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Team:EPF-Lausanne/Our Project/T7 promoter variants
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{{:Team:EPF-Lausanne/Templates/Header|title=T7 promoter variants}} | {{:Team:EPF-Lausanne/Templates/Header|title=T7 promoter variants}} | ||
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| + | Our goal is to make two families of T7 promoter variants. One family has mutations on the T7 promoter consensus sequence while the other has the same set of mutations on the consensus sequence but also has a lac operator downstream of the T7 promoter. In each family, we produce six designed variants with different predicted promoter strengths compared to the wildtype as well as three sets of randomer variants which we want to use to check the overall range of promoter strengths. | ||
=== The Making Of A Variant === | === The Making Of A Variant === | ||
| - | To produce these T7 promoter variants, we | + | To produce these T7 promoter variants, we use a two-step PCR process. The first PCR, which we call "gene-specific" PCR, is a typical PCR that adds a ribosome-binding site (rbs) in front of either RFP or the lysis operon and adds a terminator downstream. |
[[File:rbs_rfp_term.png]] | [[File:rbs_rfp_term.png]] | ||
Revision as of 17:28, 18 September 2011
T7 promoter variants
Our goal is to make two families of T7 promoter variants. One family has mutations on the T7 promoter consensus sequence while the other has the same set of mutations on the consensus sequence but also has a lac operator downstream of the T7 promoter. In each family, we produce six designed variants with different predicted promoter strengths compared to the wildtype as well as three sets of randomer variants which we want to use to check the overall range of promoter strengths.
The Making Of A Variant
To produce these T7 promoter variants, we use a two-step PCR process. The first PCR, which we call "gene-specific" PCR, is a typical PCR that adds a ribosome-binding site (rbs) in front of either RFP or the lysis operon and adds a terminator downstream.
With this PCR product now serving as the DNA template, we start a second PCR which we call the "extension" PCR. It extends the product by adding the T7 promoter, with or without a lac operator downstream. In these illustrations, we have substituted the lysis operon for the RFP gene but the same process is done for RFP.
In the last stage, we run another PCR with a set of primers that will add Gibson overhangs for the Gibson assembly that will add this promoter construct into the desired plasmid.
Characterization with RFP
With T7 and T7-lac promoter variants in hand, we want to characterize their relative strengths. To obtain the right set-up, we transform the promoter variant plasmids into a different strain of E. coli called BL21. These cells have a mutation in the promoter for the lacI gene that makes LacI protein. As a result of this mutation, LacI protein is overproduced and is found abundantly in these cells. In this same strain, the gene for the T7 RNA polymerase is preceded by a lac operator. Since LacI is a repressor and LacI is strongly present in BL21 cells, the production of T7 RNA polymerases is severely repressed. With very few T7 RNA polymerases available, there is very little recognition and binding of T7 promoters and consequently very little expression of the gene driven by the T7 promoter. Moreover, the expression of a gene driven by a T7-lac promoter would be even less, since the presence of LacI would block any action of the T7 RNA polymerase.
With such a system in place, the transformation of our T7 and T7-lac promoter variant plasmids into BL21 cells would produce little to no reporter expression. Now to induce promoter activity, we rely on the fact that the chemical IPTG blocks the production of LacI. Without these LacI proteins, the cell can resume production of T7 RNA polymerases. These in turn can bind to the T7 and T7-lac promoters and express the reporter gene without interruption. So the adding of IPTG to a BL21 cell culture containing these T7 and T7-lac promoter variant plasmids ought to produce high levels of RFP or Lysis expression. Since lysis is a rather binary process (either the cell is lysed or it is not), we use RFP fluorescence as a gauge of promoter strength and efficiency.
DNA Recovery with Lysis
Having a lysis cassette driven by a T7 promoter is an important step towards being able to recover the DNA sequences of transcription factor and promoter mutants that have strong mutual affinities. To verify that basic lysing could be induced, we would use the same IPTG experiment as for RFP, using both large samples for visual, qualitative confirmation and small samples in a platereader for quantitative, numerical confirmation.
Once the basic mechanism of cell lysing had been confirmed, the next step was to show that only cells with the functioning lysis cassette were lysing, as opposed to all cells lysing simultaneously.
