Team:Paris/August 21

From 2008.igem.org

(Difference between revisions)

Revision as of 16:55, 26 August 2008

↓ Calendar ↑

Contents

1 Cloning of FlhB promoter
- 1.1 Protocol
- 1.2 Result
2 Construction for FIFO
- 2.1 Digestion
- 2.2 Ligation
3 Screening of the cloning of E0240 and FlhDC+promotor
- 3.1 PCR screening
- 3.2 Electrophoresis
4 Construction for synchronization
- 4.1 Ligations
5 Promoter characterization plasmids
- 5.1 Ligation
- 5.2 Digestion
6 Promoter characterization plasmids
- 6.1 Ligations from digestions from 20th

Cloning of FlhB promoter

Protocol

Preparation of the template :

Resuspension of 1 colony E.coli K12 strain MG 1655 in 100µl of water.

Preparation of PCR mix :

1µl of dNTP
10µl Buffer Phusion 5X
2.5µl O 108
2.5µl O 109
1µl Template
1µl Phusion
33µL pure water

Result

[[Image:KR00019b.jpg| thumb| Vérification of pFlhB]

Well	1	2	3	4	5	6	7	8	9	10	11	12
Sample	100 bp ladder
Expected size (pb)
Measured size (pb)

Construction for FIFO

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

Digestion

Digestion

Protocol Digestion

Name	Template DNA	Description	Vol MP (µl)	Vol H2O (µl)	Enzymes
D166	MP165.1	RBS+ YFP LVA- term - FV	7.63	17	EcoRI and XbaI
D167	MP166.1	RBS+ YFP LVA+ term - FV	8.9	15.8	EcoRI and XbaI

Gel Extraction

Gel Extraction of D166-D167

Well	1	2	3	4	5	6	7	8	9	10	11	12
Sample	1kb ladder	MP165.1	MP166.1	no sample	D166	no sample	D167	no sample	100pb ladder	no sample
Expected size (pb)		2 957	2 996		2942		2981
Measured size (pb)		3 000	3 000

Measurement of the concentration of D166 & D167 purified

Protocol (it's same that for Miniprep)

Digestion Name	Concentration (µg/mL)	Ratio 260/280
D166	11	4.73
D167	10	2.84

Ligation

Ligation Name	Vector Name	Volume Vector (µL)	Insert	Volume Insert (µL)
L160	D166	3.63	D132	2.03
L161	D167	4.00	D132	2.01
Control L160	D166	3.63	-	-
Control L161	D167	4.00	-	-

Screening of the cloning of E0240 and FlhDC+promotor

We obtained single colonies with the dilution 100.
13 clones were analysed by PCR

PCR screening

reaction mixture (25 µL)

12,5 µL Quick load PCR Mixture 2X
0,5 µL O18
0,5 µL O19
11,5 µL water

PCR screening programm

elongation time: 1 min 30
primers: O18 and O19
positive control: S158 (pSB3K3)
negative control: no template

Electrophoresis

Gel n°1 (E0240 screening)

Gel n°2 (FlhDC+promotor screening)

1% agarose gel
10 µL loaded

Gel n°1 (E0240 in pSB3K3)
well n°	1	2	3	4	5	6	7	8	9	10	11	12	13	14	15	16	17
sample	1 kb DNA ladder	positive control	negative control	S159.1													100 bp DNA ladder
colonie n°				1	2	3	4	5	6	7	8	9	10	11	12	13
expected size				1192 bp
measured size				1,5 kb 1,1 kb 0,6 kb

Gel n°2 (FlhDC+promotor in pSB1A2)
well n°	1	2	3	4	5	6	7	8	9	10	11	12	13	14	15	16	17
sample	1 kb DNA ladder	positive control	negative control	S161.1													100 bp DNA ladder
colonie n°				1	2	3	4	5	6	7	8	9	10	11	12	13
expected size				1403 bp
measured size				0,3 kb

Results:

The clone of E0240 (S159.1) always have several bands amplified by PCR. It might contain different plasmids.
The clone of FlhDC+promotor (S161.1) don't have the correct size band. It also doesn't have the insert in the plasmid.

Construction for synchronization

Ligations

Ligation Name	Description	Vector Name	Volume vector (µL)	Insert Name	Volume insert(µL)
L158	rbs-TetR + gfp tripart	D110 (BV)	2	D131 (BI)	2.89
L159	rbs-lasI + Double terminator	D125 (FV)	2.08	D109 (FI)	1.15

Promoter characterization plasmids

Ligation

Our ligations from yesterday didn't work. The positive control for transformation worked.

Digestion

We had a problem with a gel extraction so we have to make again the digestions from yesterday

Other digestions made:

Protocol Digestion

Digestion name	Plasmid	Description	Miniprep used	Enzymes	Concentration after gel extraction
D179	MP3.4	B0015 (double terminator B0010-B0012) - BV	4	SpeI and PstI	9
D180	MP101.1	promoter J23101- BV	1	SpeI and PstI	7
D181	MP104.2	PTet (TetR repressible promoter) - FV	1	EcoRI and XbaI	1
D182	MP114.1	TetR - BI	1	XbaI and PstI	10
D183	MP119.3	pBad promoter - BI	1	XbaI and PstI	0
D184	MP143.1	gfp generator - FI	2	EcoRI and SpeI	13
D185	MP163.1	B0032 RBS - BV	2	SpeI and PstI	21

D179 D180 D181 D182 D183

D184 D185

Promoter characterization plasmids

Ligations from digestions from 20th

Top 10 cells were used

Ligation name	Vector digestion	Vector description	Vector conc. ug/mL	Vector volume	Insert digestion	Insert description	Insert conc. ug/mL	Insert volume	Product description	Antibiotic
L155	D164	J23101 promoter	3	16	D163	gfp generator	14	8	J23101 promoter-gfp generator	Amp
L156	D161	pTet promoter	39	1.25	D163	gfp generator	14	5	pTet promoter-gfp generator	Kana
Control L156	D161			1.25	none				Vector autoligation control	Kana
L157	D125.2	B0015	15	3	D162	tetR	11	4	tetR-B0015	Kana
Control L157	D125.2			3	none				Vector autoligation control	Kana
L166	D185	RBS B0032	21	2	D182	tetR	10	6.5	RBS B0032 - tetR	Amp
Control L166	D185			2	none				Vector autoligation control	Amp
L167	D181	pTet	1	14	D184	gfp generator	14	3	gfp generator - pTet	Amp
Control L167	D181	pTet		14	none				Vector autoligation control	Amp

Retrieved from "http://2008.igem.org/Team:Paris/August_21"