Team:Warsaw/Calendar-Main/11 July 2008

From 2008.igem.org

(Difference between revisions)
Line 31: Line 31:
5.72&deg;C 10'<br>
5.72&deg;C 10'<br>
6. keeping in 4&deg;C<br>
6. keeping in 4&deg;C<br>
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2. PCR omega in 50 µl<br>
2. PCR omega in 50 µl<br>
template DNA - pUC19 1 µl<br>
template DNA - pUC19 1 µl<br>
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Pfu turbo - 0.5 µl<br>
Pfu turbo - 0.5 µl<br>
H2o - 38.5 µl<br>
H2o - 38.5 µl<br>
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<br>
program:
program:
1. 95&deg;C 3'<br>
1. 95&deg;C 3'<br>
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6. keeping in 4&deg;C<br>
6. keeping in 4&deg;C<br>
25 cycles
25 cycles
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3. gel electrophoresis<br>
3. gel electrophoresis<br>
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4.reisolation from agarose gel<br>
4.reisolation from agarose gel<br>
</p>
</p>

Revision as of 17:12, 26 September 2008

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Preparation of constructs with OmpA protein fusions
1. Colony PCR on colonies from plates with transformations OmpA_alpha.
2. Confirmed transformant colonies inoculated to liquid LB with kanamycin.
Cloning of protein Z DNA to OmpA constructs
1. 2 colonies was inoculated to liquid LB broth with kanamycin

Preparation of construct omega-A

1. PCR A in 50 µl
template DNA - pKS-A4 1 µl
primer AP+NotI_N - 2 µl
primer AL+link10+homo2_N - 2 µl
Pfu polymerase buffer + Mg2+ (from Fermentas) - 5 µl
dNTPs - 1 µl
Pfu turbo - 0.5 µl
H2o - 38.5 µl

program:
1. 95°C 3'
2. 95°C 30"
3.62°C 45"
4.72°C 45"
5.72°C 10'
6. keeping in 4°C

2. PCR omega in 50 µl
template DNA - pUC19 1 µl
primer OmegaLS - 2 µl
primer AOmegaPli - 2 µl
Pfu polymerase buffer + Mg2+ (from Fermentas) - 5 µl
dNTPs - 1 µl
Pfu turbo - 0.5 µl
H2o - 38.5 µl

program: 1. 95°C 3'
2. 95°C 30"
3. 62°C 45"
4. 72°C 45"
5. 72°C 10'
6. keeping in 4°C
25 cycles
3. gel electrophoresis

4.reisolation from agarose gel

{{WarNotebookEnd}}

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