Literature detail

Mutational Analysis of Lassa Virus Glycoprotein Highlights Regions Required for Alpha-Dystroglycan Utilization.

Marissa Acciani¹ Jacob T Alston¹ Guohui Zhao¹ Hayley Reynolds¹ Afroze M Ali¹ Brian Xu¹ Melinda A Brindley²

Affiliations 2 institutions

Department of Infectious Diseases, College of Veterinary Medicine, University of Georgia, Athens, Georgia, USA.
Department of Infectious Diseases, Department of Population Health, Center for Vaccines and Immunology, College of Veterinary Medicine, University of Georgia, Athens, Georgia, USA [email protected].

PMID 28679759 2017 J Virol eng epublish

Article

Publication summary

Lassa virus (LASV) is an enveloped RNA virus endemic to West Africa and responsible for severe cases of hemorrhagic fever. Virus entry is mediated by the glycoprotein complex consisting of a stable-signal peptide, a receptor-binding subunit, GP1, and a viral-host membrane fusion subunit, GP2. Several cellular receptors can interact with the GP1 subunit and mediate viral entry, including alpha-dystroglycan (αDG) and lysosome-associated membrane protein 1 (LAMP1). In order to define the regions within GP1 that interact with the cellular receptors, we implemented insertional mutagenesis, carbohydrate shielding, and alanine scanning mutagenesis. Eighty GP constructs were engineered and evaluated for GP1-GP2 processing, surface expression, and the ability to mediate cell-to-cell fusion after low-pH exposure. To examine virus-to-cell entry, 49 constructs were incorporated onto vesicular stomatitis virus (VSV) pseudoparticles and transduction efficiencies were monitored in HAP1 and HAP1-ΔDAG1 cells that differentially produce the αDG cell surface receptor. Seven constructs retained efficient transduction in HAP1-ΔDAG1 cells yet poorly transduced HAP1 cells, suggesting that they are involved in αDG utilization. Residues H141, N146, F147, and Y150 cluster at the predicted central core of the trimeric interface and are important for GP-αDG interaction. Additionally, H92A-H93A, 150HA, 172HA, and 230HA displayed reduced transduction in both HAP1 and HAP1-ΔDAG1 cells, despite efficient cell-to-cell fusion activity. These mutations may interfere with interactions with the endosomal receptor LAMP1 or interfere at another stage in entry that is common to both cell lines. Insight gained from these data can aid in the development of more-effective entry inhibitors by blocking receptor interactions.<b>IMPORTANCE</b> Countries in which Lassa virus is endemic, such as Nigeria, Sierra Leone, Guinea, and Liberia, usually experience a seasonal outbreak of the virus from December to March. Currently, there is neither a preventative vaccine nor a therapeutic available to effectively treat severe Lassa fever. One way to thwart virus infection is to inhibit interaction with cellular receptors. It is known that the GP1 subunit of the Lassa glycoprotein complex plays a critical role in receptor recognition. Our results highlight a region within the Lassa virus GP1 protein that interacts with the cellular receptor alpha-dystroglycan. This information may be used for future development of new Lassa virus antivirals.

arenavirus receptor binding virus entry Cell Line DNA Mutational Analysis Dystroglycans Humans Lassa virus Lysosomal Membrane Proteins Lysosomal-Associated Membrane Protein 1 Mutagenesis, Insertional Mutagenesis, Site-Directed Mutant Proteins Receptors, Virus Recombinant Proteins Transduction, Genetic Vesiculovirus Viral Envelope Proteins

Structured evidence records

Evidence records

4 total

Molecular Adaptation 2 records

Molecular Adaptation Extraction confidence 0.90

Key finding

Mutations at residues H141, N146, F147, and Y150 within the Lassa virus GP1 glycoprotein reduce utilization of the alpha-dystroglycan receptor, indicating these residues are critical for receptor-mediated entry.

Virus

Host

Location

Supporting text

Residues H141, N146, F147, and Y150 cluster at the predicted central core of the trimeric interface and are important for GP-αDG interaction.

Genes or proteins: GP1
Receptors: alpha-dystroglycan
Mutations: H141; N146; F147; Y150
Mechanism types: receptor_binding; cell_entry

Molecular Adaptation Extraction confidence 0.90

Key finding

Mutations H92A-H93A, 150HA, 172HA, and 230HA in Lassa virus GP1 reduced viral entry efficiency, suggesting interference with LAMP1-mediated endosomal interactions or another common entry stage.

Virus

Host

Location

Supporting text

Additionally, H92A-H93A, 150HA, 172HA, and 230HA displayed reduced transduction in both HAP1 and HAP1-ΔDAG1 cells, despite efficient cell-to-cell fusion activity. These mutations may interfere with interactions with the endosomal receptor LAMP1 or interfere at another stage in entry.

Genes or proteins: GP1
Receptors: LAMP1
Mutations: H92A-H93A; 150HA; 172HA; 230HA
Mechanism types: receptor_binding; cell_entry

Receptor Usage 2 records

Receptor Usage Extraction confidence 1.00

Key finding

Mutations in the Lassa virus GP1 subunit define residues critical for interaction with the cellular receptor alpha-dystroglycan.

Virus

Host

Location

Supporting text

Seven constructs retained efficient transduction in HAP1-ΔDAG1 cells yet poorly transduced HAP1 cells, suggesting that they are involved in αDG utilization. Residues H141, N146, F147, and Y150 cluster at the predicted central core of the trimeric interface and are important for GP-αDG interaction.

Method: mutagenesis; pseudovirus assay
Receptors: alpha-dystroglycan

Receptor Usage Extraction confidence 1.00

Key finding

Certain Lassa virus GP1 mutations reduce interaction with the endosomal receptor LAMP1, indicating its involvement in virus entry.

Virus

Host

Location

Supporting text

These mutations may interfere with interactions with the endosomal receptor LAMP1 or interfere at another stage in entry that is common to both cell lines.

Method: mutagenesis; pseudovirus assay
Receptors: LAMP1

Citation context

References

59 references

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Evidence overview

Evidence 4

Types 2

Virus 1

Host 1

Evidence types

Molecular Adaptation 2 Receptor Usage 2

Linked entities

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Locations

Publication metadata

Journal: Journal of virology
Volume / Issue / Pages: 91 / 18 / -
ISSN: 1098-5514
Journal country: United States
DOI: 10.1128/JVI.00574-17