Literature DB >> 29643234

Visualization of Arenavirus RNA Species in Individual Cells by Single-Molecule Fluorescence In Situ Hybridization Suggests a Model of Cyclical Infection and Clearance during Persistence.

Benjamin R King1,2, Aubin Samacoits3,4, Philip L Eisenhauer1, Christopher M Ziegler1, Emily A Bruce1, Daniel Zenklusen5, Christophe Zimmer3,4, Florian Mueller3,4, Jason Botten6,7.   

Abstract

Lymphocytic choriomeningitis mammarenavirus (LCMV) is an enveloped, negative-strand RNA virus that causes serious disease in humans but establishes an asymptomatic, lifelong infection in reservoir rodents. Different models have been proposed to describe how arenaviruses regulate the replication and transcription of their bisegmented, single-stranded RNA genomes, particularly during persistent infection. However, these models were based largely on viral RNA profiling data derived from entire populations of cells. To better understand LCMV replication and transcription at the single-cell level, we established a high-throughput, single-molecule fluorescence in situ hybridization (smFISH) image acquisition and analysis pipeline and examined viral RNA species at discrete time points from virus entry through the late stages of persistent infection in vitro We observed the transcription of viral nucleoprotein and polymerase mRNAs from the incoming S and L segment genomic RNAs, respectively, within 1 h of infection, whereas the transcription of glycoprotein mRNA from the S segment antigenome required ∼4 to 6 h. This confirms the temporal separation of viral gene expression expected due to the ambisense coding strategy of arenaviruses and also suggests that antigenomic RNA contained in virions is not transcriptionally active upon entry. Viral replication and transcription peaked at 36 h postinfection, followed by a progressive loss of viral RNAs over the next several days. During persistence, the majority of cells showed repeating cyclical waves of viral transcription and replication followed by the clearance of viral RNA. Thus, our data support a model of LCMV persistence whereby infected cells can spontaneously clear infection and become reinfected by viral reservoir cells that remain in the population.IMPORTANCE Arenaviruses are human pathogens that can establish asymptomatic, lifelong infections in their rodent reservoirs. Several models have been proposed to explain how arenavirus spread is restricted within host rodents, including the periodic accumulation and loss of replication-competent, but transcriptionally incompetent, viral genomes. A limitation of previous studies was the inability to enumerate viral RNA species at the single-cell level. We developed a high-throughput, smFISH assay and used it to quantitate lymphocytic choriomeningitis mammarenavirus (LCMV) replicative and transcriptional RNA species in individual cells at distinct time points following infection. Our findings support a model whereby productively infected cells can clear infection, including viral RNAs and antigen, and later be reinfected. This information improves our understanding of the timing and possible regulation of LCMV genome replication and transcription during infection. Importantly, the smFISH assay and data analysis pipeline developed here is easily adaptable to other RNA viruses.
Copyright © 2018 American Society for Microbiology.

Entities:  

Keywords:  LCMV; arenavirus; cyclical; gene probes; genome replication and transcription; kinetics; persistence; smFISH

Mesh:

Substances:

Year:  2018        PMID: 29643234      PMCID: PMC5974494          DOI: 10.1128/JVI.02241-17

Source DB:  PubMed          Journal:  J Virol        ISSN: 0022-538X            Impact factor:   5.103


  52 in total

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Journal:  J Virol       Date:  1993-05       Impact factor: 5.103

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Journal:  J Gen Virol       Date:  1969-07       Impact factor: 3.891

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Journal:  Nature       Date:  1967-02-25       Impact factor: 49.962

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Journal:  Adv Immunol       Date:  1980       Impact factor: 3.543

8.  Single-RNA counting reveals alternative modes of gene expression in yeast.

Authors:  Daniel Zenklusen; Daniel R Larson; Robert H Singer
Journal:  Nat Struct Mol Biol       Date:  2008-11-16       Impact factor: 15.369

9.  Sequencing studies of pichinde arenavirus S RNA indicate a novel coding strategy, an ambisense viral S RNA.

Authors:  D D Auperin; V Romanowski; M Galinski; D H Bishop
Journal:  J Virol       Date:  1984-12       Impact factor: 5.103

10.  Analysis of Pichinde arenavirus transcription and replication in human THP-1 monocytic cells.

Authors:  S J Polyak; S Zheng; D G Harnish
Journal:  Virus Res       Date:  1995-04       Impact factor: 3.303

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Review 2.  Defective Interfering Particles of Negative-Strand RNA Viruses.

Authors:  Christopher M Ziegler; Jason W Botten
Journal:  Trends Microbiol       Date:  2020-03-26       Impact factor: 17.079

Review 3.  Hemorrhagic Fever-Causing Arenaviruses: Lethal Pathogens and Potent Immune Suppressors.

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4.  Single-Cell Profiling of Ebola Virus Disease In Vivo Reveals Viral and Host Dynamics.

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Journal:  Cell       Date:  2020-11-06       Impact factor: 41.582

5.  Sensitive visualization of SARS-CoV-2 RNA with CoronaFISH.

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Journal:  Life Sci Alliance       Date:  2022-01-07

6.  Persistent RNA virus infection is short-lived at the single-cell level but leaves transcriptomic footprints.

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Journal:  Front Immunol       Date:  2019-07-17       Impact factor: 7.561

Review 9.  Progress in Anti-Mammarenavirus Drug Development.

Authors:  Yu-Jin Kim; Victor Venturini; Juan C de la Torre
Journal:  Viruses       Date:  2021-06-22       Impact factor: 5.048

10.  Profiling the specificity of clonally expanded plasma cells during chronic viral infection by single-cell analysis.

Authors:  Daniel Neumeier; Alessandro Pedrioli; Alessandro Genovese; Ioana Sandu; Roy Ehling; Kai-Lin Hong; Chrysa Papadopoulou; Andreas Agrafiotis; Raphael Kuhn; Danielle Shlesinger; Damiano Robbiani; Jiami Han; Laura Hauri; Lucia Csepregi; Victor Greiff; Doron Merkler; Sai T Reddy; Annette Oxenius; Alexander Yermanos
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