Abstract
Soluble amyloid oligomers are potent neurotoxins that are involved in a wide range of human degenerative diseases, including Alzheimer disease. In Alzheimer disease, amyloid beta (Abeta) oligomers bind to neuronal synapses, inhibit long term potentiation, and induce cell death. Recent evidence indicates that several immunologically distinct structural variants exist as follows: prefibrillar oligomers (PFOs), fibrillar oligomers (FOs), and annular protofibrils. Despite widespread interest, amyloid oligomers are poorly characterized in terms of structural differences and pathological significance. FOs are immunologically related to fibrils because they react with OC, a conformation-dependent, fibril-specific antibody and do not react with antibodies specific for other types of oligomers. However, fibrillar oligomers are much smaller than fibrils. FOs are soluble at 100,000 x g, rich in beta-sheet structures, but yet bind weakly to thioflavin T. EPR spectroscopy indicates that FOs display significantly more spin-spin interaction at multiple labeled sites than PFOs and are more structurally similar to fibrils. Atomic force microscopy indicates that FOs are approximately one-half to one-third the height of mature fibrils. We found that Abeta FOs do not seed the formation of thioflavin T-positive fibrils from Abeta monomers but instead seed the formation of FOs from Abeta monomers that are positive for the OC anti-fibril antibody. These results indicate that the lattice of FOs is distinct from the fibril lattice even though the polypeptide chains are organized in an immunologically identical conformation. The FOs resulting from seeded reactions have the same dimensions and morphology as the initial seeds, suggesting that the seeds replicate by growing to a limiting size and then splitting, indicating that their lattice is less stable than fibrils. We suggest that FOs may represent small pieces of single fibril protofilament and that the addition of monomers to the ends of FOs is kinetically more favorable than the assembly of the oligomers into fibrils via sheet stacking interaction. These studies provide novel structural insight into the relationship between fibrils and FOs and suggest that the increased toxicity of FOs may be due to their ability to replicate and the exposure of hydrophobic sheet surfaces that are otherwise obscured by sheet-sheet interactions between protofilaments in a fibril.
Highlights
These reports of toxic oligomers are in agreement in terms of solubility, their size, morphology, and immunoreactivity varies indicating that amyloid oligomers are structurally diverse [2]
We have previously reported three antibodies, A11, OC, and ␣-annular protofibrils, that recognize mutually exclusive generic epitopes associated with prefibrillar oligomers (PFOs), fibrils, and annular protofibrils formed of different amyloid proteins, respectively [5, 24, 25]
No A11 immunoreactivity was detected under these conditions, indicating that PFOs are not formed under these conditions. 6E10 immunoreactivity was uniform over the time course, indicating that equal amounts of peptide were spotted and demonstrating the conformation-specific nature of the OC epitope
Summary
These reports of toxic oligomers are in agreement in terms of solubility, their size, morphology, and immunoreactivity varies indicating that amyloid oligomers are structurally diverse [2]. The LOC antibody was generated against the islet amyloid polypeptide fibrils, and like OC, it recognizes a variety of fibrils and FOs formed from different amyloidogenic proteins and peptides, including A, but it does not detect A monomers or PFOs [24].
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