AIDS Vaccination Studies Using an Ex Vivo Feline Immunodeficiency Virus Model: Protection from an Intraclade Challenge Administered Systemically or Mucosally by an Attenuated Vaccine

Pistello, Mauro; Matteucci, Donatella; Bonci, Francesca; Isola, Patrizia; Mazzetti, Paola; Zaccaro, Lucia; Merico, Antonio; Mauro, Daniela; Flynn, Norman; Bendinelli, Mauro

doi:10.1128/jvi.77.20.10740-10750.2003

Cited by 17 publications

(23 citation statements)

References 71 publications

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“…Viremia after HIV, SIV, and FIV infection peaks early after infection and then declines to a steady-state level, presumably due to the initiation of a host immune response (19). Proviral load has been shown to follow a similar pattern in SIV and SHIV infections of monkeys (43) and in FIV infection in cats (42). PLV proviral loads were sustained throughout the 9-month study in four of four i.v.-inoculated and one of four mucosally exposed animals, but a gradual decline was noted over time, suggesting that these animals may have eventually eliminated PBMC provirus had they been monitored over a longer period of time.…”

Section: Vol 79 2005 Mucosal Lentiviral Challenge Control In Domestmentioning

confidence: 79%

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

TerWee

Yactor

Sondgeroth

et al. 2005

J Virol

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A high percentage of free-ranging pumas (Felis concolor) are infected with feline lentiviruses (puma lentivirus, feline immunodeficiency virus Pco [FIV-Pco], referred to here as PLV) without evidence of disease. PLV establishes productive infection in domestic cats following parenteral exposure but, in contrast to domestic cat FIV, it does not cause T-cell dysregulation. Here we report that cats exposed to PLV oro-nasally became infected yet rapidly cleared peripheral blood mononuclear cell (PBMC) proviral load in the absence of a correlative specific immune response. Two groups of four specific-pathogen-free cats were exposed to PLV via the mucosal (oro-nasal) or parenteral (i.v.) route. All animals were PBMC culture positive and PCR positive within 3 weeks postinfection and seroconverted without exhibiting clinical disease; however, three or four oro-nasally infected animals cleared circulating proviral DNA within 3 months. Antibody titers reached higher levels in animals that remained persistently infected. PLV antigen-induced proliferation was slightly greater in mucosally inoculated animals, but no differences were noted in cytotoxic T-lymphocyte responses or cytokine profiles between groups. The distribution of virus was predominantly gastrointestinal as opposed to lymphoid in all animals in which virus was detected at necropsy. Possible mechanisms for viral clearance include differences in viral fitness required for crossing mucosal surfaces, a threshold dose requirement for persistence, or an undetected sterilizing host immune response. This is the first report of control of a productive feline or primate lentivirus infection in postnatally exposed, seropositive animals. Mechanisms underlying this observation will provide clues to containment of immunodeficiency disease and could prompt reexamination of vaccine-induced immunity against human immunodeficiency virus and other lentiviruses.

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Section: Vol 79 2005 Mucosal Lentiviral Challenge Control In Domestmentioning

confidence: 79%

“…Clinical monitoring was not measured intensively after this time, as all cats were consistently clinically normal. Blood samples were obtained by venipuncture of the jugular or cephalic vein on study days (relative to virus exposure) Ϫ1, 3,7,10,15,22,29,35,42,49,64,79,91,107,114,135,171,184,198,233,240,247,254, and 259.…”

Section: Methodsmentioning

confidence: 99%

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

TerWee

Yactor

Sondgeroth

et al. 2005

J Virol

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“…Prior to any procedure, the animals were sedated with ketamine-diazepam intramuscularly. The challenge virus was FIV-Pet that had been consecutively passed in vivo several times and, as a result, had reacquired virulence and neutralization characteristics typical of those of wild-type FIV (53). The preparation used was pooled plasma from acutely infected SPF cats titrated in vivo, frozen in aliquots, and diluted when used to contain 10 50% cat infectious doses (CID 50 ) in 1 ml.…”

mentioning

confidence: 99%

“…FIV Env was derived from pKKS ( Fig. 1A), a replication-competent molecular clone obtained by the cloning of env of in vivo-readapted FIV-Pet (4,53) into the p34TF10 backbone (GenBank accession no. NC_001482).…”

mentioning

confidence: 99%

Env-Expressing Autologous T Lymphocytes Induce Neutralizing Antibody and Afford Marked Protection against Feline Immunodeficiency Virus

Pistello

Bonci

Zabogli

et al. 2010

J Virol

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The envelope (Env) glycoproteins of HIV and other lentiviruses possess neutralization and other protective epitopes, yet all attempts to induce protective immunity using Env as the only immunogen have either failed or afforded minimal levels of protection. In a novel prime-boost approach, specific-pathogen-free cats were primed with a plasmid expressing Env of feline immunodeficiency virus (FIV) and feline granulocyte-macrophage colony-stimulating factor and then boosted with their own T lymphocytes transduced ex vivo to produce the same Env and interleukin 15 (3 ؋ 10 6 to 10 ؋ 10 6 viable cells/cat). After the boost, the vaccinees developed elevated immune responses, including virus-neutralizing antibodies (NA). Challenge with an ex vivo preparation of FIV readily infected all eight control cats (four mock vaccinated and four naïve) and produced a marked decline in the proportion of peripheral CD4 T cells. In contrast, five of seven vaccinees showed little or no traces of infection, and the remaining two had reduced viral loads and underwent no changes in proportions of CD4 T cells. Interestingly, the viral loads of the vaccinees were inversely correlated to the titers of NA. The findings support the concept that Env is a valuable immunogen but needs to be administered in a way that permits the expression of its full protective potential.

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“…Seven-teen animals were inoculated with Petaluma (group 1), 28 with Pisa-M2 isolate (group 2), and 11 were first inoculated with Petaluma and, one year later, superinfected with Pisa-M2 (group 3). Petaluma isolate was obtained from supernatant of persistently infected FL4 cells [19], while Pisa-M2 was a local isolate propagated in vivo by monthly passages in SPF cats and never passaged in vitro [20]. Animals were inoculated intravenously with either 2 ml of freshly collected blood (Pisa-M2) or 20 cat infectious dose 50% of FL-4 supernatant (Petaluma).…”

Section: Catsmentioning

confidence: 99%

Feline Immunodeficiency Virus (FIV) Infection in Cats: A Possible Cause of Renal Pathological Changes

Tozon¹,

Pistello²,

Poli³

2012

Immunodeficiency

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AIDS Vaccination Studies Using an Ex Vivo Feline Immunodeficiency Virus Model: Protection from an Intraclade Challenge Administered Systemically or Mucosally by an Attenuated Vaccine

Cited by 17 publications

References 71 publications

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

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

Env-Expressing Autologous T Lymphocytes Induce Neutralizing Antibody and Afford Marked Protection against Feline Immunodeficiency Virus

Feline Immunodeficiency Virus (FIV) Infection in Cats: A Possible Cause of Renal Pathological Changes

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