Team:UFMG Brazil/lab
From 2013.igem.org
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* Pipette the TMAO solutions with different concentrations, making triplicates for each one. | * Pipette the TMAO solutions with different concentrations, making triplicates for each one. | ||
* Add 100 μL of bacteria culture obtained in step 1 and add it in each well from step 4. | * Add 100 μL of bacteria culture obtained in step 1 and add it in each well from step 4. | ||
- | * Seal the plate. Read fluorescence at | + | * Seal the plate. Read fluorescence at 587 nm (excitation) 610 nm (emission) |
Revision as of 21:13, 25 October 2013