Characterization of Variant RNAs Encapsidated during Bromovirus Infection by High-Throughput Sequencing

Author:

Dexheimer Sarah1ORCID,Shrestha Nipin1,Chapagain Bandana Sharma1,Bujarski Jozef J.1,Yin Yanbin12

Affiliation:

1. Department of Biological Sciences, Plant Molecular and Bioinformatics Center, Northern Illinois University, DeKalb, IL 60115, USA

2. Nebraska Food for Health Center, Department of Food Science and Technology, University of Nebraska—Lincoln, Lincoln, NE 68588, USA

Abstract

Previously, we described the RNA recombinants accumulating in tissues infected with the bromoviruses BMV (Brome mosaic virus) and CCMV (Cowpea chlorotic mottle virus). In this work, we characterize the recombinants encapsidated inside the purified virion particles of BMV and CCMV. By using a tool called the Viral Recombination Mapper (ViReMa) that detects recombination junctions, we analyzed a high number of high-throughput sequencing (HTS) short RNA sequence reads. Over 28% of BMV or CCMV RNA reads did not perfectly map to the viral genomes. ViReMa identified 1.40% and 1.83% of these unmapped reads as the RNA recombinants, respectively, in BMV and CCMV. Intra-segmental crosses were more frequent than the inter-segmental ones. Most intra-segmental junctions carried short insertions/deletions (indels) and caused frameshift mutations. The mutation hotspots clustered mainly within the open reading frames. Substitutions of various lengths were also identified, whereas a small fraction of crosses occurred between viral and their host RNAs. Our data reveal that the virions can package detectable amounts of multivariate recombinant RNAs, contributing to the flexible nature of the viral genomes.

Funder

National Institutes of Health (NIH) AREA award

University of Nebraska—Lincoln

National Science Foundation (NSF) CAREER award

NIH R21 award

NIH R01

United States Department of Agriculture (USDA) award

National Science Foundation

Plant Molecular Biology Center and the Graduate School

Publisher

MDPI AG

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