Equine Arteritis Virus Derived from an Infectious cDNA Clone Is Attenuated and Genetically Stable in Infected Stallions

Balasuriya, Udeni B. R.; Snijder, Eric J.; Dinten, Leonie C. van; Heidner, Hans W.; Wilson, William D; Hedges, Jodi F.; Hullinger, Pamela J.; Maclachlan, Nigel J

doi:10.1006/viro.1999.9817

Cited by 56 publications

(56 citation statements)

References 26 publications

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“…The presence of EAV-specifi c antibodies in the horse blood serum is one of the evidence of the presence of the disease, which has been confi rmed also in our study by fi ndings of high antibody titre values in breeding stallions and mares [6,12,14]. High antibody titre and seroprevalence in stallions (45%) and mares (65%), without clinical signs strongly suggest the long-lasting presence of the disease at a horse stable [8].…”

Section: Discussionsupporting

confidence: 84%

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Detection Of Equine Arteritis Virus In The Semen Of Stallions In The Republic Of Serbia

et al. 2015

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The results on serological testing of blood sera from stallions and mares used for breeding and the presence of the viral genome of Equine Arteritis Virus (EAV) in stallion semen are presented. The blood and semen samples were taken from a horse stable on the territory of the Republic of Serbia during 2012, 2013 and 2014. Detection of anti-EAV specifi c antibodies in blood sera was performed by the virus neutralization test (VNT), and identifi cation of EAV genome RNA in stallion semen was done by reverse-transcriptase polymerase chain reaction (RT-PCR). In 2012, high seroprevalence of EAV was detected in the investigated stable. In total, 45% and 65 % of stallions and mares reacted positive, respectively, and the antibody titre values ranged between 2 and 10 log 2 . High seroprevalence was confi rmed in the same animals again in 2013. Out of two stallions tested semen samples in 2013, the viral genome was detected by RT-PCR in 3 examined semen samples from a seropositive stallion, while EAV was not detected in 3 semen samples of a seronegative stallion. During 2014, 11 semen samples were collected from two seropositive stallions. Again, the presence of EAV was confi rmed by RT-PCR in all 8 semen samples originating from the same stallion with the EAV genome positive semen result in 2013, whereas the virus was not detected in semen samples originating from the second anti-EAV antibody positive stallion. The presence of EAV-specifi c antibodies was confi rmed in the blood sera of the mares inseminated with the semen of seropositive stallions in 2012 and 2013.

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Section: Discussionsupporting

confidence: 84%

“…The fi rst anti-EAV antibodies can be detected 7-14 days after infection. The highest levels of antibodies are detectable in the period 2-4 months post infection, and they can persist for 3 or more years [6,12]. Antibody titre values higher than 2 log 2 are considered positive in VNT [13].…”

Section: Introductionmentioning

confidence: 99%

Detection Of Equine Arteritis Virus In The Semen Of Stallions In The Republic Of Serbia

et al. 2015

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“…The virus infects the smaller blood vessels, especially the arterioles, causing a panvasculitis (16,35,42). A number of studies have demonstrated that different strains of EAV vary significantly in their pathogenicity, with very different clinical outcomes upon experimental inoculation of horses (2,5,6,21,43). The horseadapted virulent Bucyrus (VB) strain of EAV is highly velogenic and causes severe clinical disease with a case fatality rate of 50 to 60% under experimental conditions (35,51).…”

mentioning

confidence: 99%

“…Horses inoculated with virulent strains of EAV (e.g., the VB, recombinant VB [rVBS], and KY84 strains) develop severe lymphopenia with a high-titer viremia (6 ϫ 10 3 to 1 ϫ 10 5 PFU/ml) (2,5,35,44). In contrast, horses inoculated with the attenuated modified live virus (MLV) vaccine strain or other avirulent strains of EAV (e.g., 030H and CA95G) (6,49) develop a mild, transient lymphopenia with only a very-low-titer viremia (Յ1 ϫ 10 1 PFU/ml) (20,24,(37)(38)(39)(40). The MLV vaccine (ARVAC; Fort Dodge Animal Health, Fort Dodge, IA) that is in current use in the United States and Canada (20,(37)(38)(39)(40) (24).…”

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confidence: 99%

Complex Interactions between the Major and Minor Envelope Proteins of Equine Arteritis Virus Determine Its Tropism for Equine CD3⁺T Lymphocytes and CD14⁺Monocytes

Zhang

Timoney

et al. 2010

J Virol

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Extensive cell culture passage of the virulent Bucyrus (VB) strain of equine arteritis virus (EAV) to produce the modified live virus (MLV) vaccine strain has altered its tropism for equine CD3 ؉ T lymphocytes and CD14 ؉ monocytes. The VB strain primarily infects CD14 ؉ monocytes and a small subpopulation of CD3 ؉ T lymphocytes (predominantly CD4 ؉ T lymphocytes), as determined by dual-color flow cytometry. In contrast, the MLV vaccine strain has a significantly reduced ability to infect CD14؉ monocytes and has lost its capability to infect CD3 ؉ T lymphocytes. Using a panel of five recombinant chimeric viruses, we demonstrated that interactions among the GP2, GP3, GP4, GP5, and M envelope proteins play a major role in determining the CD14 ؉ monocyte tropism while the tropism for CD3 ؉ T lymphocytes is determined by the GP2, GP4, GP5, and M envelope proteins but not the GP3 protein. The data clearly suggest that there are intricate interactions among these envelope proteins that affect the binding of EAV to different cell receptors on CD3؉ T lymphocytes and CD14؉ monocytes. This study shows, for the first time, that CD3 ؉ T lymphocytes may play an important role in the pathogenesis of equine viral arteritis when horses are infected with the virulent strains of EAV.

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“…Reverse genetic systems are a powerful tool for the molecular dissection of arteriviruses and infectious cDNA clones have been developed for equine arteritis virus and traditional PRRSV strains (Balasuriya et al, 1999(Balasuriya et al, , 2007Meulenberg et al, 1998;van Dinten et al, 1997;Wang et al, 2008). In this study, we set out to construct infectious cDNA clones of HP PRRSV to further clarify the role of this virus as the major aetiological agent of PHFS.…”

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confidence: 99%

An infectious cDNA clone of a highly pathogenic porcine reproductive and respiratory syndrome virus variant associated with porcine high fever syndrome

Zhang

Sun

et al. 2008

Journal of General Virology

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Since May 2006, a so-called ‘porcine high fever syndrome’ (PHFS) has spread all over China. The arterivirus porcine reproductive and respiratory syndrome virus (PRRSV) was believed to be the main causative agent, although the involvement of other pathogens was not formally excluded. The genome of a representative Chinese PRRSV strain, named JX143, was sequenced and used to develop infectious cDNA clones, pJX143 and pJX143M, with the latter containing an engineered MluI site that served as a genetic marker. In various virological assays, the rescued viruses, vJX143 and vJX143M, were indistinguishable from their parental virus. Animal experiments showed that these recombinant viruses retained the high pathogenicity and induced the typical clinical symptoms observed during PHFS outbreaks. This is the first report describing infectious cDNA clones of this highly pathogenic PRRSV. Our results unambiguously fulfil Koch's postulates and define highly pathogenic PRRSV as the aetiological agent of PHFS in China.

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Equine Arteritis Virus Derived from an Infectious cDNA Clone Is Attenuated and Genetically Stable in Infected Stallions

Cited by 56 publications

References 26 publications

Detection Of Equine Arteritis Virus In The Semen Of Stallions In The Republic Of Serbia

Detection Of Equine Arteritis Virus In The Semen Of Stallions In The Republic Of Serbia

Complex Interactions between the Major and Minor Envelope Proteins of Equine Arteritis Virus Determine Its Tropism for Equine CD3⁺T Lymphocytes and CD14⁺Monocytes

An infectious cDNA clone of a highly pathogenic porcine reproductive and respiratory syndrome virus variant associated with porcine high fever syndrome

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Equine Arteritis Virus Derived from an Infectious cDNA Clone Is Attenuated and Genetically Stable in Infected Stallions

Cited by 56 publications

References 26 publications

Detection Of Equine Arteritis Virus In The Semen Of Stallions In The Republic Of Serbia

Detection Of Equine Arteritis Virus In The Semen Of Stallions In The Republic Of Serbia

Complex Interactions between the Major and Minor Envelope Proteins of Equine Arteritis Virus Determine Its Tropism for Equine CD3+T Lymphocytes and CD14+Monocytes

An infectious cDNA clone of a highly pathogenic porcine reproductive and respiratory syndrome virus variant associated with porcine high fever syndrome

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Complex Interactions between the Major and Minor Envelope Proteins of Equine Arteritis Virus Determine Its Tropism for Equine CD3⁺T Lymphocytes and CD14⁺Monocytes