Literature detail

Receptor binding, fusion inhibition, and induction of cross-reactive neutralizing antibodies by a soluble G glycoprotein of Hendra virus.

Katharine N Bossart¹ Gary Crameri Antony S Dimitrov Bruce A Mungall Yan-Ru Feng Jared R Patch Anil Choudhary Lin-Fa Wang Bryan T Eaton Christopher C Broder

Affiliations 1 institutions

Department of Microbiology and Immunology, F. Edward Hébert School of Medicine, Uniformed Services University of the Health Sciences, 4301 Jones Bridge Road, Bethesda, MD 20814-4799, USA.

PMID 15890907 2005 J Virol eng ppublish

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Article

Publication summary

Hendra virus (HeV) and Nipah virus (NiV) are closely related emerging viruses comprising the Henipavirus genus of the Paramyxovirinae, which are distinguished by their ability to cause fatal disease in both animal and human hosts. These viruses infect cells by a pH-independent membrane fusion event mediated by their attachment (G) and fusion (F) glycoproteins. Previously, we reported on HeV- and NiV-mediated fusion activities and detailed their host-cell tropism characteristics. These studies also suggested that a common cell surface receptor, which could be destroyed by protease, was utilized by both viruses. To further characterize the G glycoprotein and its unknown receptor, soluble forms of HeV G (sG) were constructed by replacing its cytoplasmic tail and transmembrane domains with an immunoglobulin kappa leader sequence coupled to either an S-peptide tag (sG(S-tag)) or myc-epitope tag (sG(myc-tag)) to facilitate purification and detection. Expression of sG was verified in cell lysates and culture supernatants by specific affinity precipitation. Analysis of sG by size exclusion chromatography and sucrose gradient centrifugation demonstrated tetrameric, dimeric, and monomeric species, with the majority of the sG released as a disulfide-linked dimer. Immunofluorescence staining revealed that sG specifically bound to HeV and NiV infection-permissive cells but not to a nonpermissive HeLa cell line clone, suggesting that it binds to virus receptor on host cells. Preincubation of host cells with sG resulted in dose-dependent inhibition of both HeV and NiV cell fusion as well as infection by live virus. Taken together, these data indicate that sG retains important native structural features, and we further demonstrate that administration of sG to rabbits can elicit a potent cross-reactive neutralizing antibody response against infectious HeV and NiV. This HeV sG glycoprotein will be exceedingly useful for structural studies, receptor identification strategies, and vaccine development goals for these important emerging viral agents.

Amino Acid Sequence Animals Antibodies, Viral Base Sequence Cell Line Chlorocebus aethiops Cross Reactions DNA, Viral HeLa Cells Hendra Virus Humans Membrane Fusion Molecular Sequence Data Molecular Weight Neutralization Tests Nipah Virus Receptors, Virus Recombinant Fusion Proteins

Structured evidence records

Evidence records

3 total

Receptor Usage 2 records

Receptor Usage Extraction confidence 0.95

Key finding

Soluble Hendra virus G glycoprotein binds to a receptor present on cells permissive to both Hendra and Nipah virus infection, indicating receptor compatibility between these viruses.

Virus

Host

Location

Supporting text

Immunofluorescence staining revealed that sG specifically bound to HeV and NiV infection-permissive cells but not to a nonpermissive HeLa cell line clone, suggesting that it binds to virus receptor on host cells.

Method: immunofluorescence staining; fusion inhibition assay
Receptors: virus receptor (common cell surface receptor destroyed by protease)

Receptor Usage Extraction confidence 0.95

Key finding

Hendra virus and Nipah virus utilize a shared cell surface receptor for entry, indicating mechanistic overlap in receptor usage.

Virus

Host

Location

Supporting text

Previously, we reported on HeV- and NiV-mediated fusion activities and detailed their host-cell tropism characteristics. These studies also suggested that a common cell surface receptor, which could be destroyed by protease, was utilized by both viruses.

Method: fusion assay
Receptors: common cell surface receptor destroyed by protease

Serological Evidence 1 records

Serological Evidence Extraction confidence 0.90

Key finding

Rabbits immunized with the soluble Hendra virus G glycoprotein developed cross-reactive neutralizing antibodies against Hendra and Nipah viruses.

Virus

Host

Location

Supporting text

We further demonstrate that administration of sG to rabbits can elicit a potent cross-reactive neutralizing antibody response against infectious HeV and NiV.

Method: Neutralization Tests
Sample type: serum

Citation context

References

42 references

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Evidence overview

Evidence 3

Types 2

Virus 2

Host 2

Evidence types

Receptor Usage 2 Serological Evidence 1

Linked entities

Viruses

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Locations

Publication metadata

Journal: Journal of virology
Volume / Issue / Pages: 79 / 11 / 6690-702
ISSN: 0022-538X
Journal country: United States
DOI: 10.1128/JVI.79.11.6690-6702.2005