ViR: a tool to solve intrasample variability in the prediction of viral integration sites using whole genome sequencing data

Elisa Pischedda; Cristina Crava; Martina Carlassara; Susanna Zucca; Leila Gasmi; Mariangela Bonizzoni

doi:10.1186/s12859-021-03980-5

ViR: a tool to solve intrasample variability in the prediction of viral integration sites using whole genome sequencing data

BMC Bioinformatics. 2021 Feb 4;22(1):45. doi: 10.1186/s12859-021-03980-5.

Authors

Elisa Pischedda¹, Cristina Crava^{1

2}, Martina Carlassara¹, Susanna Zucca³, Leila Gasmi¹, Mariangela Bonizzoni⁴

Affiliations

¹ Department of Biology and Biotechnology, University of Pavia, 27100, Pavia, Italy.
² ERI BIOTECMED, Universitat de Valencia, 46010, Valencia, Spain.
³ Engenome Srl, 27100, Pavia, Italy.
⁴ Department of Biology and Biotechnology, University of Pavia, 27100, Pavia, Italy. mariangela.bonizzoni@unipv.it.

Abstract

Background: Several bioinformatics pipelines have been developed to detect sequences from viruses that integrate into the human genome because of the health relevance of these integrations, such as in the persistence of viral infection and/or in generating genotoxic effects, often progressing into cancer. Recent genomics and metagenomics analyses have shown that viruses also integrate into the genome of non-model organisms (i.e., arthropods, fish, plants, vertebrates). However, rarely studies of endogenous viral elements (EVEs) in non-model organisms have gone beyond their characterization from reference genome assemblies. In non-model organisms, we lack a thorough understanding of the widespread occurrence of EVEs and their biological relevance, apart from sporadic cases which nevertheless point to significant roles of EVEs in immunity and regulation of expression. The concomitance of repetitive DNA, duplications and/or assembly fragmentations in a genome sequence and intrasample variability in whole-genome sequencing (WGS) data could determine misalignments when mapping data to a genome assembly. This phenomenon hinders our ability to properly identify integration sites.

Results: To fill this gap, we developed ViR, a pipeline which solves the dispersion of reads due to intrasample variability in sequencing data from both single and pooled DNA samples thus ameliorating the detection of integration sites. We tested ViR to work with both in silico and real sequencing data from a non-model organism, the arboviral vector Aedes albopictus. Potential viral integrations predicted by ViR were molecularly validated supporting the accuracy of ViR results.

Conclusion: ViR will open new venues to explore the biology of EVEs, especially in non-model organisms. Importantly, while we generated ViR with the identification of EVEs in mind, its application can be extended to detect any lateral transfer event providing an ad-hoc sequence to interrogate.

Keywords: Lateral gene transfer; Non-model organisms; Repetitive DNA; Viral integration.

MeSH terms

Animals
Computational Biology
Genome, Viral
Genomics
Humans
Mosquito Vectors*
Virus Integration* / genetics
Whole Genome Sequencing*

Abstract

MeSH terms

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