Team:CIDEB-UANL Mexico/WetLab-Planning
From 2013hs.igem.org
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<p align="justify">The circuit is divided in two parts. | <p align="justify">The circuit is divided in two parts. | ||
- | Work in the lab has 3 main objectives: | + | Work in the lab has 3 main objectives:<br> |
- | 1. To test the Vip3ca3 protein production with insects. | + | 1. To test the Vip3ca3 protein production with insects.<br> |
- | 2. To test the Vip3ca3 protein production with a reporter. | + | 2. To test the Vip3ca3 protein production with a reporter.<br> |
3. To test the regulation of the Vipca3 production with the repressor.</p> | 3. To test the regulation of the Vipca3 production with the repressor.</p> | ||
<p align="justify"> | <p align="justify"> |
Revision as of 20:07, 21 June 2013
Wet Lab
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Planning
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Construction - Objectives The protein Vip3ca3 is not in the parts registry catalog so we decided to synthesize that protein in order to work with it in the lab.
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The circuit is divided in two parts.
Work in the lab has 3 main objectives:
Objectives - Return For the first objective: The part “PCC1” contains the Vip3ca3 protein and it has a lambda cI promoter. The part “PCC1” is in a vector with ampicillin resistance so we have to cut the vector with restriction enzymes in the sites of EcoRI and PstI. As we are going to pass it to another vector it needs to have a different resistance so we choose kanamycine. The new vector is also cut in the same sites: EcoRI and PstI. Then we make a digestion with the plasmid and the insert. |
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For the second objective:
We are going to bind the “PCC1” part with a GFP reporter and it has degradation tag LVA. The “PCC1” and the GFP have ampicillin resistance so we choose a vector with kanamycine resistance. We cut the vector with EcoRI and PstI restriction enzymes. The insert that goes to the right, in this case the “PCC1”, is cut with EcoRI and SpeI and the other insert, which goes to the left, is cut with XbaI and PstI. Then the 2 inserts and vector are joined with ligase.
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