| Literature DB >> 30971495 |
Gareth J Morgan1,2, Nicholas L Yan3,2, David E Mortenson3,2, Enrico Rennella4,5,6, Joshua M Blundon3,2, Ryan M Gwin3,2, Chung-Yon Lin3,2, Robyn L Stanfield7, Steven J Brown3, Hugh Rosen3, Timothy P Spicer8, Virneliz Fernandez-Vega8, Giampaolo Merlini9,10, Lewis E Kay4,5,6,11, Ian A Wilson7,12, Jeffery W Kelly1,2,12.
Abstract
In Ig light-chain (LC) amyloidosis (AL), the unique antibody LC protein that is secreted by monoclonal plasma cells in each patient misfolds and/or aggregates, a process leading to organ degeneration. As a step toward developing treatments for AL patients with substantial cardiac involvement who have difficulty tolerating existing chemotherapy regimens, we introduce small-molecule kinetic stabilizers of the native dimeric structure of full-length LCs, which can slow or stop the amyloidogenicity cascade at its origin. A protease-coupled fluorescence polarization-based high-throughput screen was employed to identify small molecules that kinetically stabilize LCs. NMR and X-ray crystallographic data demonstrate that at least one structural family of hits bind at the LC-LC dimerization interface within full-length LCs, utilizing variable-domain residues that are highly conserved in most AL patients. Stopping the amyloidogenesis cascade at the beginning is a proven strategy to ameliorate postmitotic tissue degeneration.Entities:
Keywords: dimerization; high-throughput screen; kinetic stabilizer; proteotoxicity; structural biology
Year: 2019 PMID: 30971495 PMCID: PMC6486714 DOI: 10.1073/pnas.1817567116
Source DB: PubMed Journal: Proc Natl Acad Sci U S A ISSN: 0027-8424 Impact factor: 11.205