Rational design of a conformation-specific antibody for the quantification of Aβ oligomers

Author:

Aprile Francesco A.ORCID,Sormanni PietroORCID,Podpolny MarinaORCID,Chhangur Shianne,Needham Lisa-Maria,Ruggeri Francesco S.ORCID,Perni MicheleORCID,Limbocker Ryan,Heller Gabriella T.,Sneideris Tomas,Scheidt TomORCID,Mannini BenedettaORCID,Habchi JohnnyORCID,Lee Steven F.ORCID,Salinas Patricia C.,Knowles Tuomas P. J.,Dobson Christopher M.,Vendruscolo MicheleORCID

Abstract

Protein misfolding and aggregation is the hallmark of numerous human disorders, including Alzheimer’s disease. This process involves the formation of transient and heterogeneous soluble oligomers, some of which are highly cytotoxic. A major challenge for the development of effective diagnostic and therapeutic tools is thus the detection and quantification of these elusive oligomers. Here, to address this problem, we develop a two-step rational design method for the discovery of oligomer-specific antibodies. The first step consists of an “antigen scanning” phase in which an initial panel of antibodies is designed to bind different epitopes covering the entire sequence of a target protein. This procedure enables the determination through in vitro assays of the regions exposed in the oligomers but not in the fibrillar deposits. The second step involves an “epitope mining” phase, in which a second panel of antibodies is designed to specifically target the regions identified during the scanning step. We illustrate this method in the case of the amyloid β (Aβ) peptide, whose oligomers are associated with Alzheimer’s disease. Our results show that this approach enables the accurate detection and quantification of Aβ oligomers in vitro, and inCaenorhabditis elegansand mouse hippocampal tissues.

Publisher

Proceedings of the National Academy of Sciences

Subject

Multidisciplinary

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