In Situ Transient Spectroscopy for the Study of Glucuronidase Activity within Serum Albumin

Laser flash photolysis (LFP) has shown to be an efficient technique for in situ determination of the glucuronidase activity of human serum albumin (HSA). After incubation of the steroisomeric flurbiprofen glucuronides (FBPGluc) during regular time intervals at the selected temperatures, in the presence of protein, regression analysis was applied to. the triplet decay at lambda = 360 nm. This led to a satisfactory fitting when considering a set of four lifetimes; the corresponding preexponential coefficients A(I)(FBP), A(II)(FBP), A(F)(FBPGluc), and A(B)(FBPGluc) can be correlated with the presence of flurbiprofen (FBP) within the two known binding sites (I and II), together with FBPGluc free in solution (F) and bound (B) to the protein. The new methodology based on LFP of glucuronides in the presence of HSA is fast, experimentally straightforward, and does not involve any workup. This suggests the possibility of making use of the transient triplet-triplet absorption for investigating the enzymatic-like activity of different host biomolecules and at the same time determining the distribution of the generated drug between several compartments in the protein.