2017
DOI: 10.1111/tbed.12751
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Isolation and characterization of novel goose parvovirus-related virus reveal the evolution of waterfowl parvovirus

Abstract: Short beak and dwarfism syndrome (SBDS) has been constantly breaking out in China since 2015. It is caused by a novel goose parvovirus-related virus (NGPV) and can severely restrict the growth of ducks. In this study, seven NGPV stains were isolated from different regions in China between 2015 and 2016. To better understand the correlation between NGPV and goose parvovirus (GPV), we conducted complete genome sequencing and a comprehensive analysis of the NGPV genome. The phylogenetic and alignment analysis sho… Show more

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Cited by 34 publications
(28 citation statements)
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References 40 publications
(74 reference statements)
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“…The primers were as follows: NGPV‐1F (5′‐AGA CTT ATC AACAAC CAT (C)T‐3′, position 3278–3296) and NGPV‐1R (5′‐TCA CTT ATT CCT GCT GTA G‐3′, position 4038–4056) were designed to amplify a 779‐base pair (bp) fragment, NGPV‐2R (5′‐CAT CAT CCG TAA AAA CTT GG‐3′, position 3406–3425) was designed with NGPV‐1F to amplify a 147 bp fragment. The seminested PCR assay was performed as our previous work (Li, Lin et al., ; Li, Zhang et al., ).…”
Section: Methodsmentioning
confidence: 99%
“…The primers were as follows: NGPV‐1F (5′‐AGA CTT ATC AACAAC CAT (C)T‐3′, position 3278–3296) and NGPV‐1R (5′‐TCA CTT ATT CCT GCT GTA G‐3′, position 4038–4056) were designed to amplify a 779‐base pair (bp) fragment, NGPV‐2R (5′‐CAT CAT CCG TAA AAA CTT GG‐3′, position 3406–3425) was designed with NGPV‐1F to amplify a 147 bp fragment. The seminested PCR assay was performed as our previous work (Li, Lin et al., ; Li, Zhang et al., ).…”
Section: Methodsmentioning
confidence: 99%
“…The primers were designed as described by Li et al [7] to amplify the complete genomes of the OsPV strains. The genomes were amplified using PrimeStar HS DNA polymerase (TaKaRa, Beijng, China).…”
Section: Whole Genome Amplification Of Ospvmentioning
confidence: 99%
“…These five viruses were prepared for PCR using Viral DNA Kit (Omega Bio‐Tek). All samples were subjected to PCR using specific primers (P4‐F: 5′‐ CTTGATGATGCTGAAAATGAAC‐3′ and P4‐R: 5′‐ GCCCATGGTGCCATAAGC‐3′) to amplify a partial sequence (1,446 bp) of the N‐GPV, described previously (Li et al, ). The target amplified PCR products were purified (Gel Extraction Kit; Omega Bio‐Tek), T‐A cloned (pBackZero8‐T vector cloning kit; Takara) and then sequenced in both directions (Sangon Biotech) using an ABI 3730 DNA sequencer (ABI).…”
Section: Methodsmentioning
confidence: 99%
“…The complete genome of HuN18 strain was amplified using PCR with the primers described previously (Li et al, ). The target amplified PCR products were purified, T‐A cloned and then sequenced in both directions.…”
Section: Methodsmentioning
confidence: 99%
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