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A Targetable Self-association Surface of the Huntingtin exon1 Helical Tetramer Required for Assembly of Amyloid Pre-nucleation Oligomers.
Mishra, Rakesh; Gerlach, Gabriella J; Sahoo, Bankanidhi; Camacho, Carlos J; Wetzel, Ronald.
Affiliation
  • Mishra R; Department Structural Biology, University of Pittsburgh School of Medicine Pittsburgh, PA 15260, USA. Electronic address: rakeshm2014@email.iimcal.ac.in.
  • Gerlach GJ; Department of Computational and Systems Biology, University of Pittsburgh School of Medicine Pittsburgh, PA 15260, USA.
  • Sahoo B; Department Structural Biology, University of Pittsburgh School of Medicine Pittsburgh, PA 15260, USA. Electronic address: bankanidhi@gmail.com.
  • Camacho CJ; Department of Computational and Systems Biology, University of Pittsburgh School of Medicine Pittsburgh, PA 15260, USA. Electronic address: ccamacho@pitt.edu.
  • Wetzel R; Department Structural Biology, University of Pittsburgh School of Medicine Pittsburgh, PA 15260, USA. Electronic address: rwetzel@pitt.edu.
J Mol Biol ; 436(12): 168607, 2024 Jun 15.
Article in En | MEDLINE | ID: mdl-38734203
ABSTRACT
Polyglutamine (polyQ) sequences undergo repeat-length dependent formation of disease-associated, amyloid-like cross-ß core structures with kinetics and aggregate morphologies often influenced by the flanking sequences. In Huntington's disease (HD), the httNT segment on the polyQ's N-terminal flank enhances aggregation rates by changing amyloid nucleation from a classical homogeneous mechanism to a two-step process requiring an ɑ-helix-rich oligomeric intermediate. A folded, helix-rich httNT tetrameric structure suggested to be this critical intermediate was recently reported. Here we employ single alanine replacements along the httNT sequence to assess this proposed structure and refine the mechanistic model. We find that Ala replacement of hydrophobic residues within simple httNT peptides greatly suppresses helicity, supporting the tetramer model. These same helix-disruptive replacements in the httNT segment of an exon-1 analog greatly reduce aggregation kinetics, suggesting that an ɑ-helix rich multimer - either the tetramer or a larger multimer - plays an on-pathway role in nucleation. Surprisingly, several other Ala replacements actually enhance helicity and/or amyloid aggregation. The spatial localization of these residues on the tetramer surface suggests a self-association interface responsible for formation of the octomers and higher-order multimers most likely required for polyQ amyloid nucleation. Multimer docking of the tetramer, using the protein-protein docking algorithm ClusPro, predicts this symmetric surface to be a viable tetramer dimerization interface. Intriguingly, octomer formation brings the emerging polyQ chains into closer proximity at this tetramer-tetramer interface. Further supporting the potential importance of tetramer super-assembly, computational docking with a known exon-1 aggregation inhibitor predicts ligand contacts with residues at this interface.
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Full text: 1 Collection: 01-internacional Database: MEDLINE Main subject: Exons / Protein Multimerization / Huntingtin Protein / Amyloid Limits: Humans Language: En Journal: J Mol Biol Year: 2024 Document type: Article
Fulltext
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PubMed Links
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Full text: 1 Collection: 01-internacional Database: MEDLINE Main subject: Exons / Protein Multimerization / Huntingtin Protein / Amyloid Limits: Humans Language: En Journal: J Mol Biol Year: 2024 Document type: Article