The solvatochromism and thermochromism of 4-aminophthalimide and 4-amino-N-methylphthalimide were
studied by absorption and steady state and time-resolved fluorescence emission in solvent mixtures of toluene−ethanol and toluene−acetonitrile in the temperature range 5−70 °C. The wavelengths of the maximum of
absorption and of fluorescence emission shift to the red with the increase of the proportion of the polar
component in the mixture. The greater affinity for the polar component of the mixture of the excited state
compared to the ground state enhances preferential solvation, which is the origin of this red shift. On the
other hand, a spectral shift to the blue is found upon temperature increase in solvent mixtures. This fact can
be explained by considering that association of the polar component with the excited-state solute is exothermic
and decreases with temperature. The appointed solvation change is attained by diffusion-controlled exchange
of solvent molecules between the bulk and the solvation sphere. This process leads to a time-dependent
emission spectrum in the nanosecond time domain. In this work a kinetic scheme is developed to describe
this exchange and explain the time-dependent fluorescence emission spectra. The description is based on a
Langmuir type association of the solvent molecules with the solute. The solvation equilibrium is attained by
stepwise solvent exchange. The kinetic data and the spectral information are integrated in a thermodynamic
cycle that can describe the solvation of excited and ground states at any solvent composition.
CPNs were well incorporated into glioblastoma and macrophage cells with localization in lysosomes. SW480 cells were less efficient incorporating CPNs with localization in the plasma membrane. In all cell lines PDT treatment was efficient inducing oxidative stress that triggered apoptosis.
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