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Team:Newcastle/26 July 2010
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(New page: ===Colony PCR of Genomic DNA=== ====Materials:==== # Materials added according to Colony PCR on Protocol list. # Melting temperature, Tm used for Anneal step is 59°C.) |
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===Colony PCR of Genomic DNA=== | ===Colony PCR of Genomic DNA=== | ||
| + | |||
| + | ====Aim:==== | ||
| + | |||
| + | To determine whether the genes have been inserted into the plasmid of ''B. Subtilis 168''. | ||
====Materials:==== | ====Materials:==== | ||
| + | * Pipette | ||
| + | * Microfuge | ||
| + | * Microtubes | ||
| + | * Distilled H2O | ||
| + | * Nucleotide DNTP | ||
| + | * 5x GoTaq buffer | ||
| + | * Template DNA (B. Subtilis ATCC 6633, 1:1 and 1:2) | ||
| + | * Forward and reverse primers | ||
# Materials added according to Colony PCR on Protocol list. | # Materials added according to Colony PCR on Protocol list. | ||
# Melting temperature, Tm used for Anneal step is 59°C. | # Melting temperature, Tm used for Anneal step is 59°C. | ||
| + | # | ||
Revision as of 14:02, 26 July 2010
Colony PCR of Genomic DNA
Aim:
To determine whether the genes have been inserted into the plasmid of B. Subtilis 168.
Materials:
- Pipette
- Microfuge
- Microtubes
- Distilled H2O
- Nucleotide DNTP
- 5x GoTaq buffer
- Template DNA (B. Subtilis ATCC 6633, 1:1 and 1:2)
- Forward and reverse primers
- Materials added according to Colony PCR on Protocol list.
- Melting temperature, Tm used for Anneal step is 59°C.
