Team:Paris Saclay/protocols/pcr
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- | to | + | {| class="wikitable centre" width="80%" |
+ | |+ | ||
+ | |- | ||
+ | ! scope=col | component | ||
+ | ! scope=col | volume/50µL reaction | ||
+ | ! scope=col | volume/20µL reaction | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | H2O | ||
+ | | width="34%" | | ||
+ | Add to 50 μl | ||
+ | | width="33%" | | ||
+ | Add to 20 μl | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | 5x Phusion HF Buffer High-fidelity | ||
+ | | width="34%" | | ||
+ | 10 μl | ||
+ | | width="33%" | | ||
+ | 4 μl | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | 10 mM dNTPs | ||
+ | | width="34%" | | ||
+ | 1 μl | ||
+ | | width="33%" | | ||
+ | 0.4 μl | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Primer A | ||
+ | | width="34%" | | ||
+ | x μl | ||
+ | | width="33%" | | ||
+ | x μl | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Primer B | ||
+ | | width="34%" | | ||
+ | x μl | ||
+ | | width="33%" | | ||
+ | x μl | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Template DNA: Genomic DNA of bacteria E. coli DH5α | ||
+ | | width="34%" | | ||
+ | x μl | ||
+ | | width="33%" | | ||
+ | x μl | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Phusion DNA polymerasse | ||
+ | | width="34%" | | ||
+ | 0.5 μl | ||
+ | | width="33%" | | ||
+ | 0.2 μl | ||
+ | |||
+ | |||
+ | |} | ||
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- | + | {| class="wikitable centre" width="80%" | |
+ | |+ | ||
+ | |- | ||
+ | ! scope=col | Cycle step | ||
+ | ! scope=col | temperature | ||
+ | ! scope=col | time | ||
+ | ! scope=col | cycle | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Initial denaturation | ||
+ | | width="34%" | | ||
+ | 95 - 98 °C | ||
+ | | width="33%" | | ||
+ | 30 s – 3 min | ||
+ | | width="34%" | | ||
+ | 1 | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Denaturation | ||
+ | | width="34%" | | ||
+ | 95 - 98 °C | ||
+ | | width="33%" | | ||
+ | 10 – 30 s | ||
+ | | width="34%" | | ||
+ | 25-30 | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Annealing | ||
+ | | width="34%" | | ||
+ | x °C | ||
+ | | width="33%" | | ||
+ | 30 s - 1 min | ||
+ | | width="34%" | | ||
+ | 25-30 | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Extension | ||
+ | | width="34%" | | ||
+ | 72°C | ||
+ | | width="33%" | | ||
+ | 30 s – 2 min | ||
+ | | width="34%" | | ||
+ | 25-30 | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Final extension | ||
+ | | width="34%" | | ||
+ | 72°C | ||
+ | | width="33%" | | ||
+ | 10min | ||
+ | | width="34%" | | ||
+ | 1 | ||
+ | |- | ||
+ | | width="33%" | | ||
+ | Final extension | ||
+ | | width="34%" | | ||
+ | 4-8°C | ||
+ | | width="33%" | | ||
+ | hold | ||
+ | | width="34%" | | ||
+ | 1 | ||
+ | |} | ||
3. Determine the number of oligo by electrophoresis. | 3. Determine the number of oligo by electrophoresis. | ||
- | |||
{{Team:Paris_Saclay/incl_fin}} | {{Team:Paris_Saclay/incl_fin}} |
Revision as of 20:25, 23 September 2013
PCR for the genomic DNA of bacteria
1. In a cold PCR tube (eppendrof), pipette in order the required substances in the Table 1.
component | volume/50µL reaction | volume/20µL reaction |
---|---|---|
H2O |
Add to 50 μl |
Add to 20 μl |
5x Phusion HF Buffer High-fidelity |
10 μl |
4 μl |
10 mM dNTPs |
1 μl |
0.4 μl |
Primer A |
x μl |
x μl |
Primer B |
x μl |
x μl |
Template DNA: Genomic DNA of bacteria E. coli DH5α |
x μl |
x μl |
Phusion DNA polymerasse |
0.5 μl |
0.2 μl
|
2. Program the PCR machine according to the Table 2.
Cycle step | temperature | time | cycle |
---|---|---|---|
Initial denaturation |
95 - 98 °C |
30 s – 3 min |
1 |
Denaturation |
95 - 98 °C |
10 – 30 s |
25-30 |
Annealing |
x °C |
30 s - 1 min |
25-30 |
Extension |
72°C |
30 s – 2 min |
25-30 |
Final extension |
72°C |
10min |
1 |
Final extension |
4-8°C |
hold |
1 |
3. Determine the number of oligo by electrophoresis.