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For fluorometric quantification, prepare all algal samples at the same biomass concentration, and in the same manner, as the standards used in the measurement. Do this by suspending pre-dried samples in the appropriate amount of phosphate buffer. If necessary, use a homogenizer to facilitate resuspension of dried algal cells.
For each sample, mix 80 microliters of a prepared 30% ethanol solution, 10 microliters of a prepared Nile Red solution, and 10 microliters of algae suspension, in a single well of a 96-well plate. In order to properly account for the variability of the fluorescence measurement, perform five replicates of each sample. Next, run a two-point calibration curve with standards prepared previously, in order to account for day-to-day variations in the instrument and preparation.
To perform the fluorescence measurements in a multi-well plate reader spectrophotometer, set the parameters to shake at 1,200 rpm and orbit 3 millimeters for 30 seconds, followed by incubation at 40 degrees Celsius for 10 minutes. Another shake at 1,200 rpm, and orbit 3 millimeters for 30 seconds, and to record fluorescence, with excitation at 530 nanometers and emission at 604 nanometers. Then, start the run. As a final step, convert the fluorescence measurements to oil content using the results from the internal standards.
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