Difference between revisions of "Team:UCLA/Notebook/Honeybee Silk/28 July 2015"
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− | =Redo of Expressing Honeybee Protein= | + | ='''Redo of Expressing Honeybee Protein'''= |
*Following a similar protocol to the one performed on [https://2015.igem.org/Team:UCLA/Notebook/Honeybee_Silk/18_May_2015 5/18.] | *Following a similar protocol to the one performed on [https://2015.igem.org/Team:UCLA/Notebook/Honeybee_Silk/18_May_2015 5/18.] | ||
*Growing up cells in 100ml of LB. | *Growing up cells in 100ml of LB. |
Latest revision as of 20:53, 24 August 2015
Redo of Expressing Honeybee Protein
- Following a similar protocol to the one performed on 5/18.
- Growing up cells in 100ml of LB.
- We are doing a smaller volume because we are running low on bugbuster lysis reagents, and we want to be able to do at least one more reaction after this one.
- Instead of making a starter culture, we are simply inoculating a colony into a 1L flask.
- I started incubating the culture at 12:35 pm 7/27, but I forgot to add the Kanamycin antibiotic until 1 pm. (100 ul of 1000x).
- Here are the steps for today's growth protocol.
- Inoculate one colony in 100 ml of LB in an autoclaved flask.
- Add appropriate antibiotics (kan 100 ul)
- Grow and shake at 37 until OD reaches between 0.4 and 0.6.
- The colony was inoculated at 12:20 pm, At 4 pm , the OD was 0.064, at 5:05 pm OD was 0.358, At 5:17 the OD was 0.502, when we induced with the IPTG (5:25 pm) IPTG was added to a concentration of 0.5mM
- Continue to incubate at 37 C and shake overnight.
- In the morning, spin down the cells, decant the supernatant, and freeze the pellet at -80 for storage.