Tooth enamel, the hardest tissue in the body, is formed by the evolutionarily highly conserved biomineralization process that is controlled by extracellular matrix proteins. The intrinsically disordered matrix protein ameloblastin (AMBN) is the most abundant nonamelogenin protein of the developing enamel and a key element for correct enamel formation.
AMBN was suggested to be a cell adhesion molecule that regulates proliferation and differentiation of ameloblasts. Nevertheless, detailed structural and functional studies on AMBN have been substantially limited by the paucity of the purified non-degraded protein.
Here we developed a procedure for production of a highly purified form of recombinant human AMBN in quantities that allowed its structural characterization. Using size-exclusion chromatography, analytical ultracentrifugation, transmission electron and atomic-force microscopy techniques, we show that AMBN self-associates into ribbon-like supramolecular structures with an average width and thickness of 18 and 0.34 nm, respectively.
The AMBN ribbons exhibited a length ranging from tens to hundreds of nm. Deletion analysis and NMR spectroscopy revealed that an N-terminal segment encoded by exon 5 comprises two short independently structured regions and plays a key role in self-assembly of AMBN.