| Literature DB >> 32231271 |
Daniel Lauster1,2, Simon Klenk3,4, Kai Ludwig5, Saba Nojoumi6,7, Sandra Behren3,4, Lutz Adam3,4, Marlena Stadtmüller8, Sandra Saenger8, Stephanie Zimmler8, Katja Hönzke9, Ling Yao9, Ute Hoffmann10, Markus Bardua10, Alf Hamann10, Martin Witzenrath9, Leif E Sander9, Thorsten Wolff8, Andreas C Hocke9, Stefan Hippenstiel9, Sacha De Carlo11, Jens Neudecker12, Klaus Osterrieder13, Nediljko Budisa6,7, Roland R Netz14, Christoph Böttcher5, Susanne Liese15,16, Andreas Herrmann17, Christian P R Hackenberger18,19.
Abstract
Multivalent interactions at biological interfaces occur frequently in nature and mediate recognition and interactions in essential physiological processes such as cell-to-cell adhesion. Multivalency is also a key principle that allows tight binding between pathogens and host cells during the initial stages of infection. One promising approach to prevent infection is the design of synthetic or semisynthetic multivalent binders that interfere with pathogen adhesion1-4. Here, we present a multivalent binder that is based on a spatially defined arrangement of ligands for the viral spike protein haemagglutinin of the influenza A virus. Complementary experimental and theoretical approaches demonstrate that bacteriophage capsids, which carry host cell haemagglutinin ligands in an arrangement matching the geometry of binding sites of the spike protein, can bind to viruses in a defined multivalent mode. These capsids cover the entire virus envelope, thus preventing its binding to the host cell as visualized by cryo-electron tomography. As a consequence, virus infection can be inhibited in vitro, ex vivo and in vivo. Such highly functionalized capsids present an alternative to strategies that target virus entry by spike-inhibiting antibodies5 and peptides6 or that address late steps of the viral replication cycle7.Entities:
Mesh:
Substances:
Year: 2020 PMID: 32231271 DOI: 10.1038/s41565-020-0660-2
Source DB: PubMed Journal: Nat Nanotechnol ISSN: 1748-3387 Impact factor: 39.213