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Construction of OmpR*+RBS and EnvZ*+RBS
I did some digestions (today), ligations (tommorow) and screening (the day after tommorow).
I tried to build :
RBS (B0034) + OmpR*
and
RBS (B0034) + EnvZ*
Protocol
Digestion name
| Template DNA
| Enzymes
| Volume of DNA
|
D 158
| MP 155.1 - OmpR*
| XbaI - PstI
| 5 µL
|
D 159
| MP 156.1 - EnvZ*
| XbaI - PstI
| 5 µL
|
D 102
| MP 100 - B0034
| SpeI - PstI
| 5 µL
|
- X µL of Template DNA
- Buffer (n°2) 10X : 3µL
- BSA 100X : 0.3µL
- Pure water qsp 30 µL
- 1 µL of each enzyme
- Incubate during about 3h at 37°C, then 20 minutes at 65°C (to inactivate the enzymes). Then 10°C overnight.
Transformation of the ligations we did yesterday
We transformed L 143, L 144 and the negative controls T1 and T2, using Invitrogen's TOP10 chemically competent cells standard protocol.
Creation of a registry of pFliL, pFlhDC, and FlhDC=
PCR amplification of flhDC and its promoter
List of PCRs
Name of the PCR
| PCR 136
| PCR 137
| PCR 138
| PCR 136'
| PCR 137'
| PCR 138'
| PCR 139
| PCR 140
|
Forward primer
| O 110
| O 111
| O 131
| O 110
| O 111
| O 131
| O 110
| O 131
|
Reverse primer
| O 113
| O 113
| O 132
| O 113
| O 113
| O 132
| O 113
| O 131
|
Template DNA
| MG 1655
| MG 1655
| MG 1655
| xx
| xx
| xx
| PCR 130
| PCR 130
|
Protocol
We followed the standard protocol of amplification in Two steps.
PCR program used :
PHUSION2
Results
Settings Gel 1%
- Ladder 1 kb 10 µL
- 4µL Template DNA + 2µL Loading Blue
- 1 % Agar
PCR Name
| What's in ?
| Well
| Expected size
| Measured size
|
PCR_138
| gene flhDC
| 2
| 992 bp
| 1000 bp
|
PCR_140
| gene flhDC
| 3
| 992 bp
| 1000 bp
|
PCR_138'
| gene flhDC
| 4
| X
| X
|
PCR_133
| gene flhDC + promoter
| 5
| 1227 pb
| 1200 bp
|
We managed to amplify flhDC !
Settings Gel 2%
- Ladder 100 bp 10 µL
- 4µL Template DNA + 2µL Loading Blue
- 2 % Agar
PCR Name
| What's in ?
| Well
| Expected size
| Measured size
|
PCR_136
| pflhDC (URI)
| 2
| 282 bp
| X
|
PCR_137
| pflhDC
| 3
| 428 bp
| X
|
PCR_139
| pflhDC (URI)
| 4
| 282 bp
| ~ 300 bp
|
PCR_136'
| pflhDC (URI)
| 5
| X
| X
|
PCR_137'
| pflhDC
| 6
| X
| X
|
We managed to amplify the promoter of flhDC
Digestions
After having succeded in amplifying the promoter and the gene of flhDC, we decided to clone it into a plasmid.
The first step is the digestion.
Protocol
Digestion name
| Template DNA
| Enzymes
| Volume of DNA
|
D 153
| PCR 138 - g flhDC
| EcoRI - PstI
| 5 µL
|
D 154
| PCR 140 - g flhDC
| EcoRI - PstI
| 5 µL
|
D 155
| PCR 139 - p flhDC
| EcoRI - PstI
| 5 µL
|
D 145
| MP122 - pSB1A2
| EcoRI-SpeI
| 5 µL
|
D 136
| MP103 - J61002
| EcoRI-SpeI
| 5 µL
|
- X µL of Template DNA
- Buffer (n°2) 10X : 3µL
- BSA 100X : 0.3µL
- Pure water qsp 30 µL
- 1 µL of each enzyme
- Incubate during about 3h at 37°C, then 20 minutes at 65°C (to inactivate the enzymes).
Then 10°C overnight.
Construction of pLas-TetR-GFP tripart & rbs-LasR-dble ter
Measurement of concentration of minipreps
standard protocol
Digestion
| Miniprep used
| Concentration (µg/mL)
| ratio 260/280
|
D146
| MP148.2
| 123
| 1.58
|
D147
| MP153.3
| 113
| 1.68
|
Digestion
Protocol Digestion
Ligation
Protocol Ligation
Ligation name
| Insert
| Vector
|
L150
| D146 (strongest rbs-TetR-GFP tripart)
| D105 (pLas)
|
L151
| D147 (strongest rbs-LasR activator with LVA)
| D125 (Double terminator)
|
Control 1
| /
| D105
|
Control 2
| /
| D125
|
Positive Control
| Puc19
|
PCR screening of cloning of E0240, flhD, flhC and pflhDC+flhDC
Analysis of yesterday PCR screening
Electrophoresis
- 1% agarose gel
- 10 µL loaded
Gel 1
Gel 2
Gel 3
Gel n°1
|
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 1 E0240
| positive control 2 pSB3K3
| negative control
| E0240 in pSB3K3
| 100 bp DNA ladder
| FlhD in pSB1A2
|
clone
|
|
|
|
| L139.1
| L139.2
| L139.3
| L139.4
| L139.5
| L139.6
| L139.7
| L139.8
|
| L140.1
| L140.2
| L140.3
| L140.4
|
expected size
|
|
| 316 bp
| 0 kb
| 1192 bp
|
| 589 bp
|
measured size
|
| 1,1 kb
| 1 kb
| 0 kb
| 1,5 kb 1,1 kb 0,6 kb
| 0,6 kb
| 0,6 kb
| 0,6 kb
| 0,6 kb
| 0,6 kb
| 0,6 kb
| 0,6 kb
|
| 0,4 kb 0,3 kb
| 0,4 kb 0,3 kb
| 0,4 kb 0,3 kb
| 0,4 kb 0,3 kb
|
Gel n°2
|
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 1 E0240
| positive control 2 pSB3K3
| negative control
| FlhD in pSB1A2
| 100 bp DNA ladder
| FlhC in pSB1A2
|
clone
|
|
|
|
| L140.5
| L140.6
| L140.7
| L140.8
|
| L141.1
| L141.2
| L141.3
| L141.4
| L141.5
| L141.6
| L141.7
| L141.8
|
expected size
|
|
| 316 bp
| 0 kb
| 589 bp
|
| 817 bp
|
measured size
|
| 1,1 kb
| 1 kb
| 0 kb
| 0,3 kb
| 0,3 kb
| 0,3 kb
| 0,3 kb
|
| 0,8 kb
| 0,8 kb
| 0,8 kb
| 0,8 kb
| 0,8 kb
| 0,8 kb
| 0,3 kb
| 0,8 kb
|
Gel n°3
|
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 1 E0240
| positive control 2 pSB3K3
| negative control
| FlhDC+promotor in pSB1A2
| 100 bp DNA ladder
|
|
|
|
|
clone
|
|
|
|
| L142.1
| L142.2
| L142.3
| L142.4
| L142.5
| L142.6
| L142.7
| L142.8
|
|
|
|
|
|
expected size
|
|
| 316 bp
| 0 kb
| 1403 bp
|
|
|
|
|
|
measured size
|
| 1,1 kb
| 1 kb
| 0 kb
| 0,3 kb 0,4 kb
| 0,3 kb 0,4 kb
| 0,3 kb 0,4 kb
| 0,3 kb 0,4 kb
| 0,3 kb 0,4 kb
| 0,3 kb 0,4 kb
| 1,4 kb 0,4 kb 0,3 kb
| 0,3 kb 0,4 kb
|
|
|
|
|
|
Starting the construction of the Promoter characterization plasmid
Measurement of concentration of minipreps
standard protocol
Plasmid
| Miniprep
| Concentration (µg/mL)
| ratio 260/280
|
MP3
| 3
| 152
| 1.43
|
MP3
| 4
| 775
| 1.21
|
MP101
| 1
| 317
| 1.66
|
MP101
| 2
| 389
| 1.36
|
MP101
| 4
| 209
| 1.76
|
MP104
| 1
| 173
| 1.32
|
MP104
| 3
| 43
| 1.85
|
MP104
| 4
| 52
| 1.66
|
MP114
| 1
| 173
| 1.75
|
MP114
| 2
| 263
| 1.43
|
MP143
| 1
| 133
| 1.55
|
MP143
| 2
| 132
| 1.70
|
Digestion
Protocol Digestion
Plasmid
| Description
| Miniprep used
| Enzymes
|
MP3
| B0015 (double terminator B0010-B0012) - FV
| 4
| EcoRI and XbaI
|
MP101
| promoter J23101 - BV
| 1
| SpeI and PstI
|
MP104
| PTet (Tet promoter) - BV
| 1
| SpeI and PstI
|
MP114
| TetR - FI
| 1
| EcoRI and SpeI
|
MP143
| gfp generator - BI
| 2
| SpeI and PstI
|
|