RBS-YFP-dbl ter" (pFlgA-E0430/E0432)

Transformation of the ligations we did yesterday

Protocol

Construction for synchronization

Transformation of the ligations we did yesterday

Protocol

Ligation

Protocol

Ligation Name	Description	Vector Name	Volume vector (µL)	Insert Name	Volume insert (µL)
L162	rbs-lasI + gfp generator	D107 (BV)	10	D163 (BI)	3.46
Control L162	autoligation control	D107 (BV)	10	-	-
L163	rbs-TetR + gfp generator	D110 (BV)	2.5	D163 (BI)	3.44
Control L163	autoligation control	D110 (BV)	2.5	-	-

Transformation

Protocol

Promoter characterization plasmids

Transformation of ligations from August 20th

Protocol

Top 10 cells were used