Epitranscriptomic regulation of HIV-1 full-length RNA packaging

Author:

Pereira-Montecinos Camila12,Toro-Ascuy Daniela123,Ananías-Sáez Catarina12,Gaete-Argel Aracelly12,Rojas-Fuentes Cecilia12,Riquelme-Barrios Sebastián12,Rojas-Araya Bárbara12,García-de-Gracia Francisco12,Aguilera-Cortés Paulina12,Chnaiderman Jonás1,Acevedo Mónica L13,Valiente-Echeverría Fernando123ORCID,Soto-Rifo Ricardo123ORCID

Affiliation:

1. Laboratory of Molecular and Cellular Virology, Virology Program, Institute of Biomedical Sciences, Faculty of Medicine, Universidad de Chile, Santiago, Chile

2. HIV/AIDS Workgroup (CHAIR), Faculty of Medicine, Universidad de Chile, Santiago, Chile

3. Millennium Institute on Immunology and Immunotherapy, Santiago, Chile

Abstract

Abstract During retroviral replication, the full-length RNA serves both as mRNA and genomic RNA. However, the mechanisms by which the HIV-1 Gag protein selects the two RNA molecules that will be packaged into nascent virions remain poorly understood. Here, we demonstrate that deposition of N6-methyladenosine (m6A) regulates full-length RNA packaging. While m6A deposition by METTL3/METTL14 onto the full-length RNA was associated with increased Gag synthesis and reduced packaging, FTO-mediated demethylation promoted the incorporation of the full-length RNA into viral particles. Interestingly, HIV-1 Gag associates with the RNA demethylase FTO in the nucleus and contributes to full-length RNA demethylation. We further identified two highly conserved adenosines within the 5′-UTR that have a crucial functional role in m6A methylation and packaging of the full-length RNA. Together, our data propose a novel epitranscriptomic mechanism allowing the selection of the HIV-1 full-length RNA molecules that will be used as viral genomes.

Funder

FONDECYT

ANID - ICM

CONICYT

Publisher

Oxford University Press (OUP)

Subject

Genetics

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