Molecular epidemiology of seal parvovirus, 1988-2014.

Rogier Bodewes,Marco W G Van De Bildt,Guillermo J Sánchez Contreras,Ana Rubio García,Miranda De Graaf,Thijs Kuiken,Albert D M E Osterhaus,Rebriarina Hapsari

doi:10.1371/journal.pone.0112129

Abstract

A novel parvovirus was discovered recently in the brain of a harbor seal (Phoca vitulina) with chronic meningo-encephalitis. Phylogenetic analysis of this virus indicated that it belongs to the genus Erythroparvovirus, to which also human parvovirus B19 belongs. In the present study, the prevalence, genetic diversity and clinical relevance of seal parvovirus (SePV) infections was evaluated in both harbor and grey seals (Halichoerus grypus) that lived in Northwestern European coastal waters from 1988 to 2014. To this end, serum and tissue samples collected from seals were tested for the presence of seal parvovirus DNA by real-time PCR and the sequences of the partial NS gene and the complete VP2 gene of positive samples were determined. Seal parvovirus DNA was detected in nine (8%) of the spleen tissues tested and in one (0.5%) of the serum samples tested, including samples collected from seals that died in 1988. Sequence analysis of the partial NS and complete VP2 genes of nine SePV revealed multiple sites with nucleotide substitutions but only one amino acid change in the VP2 gene. Estimated nucleotide substitution rates per year were 2.00×10−4 for the partial NS gene and 1.15×10−4 for the complete VP2 gene. Most samples containing SePV DNA were co-infected with phocine herpesvirus 1 or PDV, so no conclusions could be drawn about the clinical impact of SePV infection alone. The present study is one of the few in which the mutation rates of parvoviruses were evaluated over a period of more than 20 years, especially in a wildlife population, providing additional insights into the genetic diversity of parvoviruses.

Highlights

Parvoviruses are small, non-enveloped, viruses with linear, single-stranded DNA genomes of approximately 5 kb
Genetic analysis of seal parvovirus (SePV) Out of 12 samples in which SePV DNA was detected by realtime PCR, the partial NS (Genbank accession numbers: KM252699-KM252706) and the complete VP2 gene (Genbank accession numbers KM252691-KM252698) could be amplified in only 9 samples, possibly due to fragmentation of the DNA or inhibiting factors present in the other samples
Using the parvovirus detected in the oldest sample (SePV-PV880823.6) as a reference, 12 (1.3%) variant nucleotide positions were present in the partial NS gene (Figure 1), of which ten were transitions and two were transversions, and all 12 were synonymous

Summary

Introduction

Parvoviruses are small, non-enveloped, viruses with linear, single-stranded DNA genomes of approximately 5 kb. The family Parvoviridae comprises two subfamilies: Parvovirinae and Densovirinae. Eight genera have been recognized by the International Committee on Taxonomy of Viruses (ICTV) within the subfamily Parvovirinae: Amdoparvovirus, Aveparvovirus, Bocaparvovirus, Copiparvovirus, Dependoparvovirus, Erythroparvovirus, Protoparvovirus and Tetraparvovirus [2,3]. The genus Erythroparvovirus currently consists of six species, Primate erythroparvoviruses 1–4, Rodent erythroparvovirus 1 and Ungulate erythroparvovirus 1 [2,3]. Human parvovirus B19 or Primate erythroparvovirus 1 is the best studied member of this genus. It is prevalent worldwide; more than 15% of pre-school children, 50% of younger adults and 85% of the elderly have serologic evidence of infection based on data from Australia, Denmark, England, Japan, and the USA [4]. Chipmunk parvovirus (Rodent erythroparvovirus 1) and bovine parvovirus type 3 (Ungulate erythroparvovirus 1) are members of this genus and were identified in apparently healthy animals [10,11]

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Results

Conclusion