Study on the binding behavior of lysozyme with cephalosporin analogues by fluorescence spectroscopy
- PMID: 19343485
- DOI: 10.1007/s10895-009-0477-8
Study on the binding behavior of lysozyme with cephalosporin analogues by fluorescence spectroscopy
Abstract
It was first found that the intrinsic fluorescence of lysozyme at 340 nm can be quenched by cephalosporin analogues through the static quenching and non-radiative energy transferring procedure. In the acetate buffer solution with pH 7.0 and 298 K, the quenching fluorescence intensity was in a good linearity over the concentration of drugs in the range of 1-100 micromol L(-1), 0.1-100 micromol L(-1), 0.5-100 micromol L(-1) and 0.05-100 micromol L(-1) for cefradine, cefuroxime, cefotaxime and ceftriaxone, respectively. The quenching ability or the binding ability of the studied drugs followed the pattern: ceftriaxone > cefotaxime > cefuroxime > cefradine, which was close to the order of their antibacterial ability. The binding parameters including the association constant and the number of binding potential point were calculated at different temperatures (288, 298 and 308 K), and thermodynamic parameters DeltaH degrees, DeltaS degrees and DeltaG degrees were given. The binding mode of lysozyme with cephalosporins showed that the hydrophobic effect might play a major role. The binding distance between cephalosporin and tryptophan residue in lysozyme was obtained. The results provided the quantitative information for the binding of cephalosporin to lysozyme, and it was suggested that the drugs probably bound to the active site near Trp62 in lysozyme.
Comment in
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Fluorescence quenching to study protein-ligand binding: common errors.J Fluoresc. 2010 Mar;20(2):625-9. doi: 10.1007/s10895-009-0572-x. Epub 2009 Dec 9. J Fluoresc. 2010. PMID: 19997966
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