A-to-I editing of Malacoherpesviridae RNAs supports the antiviral role of ADAR1 in mollusks.


Journal

BMC evolutionary biology
ISSN: 1471-2148
Titre abrégé: BMC Evol Biol
Pays: England
ID NLM: 100966975

Informations de publication

Date de publication:
23 07 2019
Historique:
received: 05 11 2018
accepted: 04 07 2019
entrez: 25 7 2019
pubmed: 25 7 2019
medline: 29 9 2019
Statut: epublish

Résumé

Adenosine deaminase enzymes of the ADAR family are conserved in metazoans. They convert adenine into inosine in dsRNAs and thus alter both structural properties and the coding potential of their substrates. Acting on exogenous dsRNAs, ADAR1 exerts a pro- or anti-viral role in vertebrates and Drosophila. We traced 4 ADAR homologs in 14 lophotrochozoan genomes and we classified them into ADAD, ADAR1 or ADAR2, based on phylogenetic and structural analyses of the enzymatic domain. Using RNA-seq and quantitative real time PCR we demonstrated the upregulation of one ADAR1 homolog in the bivalve Crassostrea gigas and in the gastropod Haliotis diversicolor supertexta during Ostreid herpesvirus-1 or Haliotid herpesvirus-1 infection. Accordingly, we demonstrated an extensive ADAR-mediated editing of viral RNAs. Single nucleotide variation (SNV) profiles obtained by pairing RNA- and DNA-seq data from the viral infected individuals resulted to be mostly compatible with ADAR-mediated A-to-I editing (up to 97%). SNVs occurred at low frequency in genomic hotspots, denoted by the overlapping of viral genes encoded on opposite DNA strands. The SNV sites and their upstream neighbor nucleotide indicated the targeting of selected adenosines. The analysis of viral sequences suggested that, under the pressure of the ADAR editing, the two Malacoherpesviridae genomes have evolved to reduce the number of deamination targets. We report, for the first time, evidence of an extensive editing of Malacoherpesviridae RNAs attributable to host ADAR1 enzymes. The analysis of base neighbor preferences, structural features and expression profiles of molluscan ADAR1 supports the conservation of the enzyme function among metazoans and further suggested that ADAR1 exerts an antiviral role in mollusks.

Sections du résumé

BACKGROUND
Adenosine deaminase enzymes of the ADAR family are conserved in metazoans. They convert adenine into inosine in dsRNAs and thus alter both structural properties and the coding potential of their substrates. Acting on exogenous dsRNAs, ADAR1 exerts a pro- or anti-viral role in vertebrates and Drosophila.
RESULTS
We traced 4 ADAR homologs in 14 lophotrochozoan genomes and we classified them into ADAD, ADAR1 or ADAR2, based on phylogenetic and structural analyses of the enzymatic domain. Using RNA-seq and quantitative real time PCR we demonstrated the upregulation of one ADAR1 homolog in the bivalve Crassostrea gigas and in the gastropod Haliotis diversicolor supertexta during Ostreid herpesvirus-1 or Haliotid herpesvirus-1 infection. Accordingly, we demonstrated an extensive ADAR-mediated editing of viral RNAs. Single nucleotide variation (SNV) profiles obtained by pairing RNA- and DNA-seq data from the viral infected individuals resulted to be mostly compatible with ADAR-mediated A-to-I editing (up to 97%). SNVs occurred at low frequency in genomic hotspots, denoted by the overlapping of viral genes encoded on opposite DNA strands. The SNV sites and their upstream neighbor nucleotide indicated the targeting of selected adenosines. The analysis of viral sequences suggested that, under the pressure of the ADAR editing, the two Malacoherpesviridae genomes have evolved to reduce the number of deamination targets.
CONCLUSIONS
We report, for the first time, evidence of an extensive editing of Malacoherpesviridae RNAs attributable to host ADAR1 enzymes. The analysis of base neighbor preferences, structural features and expression profiles of molluscan ADAR1 supports the conservation of the enzyme function among metazoans and further suggested that ADAR1 exerts an antiviral role in mollusks.

Identifiants

pubmed: 31337330
doi: 10.1186/s12862-019-1472-6
pii: 10.1186/s12862-019-1472-6
pmc: PMC6651903
doi:

Substances chimiques

Antiviral Agents 0
RNA, Viral 0
RNA-Binding Proteins 0

Types de publication

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

Langues

eng

Sous-ensembles de citation

IM

Pagination

149

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Auteurs

Umberto Rosani (U)

Department of Biology, University of Padova, 32121, Padova, Italy. umberto.rosani@unipd.it.
Helmholtz Centre for Polar and Marine Research, Alfred Wegener Institute (AWI), Wadden Sea Station, 25992, List auf Sylt, Germany. umberto.rosani@unipd.it.

Chang-Ming Bai (CM)

Chinese Academy of Fishery Sciences, Yellow Sea Fisheries Research Institute, Qingdao, China.

Lorenzo Maso (L)

Department of Biology, University of Padova, 32121, Padova, Italy.

Maxwell Shapiro (M)

Department of Applied Mathematics and Statistics, Stony Brook University, Stony Brook, NY, USA.

Miriam Abbadi (M)

Istituto Zooprofilattico Sperimentale delle Venezie, 35020, Legnaro, Italy.

Stefania Domeneghetti (S)

Department of Biology, University of Padova, 32121, Padova, Italy.

Chong-Ming Wang (CM)

Chinese Academy of Fishery Sciences, Yellow Sea Fisheries Research Institute, Qingdao, China.

Laura Cendron (L)

Department of Biology, University of Padova, 32121, Padova, Italy.

Thomas MacCarthy (T)

Department of Applied Mathematics and Statistics, Stony Brook University, Stony Brook, NY, USA.

Paola Venier (P)

Department of Biology, University of Padova, 32121, Padova, Italy. paola.venier@unipd.it.

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