Misfolded protein molecules tend to self-assemble into highly-ordered aggregates, the so-called amyloid fibrils whose presence in vivo is often symptomatic of certain neurodegenerative disorders. Amyloid fibrils from different proteins share the capacity to bind a number of small planar molecules such as Congo Red (CR). The underlying docking interactions between fibrils and ligands remain poorly understood despite their importance for research on amyloid-inhibiting drugs. Here, we describe a novel approach to study binding of small ligands to amyloid fibrils. We probe dynamics of CR-amyloid interactions using two structural variants of insulin fibrils with strong quasi-opposite chiroptical properties and the ability to induce circular dichroism in bound CR molecules. We demonstrate that in mixed non-equilibrium complexes of CR with both chiral variants of fibrils, dissociation of CR-amyloid complex is the rate-determining step of the overall equilibration of the system. Kinetics of entropy-driven "hopping" of CR molecules between saturated and unoccupied binding moieties on amyloid fibrils follow exponential trajectories enabling calculation of dissociation rates of CR-amyloid complex. Temperature dependencies of CR-exchange rates reveal a heterogeneous distribution of CR-amyloid binding energies in the range of 38-53 kJ mol(-1). Our results have been discussed in the context of mechanisms of interactions between amyloid fibrils and amyloid-specific stains.

• 出版日期2016