Analysis of DNA-Protein Interactions by Intrinsic Fluorescence
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Changes in the fluorescence emission spectrum of a protein on binding to DNA can often be used to determine the stoichiometry of binding and equilibrium binding constants; in some cases the data can also give an indication of the location of particular residues within the protein. The experiments are generally quick and easy to perform, requiring only small quantities of material (1 ). Spectroscopic techniques allow one to measure binding equilibria (unlike, for example, gel retardation assays and other separation techniques, which are strictly nonequilibrium methods). Fluorescence is one of the most sensitive of spectroscopic techniques, allowing the low concentrations (typically in the μM range) required for estimation of binding constants for many protein-DNA interactions. Considerable care, however, needs to be exercised in conducting the experiment itself and in the interpretation of results. The fundamental principles of fluorescence are discussed briefly below.