Team:Heidelberg/Template/Del week16 Gibson
From 2013.igem.org
Contents |
15-08-2013
Gibson Assembly and electroporation
Assembly of our fragments
Those gel-purified fragments were added for the Gibson assembly of our construct pFSN.
Fragment | Primer | Date | Concentration (ng/µl) | Volume (µl) |
---|---|---|---|---|
pSB4K5 | FS_01 - FS_16 | 14-08-13 | 13 | 1.35 |
AF | FS_02 - FS_05 | 13-08-13 | 49.75 | 2.65 |
FG | FS_21 - FS_26 | 07-08-13 | 24.5 | 2.69 |
G | FS_35_SR_01 - FS_23 | 08-08-13 | 34.9 | 2.1 |
OP | FS_22 - FS_13 | 13-08-13 | 36.3 | 0.89 |
L | FS_14 - FS_15 | 07-08-13 | 51 | 0.31 |
Gibson MasterMix NEB | 2x | 10 |
- Gibson Assembly according to protocols of NEB, 1h at 50°C
Gibson backbone (pSB4K5)
The backbone pSB4K5 was also incubated with the Gibson mastermix. We will use this as one negative control in the electroporation to test the efficiency.
Fragment | Date | Concentration (ng/µl) | Volume (µl) |
---|---|---|---|
pSB4K5 | 14-08-13 | 13 | 1.35 |
H2O | 8.65 | ||
Gibson MasterMix NEB | 2x | 10 |
- Gibson Assembly according to protocols of NEB, 1h at 50°C
Electroporation
The following samples were electroporated
mixture | volume used | cells | |
---|---|---|---|
5 µl Gibson Assembly of pFSN construct | 10 µl H2O | 1 µl | 50 µl DH10β old |
5 µl Gibson Assembly of pFSN construct | 10 µl H2O | 14 µl | 50 µl DH10β old |
5 µl Gibson Assembly of Backbone (control) | 10 µl H2O | 1 µl | 50 µl DH10β old |
pSB4K5 14-08-13 | 1.35 µl | 50 µl DH10β old | |
pSB6A1 Hanna [69.57 ng/µl] 1:10 | 1 µl | 50 µl DH10β Fanny new |
- Cells were transdered into 400 µl SOC-medium (NEB) after electroporation
- incubation and growth of cells for 1 hour at 37°C
- cells were centrifuged for 3 min at 6000rpm, supernatant discarded and cells resuspended in remaining SOC-medium
- cells were plated on agar plates containing kanamycine, 10µl on one plate, remaining µl on another plate for electroporation of the construct pFSN and on agar plates containing ampicillin for electroporation of the control backbone pSB6A1
20130816ElectroporationA.JPG
1 µl of diluted Gibson electroporated; 10 µl of E.coli plated |
20130816ElectroporationB.jpg
1 µl of diluted Gibson electroporated; Rest of E.coli plated |
20130816ElectroporationC.jpg
14 µl of diluted Gibson electroporated; 10 µl of E.coli plated |
20130816ElectroporationD.jpg
14 µl of diluted Gibson electroporated; Rest of E.coli plated |
P1010689.JPG
1 µl of diluted Gibson (backbone control) electroporated; 10 µl of E.coli plated |
P1010690.JPG
1 µl of diluted Gibson (backbone control) electroporated; Rest of E.coli plated |
P1010692.JPG
1 µl of backbone control electroporated; 10 µl of E.coli plated |
P1010693.JPG
1 µl of backbone control electroporated; Rest of E.coli plated |
P1010704.JPG
Test of electrocompetence DH10β with 1 µl pSB6A1; 10 µl of E.coli plated |
P1010705.JPG
Test of electrocompetence DH10β with 1 µl pSB6A1; Rest of E.coli plated |
16-08-2013
Colony PCRs
As a lot of colonies grew we screened if DelL and pSB4K5 are present.
Different probes:
- A: 1 µl of diluted Gibson electroporated; 10 µl of E.coli plated
- B: 1 µl of diluted Gibson electroporated; Rest of E.coli plated
- C: 14 µl of diluted Gibson electroporated; 10 µl of E.coli plated
- D: 14 µl of diluted Gibson electroporated; Rest of E.coli plated
- Only red colonies were chosen for screening
- The expected amplicon size is 1.5 kb
- Reaction mixture
Reagent | A1, A2 | B1-B5 | C1-C3 | D1-D40 |
---|---|---|---|---|
VR-Primer: (1/10) | 2 µl | 2 µl | 2 µl | 2 µl |
FS_14: (1/10) | 2 µl | 2 µl | 2 µl | 2 µl |
Colonies | 2 red colonies A (A1, A2) | 5 red colonies B (B1-B5) | 3 red colonies C (C1-C3) | 40 red colonies D (D1-D40) |
DreamTaq | 10 µl | 10 µl | 10 µl | 10 µl |
dd H2O | 5 µl | 5 µl | 5 µl | 5 µl |
- PCR Conditions
--> T100
Cycles-PCR | temperature [°C] | Time [s] |
---|---|---|
1 | 95 | 2:00 |
12 | 95 | 1:00 |
66 ↓ 0.5 | 5 | |
72 | 1:30 min | |
18 | 95 | 1:00 |
63 | 5 | |
72 | 1:30 min | |
1 | 12 | inf |
Result:
- None of the screened colonies led to the correct amplicon, therefore the correct assembly has not worked in any of the white colonies
- screening will be repeated, with white colonies as template, as bacteria including the correct 32 kbp backbone might not be capable of expressing mRFP anymore due to the large insert between lac promotor and mRFP
17-08-2013
Colony PCRs
Different probes:
- A 1 µl of diluted Gibson Assembly electroporated; 10 µl of E.coli plated
- B 1 µl of diluted Gibson Assembly electroporated; remaining E.coli plated
- C 14 µl of diluted Gibson Assembly electroporated; 10 µl of E.coli plated
- D 14 µl of diluted Gibson Assembly electroporated; remaining E.coli plated
- Only white colonies where chosen for screening
- The expected amplicon size is 1.5 kb
- Reaction mixture
Reagent | B1w | C1w | D1w-D10w |
---|---|---|---|
VR-Primer: (1/10) | 2 µl | 2 µl | 2 µl |
FS_14: (1/10) | 2 µl | 2 µl | 2 µl |
Colonies | 1 white colony B (B1w) | 1 white colony C (C1w) | 10 white colonies D (D1w-D10w) |
DreamTaq | 10 µl | 10 µl | 10 µl |
dd H2O | 5 µl | 5 µl | 5 µl |
- PCR Conditions
--> T100
Cycles-PCR | temperature [°C] | Time [s] |
---|---|---|
1 | 95 | 2:00 |
12 | 95 | 1:00 |
66 ↓ 0.5 | 5 | |
72 | 1:30 min | |
18 | 95 | 1:00 |
63 | 5 | |
72 | 1:30 min | |
1 | 12 | inf |
Result:
- Colony D8w shows expected amplicon of 1.5kbp
- The other colonies were screened negative.
- D8w will be transfered to liquid culture to repeat screening PCR as well as for further validation beeing screening for the other insert fragments as well as test restriction digest
- Furthermore another electorporation will be carried out to yield more clones positive for screening with the Primers VR and FS_14, therefore the remaining 10µl of the Gibson assembly will be purified using isopropanol precipitation
Electroporation
We electroporated the Gibson assembly (15-08) again to increase the chance of a positive clone. We purified it by isopropanol purification.
mixture | volume used | Cells | |
---|---|---|---|
Assembled fragments (15-08) isopropanol precipitated | 15 µl | 50 µl DH10β |
- Cells were transdered into 400 µl SOC-medium (NEB) after electroporation
- incubation and growth of cells for 1 hour at 37°C
- cells were centrifuged for 3 min at 6000rpm, supernatant discarded and cells resuspended in remaining SOC-medium
- cells were plated on agar plates containing kanamycine, 10µl on one plate, remaining µl on another plate for electroporation of the construct pFSN
P1010701.JPG
15 µl of Gibson 15-08 (isopropanol precipitated) electroporated; 10 µl of E.coli plated |
P1010702.JPG
15 µl of Gibson 15-08 (isopropanol precipitated) electroporated; Rest of E.coli plated |
18-08-2013
Colony PCRs
Different probes:
- D: 14 µl of diluted Gibson Assembly electroporated; remaining E.coli plated
- E: 1 µl isopropanol precipitated Gibson Assembly (15-08) ; 10 µl of E.coli plated
- F: 1 µl isopropanol precipitated Gibson Assembly (15-08); remaining E.coli plated
- The expected amplicon size is 1.5 kb
- 3 colonies were sceened in one PCR
- Reaction mixture
Reagent | D8w | D11w-D24w | E1w-E19w | F1w-F20w | E1r-E10 | F1r-F20r |
---|---|---|---|---|---|---|
VR-Primer: (1/10) | 2 µl | 2 µl | 2 µl | 2 µl | 2 µl | 2 µl |
FS_14: (1/10) | 2 µl | 2 µl | 2 µl | 2 µl | 2 µl | 2 µl |
Colonies | Colony D8w liquid culture | 24 white colonies D (D1w-D24w) | 19 white colonies E (E1w-E19w) | 30 white colonies F (F1w-F20w) | 10 red colonies E (E1r-E10r) | 20 red colonies F (F1r-F20r) |
DreamTaq | 10 µl | 10 µl | 10 µl | 10 µl | 10 µl | 10 µl |
dd H2O | 5 µl | 5 µl | 5 µl | 5 µl | 5 µl | 5 µl |
- PCR Conditions
--> T100
Cycles-PCR | temperature [°C] | Time [s] |
---|---|---|
1 | 95 | 2:00 |
12 | 95 | 1:00 |
66 ↓ 0.5 | 5 | |
72 | 1:30 min | |
18 | 95 | 1:00 |
63 | 5 | |
72 | 1:30 min | |
1 | 12 | inf |
Result:
- colony D8w again showed the expected amplicon in the colony PCR and will therefore be further analyzed for the other fragments as well as restriction digested and partially sequenced as soon as screening primers arive
- Furthermore colonies E16w and F25w are screened positive for the fragment DelL