Team:Newcastle/Colony PCR
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{{Team:Newcastle/mainbanner}} | {{Team:Newcastle/mainbanner}} | ||
- | + | =Colony PCR= | |
- | ==== | + | ==Materials required== |
+ | Add the following according: | ||
# 37.5 µl of distilled H2O | # 37.5 µl of distilled H2O | ||
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# 1 µl template DNA | # 1 µl template DNA | ||
- | + | ==Conditions for ThermoCycler:== | |
- | + | ||
# Initialise - 95°C for 2 minutes. | # Initialise - 95°C for 2 minutes. | ||
# Denature - 95°C for 30 seconds. | # Denature - 95°C for 30 seconds. | ||
- | # Anneal - 52°C for 30 seconds (melting temperature, Tm, of template) | + | # Anneal - 52°C for 30 seconds (melting temperature, Tm, of template) |
# Extension - 75°C for 30 seconds | # Extension - 75°C for 30 seconds | ||
# Extension finish - 75°C for 5 minutes | # Extension finish - 75°C for 5 minutes |
Latest revision as of 14:52, 28 July 2010
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Colony PCR
Materials required
Add the following according:
- 37.5 µl of distilled H2O
- 10 µl of 5x GoTaq Buffer
- Nucleotide DNTP
- 2.5 µl forward primer
- 2.5 µl backward primer
- 1 µl template DNA
Conditions for ThermoCycler:
- Initialise - 95°C for 2 minutes.
- Denature - 95°C for 30 seconds.
- Anneal - 52°C for 30 seconds (melting temperature, Tm, of template)
- Extension - 75°C for 30 seconds
- Extension finish - 75°C for 5 minutes
- Hold - 4°C
Steps 2 to 4 are repeated for 30 cycles before continuing to step 5.