Rabbit haemorrhagic disease: Cross-protection and comparative pathogenicity of GI.2/RHDV2/b and GI.1b/RHDV lagoviruses in a challenge trial

Calvete, C.; Mendoza, Manuel; Alcaraz, Ana; Sarto, María Pilar; Bagüés, María Pilar Jiménez de; Calvo, A. J.; Monroy, Fernando P.; Calvo, J.H.

doi:10.1016/j.vetmic.2018.04.018

Cited by 48 publications

(90 citation statements)

References 33 publications

(29 reference statements)

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“…All of the 37 wild rabbits were also qPCR-positive for the same virus at mean (SD) Cq values of 18.7 (2.04). This value is in agreement with Calvete et al (2018), who reported Cq values ranging from 18.03 to 18.30 using the same qPCR procedures in rabbits that had died from acute RHD caused by the same virus. Although qPCR was not developed to quantify viral RNA copy numbers (Calvete et al 2018), the high Cq values found in the small mammals suggested a lower quantity of viral particles than in rabbits killed by acute disease.…”

supporting

confidence: 92%

“…The results of the qPCR analysis were negative for all tissue samples except for the liver and the spleen of the surviving rabbit challenged with the Cr-Jun15-P4 inoculum. In this instance, GI.2/RHDV2/b RNA was found with high Cq values in the spleen and liver (40.5 and 42, respectively), which were, nevertheless, out of the lowest limit of detection (Cq¼38.7) established for qPCR (Calvete et al 2018). Seroconversion was detected in two surviving rabbits: one challenged with Cr-Feb15-P1 inoculum, and the survivor from the Cr-Jun15-P4 inoculum challenge.…”

mentioning

confidence: 79%

“…Liver samples from the 37 rabbits and the four small mammals were analyzed using duplex real-time PCR (qPCR) to detect RNA from GI.1b/RHDV and GI.2/RHDV2/b lagoviruses in a single analysis (Calvete et al 2018). Each sample was amplified in duplicate in the same run, and the quantification cycle (Cq) value was calculated as an average of both amplifications.…”

mentioning

confidence: 99%

“…A subset of the same tissue samples was fixed in 10% buffered formalin and processed using standard procedures for histological examination. The entire VP60 gene of the virus was sequenced (Calvete et al 2018), from the liver samples of 37 wild rabbits, as well as from the laboratory rabbits that died from RHD. Therefore, the full capsid VP60 sequence was used to infer phylogenetic relationships in this study.…”

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confidence: 99%

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Detection of Rabbit Hemorrhagic Disease Virus GI.2/RHDV2/b in the Mediterranean Pine Vole (Microtus duodecimcostatus) and White-Toothed Shrew (Crocidura russula)

Calvete

Mendoza

Sarto

et al. 2019

Journal of Wildlife Diseases

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The European wild rabbit ( Oryctolagus cuniculus) is a key prey species on the Iberian Peninsula, and several predator species that are at risk of extinction are dependent on them as prey. A new rabbit hemorrhagic disease (RHD) virus genotype (GI.2/RHDV2/b) emerged in 2010 and posed a threat to wild rabbit populations. During a survey aimed at investigating RHD epidemiology in wild rabbits, GI.2/RHDV2/b was detected by duplex real-time PCR in carcasses of one Mediterranean pine vole ( Microtus duodecimcostatus) and two white-toothed shrews ( Crocidura russula). Laboratory New Zealand white rabbits that were challenged with inocula obtained from the liver of the small mammals died showing RHD lesions, confirming the infectiousness of the isolates. Phylogenetic analysis of the VP60 gene nucleotide sequences showed complete homology between the isolates from the two small mammal species and a high degree of similarity, but not complete homology, to GI.2/RHDV2/b sequences from wild rabbits. The GI.2/RHDV2/b genotype has not been reported in species outside the order Lagomorpha.

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confidence: 92%

mentioning

confidence: 79%

mentioning

confidence: 99%

mentioning

confidence: 99%

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Detection of Rabbit Hemorrhagic Disease Virus GI.2/RHDV2/b in the Mediterranean Pine Vole (Microtus duodecimcostatus) and White-Toothed Shrew (Crocidura russula)

Calvete

Mendoza

Sarto

et al. 2019

Journal of Wildlife Diseases

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“…A large 362 proportion of rabbits present in every shot sample were >500 days old, and may therefore confound 363 the analysis of recent virus activity. In addition, if some level of immunological cross protection 364 exists between RHDV and RHDV2 (Calvete et al, 2018), the removal of susceptible rabbits by an 365 RHDV2 outbreak from the population could result in an apparent increase of RHDV seroprevalence, 366 due to the resulting increased proportion of surviving old RHDV seropositive animals in the sample. 367…”

Section: Discussion: 310mentioning

confidence: 99%

Retrospective serological analysis reveals presence of the emerging lagovirus RHDV2 in Australian wild rabbits at least six months prior to its first detection

Strive

Piper

Huang

et al. 2019

Preprint

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SummaryThe lagovirus Rabbit Haemorrhagic Disease Virus (RHDV) has been circulating in Australia since the mid-1990s when it was deliberately released to control overabundant rabbit populations. In recent years, the viral diversity of different RHDVs in Australia has increased, and currently four different types of RHDV are known to be circulating. To allow for ongoing epidemiological studies and impact assessments of these viruses on Australian wild rabbit populations, it is essential that serological tools are updated. To this end, Reference sera were produced against all four virulent RHDVs (including RHDV2) known to be present in Australia and tested in a series of available immunological assays originally developed for the prototype RHDV, to assess patterns of cross reactivity and the usefulness of these assays to detect lagovirus antibodies, either in a generic or specific manner. Enzyme Linked Immuno Sorbent Assays (ELISAs) developed to detect antibody isotypes IgM, IgA and IgG were sufficiently cross reactive to detect antibodies raised against all four virulent lagoviruses. For the more specific detection of antibodies to the antigenically more different RHDV2, a competition ELISA was adapted using RHDV2 specific monoclonal antibodies in combination with Australian viral antigen. Archival serum banks from a long term rabbit monitoring site where rabbits were sampled quarterly over a period of six years were re-screened using this assay, and revealed serological evidence for the arrival of RHDV2 in this population at least six months prior to its initial detection in Australia in a deceased rabbit in May 2015. The serological methods and reference reagents described here will provide valuable tools to study presence, prevalence and impact of RHDV2 on Australian rabbit populations; however the discrimination of different antigenic variants of RHDVs as well as mixed infections at the serological level remains challenging.

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The impact of integrating rabbit haemorrhagic disease virus (K5) release with pindone baiting on wild rabbit populations

Patel,

Austin,

Warner

et al. 2024

Ecology and Evolution

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Several conventional and recently available tools are available for an integrated control of European rabbits in Australia. We quantified the impact of the release of rabbit haemorrhagic disease virus K5 (RHDV K5, hereafter K5) and pindone (2‐pivalyl‐1,3‐indandione) baiting at 13 sites within Cudlee Creek fire scar in the Adelaide Hills, South Australia. K5 release was followed by pindone baiting between December 2021 and March 2022; the application of both control methods followed industry best practice. We counted rabbits using spotlights before and after the application of both control methods. Fly samples and livers from dead rabbits were collected to track K5 transmission within and between sites, and to detect the natural circulation of rabbit haemorrhagic disease virus 2 (RHDV2). K5 release had minimal impact on rabbit populations, with treated populations increasing by a mean of 65.5% at 14 days post‐release and 27.9% at 77 days post‐K5 release across all sites, comparable to the changes at control sites. K5 detection in flies up to 77 days post its release, and its detection in rabbit livers, demonstrates that it can survive and transmit in the environment for prolonged periods and that it can lethally infect some rabbits. This limited impact of K5 is consistent with previous studies and may be explained by pre‐existing RHDV/RHDV2 immunity in the target populations or the presence of young rabbits with natural innate RHDV immunity. The detection of K5 in flies from control sites demonstrates that it was vectored beyond its release location. A reduction in rabbit counts post‐pindone baiting was observed at most treatment sites, with a mean population reduction of 36.6% across all sites. Landholders need to carefully and strategically plan their integrated rabbit control programmes. Not all combinations of controls, even if theoretically logical, achieve meaningful outcomes for rabbit management.

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Rabbit haemorrhagic disease: Cross-protection and comparative pathogenicity of GI.2/RHDV2/b and GI.1b/RHDV lagoviruses in a challenge trial

Cited by 48 publications

References 33 publications

Detection of Rabbit Hemorrhagic Disease Virus GI.2/RHDV2/b in the Mediterranean Pine Vole (Microtus duodecimcostatus) and White-Toothed Shrew (Crocidura russula)

Detection of Rabbit Hemorrhagic Disease Virus GI.2/RHDV2/b in the Mediterranean Pine Vole (Microtus duodecimcostatus) and White-Toothed Shrew (Crocidura russula)

Retrospective serological analysis reveals presence of the emerging lagovirus RHDV2 in Australian wild rabbits at least six months prior to its first detection

The impact of integrating rabbit haemorrhagic disease virus (K5) release with pindone baiting on wild rabbit populations

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