Elsevier, Journal of Biological Chemistry, 9(291), p. 4626-4637, 2016
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β2-microglobulin (β2m), a key component of the major histocompatibility class I complex , can aggregate into fibrils with severe clinical consequences. As such, investigating structural aspects of the formation of oligomeric intermediates of β2m and their subsequent progression towards fibrillar aggregates is of great importance. However β2m aggregates are challenging targets in structural biology, primarily due to their inherent transient and heterogeneous nature. Here we study the oligomeric distributions and structures of the early intermediates of amyloidogenic β2m and its truncated variant ΔN6-β2m. We established compact oligomers for both variants by integrating advanced mass spectrometric techniques with available electron microscopy maps and atomic-level structures from NMR spectroscopy and X-ray crystallography. Our results revealed a stepwise assembly mechanism by monomer addition and domain swapping, for the oligomeric species of (ΔN6)-β2m. The observed structural similarity and common oligomerization pathway between the two variants is likely to enable ΔN6-β2m to cross-seed β2m fibrillation and allow the formation of mixed fibrils. We further determined the key subunit interactions in ΔN6-β2m tetramer, revealing the importance of a domain-swapped hinge region for formation of higher-order oligomers. Overall, we deliver new mechanistic insights into β2m aggregation paving the way for future studies on the mechanisms and cause of amyloid fibrillation.