Revision as of 09:58, 26 August 2008

Construction for Synchronization

Transformation of the ligations we did yesterday

Ligation Name	Description	Antibio
L159	D125 (FV) + D109 (FI)	Kan
Control L159	D125	Kan
L162	D107 (BV) + D163 (BI)	Amp
Control L162	D107	Amp
L163	D110 (BV) + D163 (BI)	Amp
Control L163	D110	Amp

Construction of pFlgA - GFP Generator

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

Results of the transformation we did the day before yesterday

Ligation name	Description	Antibio	Number Colonies observed	Fluorescence	Comments
Ligations
L164	D168(FV) - D132(FI) pFlgA - gfp generator	Amp	125	No	ok
Controls
TL164	D168(FV)	Amp	8	No	ok
Positive Control	pUC19	Amp	2000 (efficiency 2.10^8)	No	OK

=> Need to screen to know which clones we can use for the  of  pFlgA promotor characterization.

Cloning of EnvZ*

The sequencing of EnvZ* previously cloned, revealed a loss of about 300 bp. EnvZ* contains indeed an EcoRI restriction site within its sequence. So we can't use this enzyme during the cloning.

Digestion

name	sample	digestion	digestion number
EnvZ*	PCR129 from August 8th	XbaI & PstI	D159
pSB1A2	MP108 (C0179 (lasR-pSB1A2))	XbaI & PstI	D116

Reaction mixture

4 µL of PCR129 (or 2 µL of MP108)
3 µL of 10X buffer n°2
0,3 µL of 100X BSA
1 µL of XbaI
1 µL of PstI
20,7 µL (or 22,7 µL) of water

Incubation at 37°C during 2H25, and then ~20 min at 65°C

Electrophoresis

1% agarose gel

EnvZ*: 3 µL of digestion products + 1 µL of loading blue + 2 µL of water
pSB1A2: 30 µL of digestion products + 6 µL of loading blue

Gel after excision

well n°	1	2	3	4	5	6
sample	1 kb DNA ladder	D159 (EnvZ*)		D116 (pSB1A2 & lasR)		100 bp DNA ladder
expected size		1421 bp		2057 bp & 707 bp
measured size		1,4 kb		2 kb & 0.7 kb

@@ Line 131: / Line 131: @@
 |1 kb DNA ladder
 |D159 (EnvZ*)
-|
+|<br>
 |D116 (pSB1A2 & lasR)
-|
+|<br>
 |100 bp DNA ladder
 |-

Team:Paris/August 25

From 2008.igem.org