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Team:Warsaw/Calendar-Main/23 September 2009
From 2009.igem.org
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Gradient PCR PhoP/PhoQ
Kama
Kama
Tasks:
- Amplification of phoP/phoQ
Methods:
PCR mixture's composition:
1μl Pfu buffer (EURX) 0,25μl primer phoPF 0,25μl primer phoQR 0,5μl dNTPs (10 mM) 0,25μl Pfu turbo polymerase (EURX) 0,5μl template DNA from Salmonella (unknown strain) 0,75μl DMSO The solution was topped up with H2O to 10μl.
- PCR programs:
pho
4min 95°C
(30s 95°C, 1min 55-65°C, 5min 10s 72°C)x35
10min 72°C
~ 7°C
- Electrophoretic separation on 1% agarose gel
Results:
- Gel (from left)
- M - GeneRuler DNA Ladder Mix #SM0333 (Fermentas)
- control -
- 3-5 - samples (annealing temperature increases to from the left to the right)
Notes:PhoP/PhoQ was succesfully amplified
Insertion of the pho gene into the pSB plasmid
Kama
- Isolation of plasmid containing an insert was performed with the A&A plasmid mini kit
Notes
Contents |
Isolation of BBa_J63010 from 2009 Kit
Monika
Tasks:
- Isolate BioBrick BBa_J63010 from 2009 Kit Plate 1
Methods:
- 2009 Kit: resuspension of DNA from selected wells with 15ul of H2O
- Transformation of chemocompetent cells with 3ul of DNA solution - procedure destribed here
- Planting on LB-agar medium supplemented with ampicilin
Results:
- Will be determined tomorrow.
PCR of phoQ
Monika
Task:
- amplification of phoQ (1464 bp)
Methods:
- PCR mixture:
5μl Pfu polymerase buffer 1μl forward primer and 1μl reverse primer 2μl dNTPs (10 mM) 2,5μl Pfu turbo polymerase (EURX) 2μl template DNA from Salmonella enterica typhimurium LT2 The solution was topped up with H2O to 50μl
- PCR conditions:
1. 5min 95°C 2. 30s 95°C 3. 2min 72°C 4. go to step 2 x30 5. 10min 72°C 6. forever 4°C
Results:
- Will be seen tomorow
Assembly of endosome detection operon
Marcin
Task 1: Gel-out of the following biobricks (digested in 22.09.09):
- BBa_K177035 - PstI, SpeI
- BBa_K177035 - PstI, XbaI
- BBa_K177036 - PstI, SpeI
- BBa_K177044 - PstI, XbaI
Methods:
All gel-outs were performed using the A&A kit according to the manual
Task 2: Prepare the following ligations:
- BBa_K177035 with BBa_K177036 to obtain BBa_K177037
- BBa_K177035 with BBa_K177043 to obtain BBa_K177044
Methods
- Reaction mixtures composition:
11 μl insert 7 μl vector 1 μl T4 ligase (Fermentas) 2.4 μl Buffer Tango (Fermentas) 2.5 μl dNTPs mixture (EurX, concentration 5 mM)
- Ligation was carried out 10 hours in 16 °C. Subsequently mixtures were thermally inactivated
Task 3: Transformation of TOP10 chemocompetent bacteria with following constructs:
Methods:
- Ligation mixture was thermally inactivated
- Detailed protocol of transformation is described here
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