First Report of Little Cherry Virus 1 Infecting Sweet Cherry in Ontario, Canada

HomePlant DiseaseVol. 105, No. 12First Report of Little Cherry Virus 1 Infecting Sweet Cherry in Ontario, Canada PreviousNext DISEASE NOTE OPENOpen Access licenseFirst Report of Little Cherry Virus 1 Infecting Sweet Cherry in Ontario, CanadaA. Simkovich, S. E. Kohalmi, and A. WangA. SimkovichLondon Research and Development Centre, Agriculture and Agri-Food Canada, London, Ontario, CanadaDepartment of Biology, University of Western Ontario, London, Ontario, CanadaSearch for more papers by this author, S. E. KohalmiDepartment of Biology, University of Western Ontario, London, Ontario, CanadaSearch for more papers by this author, and A. Wang†Corresponding author: A. Wang; E-mail Address: Aiming.Wang@AGR.GC.CAhttps://orcid.org/0000-0003-2233-0652London Research and Development Centre, Agriculture and Agri-Food Canada, London, Ontario, CanadaSearch for more papers by this author AffiliationsAuthors and Affiliations A. Simkovich1 2 S. E. Kohalmi2 A. Wang1 † 1London Research and Development Centre, Agriculture and Agri-Food Canada, London, Ontario, Canada 2Department of Biology, University of Western Ontario, London, Ontario, Canada Published Online:2 Dec 2021https://doi.org/10.1094/PDIS-04-21-0798-PDNAboutSectionsView articlePDFSupplemental ToolsAdd to favoritesDownload CitationsTrack Citations ShareShare onFacebookTwitterLinked InRedditEmailWechat View articleThe Niagara fruit belt is one of the richest fruit-producing areas in Canada, contributing to 90% of Ontario’s tender fruits such as peach, plum, and sweet cherry. Little cherry virus 1 (LCV1) of the genus Velarivirus is a causal agent of little cherry disease, which has devastated cherry crops in many regions (Eastwell and Bernardy 1998; Jelkmann and Eastwell 2011). From 2013 to 2018, foliar symptoms indicative of viral infection such as leaf deformation, ringspot, mottling, vein clearing, and reddening were found on sweet cherry trees grown in the Niagara region. To determine if these trees were infected by a virus, small RNAs (sRNAs) were isolated from separately pooled asymptomatic and symptomatic leaves using the mirPremier microRNA isolation kit (Sigma Aldrich Canada, Oakville, ON). The sRNAs were used to create two libraries (four leaves per library) with the TruSeq Small RNA Sample Prep Kit (Illumina, San Diego, CA). The sRNA libraries were separately sequenced with the MiSeq Desktop Sequencer (Illumina). In total, 5,380,196 reads were obtained, and Trimmomatic (Bolger et al. 2014) was used to remove adaptors. The remaining 4,733,804 clean reads were assembled into contigs using Velvet 0.7.31 (Zerbino and Birney 2008) and Oases 0.2.09 (Schulz et al. 2012) with minimum length of 75 nt. A BLASTn search (Altschul et al. 1997) of the contigs identified the presence of cherry virus A (CVA; genus: Capillovirus) and two members of the Ilarvirus genus (Prunus necrotic ringspot virus [PNRSV] and prune dwarf virus [PDV]) in both libraries. LCV1 was only found in contigs derived from the symptomatic library. Of the clean reads, 22,016 were assembled into six contigs (with lengths ranging from 86 to 116 nt) mapping to LCV1, covering 7.07% of the viral genome. To confirm LCV1 infection, primers were designed from the assembled contigs and used for reverse transcription polymerase chain reaction (RT-PCR). Amplicons were sequenced, and the terminal sequences were determined using 5′ and 3′ RACE Systems (Invitrogen, Burlington, ON). Degenerate primers were designed from multiple sequence alignments of published LCV1 genomes for amplification and primer walking to obtain the sequence of LCV1. The complete genome sequence of LCV1 has a length of 16,934 nt and was deposited in GenBank (accession no. MN508820). A BLASTn search showed that this isolate is nearly identical (99.6% sequence identity) to an isolate from California (accession no. MN131067). To determine the incidence of infection, a field survey was performed at the same location during the spring months of 2014 to 2018 using RT-PCR with primers specific to the viral coat protein gene. Among 46 cherry trees sampled, two (4.3%) trees were infected with LCV1 and showed negative results with CVA, PNRSV, and PDV. Both trees displayed mild suturing of primary and secondary veins. LCV1 has been identified in Western stone fruit producing regions (British Columbia in Canada, and Washington, California, and Oregon in the United States of America). To the best of our knowledge, this is the first report of LCV1 in any eastern region of Canada. The low incidence of LCV1 suggests that this virus is not widespread in this region. Routine monitoring and detection of LCV1 is required to prevent this devastating cherry disease from spreading in this region.The author(s) declare no conflict of interest.References:Altschul, S. F., et al. 1997. 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Genome Res. 18:821. https://doi.org/10.1101/gr.074492.107 Crossref, ISI, Google ScholarFunding: Funding was provided by Agriculture and Agri-Food Canada.The author(s) declare no conflict of interest.DetailsFiguresLiterature CitedRelated Vol. 105, No. 12 December 2021SubscribeISSN:0191-2917e-ISSN:1943-7692 DownloadCaptionLeaf dieback caused by Stemphylium leaf blight on onion in Elba, New York State (F. Hay et al.). Photo credit: C. A. Hoepting. Symptoms of wilt observed on inflorescences of a coconut tree in Antsohyhi, Madagascar (sample MG16-004) (F. Pilet et al.). Photo credit: F. Pilet. Metrics Downloaded 596 times Article History Issue Date: 23 Jan 2022Published: 2 Dec 2021First Look: 14 Jul 2021Accepted: 12 Jul 2021 Page: 4173 InformationCopyright © 2021 Her Majesty the Queen in Right of Canada as Represented by the Minister of Agriculture and Agri-Food Canada.FundingAgriculture and Agri-Food CanadaKeywordsfruit tree viruspathogen detectionPrunusviruses and viroidsThe author(s) declare no conflict of interest.PDF download