Team:British Columbia/Notebook Biofilm
From 2010.igem.org
Protocol
Day 1
1. PIck an isolated colony from a Trypticase Soy Agar (TSA) plate and incubate in 5 mL of Trypticase Soy Broth (TSB) without shaking overnight
Day 2
1. Vortex the overnight culture and dilute 30 uL of culture by 1:100 in a 1% glucose solution diluted with TSB
2. Vortex to mix bacteria sample
3. Innoculate 200 uL of dilute sample into pre-determined wells of a microtiter plate
4. Use 1% glucose solution diluted with TSB, but without bacterial sample, as control and test samples in triplicate
5. Place lid onto microtiter plate and place in a non-shaking incubator for 24 hours at 37C
Day 3
1. Take microtiter plate out of the incubator and decant all liquid from the wells into a biohazard container
2. Wash each well with 3 x 300 uL of Phosphate Buffered Saline (PBS) at room temperature
3. Heat fix remaining bacteria through exposure for 1 hour to 60C air using a heat block
4. Leave plate inverted overnight at room temperature
Day 4
1. Add 150 uL of 0.1% crystal violet dye diluted with deionized water to each well
2. Allow staining to occur for 15 minutes
3. Decant crystal violet dye from each well into a biohazard container
4. Wash wells with deionized water until crystal violet is no longer present in the water
5. Air dry plate
6. Take OD readings at an absorbance of 550 nm on a plate reader