15th of October luciferase assay protocol

Pellet 750 ul of grown culture when the culture is around OD=0.9 by centrifuging 5 min at 10000 rpm in a tabletop centrifuge.
Resuspend the cells in 1x PBS.
Lyse the cells by 2 times 15 second sonication at max amplitude, with a 15 second interval.
Freeze the cells at -20 until measurements will be done.

Mix 1 ul of 100X luciferase substrate in 100 ul of assay buffer per sample in the luminometer's reagent tube no. 1
Put 20 ul of lysed cells in a white 96 wells plate.
Put the prime plate in the luminometer (usually on top)
Put the tube with assay buffer under reagent needle no. 1, make sure the tip of the needle is in a position to reach all the assay buffer.
Prime the luminometer with 1000 ul assay buffer in the priming plate(make sure the tubing is rinsed before)
Measure luciferase activity by:
- Adding 100 ul of assay buffer to a well
- Wait 2 seconds
- Integrate luminescence for 10 seconds.
- Repeat for every well
- There is a standard protocol on the computer in which you only have to indicate the wells to be assayed.
Purge the tubing (Assay buffer can be stored and frozen for short periods (1 week at most) according to the technical manual)
Rinse the tubing with 5000 ul of ethanol, and purge it.
Rinse the tubing with 5000 ul of H2O, and purge it.
The tubing and injector should be clean and empty now.

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