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Species H Rotavirus Detected in Piglets with Diarrhea, Brazil, 2012 - Volume 20, Number 6—June 2014 - Emerging Infectious Disease journal - CDC

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Species H Rotavirus Detected in Piglets with Diarrhea, Brazil, 2012 - Volume 20, Number 6—June 2014 - Emerging Infectious Disease journal - CDC



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Volume 20, Number 6—June 2014

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Species H Rotavirus Detected in Piglets with Diarrhea, Brazil, 2012

Bruna L.D. Molinari, Elis Lorenzetti, Rodrigo A.A. Otonel, Alice F. Alfieri, and Amauri A. AlfieriComments to Author 
Author affiliations: UniversidadeEstadual de Londrina, Londrina, Parana, Brazil

Abstract

We determined nucleotide and deduced amino acid sequences of the rotavirus gene encoding viral protein 6 from 3 fecal samples collected from piglets with diarrhea in Brazil, 2012. The analyses showed that the porcine rotavirus strains in Brazil are closely related to the novel species H rotavirus.
Rotaviruses (RVs) form a genus of the family Reoviridae and are a common cause of viral gastroenteritis in humans and animals (1). The RV genome consists of 11 segments of double-stranded RNA that encode 6 structural viral protein (VP1–4, VP6, and VP7) and 6 nonstructural proteins (NSP1–6) (1). RVs have been classified into 7 species, which are also known as groups, termed A–G, on the basis of the antigenicity and genetic characteristics of VP6 (2,3). Rotavirus A (RVA) infections cause severe diarrhea in infants and young children worldwide but can also infect adults, other mammals, and birds (1). Rotavirus B (RVB) infections were first associated with severe diarrhea in adults (4) and have also been detected in cattle, pigs, sheep, and rats (57).
In addition to the 7 established species of RV, Matthijnssens et al. (2) recently proposed the new Rotavirus H (RVH) on the basis of VP6 sequence analysis. This species includes the following: the novel adult diarrhea RV strain (ADRV-N) isolated from specimens collected during an outbreak of gastroenteritis among adults during 1997 in China (8); strain J19, identified during the same outbreak in China in 1997 (9); the human Rotavirus B219, detected in a sporadic case of diarrhea in Bangladesh during 2002 (10,11); and the porcine RV strain SKA-1 that was isolated from a pig with diarrhea in Japan (12).
In this study, we determined the VP6 nucleotide sequence for 3 RV-positive fecal samples obtained from piglets with diarrhea in Brazil during 2012. A comparative analysis with other VP6 genes showed that the porcine RV strain from Brazil is closely related to the novel RVH.
A molecular study of RVB infection on a pig farm in Mato Grosso do Sul in the Central-West region of Brazil was performed during an outbreak of diarrheal illness in 2012. A total of 59 diarrheic fecal specimens were collected from 59 piglets whose ages ranged from 12 to 35 days, and the presence of RV was investigated by using polyacrylamide gel electrophoresis (13). Eight samples that showed RVB dsRNA pattern (4:2:2:3) and 2 that showed polyacrylamide gel electrophoresis inconclusive results were subjected to reverse transcription PCR (RT-PCR) by using the primer pair described by Gouvea et al. (14), which were designed to amplify a partial fragment of the NSP2 gene of RVB. All 10 samples were positive for RVB on the basis of the amplification of the 434-bp target fragment. To amplify larger fragments of the distinctive RVB NSP2 gene, we submitted the 10 fecal samples to RT-PCR using the primer pairs NSP2–1 F/R (993 bp), and NSP2–2 F/R (938 bp) as described by Suzuki et al. (15). Products of 993 bp expected for amplification reaction with a NSP2–1 primer pair were obtained for 7 of the samples. The remaining 3 samples (BR59, BR60, and BR63), from 35-day-old piglets, did not generate the expected fragments with any of the primer pairs. However, because of an unexpected annealing of the NSP2–2 primer pair in RT-PCR, shorter (≈750 bp) amplicons were generated for these 3 samples.
The nonspecific amplification products of the 3 samples were purified and sequenced with NSP2–2 forward and reverse primers by using the BigDye Terminator v3.1 Cycle Sequencing Reaction Kit (Applied Biosystems, Foster City, CA, USA) on an automated sequencer (ABI3500). Similarity searches were performed with sequences deposited in GenBank by using BLAST software (http://blast.ncbi.nlm.nih.gov/Blast.cgi?CMD=Web&PAGE_TYPE=BlastHomeExternal Web Site Icon). Of note, the highest nucleotide identities were obtained for the VP4 genes of the RVH strains SKA-1 (89%), B219 (72%), and J19 (70%). The VP4 nucleotide sequence alignment of the RVH SKA-1 strain and the nonspecific product was performed from the nucleotide positions 1792–2433 by using MEGA (v. 6) (http://www.megasoftware.net/External Web Site Icon).
To confirm the similarity of the samples BR59, BR60, and BR63 with RVH, we performed an additional set of RT-PCRs using 2 new primer pairs designed on the basis of the complete sequence of the VP6 gene of the porcine RVH strain SKA-1 (12) (Table 1). Phylogenetic analysis and nucleotide distance calculations were performed by using MEGA (v. 6) and BioEdit (v. 7.0.8.0) software (http://www.mbio.ncsu.edu/bioedit/bioedit.htmlExternal Web Site Icon).

Ms Molinari is a graduate student at Universidade Estadual de Londrina, Brazil. Her research interest is the genomic characterization of rotavirus.

Acknowledgments

This work was supported by the Brazilian Institutes National Council for Scientific and Technological Development (CNPq), Coordination for the Improvement of Higher Education Personnel (CAPES), and Araucária Foundation (FAP/PR).
A.A.A., A.F.A., and E.L. are the recipients of CNPq fellowships.

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Tables

Suggested citation for this article: Molinari BLD, Lorenzetti E, Otonel RAA, Alfieri AF, Alfieri AA. Species H rotavirus detected in piglets with diarrhea, Brazil, 2012. Emerg Infect Dis. 2014 Jun [date cited]. http://dx.doi.org/10.3201/eid2006.130776External Web Site Icon
DOI: 10.3201/eid2006.130776

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