Today:
- Pool the colonies (from each of 6 original mutagenized cultures).
- Freeze part.
- Make chromosomal DNA preps from the rest. These will be used for sequencing and for the backcrosses (steps 5 & 6)
- As controls also make DNA from the pooled NovR colonies from yesterday.
- Use the 2 DNAs from the StrR parent and the 2 DNAs from the CmR parent to transform KW20 to StrR and to CmR.
- Maybe use the DNAs from the wildtype parent to transform KW20 to KanR.
- (Incidentals: make lots more BHI agar, pour plates, use frozen competent KW20, test transformation by NalR fragment, wash and autoclave flasks again.)
- Pool the backcross colonies derived from each of 6 original mutagenized cultures.
- Freeze part.
- Grow part in log phase for at least 2 hr (like yesterday)
- Transform with a different marker (NalR fragment, or MAP7 DNA with selection for NalR or SpcR).
- Pool the transformant colonies (from each of 6 original mutagenized cultures).
- Make chromosomal DNA preps from them for sequencing.
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