Team:EPF-Lausanne/Notebook/June2011

From 2011.igem.org

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(Thursday, 30 June 2011)
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Henrike and Irina designed primers for both plasmids, with the goal of amplifying the following four parts:
Henrike and Irina designed primers for both plasmids, with the goal of amplifying the following four parts:
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1) a pTet-RFP segment (820 bp)
1) a pTet-RFP segment (820 bp)
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*Primer 1: J61002-Ptet-RFP-r
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*Primer 2: J61002-RFP-f
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*DNA template: Plate 1, 18 C
2) a J61002 plasmid backbone with a terminator (2334 bp)
2) a J61002 plasmid backbone with a terminator (2334 bp)
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*Primer 1: J61002-f
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*Primer 2: J61002-term-r
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*DNA template: Plate 1, 18 C
3) a constitutive promoter for TetR (725 bp)  
3) a constitutive promoter for TetR (725 bp)  
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*Primer 1: Pconst-tetR-f
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*Primer 2: TetR-r
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*DNA template: TetR Repressilator plasmid
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4) P23019 plasmid (2242 bp)
 
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4) P23019 plasmid (2242 bp)
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*Primer 1: P23019-r
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*Primer 2: P23019-f
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*DNA template: Plate 4, 14E
With a first PCR, we were able to amplify the pTet-RFP segment and the promoter for TetR, but neither of the backbones was amplified. The iProof PCR was done using 40 seconds of elongation time at 55 C.  
With a first PCR, we were able to amplify the pTet-RFP segment and the promoter for TetR, but neither of the backbones was amplified. The iProof PCR was done using 40 seconds of elongation time at 55 C.  

Revision as of 17:06, 8 July 2011