Team:Aachen/Interlab Study
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The cultivation of our cultures was performed in 50 ml [https://2014.igem.org/Team:Aachen/Notebook/Protocols#LB_medium LB Media] in 500 ml shake flasks at 37 degrees Celsius and 300rpm shaking frequency. Appropiate antibiotics were added to each media (Kanamycin for I20260, Chloramphenicol for B0015, J23101.E0240 and J23115.E0240). Both antibiotics were added from a 1000* stock stored at -20 degrees Celsius for a final concentration of 35µg/ml Chloramphenicol and 50µg/ml for Kanamycin respectively. | The cultivation of our cultures was performed in 50 ml [https://2014.igem.org/Team:Aachen/Notebook/Protocols#LB_medium LB Media] in 500 ml shake flasks at 37 degrees Celsius and 300rpm shaking frequency. Appropiate antibiotics were added to each media (Kanamycin for I20260, Chloramphenicol for B0015, J23101.E0240 and J23115.E0240). Both antibiotics were added from a 1000* stock stored at -20 degrees Celsius for a final concentration of 35µg/ml Chloramphenicol and 50µg/ml for Kanamycin respectively. | ||
- | The precultures were inoculated from the same cryo stock every time. They were cultivated for 16 hours and then sampled for OD measurement with a Spektrophotometer. Then 2 ml of each preculture were centrifuged (5 minutes, 6000 g) and then washed twice with PBS buffer. Afterwards all cultures were inoculated to have the same starting OD. | + | The precultures were inoculated from the same cryo stock every time under a sterile clean bench. They were cultivated for 16 hours and then sampled for OD measurement with a Spektrophotometer. Then 2 ml of each preculture were centrifuged (5 minutes, 6000 g) and then washed twice with PBS buffer. Afterwards all cultures were inoculated to have the same starting OD once again done under sterile conditions inside a clean bench. |
===Sampling=== | ===Sampling=== |
Revision as of 12:04, 25 September 2014
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