The RGD-binding integrins αvβ6 and αvβ8 are receptors for mouse adenovirus-1 and -3 infection

Manuela Bieri; Rodinde Hendrickx; Michael Bauer; Bin Yu; Tania Jetzer; Birgit Dreier; Peer R E Mittl; Jens Sobek; Andreas Plückthun; Urs F Greber; Silvio Hemmi

doi:10.1371/journal.ppat.1010083

The RGD-binding integrins αvβ6 and αvβ8 are receptors for mouse adenovirus-1 and -3 infection

PLoS Pathog. 2021 Dec 15;17(12):e1010083. doi: 10.1371/journal.ppat.1010083. eCollection 2021 Dec.

Authors

Manuela Bieri^{1

2}, Rodinde Hendrickx^{1

2}, Michael Bauer¹, Bin Yu³, Tania Jetzer¹, Birgit Dreier⁴, Peer R E Mittl⁴, Jens Sobek⁵, Andreas Plückthun⁴, Urs F Greber¹, Silvio Hemmi¹

Affiliations

¹ Department of Molecular Life Sciences, University of Zurich, Zurich, Switzerland.
² Molecular Life Sciences Graduate School, ETH and University Of Zurich, Switzerland.
³ National Engineering Laboratory for AIDS Vaccine, School of Life Sciences, Jilin University, Changchun, China.
⁴ Department of Biochemistry, University of Zurich, Zurich, Switzerland.
⁵ Functional Genomics Center Zurich, Eidgenössische Technische Hochschule (ETH) Zurich and University of Zurich, Zurich, Switzerland.

Abstract

Mammalian adenoviruses (AdVs) comprise more than ~350 types including over 100 human (HAdVs) and just three mouse AdVs (MAdVs). While most HAdVs initiate infection by high affinity/avidity binding of their fiber knob (FK) protein to either coxsackievirus AdV receptor (CAR), CD46 or desmoglein (DSG)-2, MAdV-1 (M1) infection requires arginine-glycine-aspartate (RGD) binding integrins. To identify the receptors mediating MAdV infection we generated five novel reporter viruses for MAdV-1/-2/-3 (M1, M2, M3) transducing permissive murine (m) CMT-93 cells, but not B16 mouse melanoma cells expressing mCAR, human (h) CD46 or hDSG-2. Recombinant M1 or M3 FKs cross-blocked M1 and M3 but not M2 infections. Profiling of murine and human cells expressing RGD-binding integrins suggested that αvβ6 and αvβ8 heterodimers are associated with M1 and M3 infections. Ectopic expression of mβ6 in B16 cells strongly enhanced M1 and M3 binding, infection, and progeny production comparable with mαvβ6-positive CMT-93 cells, whereas mβ8 expressing cells were more permissive to M1 than M3. Anti-integrin antibodies potently blocked M1 and M3 binding and infection of CMT-93 cells and hαvβ8-positive M000216 cells. Soluble integrin αvβ6, and synthetic peptides containing the RGDLXXL sequence derived from FK-M1, FK-M3 and foot and mouth disease virus coat protein strongly interfered with M1/M3 infections, in agreement with high affinity interactions of FK-M1/FK-M3 with αvβ6/αvβ8, determined by surface plasmon resonance measurements. Molecular docking simulations of ternary complexes revealed a bent conformation of RGDLXXL-containing FK-M3 peptides on the subunit interface of αvβ6/β8, where the distal leucine residue dips into a hydrophobic pocket of β6/8, the arginine residue ionically engages αv aspartate215, and the aspartate residue coordinates a divalent cation in αvβ6/β8. Together, the RGDLXXL-bearing FKs are part of an essential mechanism for M1/M3 infection engaging murine and human αvβ6/8 integrins. These integrins are highly conserved in other mammals, and may favour cross-species virus transmission.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Adenoviridae / metabolism*
Adenoviridae Infections / metabolism*
Animals
Antigens, Neoplasm / metabolism*
Humans
Integrins / metabolism*
Mice
Receptors, Virus / metabolism*

Substances

Antigens, Neoplasm
Integrins
Receptors, Virus
integrin alphavbeta6
integrin alphavbeta8

Grants and funding

SH and UFG were funded by an Initial grant from Training Network grant supporting RH “ADVance” from the FP7 of the European Commission (no. 290002ADVance); SH was funded by the Swiss National Science Foundation (31003A_146286) supporting MBi; UFG was funded by the Swiss National Science Foundation 31003A_179256 / 1; MBi was partly supported from Novartis foundation for medical-biological research (16C222). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.