Difference between revisions of "Part:BBa K4604035:Design"
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<caption><b>Fig. 1:</b> table showing parameters varying from PCR protocol for piG_08</caption> | <caption><b>Fig. 1:</b> table showing parameters varying from PCR protocol for piG_08</caption> | ||
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Since regular Golden Gate cloning did not work with the plasmid we used a different approach. We fused the single parts (see in the table above) together via PCR to one large fragment. Therefore we designed complementary overhangs attached to the primers used to amplify the single fragments. First we fused the amp promoter with <i>mazE</i> and then added the terminator. This insert was amplified according to the Q5 protocol with 62°C annealing temperature and an elongation time of 1 minute. The backbone pGGAselect and this PCR fragment were then digested with PacI and NotI for approximately 30 minutes. Afterwards the fragments were purified from gel. A ligation was set up according to the protocol, afterwards a transformation was done. The resulting colonies after an approximate 12-14h incubation time were screened by colony PCR. DNA of potential colonies containing the insert was isolated from overnight cultures (5mL LB-medium, 34 mg/mL chloramphenicol) and sent for sequencing for correct insertion and no mutation. | Since regular Golden Gate cloning did not work with the plasmid we used a different approach. We fused the single parts (see in the table above) together via PCR to one large fragment. Therefore we designed complementary overhangs attached to the primers used to amplify the single fragments. First we fused the amp promoter with <i>mazE</i> and then added the terminator. This insert was amplified according to the Q5 protocol with 62°C annealing temperature and an elongation time of 1 minute. The backbone pGGAselect and this PCR fragment were then digested with PacI and NotI for approximately 30 minutes. Afterwards the fragments were purified from gel. A ligation was set up according to the protocol, afterwards a transformation was done. The resulting colonies after an approximate 12-14h incubation time were screened by colony PCR. DNA of potential colonies containing the insert was isolated from overnight cultures (5mL LB-medium, 34 mg/mL chloramphenicol) and sent for sequencing for correct insertion and no mutation. | ||
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===Source=== | ===Source=== | ||
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− | The Amp promoter was taken by iGEM ECUST 2017 (BBa_K2308010). | + | The Amp promoter was taken by iGEM ECUST 2017 (<a href="https://parts.igem.org/Part:BBa_K2308010">BBa_K2308010</a>).</html> |
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Latest revision as of 01:02, 12 October 2023
piG_08 (ampProm_mazE)
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21INCOMPATIBLE WITH RFC[21]Illegal BamHI site found at 226
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000INCOMPATIBLE WITH RFC[1000]Illegal BsaI site found at 515
Design Notes
Choice of a constitutive promoter to ensure baseline expression of MazE (antitoxin).
Cloning of piG_08
The amp promoter as well as the rrnB terminator were used for cloning from a plasmid of iGEM2022 Freiburg team. The mazE was synthesized by IDT, the sequence for that was taken from the Library of Medicine (gene ID:947245) out of E. coli K12 MG1655 . For the PCR we used the general protocol for the Q5 polymerase with varying parameters for elongation time and annealing temperature:
fragment | Annealing temp. | Elongation time | Fragment size (in bp) |
---|---|---|---|
Amp promoter | 61°C | 15 s | 100 |
mazE | 61°C | 20 s | 320 |
rrnB terminator | 61°C | 30 s | 450 |
Since regular Golden Gate cloning did not work with the plasmid we used a different approach. We fused the single parts (see in the table above) together via PCR to one large fragment. Therefore we designed complementary overhangs attached to the primers used to amplify the single fragments. First we fused the amp promoter with mazE and then added the terminator. This insert was amplified according to the Q5 protocol with 62°C annealing temperature and an elongation time of 1 minute. The backbone pGGAselect and this PCR fragment were then digested with PacI and NotI for approximately 30 minutes. Afterwards the fragments were purified from gel. A ligation was set up according to the protocol, afterwards a transformation was done. The resulting colonies after an approximate 12-14h incubation time were screened by colony PCR. DNA of potential colonies containing the insert was isolated from overnight cultures (5mL LB-medium, 34 mg/mL chloramphenicol) and sent for sequencing for correct insertion and no mutation.
Source
The Amp promoter was taken by iGEM ECUST 2017 (BBa_K2308010).