Puma Lentivirus Is Controlled in Domestic Cats after Mucosal Exposure in the Absence of Conventional Indicators of Immunity

TerWee, Julie A.; Yactor, Jennifer K.; Sondgeroth, Kerry S.; VandeWoude, Sue

doi:10.1128/jvi.79.5.2797-2806.2005

Cited by 28 publications

(43 citation statements)

References 50 publications

(57 reference statements)

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“…Barr, et al (1989) considered a single band on immunoblot to be equivocal with a high probability that the sample was positive. The four aforementioned experimental studies in domestic cats (VandeWoude et al, 1997a(VandeWoude et al, , 2003Sondgeroth et al, 2005;TerWee et al, 2005) had 100% specificity using one band as a positive indicator. Further, the sensitivity was high because 25 of 27 domestic cats that were inoculated with PLV were positive by PLV immunoblot, viral coculture, and PCR.…”

Section: Discussionmentioning

confidence: 98%

“…All positive samples, including positive controls, had similar banding patterns characterized by greater affinity for the p24 antigen than any other antigen, suggesting that all positive results were true positives and not unspecific antibody binding. Further, during experimental infection of domestic cats with PLV, PLV immunoblots were 100% specific for PLV infection because none of the 19 sham-inoculated animals used in controlled studies were positive by PLV immunoblot, coculture, or PCR (VandeWoude et al, 1997a;VandeWoude et al, 2003;Sondgeroth et al, 2005;TerWee et al, 2005).…”

Section: Discussionmentioning

confidence: 99%

“…Antigens were prepared from viral cultures of domestic cat FIV (FIV-B2546), puma lentivirus (PLV-1695), and lion lentivirus (LLV-438). Stocks were grown in domestic cat origin cell line Mya-1 (Miyazawa et al, 1989), and viral proteins were isolated as previously described (VandeWoude et al, 1997b;TerWee et al, 2005). Reverse-transcriptase positive tissue culture supernatant was centrifuged at 200 3 G (GPR centrifuge, Beckman Instruments, Inc., Fullerton, California, USA) for 10 min at 5 C to remove cellular material.…”

Section: Immunoblot Analysismentioning

confidence: 99%

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Variability in assays used for detection of lentiviral infection in bobcats (Lynx rufus), pumas (Puma concolor), and ocelots (Leopardus pardalis)

Franklin

Troyer

TerWee

et al. 2007

Journal of Wildlife Diseases

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ABSTRACT:Although lentiviruses similar to feline immunodeficiency virus (FIV) are known to infect numerous felid species, the relative utility of assays used for detecting lentiviral infection has not been compared for many of these hosts. We tested bobcats (Lynx rufus), pumas (Felis concolor), and ocelots (Leopardus pardalis) for exposure to lentivirus using five different assays: puma lentivirus (PLV), African lion lentivirus (LLV), and domestic cat FIV-based immunoblots, a commercially available enzyme-linked immunosorbent assay (ELISA) kit, and nested polymerase chain reaction (PCR). Puma lentivirus immunoblots identified more seropositive individuals than the other antibody-detection assays. The commercial ELISA provided a fair ability to recognize seropositive samples when compared with PLV immunoblot for screening bobcats and ocelots, but not pumas. Polymerase chain reaction identified fewer positive samples than PLV immunoblot for all three species. Immunoblot results were equivalent whether the sample tested was serum, plasma, or whole blood. The results from this study and previous investigations suggest that the PLV immunoblot has the greatest ability to detect reactive samples when screening wild felids of North America and is unlikely to produce false positive results. However, the commercial ELISA kit may provide an adequate alternative for screening of some species and is more easily adapted to field conditions.

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Section: Discussionmentioning

confidence: 98%

Section: Discussionmentioning

confidence: 99%

Section: Immunoblot Analysismentioning

confidence: 99%

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Variability in assays used for detection of lentiviral infection in bobcats (Lynx rufus), pumas (Puma concolor), and ocelots (Leopardus pardalis)

Franklin

Troyer

TerWee

et al. 2007

Journal of Wildlife Diseases

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“…Cats can be persistently infected with PLV by either the oral nasal (ON) or intravenously (IV) routes but there are no clinical consequences of the infection (VandeWoude et al, 1997;Terwee et al, 2005). Despite the fact that in the majority of ON-inoculated cats the virus levels dropped below the level of detection at time points when viremia was still apparent in IV-inoculated cats, there were no differences in immunological profiles of cats.…”

Section: Fivpco In a New Hostmentioning

confidence: 93%

The molecular biology and evolution of feline immunodeficiency viruses of cougars

Poss

Ross

Rodrigo

et al. 2008

Veterinary Immunology and Immunopathology

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Feline immunodeficiency virus (FIV) is a lentivirus that has been identified in many members of the family Felidae but domestic cats are the only FIV host in which infection results in disease. We studied FIVpco infection of cougars (Puma concolor) as a model for asymptomatic lentivirus infections to understand the mechanisms of host-virus coexistence. Several natural cougar populations were evaluated to determine if there are any consequences of FIVpco infection on cougar fecundity, survival, or susceptibility to other infections. We have sequenced full length viral genomes and conducted a detailed analysis of viral molecular evolution on these sequences and on genome fragments of serially sampled animals to determine the evolutionary forces experienced by this virus in cougars. In addition, we have evaluated the molecular genetics of FIVpco in a new host, domestic cats, to determine the evolutionary consequences to a host-adapted virus associated with crossspecies infection. Our results indicate that there are no significant differences in survival, fecundity or susceptibility to other infections between FIVpco-infected and uninfected cougars. The molecular evolution of FIVpco is characterized by a slower evolutionary rate and an absence of positive selection, but also by proviral and plasma viral loads comparable to those of epidemic lentiviruses such as HIV-1 or FIVfca. Evolutionary and recombination rates and selection profiles change significantly when FIVpco replicates in a new host.

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“…Lentiviral infections have also been detected in several nondomestic feline species, including in African lion (FIVple) populations in eastern and southern Africa (Panthera leo), but significant sequence divergence exists among the feline lentiviruses of different host species, with as much as 30% diversity in the conserved regions of the polymerase gene (Pol), and even higher diversity in the regions encoding the envelope glycoprotein and core protein (Brown et al 1994;Langley et al 1994;Carpenter et al 1998;Terwee et al 2005;Troyer et al 2005). Diversity is also pronounced among the feline lentiviruses infecting a single nondomestic host species, where as much as a 20% divergence may exist in the Pol region among different isolates (Brown et al 1994;Carpenter et al 1998;Terwee et al 2005;Troyer et al 2005). These findings are in contrast to FIVfca, where viral subtypes, or clades, differ in their nucleotide sequences by only 5-10% across the entire genome (Sodora et al 1995;Carpenter et al 1998).…”

Section: Introductionmentioning

confidence: 99%

Detection and Genetic Analysis of Feline Immunodeficiency Virus (FIVple) in Southern African Lions (Panthera leo)

Adams

Vuuren

Bosman

et al. 2011

South African Journal of Wildlife Research

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Feline immunodeficiency virus is a retrovirus of domestic cats that causes immunosuppressive disease and lifelong infection. Lentivirus has also been detected in African lions (Panthera leo). The lentivirus infecting lions in southern Africa has never been isolated; thus, knowledge about its molecular characteristics in these populations is limited. Our investigation used whole blood samples collected opportunistically from free-ranging southern African lions in Kruger National Park, South Africa, and from Hlane Royal National Park in Swaziland to analyse the lentivirus. Whole blood samples from captive exotic felids from zoos in South Africa and the United States, and from domestic cats in South Africa were analysed for comparison. A nested polymerase chain reaction (PCR) assay was used to amplify a portion of the proviral DNA encoding the reverse transcriptase. The nucleotide sequence of all products was determined and examined. The PCR assay was successful in amplifying lion lentivirus, with 52 positive and 65 negative samples. Of the 34 sequences amplified from a variety of felids, six showed an average of 96% homology to domestic feline lentivirus, and 28 showed an average of 94% homology to lion lentivirus. In addition, domestic cat lentivirus nucleic acid was amplified from a captive tiger, demonstrating the possibility of cross-species transmission.

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Puma Lentivirus Is Controlled in Domestic Cats after Mucosal Exposure in the Absence of Conventional Indicators of Immunity

Cited by 28 publications

References 50 publications

Variability in assays used for detection of lentiviral infection in bobcats (Lynx rufus), pumas (Puma concolor), and ocelots (Leopardus pardalis)

Variability in assays used for detection of lentiviral infection in bobcats (Lynx rufus), pumas (Puma concolor), and ocelots (Leopardus pardalis)

The molecular biology and evolution of feline immunodeficiency viruses of cougars

Detection and Genetic Analysis of Feline Immunodeficiency Virus (FIVple) in Southern African Lions (Panthera leo)

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