Difference between revisions of "Template:Groningen/Labjournal/Cipro-in-pSB1C3"
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| − | <h3> | + | <h3>Ciprofloxcacin cassette in pSB1C3</h3> |
| − | <p>To design a qnrS1 resistance cassette biobrick we designed a gBlock that | + | <p>To design a qnrS1 resistance cassette biobrick we designed a gBlock that contains the Bacillus subtilis promoter PatpI, which is active from a very early stage of germination and includes a ribosome binding site. The gBlock also contains the original qnrS1 gene sequence from E. coli, the double terminator BBa_B0015 from iGEM as well as the prefix and suffix for BioBricks. In summary the ciprofloxacin cassette consists of the following parts PatpI+RBS+QnrS1+Ter2, see plasmid map.</p> |
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<h5>Experiment:</h5> | <h5>Experiment:</h5> | ||
| − | <p>28 | + | <p>28/9 After ligation 2 µl of ligation were transformed into E. |
coli Top10. The transformation was plated on plates containing 50 µg/ml | coli Top10. The transformation was plated on plates containing 50 µg/ml | ||
chloramphenicol. The transformation was performed according to the | chloramphenicol. The transformation was performed according to the | ||
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<h5>Experiment:</h5> | <h5>Experiment:</h5> | ||
| − | <p>29 | + | <p>29/09 To analyze the success of the transformation 12 samples |
were picked and and a colony PCR was performed according to the colony | were picked and and a colony PCR was performed according to the colony | ||
PCR protocol <a href="/Team:Groningen/Protocols#Colony-PCR">Colony PCR</a>. The primers F-qnrs1 e.coli and R-qnrs1 | PCR protocol <a href="/Team:Groningen/Protocols#Colony-PCR">Colony PCR</a>. The primers F-qnrs1 e.coli and R-qnrs1 | ||
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<h5>Experiment:</h5> | <h5>Experiment:</h5> | ||
| − | <p>30 | + | <p>30/9 To further analyze the success of the transformation |
four colonies were grown as overnight cultures (started on 29.09.2016) | four colonies were grown as overnight cultures (started on 29.09.2016) | ||
in LB and 50 µg/ml chloramphenicol and were digested using the enzymes | in LB and 50 µg/ml chloramphenicol and were digested using the enzymes | ||
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(Figure 4).</p> | (Figure 4).</p> | ||
| − | < | + | <h4>Validation:</h4> |
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| + | <p>The two samples that showed the correct digestion pattern in the restriction digestion control were sent for sequencing with the primers VF2 and VR, see {{primerlist}} and {{sequencing}}. These two samples showed the correct sequence (Figure 5.1-5.4, 5.1 mutant 1 forward, 5.2: mutant 2 forward, 5.3: mutant 1 reverse, 5.4: mutant 2 reverse ).Thus the qnrS1 resistance cassette could successfully be integrated into the iGEM shipping backbone pSB1C3.</p> | ||
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Revision as of 13:23, 16 October 2016
To design a qnrS1 resistance cassette biobrick we designed a gBlock that contains the Bacillus subtilis promoter PatpI, which is active from a very early stage of germination and includes a ribosome binding site. The gBlock also contains the original qnrS1 gene sequence from E. coli, the double terminator BBa_B0015 from iGEM as well as the prefix and suffix for BioBricks. In summary the ciprofloxacin cassette consists of the following parts PatpI+RBS+QnrS1+Ter2, see plasmid map. The sequence of the qnrS1 gene was amplified from the gBlock qnrS1
E. coli ordered from IDT (link to sponsors). Primers used for the
amplification were F-qnrs1 e.coli and R-qnrs1 e.coli. See the primer
listhere. 50 μl PCR assay was performed according to the following protocol:
PCR (Q5® High-Fidelity) The PCR samples were loaded on a 1 % agarose gel. For detailed
information on how to prepare and run agarose gels see following
protocol DNA electrophoresis.The amplified qnrS1 sequence has a
size of 1194 bps. The PCR of the qnrS1 sequence from the IDT gBlock was successful. It
was verified by DNA electrophoresis (Figure 1). A band with the correct
size of 1194 bps could be seen. The PCR product was subsequently cleaned with the Gel extraction kit
Gel extraction (Agarose Gel Extraction Kit – Jena Bioscience). 28/09 The qnrS1 gene should be cloned into the biobrick shipping
vector BBa_pSB1C3. For this case the vector with BBa_J04450 was used.
It consists of a red fluorescent protein in the shipping vector
BBa_pSB1C3. The qnrS1 gene and BBa_J04450 were cut with the restriction enzymes
EcoRI and PstI. The restriction was performed in 20 μl RD assay according to the
restriction digestion assay Restriction digestion (FastDigest enzymes). The restricted samples were analyzed on a 1 % agarose gel. For
detailed information on how to prepare and run agarose gels see
following protocol DNA electrophoresis. Bands of the sizes 2029 bps for the vector and 1176 for the gene
were expected. The digestion was successful because bands for both expected
fragments could be seen on the gel, namely RFP insert is 1069bp and the
pSB1C3 backbone is 2019 bp. The digested samples were cut out from the gel and the DNA was
extracted using the Nucleospin Gel Extraction Kit Gel extraction (Agarose Gel Extraction Kit – Jena Bioscience) 28.9.2016: After restriction digestion ligation was performed. 6 µl
qnrS1 insert DNA were ligated to to 4 µl pBS1C3 vector DNA. The
ligation took place for 2 h at room temperature. 20 μl ligation assay was performed according to the ligation
protocol .Ligation 28/9 After ligation 2 µl of ligation were transformed into E.
coli Top10. The transformation was plated on plates containing 50 µg/ml
chloramphenicol. The transformation was performed according to the
transformation protocol 29/09 To analyze the success of the transformation 12 samples
were picked and and a colony PCR was performed according to the colony
PCR protocol Colony PCR. The primers F-qnrs1 e.coli and R-qnrs1
e.coli were used. here The colony PCR was loaded on a 1 % agarose gel. For detailed
information on how to prepare and run agarose gels see following
protocol. DNA electrophoresis The colony PCR did not bring clear results about the efficiency of
the transformation (Figure 3). 30/9 To further analyze the success of the transformation
four colonies were grown as overnight cultures (started on 29.09.2016)
in LB and 50 µg/ml chloramphenicol and were digested using the enzymes
EcoRI and PstI according to the restriction digestion protocol Restriction digestion (FastDigest enzymes) The digested samples were loaded on a 1 % agarose gel. For detailed
information on how to prepare and run agarose gels see following
protocol DNA electrophoresis. Two out of the four digested samples showed bands of the expected
sizes 2029 bps for the vector and 1184 for the gene could be seen
(Figure 4). The two samples that showed the correct digestion pattern in the restriction digestion control were sent for sequencing with the primers VF2 and VR, see {{primerlist}} and {{sequencing}}. These two samples showed the correct sequence (Figure 5.1-5.4, 5.1 mutant 1 forward, 5.2: mutant 2 forward, 5.3: mutant 1 reverse, 5.4: mutant 2 reverse ).Thus the qnrS1 resistance cassette could successfully be integrated into the iGEM shipping backbone pSB1C3.Ciprofloxcacin cassette in pSB1C3
Amplification of the qnrS1 sequence
Experiment:
PCR mixture:
PCR set-up:
95ºC 2:00 min 95ºC 30s (12X) 60ºC 30s (12X) 72ºC 1:30 min (12X) 72ºC 2:00 min 10ºC on hold DNA Electrophoresis:
Conclusion:
Procedure after gel validation:
Restriction Digestion:
Experiment:
RD mixture:
DNA Electrophoresis:
Conclusion:
Procedure after gel validation:
Ligation:
Experiment:
Ligation mixture:
Transformation:
Experiment:
Colony PCR:
Experiment:
DNA electrophoresis:
Conclusion:
Control restriction digestion:
Experiment:
DNA electrophoresis:
Conclusion:
Validation:
