J-Aggregation of Anionic Ethyl meso-Thiacarbocyanine Dyes Induced by Binding to Proteins

The effects of ribonuclease A (RNase), lysozyme, trypsin, and bovine serum albumin (BSA) on the J-aggregation behavior of 3,3‘-bis[sulfopropyl]-5-methoxy-4‘,5‘-benzo-9-ethylthiacarbocyanine (1), 3,3‘-bis[sulfopropyl]-4,5,4‘,5‘-dibenzo-9-ethylthiacarbocyanine (2), and 3,3‘-bis[sulfopropyl]-5,5‘-dimethoxy-9-ethylthiacarbocyanine (3) were studied in aqueous solution. The formation of J-aggregates at pH 6 is induced by RNase for 1 − 3, by lysozyme for 1 and 2, and by trypsin for 2. The formation of J-aggregates correlates with decay of the dimers and is supported by induced circular dichroism spectra. The concentration of J-aggregates for lysozyme/1 increases with an increase in the protein/dye concentration ratio, reaches a plateau, and then gradually decreases. J-aggregates are characterized by relatively weak fluorescence; e.g., Φf = 0.01 for lysozyme/1, and by a small Stokes shift of 6−8 nm, indicating almost resonance fluorescence. J-aggregation proceeds in the range of seconds to minutes with sigmoidal type kinetic curves for trypsin/2 and nonsigmoidal kinetics in the other cases. The presence of BSA, in contrast to RNase, lysozyme, and trypsin, results in deaggregation of dimers of 1 − 3 and formation of bound monomers and exhibits intense fluorescence from the trans-monomer; e.g., Φf = 0.22 for BSA/1. Generally, the binding of 1 − 3 to the proteins is a cooperative process, where the number of binding sites changes from n = 15 for lysozyme/1 to n = 6 for trypsin/2 and n = 0.3 and 1 for BSA/3.