Hi,

I wanted to study the conformation changes in BSA using Three dimensional fluorescence spectroscopic analysis in a spectrofluorometer. I am using BSA (10 uM) for this analysis and my parameters for scan are emission wavelength scanning range is from 200 to 600 nm and the excitation wavelength scan range is recorded from 200 to 400 nm at 5 nm increments. 

I am not getting the 4 characteristic peaks that are Peak 1, the Rayleigh scattering peak, Peaks 2 and 3 which are the two typical fluorescence peaks of BSA and peak 4 which is the second order scattering peak. Instead I always end up getting multiple peaks of equal heights at random wavelengths.  What could be the reason for this? I feel my protocol may not be correct or some scan settings need to be changed.

Thanks in advance :)

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