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Team:Warsaw/Calendar-Main/7 September 2009
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(New page: {{WarNotebook}} <!-- do not edit above me! --> ===<div style="text-align: center;">Acquiring the internaline A gene from ''Listeria monocytogenes'' st. EDG-e genome </div>=== '''Jarek''...) |
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| + | <h3><div style="text-align: center;">Assembly of endosomal detection operon</div></h3> | ||
| + | <h4>Marcin</h4> | ||
| + | Task 1: | ||
| + | * Digest pKSII cloning vector using SmaI: | ||
| + | Methods: | ||
| + | * Reaction mixture composition: | ||
| + | <pre> | ||
| + | 15 μl purified plasmid DNA product | ||
| + | 0.5 μl SmaI (Fermentas) | ||
| + | 2 μl Buffer Tango (Fermentas) | ||
| + | 12.5 μl MQ water | ||
| + | </pre> | ||
| + | * Digestion was performed 6 hours and in next step enzyme was inactivated in 65 °C for 20 minutes | ||
| + | Task 2: | ||
| + | * Phosphorylation of previously purified sequence of mitochondrial signal peptide from Cox1 : | ||
| + | Methods: | ||
| + | * Reaction mixture composition: | ||
| + | <pre> | ||
| + | 15 μl purified plasmid DNA product | ||
| + | 2 μl PNK Buffer (NEB) | ||
| + | 0.5 μl PNK (NEB) | ||
| + | 2.5 μl dNTPs mixture (EurX, concentration 5 mM) | ||
| + | </pre> | ||
| + | * Reaction was performed 45 minutes and subsequently inactivate via heating (65 °C) | ||
| + | |||
| + | |||
| + | Task 3: Ligate of mitochondrial signal peptide to pKSII vector | ||
| + | *Methods: | ||
| + | * Ligation mixtures composition: | ||
| + | <pre> | ||
| + | 10 μl phosphorylated insert | ||
| + | 8 μl digested vector | ||
| + | 2.5 μl Tango buffer(Fermentas) | ||
| + | 2.5 μl dNTPs mixture (EurX, concentration 5 mM) | ||
| + | 1 μl ligase T4 (Fermentas) | ||
| + | </pre> | ||
| + | * Ligation was carry out about 15 hours | ||
Revision as of 19:39, 8 September 2009
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Acquiring the internaline A gene from Listeria monocytogenes st. EDG-e genome
Jarek
Tasks:
- Electrophoretical segregation of PCR products from previous day in 0,8% agarosis gel (sample containing 10 microL was used).
- Purifing DNA from agarose block with A&A Gel-Out kit.
Results:
- Finally I have the correct PCR product (at least I hope it's that one).
Assembly of endosomal detection operon
Marcin
Task 1:
- Digest pKSII cloning vector using SmaI:
Methods:
- Reaction mixture composition:
15 μl purified plasmid DNA product 0.5 μl SmaI (Fermentas) 2 μl Buffer Tango (Fermentas) 12.5 μl MQ water
- Digestion was performed 6 hours and in next step enzyme was inactivated in 65 °C for 20 minutes
Task 2:
- Phosphorylation of previously purified sequence of mitochondrial signal peptide from Cox1 :
Methods:
- Reaction mixture composition:
15 μl purified plasmid DNA product 2 μl PNK Buffer (NEB) 0.5 μl PNK (NEB) 2.5 μl dNTPs mixture (EurX, concentration 5 mM)
- Reaction was performed 45 minutes and subsequently inactivate via heating (65 °C)
Task 3: Ligate of mitochondrial signal peptide to pKSII vector
- Methods:
- Ligation mixtures composition:
10 μl phosphorylated insert 8 μl digested vector 2.5 μl Tango buffer(Fermentas) 2.5 μl dNTPs mixture (EurX, concentration 5 mM) 1 μl ligase T4 (Fermentas)
- Ligation was carry out about 15 hours
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