Team:Paris/August 27
From 2008.igem.org
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=Cloning of EnvZ* in pSB1A2= | =Cloning of EnvZ* in pSB1A2= | ||
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'''Results''': All the clones analysed were not correct. | '''Results''': All the clones analysed were not correct. | ||
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=Cloning of OmpR*= | =Cloning of OmpR*= | ||
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* 1 µL T4 DNA ligase at 400 000 U/mL concentration | * 1 µL T4 DNA ligase at 400 000 U/mL concentration | ||
* O/N at 16°C | * O/N at 16°C | ||
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=Checking mutagenesis FliA= | =Checking mutagenesis FliA= |
Revision as of 18:51, 9 September 2008
Construction of pFlhB - mRFP Tripart (LVA+)Aim : Construction of "pFlhB-RBS-mRFP-dbl ter" (pFlhB-I732078)
DigestionMeasurement of the concentration of D187 purifiedProtocol (it's same that for Miniprep) => the experiments of Gel Extraction have failed, so we need to repeat the step of digestion. Digestion
Gel Verification
Cloning of EnvZ* in pSB1A2Transformation results
PCR screening
Electrophoresis
PCR
elongation time: 2 min 30
Results: All the clones analysed were not correct.
Cloning of OmpR*DigestionDetermination of the concentration of DNAWe used the biophotometer
Name of the digestions
Protocol of digestion
Cleaning of the digestion productsLigationDetermination of the concentration of DNAWe used the biophotometer
Protocol of ligation L171
Checking mutagenesis FliAFor this, i digested mutated FliA and non-mutated FliA with EcoRI and PstI and put in migration the digestion products running on gels. Results : No digestion for the mutated sequence --> successful mission ! |