Genomic characterization and phylogenetic analysis of Chinese sacbrood virus isolated from Loess Plateau, China

Yu, Hao; Liu, T.X.; Wang, Dan

doi:10.4238/gmr.15036928

Cited by 2 publications

(3 citation statements)

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“…Healthy larvae treated by the same method were used as the negative control. CSBV was subsequently identified by reverse-transcription polymerase chain reaction (RT-PCR) to exclude black queen cell virus (BQCV), acute bee paralysis virus (ABPV), chronic bee paralysis virus (CBPV), deformed wing virus (DWV), Kashmir bee virus (KBV), and Israeli acute paralysis virus (IAPV), following the method reported by Yu, Liu & Wang (2016). CSBV virus samples free of other viruses were stored at −80 °C until further use.…”

Section: Methodsmentioning

confidence: 99%

“…The differences between the AC and AM genotypes may result from the adaptation of the virus to different hosts and the existence of different subgroups of the AC genotype based on regional variations (Choe et al, 2012a; Grabensteiner et al, 2001; Ma et al, 2013b). The AC genotype SBV strains were mainly isolated from Asian countries, and their hosts include A. cerana (Zhang et al, 2001; Zhang, 2012; Reddy et al, 2016, 2017; Ma et al, 2011c; Nguyen & Le, 2013; Choe et al, 2012b; Xia, Zhou & Wei, 2015; Hu et al, 2016; Yu, Liu & Wang, 2016). However, the AM genotype SBV persists in the bee colony and may cause infection of A. mellifera (Allen & Ball, 1996; Berenyi et al, 2006; Ellis & Munn, 2005; Cavigli et al, 2016; Tsevegmid, Neumann & Yañez, 2016; Desai & Currie, 2016).…”

Section: Introductionmentioning

confidence: 99%

“…The genetic characterization and phylogenetic relationship of SBV-infected honeybees collected from different hosts and various geographic regions have recently attracted attention. Previous studies have focused on the alignment, basic structure, and composition of SBV/CSBV genomes, and host-specificity and geographic differences of SBV/CSBV (Choe et al, 2012a, 2012b; Grabensteiner et al, 2001; Reddy et al, 2016, 2017; Ma et al, 2011c, 2013b; Nguyen & Le, 2013; Xia, Zhou & Wei, 2015; Hu et al, 2016; Yu, Liu & Wang, 2016; Zhang et al, 2001); however, it is unclear whether there is recombination between SBV and CSBV and if CSBV breaks through the species barrier, develops cross-infection, and causes disease (kills larvae) in A. mellifera . Using artificial infection experiments, Gong et al (2016) demonstrated that CSBV is able to infect A. mellifera , but did not observe obvious signs of the disease, which indicated low pathogenicity.…”

Section: Introductionmentioning

confidence: 99%

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Genetic and phylogenetic analysis of Chinese sacbrood virus isolates fromApis mellifera

Li¹,

Fei²,

Sun³

et al. 2019

PeerJ

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BackgroundSacbrood virus (SBV) is one of the most pathogenic honeybee viruses that exhibits host specificity and regional variations. The SBV strains that infect the Chinese honeybee Apis cerana are called Chinese SBVs (CSBVs).MethodsIn this study, a CSBV strain named AmCSBV-SDLY-2016 (GenBank accession No. ) infecting A. mellifera was identified by electron microscopy, its protein composition was analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis and agar gel immunodiffusion assay, and its nucleotide sequence was identified using a series of reverse-transcription polymerase chain reaction fragments of AmCSBV-SDLY-2016 generated using SBV/CSBV-specific primers. To investigate phylogenetic relationships of the CSBV isolates, a phylogenetic tree of the complete open reading frames (ORF) of the CSBV sequences was constructed using MEGA 6.0; then, the similarity and recombination events among the isolated CSBV strains were analyzed using SimPlot and RDP4 software, respectively.ResultsSequencing results revealed the complete 8,794-nucleotide long complete genomic RNA of the strain, with a single large ORF (189–8,717) encoding 2,843 amino acids. Comparison of the deduced amino acid sequence with the SBV/CSBV reference sequences deposited in the GenBank database identified helicase, protease, and RNA-dependent RNA polymerase domains; the structural genes were located at the 5′ end, whereas the non-structural genes were found at the 3′ end. Multiple sequence alignment showed that AmCSBV-SDLY-2016 had a 17-amino acid (aa) and a single aa deletion at positions 711–729 and 2,128, respectively, as compared with CSBV-GD-2002, and a 16-aa deletion (positions 711–713 and 715–728) as compared with AmSBV-UK-2000. However, AmCSBV-SDLY-2016 was similar to the CSBV-JLCBS-2014 strain, which infects A. cerana. AmCSBV-SDLY-2016 ORF shared 92.4–97.1% identity with the genomes of other CSBV strains (94.5–97.7% identity for deduced amino acids). AmCSBV-SDLY-2016 was least similar (89.5–90.4% identity) to other SBVs but showed maximum similarity with the previously reported CSBV-FZ-2014 strain. The phylogenetic tree constructed from AmCSBV-SDLY-2016 and 43 previously reported SBV/CSBV sequences indicated that SBV/CSBV strains clustered according to the host species and country of origin; AmCSBV-SDLY-2016 clustered with other previously reported Chinese and Asian strains (AC genotype SBV, as these strains originated from A. cerana) but was separate from the SBV genomes originating from Europe (AM genotype SBV, originating from A. mellifera). A SimPlot graph of SBV genomes confirmed the high variability, especially between the AC genotype SBV and AM genotype SBV. This genomic diversity may reflect the adaptation of SBV to specific hosts, ability of CSBV to cross the species barrier, and the spatial distances that separate CSBVs from other SBVs.

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Section: Methodsmentioning

confidence: 99%