Difference between revisions of "Team:Freiburg/Labjournals/Cloning/August"
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+ | <h1>Cloning</h1> | ||
<h1 class="sectionedit1">2015/08/01</h1> | <h1 class="sectionedit1">2015/08/01</h1> | ||
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<strong>antigen 18</strong>:~570bp. | <strong>antigen 18</strong>:~570bp. | ||
For pRIG15_8, clone 3 shows correct bands, for pIRG15_10 clone 3, pRIG15_17 clone 1 and pRIG15_18 clone 2 and 3 are correct. Correct clones were sent for sequencing.</div></div></div><hr/> | For pRIG15_8, clone 3 shows correct bands, for pIRG15_10 clone 3, pRIG15_17 clone 1 and pRIG15_18 clone 2 and 3 are correct. Correct clones were sent for sequencing.</div></div></div><hr/> | ||
− | <p> | + | <p id="PCR5_7_9_11"> |
<strong> PCR for amplification of antigens 5, 7, 9 and 11 (RE) </strong> | <strong> PCR for amplification of antigens 5, 7, 9 and 11 (RE) </strong> | ||
</p> | </p> | ||
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</li> | </li> | ||
</ul> | </ul> | ||
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<strong> Test Digests (RE) </strong> | <strong> Test Digests (RE) </strong> | ||
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</table></div> | </table></div> | ||
<!-- EDIT44 TABLE [19194-19490] --> | <!-- EDIT44 TABLE [19194-19490] --> | ||
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<strong> Test digest of all clones above (LS)</strong> | <strong> Test digest of all clones above (LS)</strong> | ||
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<strong>PCR: Salmonella mutagenesis (LS)</strong> | <strong>PCR: Salmonella mutagenesis (LS)</strong> | ||
</p> | </p> | ||
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</li> | </li> | ||
</ul> | </ul> | ||
− | <p> | + | <p id="TDbb15"> |
<strong> Test digest of pRIG15_15 (RE) </strong> | <strong> Test digest of pRIG15_15 (RE) </strong> | ||
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</li> | </li> | ||
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<strong>Repetition: PCR for Salmonella antibody (LS)</strong> | <strong>Repetition: PCR for Salmonella antibody (LS)</strong> | ||
</p> | </p> | ||
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Latest revision as of 07:59, 10 September 2015
Cloning
2015/08/01
Mini-Prep of the ligations for untagged antigens, pET_804 (3) and pIG15_804 (3) (RE)
- Qiagen-kit
- eluted in 30 µl dH2O
- NanoDrop:
plasmid | concentration [ng/µl] |
---|---|
pET_802 - 1 | 234.4 |
pET_802 - 2 | 204.0 |
pET_1002 - 1 | 223.2 |
pET_1002 - 2 | 214.6 |
pET_1102 - 1 | 220.3 |
pET_1102 - 2 | 236.4 |
pET_1502 - 1 | 199.0 |
pET_1502 - 2 | 250.0 |
pET_1702 - 1 | 238.9 |
pET_1702 - 2 | 213.7 |
pET_804 - 3 | 254.4 |
pET_804 - 3 | 257.7 |
pIG15_804 - 3 | 241.2 |
pIG15_804 - 3 | 322.3 |
Digest of the ILS plasmids (RE)
- Bba_K823013 with SpeI and PstI-HF
- Bba_K823008 with SpeI and PstI-HF
- Bba_K823005 with SpeI and PstI-HF
- Bba_I13504 with XbaI and PstI-HF
- 1 µl of each restr. enzyme
- 5 µl CutSmart
- 10 µl DNA
- 33 µl dH2O
- incubated for 1 h at 37°C
analysis on 1 % agarose gel:
Digest of pET_804 and pIG15_804 (RE)
Both plasmids were digested with BamHI and HindIII (to insert other antigens) as well as HindIII and AflII (to insert the Halo-tag instead of Spy)
- 1 µl of each restr. enzyme
- 5 µl FD Green Buffer
- 14 µl DNA
- 33 µl dH2O
- incubated for 5 min at 37°C
analysis on 1 % agarose gel: DNA is totally destructed by the enzymes
Repetition of the digest with NEB enzymes (RE)
- incubated for 1 h at 37°C
analysis on 1 % agarose gel: digest worked and the backbones were extracted from the gel (TAE buffer was exchanged before running the gel, maybe it caused the problems with DNA destruction instead of the restriction enzymes)
Test digest of pET_SpyC_GST (RE)
- 1 µl HindIII
- 1 µl PstI-HF
- 2 µl CutSmart
- 5 µl DNA
- 11 µl dH2O
- incubated for 1 h at 37°C
- expected fragment sizes: ~1700 and ~4100 bp
Test digest of pET_x02 (untagged antigens) (RE)
- 1 µl BamHI
- 1 µl PstI-HF
- 2 µl CutSmart
- 5 µl DNA
- 11 µl dH2O
- incubated for 1 h at 37°C
- expected fragment sizes:
Plasmid | Backbone | Antigen-containing fragment |
---|---|---|
pET_802 | ~4100 bp | ~1700 bp |
pET_1002 | ~4100 bp | ~1900 bp |
pET_1102 | ~4100 bp | ~3000 bp |
pET_1502 | ~4100 bp | ~3400 bp |
pET_1702 | ~4100 bp | ~1800 bp |
analysis of both test digests on 1 % agarose gel: DNA is destructed by the enzymes (TAE buffer was exchanged afterwards); only for pET_1502 and pET_1702, correct fragments are visible among the smeer
Ligations (RE)
- InterLab study:
Backbone | Bba_K823013 | Bba_K823008 | Bba_K82_3005 |
Backbone amount [µl] | 2.17 | 1 | 2.08 |
GFP (Bba_I13504) amount [µl] | 3.09 | 3.09 | 3.09 |
- Halo-tag:
Backbone | pIG15_804 |
Backbone amount [µl] | 0.93 |
Halo-tag amount [µl] | 4.5 |
- Antigens:
Backbone | pET_804 | pIG15_804 |
Backbone amount [µl] | 0.83 | 0.43 |
10 (HCV) amount [µl] | 2.12 | 1.18 |
11 (Tetanus) amount [µl] | 1.12 | 0.62 |
15 (Salmonella) amount [µl] | 1.21 | 0.67 |
17 (HIV) amount [µl] | 2.27 | 1.26 |
- 1 µl T4 ligase
- 2 µl T4 ligase buffer
- up to 20 µl dH20
- incubated for 1 h at RT
Transformation of the ligation products (5 µl) into E.coli TOP10 (RE)
- pILS1-3, pIG15_805 and pIG15_1004-1704 were plated on LB-cml
- pET_1004-1704 were plated on LB_amp
2015/08/03
Sequencing results (LS)
- pET_804 (3): correct
- pET_804 (4): correct
- pIG15_804 (3): correct
- pIG15_804 (4): correct
Test digest: pEtX04, pIG15_X04, pILS1-3 and pIG15_805 (LS)
- Interlab Study: pILS1, 2 and 3–>EcoRI HF and SpeI HF
6xMasterMix | |
---|---|
6µl | EcoRI HF |
6µl | SpeI Hf |
12µl | Cut smart |
66µl | dH2O |
- pETX04, pIG15_X04, pIG15_805–>BamHI HF and PstI HF
18xMasterMix | |
---|---|
18µl | BamHI HF |
18µl | PstI HF |
36µl | Cut smart |
198µl | dH2O |
- addition of 5µl plasmid each
- incubation at 37°C, 1h
- analysis on 1% agarose gel:
PCR for biobricks + PCR for GFP insert (LS)
Antigens 6, 8, 10, 11, 17 and 18 will be amplified using primers with matching overlap for pSB1C3 for Gibson cloning. The plasmids pIG15_X01 containg antigen fragments will be used as template. For GFP amplification pQE-60 GFP will be used as template.
MasterMix | |
---|---|
high GC buffer | 60µl |
dNTPs | 6µl |
DMSO | 9µl |
Polymerase | 3µl |
dH2O | 190,5µl |
+0,1µ template (~100ng/µl) +1µl of each primer
Cycling | |
---|---|
98°C | 3min |
98°C | 30s |
60°C | 30s |
72°C | 40s |
72°C | 10 min |
4°C | – |
- analysis on 1% agarose gel:
Gel-ex: PCR products (LS)
- qiagen kit
concentrations [ng/µl] | |
---|---|
GFP | 37,8 |
frg. 8 | 30,9 |
frg. 10 | 41,1 |
frg. 11 | 11,6 |
frg. 17 | 42,5 |
frg. 18 | 39,0 |
2015/08/04
Digest: pIG15_104 with EcoRI HF and SpeI HF (LS)
For Gibson assembly of the biobricks containing the antigens, digested backbone is needed. pIG15_104 is the cellfree expression vector inside the pSB1C3 standard and can thus be used for digestion.
Digest | |
---|---|
10µl | pIG15_104 |
1µl | SpeI HF |
1µl | EcoRI HF |
5µl | Cut Smart |
33µl | dH2O |
- 1h, 37°C
- analysis on 1% agarose gel
- gel-ex: 45,0ng/µl
Inoculation of Gly-Stocks in liquid LB-Amp (LS)
To build biobricks with all antigens some of the Gly-stocks have to be inoculated again, followed by miniprep of the respective plasmids. The following E.coli Gly-stocks were inoculated:
- pIG15_301
- PIG15_401
- pIG15_501
- pIG15_701
- pIG15_901
- incubation at 37°C, shaking
Gibson-Assembly (RE)
- inserts: PCR products of the antigens 8, 10, 11, 17 and 18
- backbone: pSB1C3, EcoRI and SpeI digested
- DNA-Mix:
Antigen | Backbone [µl] | Antigen [µl] |
---|---|---|
8 | 0.53 | 1.24 |
10 | 0.53 | 1.4 |
11 | 0.24 | 4.76 |
17 | 0.53 | 1.14 |
18 | 0.53 | 1.23 |
- 5 µl were directly transformed into E. coli TOP10
Transformation (RE)
- pET_804
- pIG15_804
- pET_SpyC_GST
- pIG15_1104
- pILS_1
- pILS_2
- pILS_3
- pET_804 and pET_SpyC_GST were plated on LB_amp
- all the others were plated on LB_cml
2015/08/05
Inocculation of 5 ml liquid culture (RE)
- pET_804 (LB_amp, 2x)
- pIG15_804 (LB_cml, 2x)
- pET_SpyC_GST (LB_amp)
- pIG15_1104 (LB_cml)
- pILS_1 (LB_cml)
- pILS_2 (LB_cml)
- pILS_3 (LB_cml)
Preparation of Gibson MasterMix (RE)
- according to the protocol of AG Weber
- 100 µl 5X ISO Buffer
- 50 µl Taq ligase
- 6.25 µl Phusion polymerase
- 0.2 µl T5 Exonuclease
- 218.55 µl ddH2O
- –> 15 µl aliquots stored at -20°C
Mini-Prep (LS)
- qiagen kit
concentrations | |
---|---|
pIG15_401 | 715,8 |
pIG15_301 | 243,1 |
pIG15_501 | 437,3 |
pIG15_701 | 329,3 |
pIG15_901 | 606,5 |
PCR for amplification of the antigens (LS)
- amplification of the following antigens: 3,4,5,6,7,9
- 2×20µl each (antigen 6: 4×20µl)
- PCR mix and cycling protocol same way as last time (3.8.2015)
Inoculation (LS)
- 3 colonies from Gibson-Assembly plates each
- 5ml LB-Amp
- incubation at 37°C o/n
Mini-Prep (RE)
- Qiagen-Kit
- eluted in 30 µl dH2O
- pET_804
- pIG15_804
- pET_SpyC_GST
- pIG15_1104
2015/08/06
Digest of pET_804 and pIG15_804 (RE)
- ~2 µg per construct were digested with BamHI and HindIII for insertion of antigens
- ~1 µg per construct was digested with HindIII and AflII for insertion of the Halo-tag
- 1 µl of each restriction enzyme (Fermentas)
- 5 µl FD Green Buffer
- ad 50 µl dH2O
Analysis of PCR (from yesterday) on 1% agarose gel (LS)
Gel-ex: PCR products for biobricks (LS)
- qiagen kit
concentrations [ng/µl] | |
---|---|
antigen 6 | 59,1 |
antigen 4 | 54,1 |
antigen 5 | 6,9 |
antigen 3 | 109,9 |
Digest: pET804 with BamHI+HindIII and HindIII+AflII (LS)
Digest | |
---|---|
1µl | FD BamHI/AflII |
1µl | FD HindIII |
5µl | FD buffer |
5/3µl | DNA |
- incubation at 37°C, 30 min
Mini-Prep of Gibson products for standardized plasmids (LS)
- Zymo Research kit
concentrations | ||
---|---|---|
pRIG15_8 | 1 | 429,5 |
2 | 180,2 | |
3 | 190,9 | |
pRIG15_10 | 1 | 176,4 |
2 | 352,5 | |
3 | 184,5 | |
pRIG15_18 | 1 | 231,0 |
2 | 199,4 | |
3 | 189,1 |
Test digest of standardized plasmids (LS)
- digest with: EcoRI HF and PstI HF
Master Mix | |
---|---|
5,5µl | EcoRI HF |
5,5µl | PstI HF |
22µl | buffer |
132µl | dH2O |
+5µl plasmid DNA |
- incubation at 37°, 1h
- analysis on 1% agarose gel
PCR for amplification of antigens 5, 7, 9 and 11 (RE)
- gradient for annealing temp., because the PCR did not work for those antigens the last time
- 5X Master-Mix per antigen
- 20 µl Phusion High GC Buffer
- 5 µl of each primer
- 2 µl dNTPs
- 3 µl DMSO
- 1 µl Phusion polymerase
- 0.5 µl Template (100 ng/µl)
- 63.5 µl dH2O
cycling:
- the same cycling conditions as before were used, except the gradient for the annealing temperature (55°C-65°C)
analysis on 1% agarose gel:
- amplification of 5, 7 and 9 was successful for every annealing temperature
- amplification of 11 did not work again
Gel-Ex of the PCR products (RE)
- Qiagen-Kit
- eluted in 20 µl dH2O
- 5: 72.4 ng/µl
- 7: 98.3 ng/µl
- 9: 76.7 ng/µl
Ligations (RE)
- 1 µl T4 ligase
- 2 µl T4 ligase buffer
- ad 20 µl dH2O
- incubation 1 h at RT
- transformation of 5 µl ligation product into E. coli TOP10
Backbone | Backbone amount [µl] | Insert | Insert amount [µl] |
---|---|---|---|
pET_804 (BamHI and HindIII digested ) | 6 | 10 | 10.77 |
pET_804 (BamHI and HindIII digested ) | 6 | 11 | 10.84 |
pET_804 (BamHI and HindIII digested ) | 6 | 15 | 10.84 |
pET_804 (BamHI and HindIII digested ) | 6 | 17 | 10.66 |
pIG15_804 (BamHI and HindIII digested ) | 5.43 | 10 | 1.55 |
pIG15_804 (BamHI and HindIII digested ) | 5.43 | 15 | 1.06 |
pIG15_804 (BamHI and HindIII digested ) | 5.43 | 17 | 2.31 |
pET_804 (HindIII and AflII digested ) | 10.42 | Halo | 0.66 |
pIG15_804 (HindIII and AflII digested ) | 3.09 | Halo | 1.2 |
Gibson-Assembly (JN)
- assembly of pSB1C3 backbone with different antigens for standardization
Backbone amount [µl] | Insert | Insert amount [µl] | H2O [µl] |
---|---|---|---|
0.53 | 3 | 0.88 | 3.59 |
0.53 | 4 | 1.75 | 2.69 |
0.53 | 5 | 1.33 | 3.13 |
0.53 | 6 | 0.41 | 4.06 |
0.53 | 7 | 1.47 | 3.00 |
0.53 | 9 | 1.52 | 2.95 |
2015/08/07
Inoculation of ligation/gibson clones (LS)
- 2x each
- 5ml LB-Amp/Cml
- 37°C, shaking
Repetition of PCR for biobrick fragments: 10, 11, and 18 (LS)
- 4×20µl, gradient PCR
Master Mix | |
---|---|
high GC buffer | 16µl |
primer 1 | 4µl |
primer 3 | 4µl |
dNTPs | 1,6µl |
DMSO | 2,4µl |
Phusion Polymerase | 0,8µl |
template | 0,4µl |
dH2O | 50,8µl |
cycling | |
---|---|
98°C | 3min |
98°C | 30s |
55°C-65°C | 30s |
72°C | 1min |
72°C | 10min |
4°C | – |
- analysis on 1% agarose gel
- 11 did not work…
Mini-Prep (JN)
- pRIG15_06/07, pIG15_1004/1504/1704, pET_1004/1104
- Qiagen kit
- eluted in 30µl dH2O
plasmid | concentration [ng/µl] |
---|---|
pRIG15_06 - 1 | 72.5 |
pRIG15_06 - 2 | 82.8 |
pRIG15_07 - 1 | 92.1 |
pRIG15_07 - 2 | 111.4 |
pIG15_1004 - 1 | 144.5 |
pIG15_1004 - 2 | 147.9 |
pIG_1504 - 1 | 130.4 |
pIG_1504 - 2 | 151.2 |
pIG_1704 - 1 | 74.1 |
pIG_1704 - 2 | 69.3 |
pET_1004 - 1 | 78.0 |
pET_1004 - 2 | 57.0 |
pET_1104 - 1 | 100.8 |
pET_1104 - 2 | 125.0 |
2015/08/08
Mini-Prep (RE)
- Biozym-kit (Solution 2 from Peqlab-kit was used, because it was empty in the Biozym-kit)
- eluted in 30 µl dH2O
- pET_1504 - 1: 156.4 ng/µl
- pET_1505 - 2: 84.2 ng/µl
- pET_1704 - 1: 104.8 ng/µl
- pET_1704 - 2: 144.7 ng/µl
- pIG15_805 - 1: 189.1 ng/µl
Test Digests (RE)
- pRIG15_06 and pRIG15_07 with EcoRI-HF and PstI-HF (NEB –> 1 h incubation at 37°C)
- pET_1001, pET_1104, pET_1504, pET_1704, pIG15_1004, pIG15_1504, pIG15_1704 with BamHI and HindIII (Fermentas FD –> 30 min incubation at 37°C)
- pIG15_805 with HindIII and AflII (Fermentas FD –> 30 in incubation at 37°C)
Repetition of Test Digests (JN)
- pET_1001, pET_1104, pET_1504, pET_1704, pIG15_1004, pIG15_1504, pIG15_1704 with BamHI and HindIII (Fermentas FD –> 15 min incubation at 37°C)
Gel-ex: PCR product for biobricks 10 and 18 (LS)
- qiagen kit
- eluted in 20µl
concentrations [ng/µl] | |
---|---|
fragment 10 | 50,9 |
fragment 18 | 55,3 |
Repetition of PCR for biobrick 11 (LS)
Q5 Master Mix | |
---|---|
Q5 2x Master Mix | 50µl |
oIG15_b1101 | 5µl |
oIG15_b1102 | 5µl |
dH2O | 19,6µl |
pIG15_1101 | 0,4µl |
- 4×25µl
cycling | |
---|---|
98°C | 3min |
98°C | 30s |
55°C-65°C | 30s |
72°C | 1min |
72°C | 10min |
4°C | – |
- analysis on 1% agarose gel
Transformation (LS)
blunt-end ligation: GFP ind pJet | |
---|---|
0,3µl | GFP (PCR product |
1µl | T4 DNA Ligase |
10µl | 2x buffer |
1µl | pJet |
up to 20µl | dH2O |
- 5min, RT
Gibson | |
---|---|
1.15µl | |
0.53µl | pSB1C3 |
+Gibson mix |
- transformation of blunt-end ligation/ gibson (7µl) in E.coli T10
- transformation of pIG15_105 (1µl) in E.coli T10
- transformation according to protocol
PCR for fragment 17 with HA-tag (LS)
Primer combination | ||
---|---|---|
resulting plasmid | primer 1 | primer2 |
pET_1703-HA | oIG15_17_HA002 | oIG15_17_HA004 |
pET_1704-HA | oIG15_17_HA001 | oIG15_17_HA005 |
pET_1705-HA | oIG15_17_HA001 | oIG15_17_HA006 |
pIG15_1704-HA | oIG15_17_HA003 | oIG15_17_HA005 |
pIG15_1705-HA | oIG15_17_HA003 | oIG15_17_HA006 |
Q5 PCR (x25µl) | |
---|---|
25µl | Q5 MM |
2.5µl | primer 1 |
2.5µl | primer 2 |
0.4µl | pIG15_1701 |
9.6µl | dH2O |
cycling | |
---|---|
98°C | 3min |
98°C | 30s |
55°C-65°C | 30s |
72°C | 1min |
72°C | 10min |
4°C | – |
- analysis on 1% agarose gel
- gel-ex:qiagen kit
Inoculation: pIG15_105 and pIG15_805 (LS)
- 5ml LB-ml
- 37°C, shaking o/n
2015/08/09
Inoculation: pRIG15_10, pRIG15_18, ligation of pJet_GFP (JN)
- 3 clones for each
- 5ml LB-medium (pRIG with Cml, pJet with Amp)
- 37°C, shaking, until evening
Gibson Assembly (JN)
- antigen 11 with pSB1C3 backbone to send it in
- pET_803 backbone with 1703-HA
- pET_804 backbone with 1704-HA
ingredient | pRIG15_11 | pET_1703-HA | pET_1704-HA |
---|---|---|---|
backbone | 0.53µl | 0.94µl | 1.47µl |
insert | 1.21µl | 2.32µl | 0.75µl |
H2O | 3.26µl | 1.73µl | 2.78µl |
- transformation into E.coli Top10 and plating (pRIG on Cml, pET on Amp)
Mini-Prep of pIG15_105 and pIG15_805 (JN)
- Zymo Research kit
- eluted in 30 µl dH2O
- NanoDrop:
plasmid | concentration [ng/µl] |
---|---|
pIG15_105 | 23.2 |
pIG15_805 | 28.8 |
Digest: pIg15_105, pIG15_804 and pIG15_805 (LS)
- pIG15_105: HindIII + AflII
- pIG15_804:BamHI + HindIII
- pIg15_805: BamHI + HindIII
- 5µl FD green buffer
- 1µl of Enzyme 1 and 2 each
- up to 50µl dH2O
- incubation at 37°C for approx. 45min
- analysis on 1% agarose gel: no results for pIG15_105 and pIG15_805
- gel-ex (qiagen kit): pIg15_804 backbone. 65,8ng/µl
Blunt-end ligation: Antigen 15 (Salmonella) in pJET + Transformation (LS)
Ligation | |
---|---|
volume [µl] | component |
0,6 | PCR product antigen 15 |
1µl | linearized pJET |
10µl | 2x reaction buffer |
1µl | T4 DNA ligase |
up to 20µl | dH2O |
- 5min, RT
- transformation in E.coli T10 (transformation according to protocol)
Mini-prep of pJet_GFP and pRIG15_10 (RE)
- Zymo-kit
- pelleted cells were resuspended in LB medium
- elution in 30 µl dH2O
- NanoDrop:
plasmid | concentration [ng/µl] |
---|---|
pJet_GFP - 1 | 233.9 |
pJet_GFP - 2 | 154.9 |
pJet_GFP - 3 | 195.6 |
pRIG15_10 - 1 | 39.6 |
pRIG15_10 - 2 | 141.5 |
pRIG15_10 - 3 | 46.1 |
Test digest of pJet_GFP and pRIG15_10 (RE)
- pJet_GFP was digested with BamHI and HindIII (FastDigest; 30 min incubation)
- pRIG15_10 was digested with EcoRI-HF and PstI-HF (NEB; 1 h incubation)
- 1 µl of each restriction enzyme
- 2 µl of the respective buffer
- 5 µl DNA
- 11 µl dH2O
- incubation at 37°C
Inocculation of liquid cultures (RE)
- pRIG15_11 (LB_cml)
- pET_1703_HA (LB_amp)
- pET_1704_HA (LB_amp)
- 3 clones each
2015/08/10
Mini-Prep of pRIG15_11 (antigen 11 for iGEM Registry), pET_1703-HA and pET_1704-HA (JN)
- Zymo Research kit
- eluted in 30 µl dH2O
- NanoDrop:
plasmid | concentration [ng/µl] |
---|---|
pRIG15_11 - 1 | 132.6 |
pRIG15_11 - 2 | 350.3 (strange curve) |
pRIG15_11 - 3 | 93.4 |
pET_1703-HA - 1 | 92.7 |
pET_1703-HA - 2 | 119.0 |
pET_1703-HA - 3 | 89.4 |
pET_1704-HA - 1 | 121.3 |
pET_1704-HA - 2 | 102.1 |
pET_1704-HA - 3 | 122.4 |
Test digest of all clones above (LS)
- pRIG15_11. EcoRI + PstI (1h incubation at 37°C)
- pET1703/4-_HA: BamHI + AflII (30 min incubation at 37°C)
- 5µl plasmid
- 1µl of each restriction enzyme
- 2µl 10x buffer
- up to 20µl dH2O
- analysis on 1% agarose gel
2015/08/11
Digest of pJet_GFP 1-3, pET_1703_HA and pET_1704_HA (RE)
- 1 µl BamHI
- 1 µl HindIII
- 5 µl FD Green Buffer
- 10 µl DNA
- 33 µl dH2O
- incubation for 30 min at 37°C
Ligation (LS)
Backbone | Insert | ||||
---|---|---|---|---|---|
concentration [ng/µl] | volume [µl] | concentration [ng/µl] | volume [µl] | ||
pET_1703-HA (BamHI+HindIII) | 21,7 | 2,3 | Tetanus (antigen 11) | 58,9 | 0,25 |
GFP | 17,7 | 1,19 | |||
pET_1704-HA (BamHI+HindIII) | 16,0 | 3,31 | Tetanus (antigen 11) | 58,9 | 0,36 |
GFP | 17,7 | 1,19 | |||
pET_804 (HindIII+AflII) | 4,8 | 10,34 | Halo-tag | 37,6 | 0,56 |
pIG15_804 (HindIII+AflII | 16,2 | 3,09 | Halo-tag | 37,6 | 0,93 |
pET_804 (BamHI+HindIII | 116,4 | 0,43 | HIV(antigen 17 | 10,8 | 1,39 |
Salmonella (antigen 15 | 70,7 | 0,72 | |||
Tetanus (antigen 11) | 58,9 | 0,25 | |||
HCV (antigen 10 | 12,9 | 1,37 | |||
GFP | 17,7 | 1,19 | |||
pIG15_804 (BamHI and HindIII) | 65,9 | 0,76 | HIV (antigen 17) | 10,8 | 2,31 |
Salmonella (antigen 15 | 70,7 | 1,2 | |||
HCV (antigen 10 | 12,9 | 1,94 | |||
GFP | 17,7 | 1,98 |
- added 2µl T4 DNa Ligase buffer
- 1µl T4 DNA Ligase
- up to 20µl dH2O
- incubation at Rt for 1h
- Transformation into E.coli T10 (according to protocol)
Retrafo: pET_1703-HA in E.coli T10 (LS)
- 1µl plasmid
- transformation according to protocol
Inoculation of pSB1C3_SpyC (JN)
- 3 colonies were picked and inoculated in 5ml each of LB-medium with Cml
Mini-prep of pJet_15 (JN)
- ZymoResearch kit
- eluted in 30µl dH2O
- concentrations
plasmid | concentration [ng/µl] |
---|---|
pJet_15-1 | 240.9 |
pJet_15-2 | 259.2 |
Digest with BamHI and HindIII of pJet_15 (JN)
ingredient | amount [µl] |
---|---|
DNA | 5 |
buffer | 5 |
BamHI | 1 |
HindIII | 1 |
H2O | 38 |
- 37°C for 30min
- analysis on 1% agarose gel
Gel-ex of fragment 15 (JN)
- fragment 15, digested with BamHI and HindIII, was extracted out of the gel
- Qiagen gel extraction kit
- concentrations
fragment 15 -1 | 16.7 ng/µl |
fragment 15 -2 | 16.6 ng/µl |
2015/08/12
Inoculation of many colonies (RE/JN)
- Gibson and ligation
- in 5ml LB medium
- 2 colonies each
Mini-prep of pSB1C3_SpyC_correct (JN)
- ZymoResearch kit
- eluted in 30µl dH2O
- concentrations
plasmid | concentration [ng/µl] |
---|---|
pSB1C3_SpyC_correct-1 | 76.3 |
pSB1C3_SpyC_correct-2 | 263.5 |
pSB1C3_SpyC_correct-2 | 89.4 |
Test-digest of pSB1C3_SpyC_correct (JN)
ingredient | amount [µl] |
---|---|
DNA | 5 |
EcoRI | 0.5 |
PstI | 0.5 |
buffer | 2 |
dH2O | 12 |
- 37°C for 1 hour
- analysis on 1% agarose gel
Mini-prep (JN)
- Qiagen kit
- eluted in 30dH2O
- concentrations
plasmid | concentration [ng/µl] |
---|---|
pET_1704-1 | 129.0 |
pET_1704-2 | 94.2 |
pET_805-1 | 84.6 |
pET_805-2 | 119.7 |
pET_203-HA-1 | 68.6 |
pET_203-HA-2 | 77.6 |
pET_1504-1 | 50.1 |
pET_1504-2 | 47.5 |
pET_1103-HA-2 | 48.8 |
pET_1104-HA-1 | 39.4 |
pET_1104-HA-2 | 56.8 |
pRIG15_10-1 | 106.8 |
pRIG15_10-2 | 145.6 |
Test digests (RE)
- pRIG15_10
–> EcoRI + PstI
- pET_805
- pIG15_805
–> HindIII + AflII
- pET_1704
- pET_203_HA
- pET_1103_HA
- pET_1104_HA
- pET_1504
- pET_1004
- pET_1104
- pET_204
- pET_204_HA
- pIG15_1504
- pIG15_1704
- pIG15_204
–> BamHI + HindIII
Mini-Prep (LS)
- qiagen kit
plasmid | concentration [ng/µl] |
---|---|
pET_1104 (1) | 172,8 |
pET_1104 (2) | 116,2 |
pET_204(1) | 160,6 |
pET_204 (2) | 172,2 |
pET_204-HA (1) | 228,6 |
pET_204-HA (2) | 146,5 |
pIG15_805 (1) | 394,0 |
pIG15_805 (2) | 463,2 |
Sequencing (RE)
- pET_203_HA - 1
- pET_204 - 1
- pET_204_HA - 1
- pET_1104 - 1
- pET_1104_HA - 1
- pET_1704 - 1
- pIG15_204_HA - 1
- pIG15_1704 - 1
- pIG15_805 - 1
- pRIG15_10 - 2
edit 08/13: all results are positive, except pRIG15_10. pIG15_805 should be sequenced with a reverse primer again to verfiy the whole Halo-tag sequence.
Ligations (RE)
Backbone | Insert | ||||||
---|---|---|---|---|---|---|---|
new plasmid | name | c [ng/µl] | V [µl] | name | c [ng/µl] | V [µl] | dH2O [µl] |
pET_1504 | pET_804 (BamHI+HindIII) | 127.6 | 0.39 | fragment 15 (from pJet) | 16.7 | 2.45 | 14.16 |
pET_1004 | pET_804 (BamHI+HindIII) | 127.6 | 0.39 | fragment 10 | 26.7 | 0.59 | 16.02 |
pIG15_1504 | pIG15_804 (BamHI+HindIII) | 65.9 | 0.76 | fragment 15 (from pJet) | 16.7 | 2.45 | 11.83 |
pIG15_1004 | pIG15_804 (BamHI+HindIII) | 65.9 | 0.76 | fragment 10 | 26.7 | 1.06 | 15.18 |
pET_805 | pET_804 (HindIII+AflII) | 57.5 | 0.88 | Halo tag | 37.6 | 0.66 | 15.46 |
- 1 µl T4 ligase
- 2 µl T4 ligase buffer
- incubated for 1h at RT
- directly transformed into E. coli TOP10 (pET constructs plated on LB_amp; pIG15 constructs plated on LB_cml)
2015/08/13
Inocculation of liquid cultures (RE)
- yesterday's ligations
- 2 single colonies per construct
Test digest: pIG15_1704 (LS)
- 5µl plasmid
- 1µl BamHI + HindIII
- 2µl buffer
- up to 20µl dH2O
- analysis on 1% agarose gel
2015/08/14
Inoculation of pIG15_1504/10004, pET_1004/805/1504 (JN)
- 5ml LB-medium each
Mini-Prep of pIG15_1704-HA (JN/LS)
- Zymo Research kit
- eluted in 30µl H2O
- concentrations
plasmid | concentration [ng/µl] |
---|---|
pIG15_1704-HA-1 | |
pIG15_1704-HA-2 |
Test-Digest pIG15_1704-HA (LS)
Mini-Prep of pIG15_1504/10004, pET_1004/805/1504 (JN)
- Zymo Research kit
- eluted in 30µl H2O
- concentrations
plasmid | concentration [ng/µl] |
---|---|
pIG15_1504-1 | 71.6 |
pIG15_1504-2 | 34.8 |
pIG15_1004-1 | 79.9 |
pIG15_1004-2 | 80.2 |
pET_1004-1 | 68.9 |
pET_1004-2 | 54.8 |
pET_805-1 | 53.0 |
pET_805-2 | 58.1 |
pET_1504-1 | 63.4 |
pET_1504-2 | 60.3 |
Digest of pIG15_805 (RE)
- 1 µl BamHI
- 1 µl HindIII
- 5 µl FD Green Buffer
- 5 µl DNA
- 38 µl dH2O
- incubation for 30 min at 37°C
Gel-Ex of pIG15_805 backbone (RE)
- Qiagen-kit
- eluted in 20 µl dH2O
- NanoDrop: 39.6 ng/µl
2015/08/15
Ligations (RE)
- Backbone: pIG15_805 (BamHI and HindIII digested; 39.6 ng/µl) 1.25 µl
- Inserts:
- fragment 10: 0.87 µl
- fragment 11: 0.9 µl
- fragment 15: 3.78 µl
- fragment 17: 2.14 µl
- GFP: 1.67 µl
- + ligation control
- Backbone: pET_804 (HindIII and AflII digested) 0.86 µl
- Insert: Halo-tag 0.66 µl
- incubation for 1 h at RT
- 5 µl ligation product were directly transformed into E. coli TOP10
Transformation for ProtPur (RE)
- pET_203_HA into E. coli BL21 pLys
- pET_1104_HA into E. coli C43
- pET_1704_HA into E. coli BL21 pLys
Mini-Prep of Retrafo pET_1703-HA (JN)
- Zymo Research kit
- eluted in 30µl dH2O
- concentration: 57.1ng/µl
Test-Digest of pET_805/1004/1504, pIG15_1004/1504 (JN)
ingredient | pET_805 | all the others |
---|---|---|
DNA | 5µl | 5µl |
BamHI | - | 1µl |
HindIII | 1µl | 1µl |
AflII | 1µl | - |
buffer | 2µl | 2µl |
DNA | 11µl | 11µl |
- 30min at 37°C
- analysis on 1% agarose gel but with unknown ladder –> no reliable statement about digest possible
2015/08/16
Digest (RE)
- analysis on 1% agarose gel
Gel-ex of fragment 15, backbones pET_1104/1704-HA, pIG15_804/805/1704-HA (JN)
- Qiagen kit
- eluted in 20µl dH2O
DNA | concentration [ng/µl] |
---|---|
fragment 15 | 12.5 |
pET_1104 | 12.9 |
pET_1704-HA | 9.3 |
pIG15_804 | 19.7 |
pIG15_805 | 7.2 |
pIG15_1704-HA | 12.8 |
Ligation of fragment 15 into different backbones, GFP into pIG15_805, Halo into pET_804 (JN)
Backbone | Insert | ||||
---|---|---|---|---|---|
new plasmid | name | V [µl] | name | V [µl] | dH2O [µl] |
pET_1504 | pET_1104 (BamHI+HindIII) | 3.9 | fragment 15 (from pJet) | 3.7 | 9.4 |
pET_1504-HA | pET_1704-HA (BamHI+HindIII) | 5.4 | fragment 15 (from pJet) | 2.8 | 8.8 |
pIG15_1504 | pIG15_804 (BamHI+HindIII) | 2.5 | fragment 15 (from pJet) | 8.5 | 6 |
pIG15_1504-HA | pIG15_1704-HA (BamHI+HindIII) | 3.9 | fragment 15 (from pJet) | 8.5 | 4.6 |
pIG15_1505 | pIG15_805 (BamHI+HindIII) | 6.9 | fragment 15 (from pJet) | 6.9 | 3.7 |
pIG15_205 | pIG15_805 (BamHI+HindIII) | 6.9 | GFP (PCR product) | 6.9 | 8.1 |
pET_805 | pET_804 (HindIII+AflII) | 0.9 | Halo tag | 1.2 | 14.9 |
- 1 µl T4 ligase
- 2 µl T4 ligase buffer
- incubated for 1h at RT
Transformation (RE)
- 5 µl of the ligation products and the Gibson Mix into E. coli TOP10
- pET constructs were plated on LB_amp
- pIG15 constructs were plated on LB_cml
Mini-prep (RE)
- Zymo-Kit; elution into 30 µl dH2O
- pIG15_1005 - 1: 230.9 ng/µl
- pIG15_1005 - 2: 162.1 ng/µl
- pIG15_1105 - 1: 121.3 ng/µl
- pIG15_1105 - 2: 117.8 ng/µl
- pIG15_1505 - 1: 96.6 ng/µl
- pIG15_1505 - 2: 139.1 ng/µl
2015/08/17
Test digests (RE)
- pIG15_1005, pIG15_1105 and pIG15_1505 with BamHI and HindIII (FastDigest)
- pRIG15_10 with EcoRI and SpeI (NEB)
- 0.5 µg DNA
- 1 µl of each RE
- 2 µl of the respective buffer
- ad 20 µl dH2O
- incubation for 30 min (FastDigest) or 1 h (NEB) at 37°C
Seuencing (RE) The following constructs have been send in for sequencing:
- pIG15_1005 - 2
- pIG15_1105 - 1
- pIG15_1505 - 1
- pIG15_805 - 2 (again with the pET_RP to verfiy the sequence of the Halo-tag)
Re-trafo (RE)
- of pIG15_1704_HA into E. coli TOP10
Inoculation of pET_1504/1504-HA, pIG15_1504/1504-HA/1505/1705-HA/205 (JN)
- 2 single colonies were picked of each plate
- in 5ml LB medium (pET with Amp, pIG15 with Cml)
Resuspension of IDT gBlocks (JN)
- pOP fragment 1 was eluted in 50µl dH2O, pOP fragment 2/3/4/5 were eluted in 100µl dH2O after short centrifugation
- according to the protocol delivered by IDT the fragments were incubated at 50°C for 20min and afterwards vortexed and centrifuged again
Ligation of pOP fragments into blunt end pJet (JN)
- the delivered fragments were cloned into blunt end pJet according to protocol
ingredient | amount [µl] |
---|---|
DNA | 1 |
pJet | 0.5 |
T4 buffer | 2 |
T4 ligase | 1 |
dH2O | 5.5 |
- incubation for 5min at RT
- directly afterwards trafo with 5 µl according to protocol into E.coli TOP10
Gibson Assembly 1 of pOP (JN)
- pOP fragments 2+3+4 were assembled via Gibson according to protocol
ingredient | amount [µl] |
---|---|
fragment 2 | 2 |
fragment 3 | 2 |
fragment 4 | 1 |
- trafo with 5µl according to protocol into E.coli TOP10 followed directly after short incubation
Mini-Prep (JN)
- Zymo Research kit
- eluted in 30µl dH2O
plasmid | concentration [ng/µl] |
---|---|
pET_1504-1 | 54.8 |
pET_1504-2 | 63.3 |
pET_1504-HA-1 | 85.5 |
pET_1504-HA-2 | 59.3 |
pIG15_1705-HA-1 | 64.3 |
pIG15_1705-HA-2 | 114.8 |
pIG15_205-1 | 140.6 |
pIG15_205-2 | 66.9 |
pIG15_1504-1 | 77.5 |
pIG15_1504-2 | 77.2 |
pIG15_1504-HA-1 | 64.1 |
pIG15_1504-HA-2 | 92.5 |
pIG15_1505-1 | 80.4 |
pIG15_1505-2 | 119.2 |
2015/08/18
Inoculation (JN)
- pJet_pOP fragments in 5ml LB-Amp
- Re-trafo pIG15_1704-HA in LB Cml
- Gibson 1 pOP in LB without antibiotics
Test-digest of pET_1504/1504-HA, pIG15_1504/1504-HA/1505/1705-HA/205 (JN)
- all prepared the same way with BamHI and HindIII
ingredient | amount [µl] |
---|---|
DNA | 5 |
BamHI | 1 |
HindIII | 1 |
FD buffer | 2 |
dH2O | 11 |
- incubation for 30min at 37°C
- analysis on 1% agarose gel
Mini-Prep of pOP Gibson 1 (JN)
- Qiagen kit
- eluted in 30µl dH2O
plasmid | concentration [ng/µl] |
---|---|
pOP Gibson 1 (1) | 61.8 |
pOP Gibson 1 (2) | 41.3 |
pOP Gibson 1 (3) | 40.7 |
pOP Gibson 1 (4) | 20.4 |
pOP Gibson 1 (5) | 6.1 |
pOP Gibson 1 (6) | 20.4 |
pOP Gibson 1 (7) | 46.2 |
pOP Gibson 1 (8) | 68.0 |
pOP Gibson 1 (9) | 61.6 |
pOP Gibson 1 (10) | 63.6 |
pOP Gibson 1 (11) | 61.0 |
Digest of pOP Gibson 1 (8) and (10) (JN)
ingredient | amount (8) [µl] | amount (10) [µl] |
---|---|---|
DNA | 14.7 | 15.7 |
BamHI | 1 | 1 |
HindIII | 1 | 1 |
FD buffer | 5 | 5 |
dH2O | 28.3 | 27.3 |
- 30min at 37°C
- analysis on 1% agarose gel
Digest of fragment 2 + 4 of pOP for 5-fragment Gibson (JN)
ingredient | amount [µl] |
---|---|
fragment | 44 |
enzyme | 1 |
FD buffer | 5 |
- fragment 2 digested with HindIII
- fragment 4 digested with BamHI
- 30min at 37°C
- analysis on 1% agarose gel
Gel-ex fragment 2+4 digest (RE)
- Qiagen-Kit
- eluted in 15 µl dH2O
- fragment 2: 6.7 ng/µl
- fragment 4: 8.1 ng/µl
Gibson assembly for pOP (JN)
- fragment 1, digested fragment 2, fragment 3, digested fragment 4, fragment 5
fragment | amount [µl] |
---|---|
1 | 0.5 |
2 | 2 |
3 | 1 |
4 | 0.5 |
5 | 1 |
- DNA added to Gibson Master Mix
- after 5min of incubation at RT, 5µl were used for a transformation into E.coli TOP10 according to protocol
- the rest was incubated for 1h at 50°C, 3min at RT, 3min on ice
- then another transformation was performed
- both were plated on Amp plates
Mini-Prep of pJet_pOP fragments and pIG15_1704-HA (JN)
- Zymo Research kit
- eluted in 30µl dH2O
plasmid | concentration [ng/µl] |
---|---|
pJet_pOP1 (1) | 132.9 |
pJet_pOP1 (2) | 194.9 |
pJet_pOP2 (1) | 189.0 |
pJet_pOP2 (2) | 193.3 |
pJet_pOP3 (1) | 130.6 |
pJet_pOP3 (2) | 183.9 |
pJet_pOP4 (1) | 205.9 |
pJet_pOP4 (2) | 116.4 |
pJet_pOP5 (1) | 213.8 |
pJet_pOP5 (2) | 91.3 |
pIG15_1704-HA (1) | 83.0 |
pIG15_1704-HA (2) | 138.6 |
2015/08/19
PCR for pOP Gibson (JN)
As the fragments for the pOP vector were wrongly cloned, there is a antibiotic resistance missing after the first Gibson Assembly. Therefore, colonies cannot be selected for taking up the plasmid. Yesterday we tried an approach with a 5 fragment Gibson Assembly but no colonies were growing on the plate overnight. The next approach is to assemble two and accordingly 3 fragments via PCR. We decided to use fragments 5, 1 and 2 for one reaction, where the antibiotic resistance would be restored. The other reaction should assemble fragments 3 and 4. The PCR reaction mixes were prepared as follows. For the first reactions, the primers pOOP_5fw and pOOP_2rv were used, for the second pOOP_3fw and pOOP_4rv. As template a 1:10 dilution of the prepped pJet constructs (1) from yesterday was prepared. From this dilution 1µl per fragment was used.
ingredient | fr. 5,1,2 | fr. 3,4 |
---|---|---|
template | 3µl | 2µl |
Phusion | 0.5µl | 0.5µl |
dNTP | 1µl | 1µl |
primer fw | 2.5µl | 2.5µl |
primer rv | 2.5µl | 2.5µl |
DMSO | 1.5µl | 1.5µl |
buffer | 10µl | 10µl |
dH2O | 29µl | 30µl |
Cycling | |
---|---|
98°C | 3min |
98°C | 30s |
60°C | 20s |
72°C | 1min |
72°C | 10 min |
4°C | – |
- analysis on 1% agarose gel
Gel-ex of pOP_512 and pOP_34 (JN)
- Qiagen kit
- eluted in 20µl dH2O
plasmid | concentration [ng/µl] |
---|---|
pOP_512 | 6.3 |
pOP_34 | 4.3 |
Gibson Assembly of PCR products pOP_512 and pOP_34 for pOP (JN)
- 1.5µl of pOP_512 and 3.5µl of pOP_34 were added to Gibson Master Mix
- after 5min of incubation at RT, 5µl were used for a transformation into E.coli TOP10 according to protocol
- the rest was incubated for 1h at 50°C, 3min at RT, 3min on ice
- then another transformation was performed
- both were plated on Amp plates
PCR for SpyCatcher amplification (RE)
- The SpyCatcher was amplified with two different reverse primers. oIG15_SpyC_02 a HindIII restrcition site, oIG15_SpyC_03 a BamHI site. PCR fragments obtained by 02 are named 1-2, the others 1-3.
Ingredient | Volume [µl] |
---|---|
Template (pSB1C3 with SpyC (Munich)) | 0.25 |
Fwd primer (oIG15_SpyC_01) | 2.5 |
Rev primer (oIG15_SpyC_02 or _03) | 2.5 |
dNTPs | 1 |
DMSO | 1.5 |
High GC Buffer | 1 |
Phusion polymerase | 0.5 |
dH2O | 31.75 |
Cycling (25 cycles):
98°C | 180 s |
98°C | 30 s |
60°C | 20 s |
72°C | 25 s |
72°C | 600 s |
4°C | infinite |
Digest of pET_SpyC and pET_SpyC_GST (RE)
- digests to open the backbone for insertion of the real SpyC sequence (wrong sequence is excised)
- pET_SpyC was digested with BamHI and HindIII
- pET_SpyC_GST was digested with BamHI
- 1 µl of each RE
- 5 µl FD Green Buffer
- 1 µg DNA
- 1 µl Antarctic phosphatase
- ad 50 µl dH2O
Analysis of the SpyC PCR products and the backbone digests (RE)
- 1 % agarose gel
- both amplifications were successful
- both digests were successful
- all fragments were extracted from the gel
- Qiagen-kit
- elution in 30 µl dH2O
- NanoDrop:
Fragment | Concentration [ng/µl] |
---|---|
SpyC PCR product 1-2 | 30 |
SpyC PCR product 1-3 | 30 |
pET_SpyC backbone | 31 |
pET_SpyC_GST backbone | 14 |
Digest of the purified SpyCatcher PCR products (RE)
- 1-2 was digested with BamHI and HindIII
- 1-3 was digested with BamHI
- 1 µl of each RE
- 5 µl FD Green Buffer
- 17 µl DNA
- 26 µl dH2O
- incubated for 30 min at 37°C
Gel-Ex (RE)
- of the digested SpyC PCR products
- Qiagen-kit
- eluted in 20 µl dH2O
Blunt end ligation of the SpyCatcher PCR products (undigested!) into pJET (RE)
- 1 µl pJet
- 10 µl reaction buffer
- 1.5 µl PCR product
- 1 µl T4 ligase
- 6.5 µl dH2O
- incubated for 5 min at RT and subsequently transformed into E. coli TOP10 (plated on LB_amp)
Transformation (RE)
- pOP 2-fragment Gibson (50°C incubation) after fusion PCR (JN)
- E. coli TOP10; plated on LB_amp
Ligations (SpyCatcher) (RE)
1.:
- pET_SpyC (BamHI / HindIII digested): 1.61 µl
- PCR product 1-2 (same digest): 0.52 µl
- dH2O: 14.87 µl
- T4 ligase: 1 µl
- T4 ligase buffer: 2 µl
2.:
- pET_SpyC_GST (BamHI digested): 3.33 µl
- PCR product 1-2 (same digest): 0.42 µl
- dH2O: 13.25 µl
- T4 ligase: 1 µl
- T4 ligase buffer: 2 µl
Incubated at 16°C over night
2015/08/20
Transformation: Ligation pET_Spy-C (LS)
- 7µl of ligation mix
- transformation according to protocol
- incubation on LB-Amp plates at 37°C
Miniprep: pOP and pIG15_1504-HA (LS)
- qiagen kit
concentrations | |
---|---|
pIG15_1504-HA (1) | 89,1 |
pIG15_1504-HA (2) | 159,0 |
pOP after F-PCR (5min) (1) | 161,8 |
pOP after F-PCR (5min) (2) | 100,8 |
pOP after F-PCR (5min) (3) | 216,9 |
Picked clones from ligation plate (LS)
- 3x pET_SpyC
- 3x pET_SpyC-GST
- incubation in 5ml LB-Amp at 37°C o/n
Pelleting of liquid culure (LS)
- 5ml liquid culture
- pJET-Spy-C
- frozen at -20°C
2015/08/21
Mini-Prep (RE)
- 6 cultures pelleted yesterday by LS (pJet_SpyC 1-2; pJet_SpyC 1-3)
- 3 cultures of pET_SpyC (ligation after PCR product digest)
- 3 cultures of pET_SpyC_GST (ligation after PCR product digest)
(Test)Digest (RE)
- pET_SpyC_GST and pJet_SpyC 1-3 with BamHI
- pET_SpyC and pJet_SpyC 1-2 with BamHI and HindIII
- pOP with PstI and MluI
- DNA: 1 µg for pJets; 0.5 µg for pET and pOP
- Buffer: 5 µl CutSmart for pOP; FD Green for the others
- 1 µl of each RE
- ad 50 µl dH2O
- incubation for 1 h (pOP) or 30 min at 37°C
Dilution of primers (LS)
- biobrick SpyC (GST)
- Salmonella mutagenesis
PCR: Salmonella mutagenesis (LS)
2x MM | |
---|---|
25µl | Q5 MM |
2,5µl | primer 1 |
2,5µl | primer2 |
3µl | pIG15_1501 |
18µl | dH2O |
- first part: oIG15_1503f + oIG15_1504r
- second part: oIG15_1505f + oIG15_1506r
- third part: oIG15_1507f + oIG15_1508r
cycling | |
---|---|
98°C | 5min |
98°C | 10s |
60°C | 30s |
72°C | 40s |
72°C | 10min |
4°C | – |
Gel-ex: Spy-Catcher (LS)
1. Spy-C: BamHI digested 2. Spy-C: BamHI and HindIII digested
- qiagen kit:
concentration [ng/µl] | |
---|---|
1. | 5,5 |
2. | 25,6 |
Fusions PCR for pOOP fragments (RE)
Fragment 5-1:
Ingredient | Volume [µl] |
---|---|
Template (pJet_pOOP_5) | 1 |
Template (pJet_pOOP_1) | 1 |
Fwd primer (oIG15_pOOP5_fw) | 2.5 |
Rev primer (oIG15_pOOP1_rv) | 2.5 |
dNTPs | 1 |
DMSO | 1.5 |
High GC Buffer | 10 |
Phusion polymerase | 0.5 |
dH2O | 30 |
Fragment 2-3-4:
Ingredient | Volume [µl] |
---|---|
Template (pJet_pOOP_2) | 1 |
Template (pJet_pOOP_3) | 1 |
Template (pJet_pOOP_4) | 1 |
Fwd primer (oIG15_pOOP2_fw) | 2.5 |
Rev primer (oIG15_pOOP4_rv) | 2.5 |
dNTPs | 1 |
DMSO | 1.5 |
High GC Buffer | 10 |
Phusion polymerase | 0.5 |
dH2O | 29 |
Cycling (25 cycles):
98°C | 180 s |
98°C | 30 s |
60°C | 20 s |
72°C | 90 s |
72°C | 600 s |
4°C | infinite |
Gel-ex: PCR product for Salmonella mutagenesis (LS)
- qiagen kit
- eluted in 20µl
concentration [ng/µl | |
---|---|
1.part | 65,6 |
2.part | 132,3 |
3.part | 115,3 |
Digest of pIG15_104 to get pSB1C3 backbone (RE)
- 10 µl DNA
- 5 µl CutSmart
- 1 µl XbaI
- 1 µl PstI-HF
- 33 µl dH2O
- incubation for 1 h at 37°C
Ligation: Spy-Catcher (LS)
- backbone: pET_SpyC(old) BamHI or BamHI+HindIII digested
- insert: gel-ex of SpyC (GST) fragment
Ligation mix | ||
---|---|---|
pET_SpyC | pET_SpyC-GST | |
backbone | 3,47 | 1,58 |
insert | 1,64 | 0,35 |
buffer | 2 | 2 |
T4 Ligase | 0,5 | 0,5 |
dH2O | 12 | 15 |
- 1h, RT
Transformation: Ligation of pET_SpyC (-GST) into E.coli T10 (LS)
- 10µl of ligation mix
- transformation according to protocol
- plated on LB-Amp
- incubation at 37°C o/n
2015/08/22
Picking colonies from pET_SpyC (-GST) Ligation (LS)
- 3x 5ml LB-Amp each
- incubation at37°C
Gel-ex: pSB1C3 XbaI and PstI digested (LS)
- qiagen kit
- concentration (20µl): 14,3ng/µl
Fusion-PCR: pOOP (LS)
1.PCR | frg.1 + frg.5 | frg.2 + frg.3 | ||
---|---|---|---|---|
frg.1 | 3µl | frg.2 | 3µl | |
frg.5 | 3µl | frg.3 | 3µl | |
Phusion Polymerase | 0,5 | |||
high GC buffer | 10µl | |||
dNTPS | 2µl | |||
DMSO | 2µl | |||
dH2O | 30µl |
cycling | |||
---|---|---|---|
frg. 1+ frg.5 | frg.2 + frg.3 | ||
98°C | 5min | 98°C | 5min |
98°C | 1min | 98°C | 1min |
72°C | 30s | 78°C | 30s |
72°C | 45s | 72°C | 1min 15s |
72°C | 5min | 72°C | 5min |
4°C | – | ||
addition of frg. 4 | |||
– | 98°C | 5min | |
– | 98°C | 1min | |
– | 78°C | 30s | |
– | 72°C | 2min | |
– | 72°C | 5min | |
– | 4°C | – | |
addition of primers | |||
primer 1 rev | 2,5ml | primer 4 rev | 2,5µl |
primer 5 fw | 2,5µl | primer 2fw | 2,5µl |
98°C | 5min | ||
98°C | 1min | ||
60°C | 30s | ||
72°C | 1/2min | ||
72°C | 5min | ||
4°C | – |
- analysis on 1%agarose gel
- fusion of frg. 1+5 worked, fusion of frg. 2+3+4 did not work
Gibson: Salmonella mutagenesis (LS)
fragment | concentration [ng/µl] | volume [µl] |
---|---|---|
pSB1C3 (XbaI+PstI | 14,3 | 2,52 |
fragment 1 | 65,5 | 0,22 |
fragment 2 | 132,3 | 0,44 |
fragment 3 | 115,3 | 0,83 |
- added 15µl Gibson mix
- incubation at RT, 5 min
- transformation in E.coli T10
- plated on LB-Cml
Gel-ex of fusion PCR product 5-1 (RE)
- qiagen kit
- eluted in 20µl dH2O
- NanoDrop: 11.8ng/µl
2015/08/23
Repetition of Fusion PCR (RE)
- assembly of pOP fragments 2 and 3
Ingredient | Volume [µl] |
---|---|
Fragment 2 | 2 |
Fragment 3 | 2 |
dNTPs | 2 |
DMSO | 3 |
High GC Buffer | 10 |
Phusion polymerase | 0.5 |
dH2O | 30.5 |
Cycling (4 cycles):
98°C | 180 s |
98°C | 30 s |
75°C | 20 s |
72°C | 120 s |
72°C | 300 s |
4°C | infinite |
Addition of Primers oIG15_pOOP2_fw and oIG15_pOOP3_rv (2.5 µl each)
Cycling (20 cycles):
98°C | 180 s |
98°C | 30 s |
60°C | 20 s |
72°C | 120 s |
72°C | 300 s |
4°C | infinite |
PCR clean-up of fragment 2-3 (RE)
- Qiagen-kit
- elution in 20 µl dH2O
- NanoDrop: 7.2 µl
Fusion PCR of frg. 2-3 and 4 (RE)
^ Ingredient ^ Volume [µl] ^
Fragment 2-3 | 2 |
Fragment 4 | 2 |
dNTPs | 2 |
DMSO | 3 |
High GC Buffer | 10 |
Phusion polymerase | 0.5 |
dH2O | 30.5 |
Cycling (4 cycles):
98°C | 180 s |
98°C | 30 s |
75°C | 20 s |
72°C | 120 s |
72°C | 300 s |
4°C | infinite |
Addition of Primers oIG15_pOOP2_fw and oIG15_pOOP4_rv (2.5 µl each)
Cycling (20 cycles):
98°C | 180 s |
98°C | 30 s |
60°C | 20 s |
72°C | 120 s |
72°C | 300 s |
4°C | infinite |
Mini-Prep (RE)
- pET_SpyC (3x; ligation with pJet digest product)
- pET_SpyC_GST (3x; ligation with pJet digest product)
- Zymo-kit
- elution in 30 µl dH2O
Construct | Concentration [ng/µl] |
---|---|
pET_SpyC-1 | 33.1 |
pET_SpyC-2 | 28.3 |
pET_SpyC-3 | 23.0 |
pET_SpyC_GST-1 | 30.1 |
pET_SpyC_GST-2 | 24.6 |
pET_SpyC_GST-3 | 29.8 |
Test-Digest of pET_SpyC and pET_SpyC-GST (RE)
- 8 µl DNA
- 2 µl FD Green Buffer
- 1 µl BamHI
- (1 µl HindIII - only for pET_SpyC)
- ad 20 µl dH2O
- incubation for 30 min at 37°C
Repetition of Fusion PCR (LS)
- same components/cycling as last time
- 2×25µl
Ingredient | Volume [µl] |
---|---|
Fragment 2 | 2 |
Fragment 3 | 2 |
dNTPs | 2 |
DMSO | 2 |
High GC Buffer | 10 |
Phusion polymerase | 0.5 |
dH2O | 30 |
Cycling (4 cycles):
98°C | 180 s |
98°C | 30 s |
75°C | 20 s |
72°C | 120 s |
72°C | 300 s |
4°C | infinite |
Addition of Primers oIG15_pOOP2_fw and oIG15_pOOP3_rv (1µl each)
Cycling (20 cycles):
98°C | 180 s |
98°C | 30 s |
60°C | 20 s |
72°C | 120 s |
72°C | 300 s |
4°C | infinite |
- analysis on 1% agarose gel
- correct band at ~2700bp visible
- gel-ex (qiagen kit): 20µl –>18.5ng/µl
- second PCR: fusion of frg. 4 to frg.2-3 (2×25µl)
Ingredient | Volume [µl] |
---|---|
Fragment 2-3 | 2 |
Fragment 4 | 2 |
dNTPs | 2 |
DMSO | 3 |
High GC Buffer | 10 |
Phusion polymerase | 0.5 |
dH2O | 30.5 |
Cycling (4 cycles):
98°C | 180 s |
98°C | 30 s |
75°C | 20 s |
72°C | 120 s |
72°C | 300 s |
4°C | infinite |
Addition of Primers oIG15_pOOP2_fw and oIG15_pOOP4_rv (1µl µl each)
Cycling (20 cycles):
98°C | 180 s |
98°C | 30 s |
60°C | 20 s |
72°C | 120 s |
72°C | 300 s |
4°C | infinite |
- analysis on 1% agarose gel
- correct band at ~3400bp visible
- excision/ frozen at -20°C
Picking clones from Gibson: Salmonella mutagenesis (LS)
2015/08/24
Mini-prep of pRIG15_15 (RE)
- Zymo-Kit
- eluted in 30 µl dH2O
- pRIG15_15 - 1: 54.9 ng/µl
- pRIG15_15 - 2: 47.2 ng/µl
- pRIG15_15 - 3: 37.8 ng/µl
Gel-Ex of Fusion PCR product 2-3-4 (RE)
- Qiagen-Kit
- eluted in 20 µl dH2O
- NanoDrop: 7.4 ng/µl
Test digest of pRIG15_15 (RE)
- 7 µl DNA
- 1 µl EcoRI-HF
- 1 µl SpeI
- 2 µl CutSmart
- 9 µl dH2O
- incubation for 1 h at 37°C
2015/08/25
Mini-Prep of pOOP (3x) (RE)
2015/08/26
Colony PCR (LS)
- 12 colonies from ligation plate + control (pSB1C3 with Spy-Catcher from munich)
- dipped sterile filter tip in colony, put some of the colony in PCR tube, streaked the rest of th colony on new LB-Amp plate
PCR Master Mix | |
---|---|
32,5µl | Dream Taq buffer |
32,5µl | dNTPs |
13µl | oIG15_SpyC-01 |
13µl | oIG15_SpyC-02 |
4µl | Dream Taq |
162,5µl | dH2O |
cycle (20x) | |
---|---|
95°C | 10min |
95°C | 30s |
60°C | 30s |
72°C | 40s |
72°C | 5min |
4°C | – |
- analysis on 1%agarose gel
PCR for Salmonella antibody (JN)
Q5 2x Master Mix | 25µl |
oIG15_b1101 | 2,5µl |
oIG15_b1102 | 2,5µl |
dH2O | 19.8µl |
pIG15_1302 | 0.2µl |
- 2×25µl
cycling (20x) | |
---|---|
98°C | 5min |
98°C | 30s |
60°C | 30s |
72°C | 30s |
72°C | 10min |
4°C | – |
- analysis on 1% agarose gel
- no bands were visible at all
Repetition: PCR for Salmonella antibody (LS)
Q5 Master Mix | |
---|---|
Q5 2x Master Mix | 25µl |
oIG15_1303f | 2,5µl |
oIG15_1304r | 2,5µl |
dH2O | 18µl |
pIG15_1301 | 2µl |
- 2×25µl
cycling (20x) | |
---|---|
98°C | 3min |
98°C | 10s |
60°C | 30s |
72°C | 40s |
72°C | 10min |
4°C | – |
- analysis on 1% agarose gel
- correct bands visible: gel-ex (qiagen kit)
Gibson assembly for pRIG15_13 (LS)
- 2,13 µl pSB1C3 (PstI+XbaI)
- 0,74µl frg. 13
- added to Gibson mix
- 5 min, RT
- transformation into E.coli Top 10
2015/08/27
Repetition of transformation of E.coli Top 10 with Gibson mix for pRIG15_13 (LS)
2015/08/28
Miniprep of pET_SpyC 8-12 (RE)
2015/08/29
Picked one clone from Gibson plate for pRIG15_13 (LS)
Repetition of PCR for frg. 13 (LS)
- same as last tim
- analysis on 1% agarose gel: correct
- gel-ex (qiagen): 138,3ng/µl
Miniprep: pRIG15_13 (1) (LS)
- 5ml
- Zymo kit: 216,5 ng/µl
Test Digest: pRIG15_13(1) with EcoRI HF and SpeI HF (LS)
5µl | pRIG15_13 (1) |
0,5µl | EcoRI HF |
0,5µl | SpeI HF |
14µl | dH2O |
- 37°C, 1h
- analysis on 1% agarose gel: not convincing
Repetition of Gibson assembly for pRIG15_13 (LS)
- 2,03µl pSB1C3 (XbaI + PstI)
- 0,60µl frg. 13
- added Gibson MasterMix
- 5min, RT
- transformation into E.coli Top 10
Transformation: pOP (2) + (LS)
- 2µl plasmid
- transformation according to protocol
2015/08/30
Digest of pOP, BBa_I712669 and BBa_K592009 (JN)
DNA | 5µl |
EcoRI | 1µl |
Spe | 1µl |
CutSmart | 5µl |
dH2O | 38µl |
- analysis on 1% agarose gel, correct fragments for pOP and BBa_I712669 were cut out of the gel
Gel-ex of pOP and BBa_I712669 (JN)
- Qiagen kit
- eluted in 20µl dH2O
pOP | 20.3ng/µl |
BBa_I712669 | 2.6ng/µl |
Ligation of pOP and BBa_I712669 (JN)
pOP backbone | 2.46µl |
BBa_I712669 insert | 16.15µl |
T4 buffer | 2µl |
T4 ligase | 1µl |
- 1h at RT
Trafo of ligation product (10µl) into E.coli TOP10 (JN)
- plated on LB-Amp plates