Difference between revisions of "Part:BBa K3440018"
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The colonies for which the size seemed correct were sent for sequencing at Microsynth AG. The sequence obtained for colony 4 corresponded to the expected part, but it was not fully sequenced due to the limitations of the Sanger sequencing method. | The colonies for which the size seemed correct were sent for sequencing at Microsynth AG. The sequence obtained for colony 4 corresponded to the expected part, but it was not fully sequenced due to the limitations of the Sanger sequencing method. | ||
− | This construct was further analysed by Western Blot to check whether we obtained protein expression of bphR2 thanks to the added myc-tag (Figure 2). Additionally, | + | This construct was further analysed by Western Blot to check whether we obtained protein expression of bphR2 thanks to the added myc-tag (Figure 2). Additionally, 10e-4 M 1,1-biphenyl was added to BBa_K3440018 to compare the differences in protein expression. No bands of the correct size (35.1 kDa) were obtained for BBa_K3440018 in uninduced nor induced conditions, therefore we could not prove that this construct can express bphR2 constitutively. |
[[File:T--Stockholm--BBa_K3440000_WB.png|thumb|center|500px|Figure 2: Western blot with p3.2 and p3.2+biphenyl as BBa_K3440018]] | [[File:T--Stockholm--BBa_K3440000_WB.png|thumb|center|500px|Figure 2: Western blot with p3.2 and p3.2+biphenyl as BBa_K3440018]] |
Revision as of 18:26, 26 October 2020
PCB detection
Pconst(BBa_J23100)-RBS(BBa_B0034)-bphR2(BBa_K1413021)-Myc(BBa_K823036)-DT(BBa_B0015)-Pbphr1(BBa_K1155001)-RBS(BBa_B0034)-LuxI(BBa_C0061)
Usage and Biology
This is the final construct to detect a PCB and consequently produce a quorum sensing molecule. bphR2 is produced constitutively and can bind to a PCB. The complex PCB:bphR2 can activate bphR1 promoter, under which LuxI is placed. LuxI produces the 3OC6-HSL quorum sensing molecule.
Characterization
Due to the pandemics, we haven’t been able to use biobricks to create the iGEM Stockholm 2020 parts. Those parts were ordered as gene blocks from Integrated DNA Technologies Inc.. As a result, the sequences of the biobricks used are the same, but the scars between biobricks might differ, as well as the final size of the part.
After insertion into a pSB1C3 plasmid and transformation of E. coli TOP10 cells using heat shock, we picked several colonies corresponding to this part and PCR-amplified them using the VR and VF2 primers contained in the plasmid backbone pSB1C3.
We then ran electrophoretic gels at 180V for 30 mins (Figure 1). Ten colonies were picked from the plate and we obtained five bands for which the band height corresponded to the expected length of the construct (2493bp).
The colonies for which the size seemed correct were sent for sequencing at Microsynth AG. The sequence obtained for colony 4 corresponded to the expected part, but it was not fully sequenced due to the limitations of the Sanger sequencing method.
This construct was further analysed by Western Blot to check whether we obtained protein expression of bphR2 thanks to the added myc-tag (Figure 2). Additionally, 10e-4 M 1,1-biphenyl was added to BBa_K3440018 to compare the differences in protein expression. No bands of the correct size (35.1 kDa) were obtained for BBa_K3440018 in uninduced nor induced conditions, therefore we could not prove that this construct can express bphR2 constitutively.
We checked that a potential toxicity of the plasmid for E .coli was not the reason behind proteins not appearing on the Western Blot by making viability tests (see Figure 3 for the layout and Figure 4 for the results). We made growth curves by measuring OD600 of E. coli containing the part and different concentrations of pollutants. It appeared that only the highest concentration of 10e-3M of 1,1-dibiphenyl retarded the growth of E. coli. We therefore concluded that this was not the reason why the band did not appear on the Western Blot.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12INCOMPATIBLE WITH RFC[12]Illegal NheI site found at 7
Illegal NheI site found at 30 - 21INCOMPATIBLE WITH RFC[21]Illegal BglII site found at 996
Illegal BglII site found at 2108
Illegal BamHI site found at 1301
Illegal BamHI site found at 1384
Illegal XhoI site found at 1191 - 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal NgoMIV site found at 536
- 1000INCOMPATIBLE WITH RFC[1000]Illegal SapI.rc site found at 320
Illegal SapI.rc site found at 1284