Antigen‐specific cytotoxic T lymphocytes protect against lethal West Nile virus encephalitis

Purtha, Whitney E.; Myers, Nancy B.; Mitaksov, Vesselin; Sitati, Elizabeth; Connolly, Jennifer M.; Fremont, Daved H.; Hansen, Ted H.; Diamond, Michael S.

doi:10.1002/eji.200737192

Cited by 98 publications

(131 citation statements)

References 47 publications

(65 reference statements)

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“…Intracellular IFN-γ staining was performed on splenocytes at indicated days after infection or vaccination as previously described [37,38]. Briefly, splenocytes from infected or vaccinated mice were stimulated with 1μg/ml of the WNV NS4B peptide (#33, D b -restricted, SSVWNATTAI) or WNV E peptide (#3, K b -restricted, IALTFLAV) and WNV E peptide (#28, D b -restricted, TVWRNRETL) [38,39] for four hours at 37ºC with the addition of Golgi plug ™ (1μl/ml, BD Biosciences), washed and stained with fluorescein isothiocyanate (FITC)-conjugated mAbs to CD8 or a FITC-conjugated isotype control mAb (BD Biosciences) at 4ºC for 30 minutes.…”

Section: Intracellular Ifn-γ Stainingmentioning

confidence: 99%

“…Briefly, splenocytes from infected or vaccinated mice were stimulated with 1μg/ml of the WNV NS4B peptide (#33, D b -restricted, SSVWNATTAI) or WNV E peptide (#3, K b -restricted, IALTFLAV) and WNV E peptide (#28, D b -restricted, TVWRNRETL) [38,39] for four hours at 37ºC with the addition of Golgi plug ™ (1μl/ml, BD Biosciences), washed and stained with fluorescein isothiocyanate (FITC)-conjugated mAbs to CD8 or a FITC-conjugated isotype control mAb (BD Biosciences) at 4ºC for 30 minutes. After washing and fixing with 1% PFA in PBS, cells were permeabilized with saponin and stained with an allophycocyanin (APC)-conjugated IFN-γ antibody or an isotype control (BD Biosciences) at 4ºC for 30 minutes, washed and analyzed by flow cytometry.…”

Section: Intracellular Ifn-γ Stainingmentioning

confidence: 99%

“…CD8 + T cells that are generated during WNV infection protect mice against challenge [38,39,43,44]. Prior immunization studies with live attenuated, DNA plasmid, or protein subunit vaccines against WNV have demonstrated the induction of memory T cell responses [21,25,32], although their role in protection against challenge was not evaluated.…”

Section: Vaccination Induces Antigen-specific Cd8 + T Cell Responsesmentioning

confidence: 99%

“…Prior immunization studies with live attenuated, DNA plasmid, or protein subunit vaccines against WNV have demonstrated the induction of memory T cell responses [21,25,32], although their role in protection against challenge was not evaluated. To begin to address this question, we first assessed the efficiency of induction of WNV-specific CD8 + T cells after immunzation by analyzing intracellular IFN-γ production ex vivo after antigen-specific restimulation with D b and K b -restricted WNV NS4B and E peptides [37,38]. Splenocytes were harvested from mice on day 14 or 60 after primary immunization or infection or on day 70, 10 days after boosting and the level of CD8 + T cell activation was analyzed by flow cytometry (Fig 3A).…”

Section: Vaccination Induces Antigen-specific Cd8 + T Cell Responsesmentioning

confidence: 99%

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The relative contribution of antibody and CD8+ T cells to vaccine immunity against West Nile encephalitis virus

Shrestha

Chu

et al. 2008

Vaccine

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West Nile virus (WNV) is a mosquito borne, neurotropic flavivirus that causes a severe central nervous system (CNS) infection in humans and animals. Although commercial vaccines are available for horses, none is currently approved for human use. In this study, we evaluated the efficacy and mechanism of immune protection of two candidate WNV vaccines in mice. A formalin-inactivated WNV vaccine induced higher levels of specific and neutralizing antibodies compared to a DNA plasmid vaccine that produces virus-like particles. Accordingly, partial and almost complete protection against a highly stringent lethal intracranial WNV challenge were observed in mice 60 days after single dose immunization with the DNA plasmid and inactivated virus vaccines, respectively. In mice immunized with a single dose of DNA plasmid or inactivated vaccine, antigenspecific CD8 + T cells were induced and contributed to protective immunity as acquired or genetic deficiencies of CD8 + T cells lowered the survival rates. In contrast, in boosted animals, WNVspecific antibody titers were higher, survival rates after challenge were greater, and an absence of CD8 + T cells did not appreciably affect mortality. Overall, our experiments suggest that in mice, both inactivated WNV and DNA plasmid vaccines are protective after two doses, and the specific contribution of antibody and CD8 + T cells to vaccine immunity against WNV is modulated by the prime-boost strategy.

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Section: Intracellular Ifn-γ Stainingmentioning

confidence: 99%

Section: Intracellular Ifn-γ Stainingmentioning

confidence: 99%

Section: Vaccination Induces Antigen-specific Cd8 + T Cell Responsesmentioning

confidence: 99%

Section: Vaccination Induces Antigen-specific Cd8 + T Cell Responsesmentioning

confidence: 99%

See 2 more Smart Citations

The relative contribution of antibody and CD8+ T cells to vaccine immunity against West Nile encephalitis virus

Shrestha

Chu

et al. 2008

Vaccine

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“…La réponse des lymphocytes T est donc importante pour combattre l'infection [9]. Chez la souris, il a été montré que les lymphocytes T CD4 + et CD8 + participent à l'élimination du virus en périphérie et dans le système nerveux central [28,29]. Le transfert de lymphocytes T CD8 + chez des souris défi-cientes en lymphocytes permet de contrôler l'infection par le WNV [30].…”

Section: Réponse Immunitaire Cellulaireunclassified

Infection par le virusWest Nilechez l’homme

et al. 2011

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> Depuis son émergence en 1999, le virus West Nile (WNV) est devenu la principale cause d'encépha-lite arbovirale aux États-Unis. L'infection est souvent asymptomatique mais, lorsqu'elle est cliniquement apparente, les symptômes vont d'un symptôme grippal à des désordres neurologiques plus graves pouvant parfois entraîner la mort. Les études en cours, menées en parallèle chez l'animal et chez l'homme, cherchent à comprendre la dynamique hôte-virus et les mécanismes conduisant au développement de symptômes neurologiques dans approximativement 1 % des cas. La comparaison des individus asymptomatiques et symptomatiques et l'utilisation des données disponibles pour d'autres Flavivirus ont amélioré nos connaissances et laissent espérer le déve-loppement de solutions thérapeutiques actuellement absentes et de mesures prophylactiques. C'est la synthèse de ces connaissances que nous présentons dans cette seconde partie. < Le récepteur cellulaire utilisé par le WNV à la surface des cellules cibles n'a pas encore été caractérisé mais, après s'être attaché à la surface cellulaire, le virus est internalisé dans le cytoplasme par un mécanisme qui fait intervenir la clathrine et une fusion avec les endosomes. À pH acide, l'enveloppe virale fusionne avec la membrane cellulaire de l'endosome, libérant la nucléocapside et le maté-riel génétique viral dans le cytoplasme cellulaire. La machinerie cellulaire traduit l'ARN viral dont le cadre de lecture d'environ 10,7 kb code pour une polyprotéine virale. Cette dernière est clivée au cours d'une étape post-traductionnelle et produit trois protéines de structure (C pour capside, prM pour pré-membrane et E pour enveloppe) suivies de sept protéines non structurales (NS1, NS2a, 2b, NS3, NS4a, NS4b et NS5), lesquelles participent au cycle de réplication du virus. La capside est associée au matériel génétique dans la nucléocap-side, la pré-membrane sert de protéine chaperonne pour l'enveloppe durant la maturation des virions et empêche la fusion lors de la sécrétion. L'enveloppe permet la liaison au récepteur et la fusion avec la membrane de l'endosome. Parmi les rôles potentiels des protéines non structurales, NS1 est impliquée dans la réplication de l'ARN, dans l'échappement viral [2] et la virulence [3]. NS3 participe à la maturation post-traductionnelle des protéines virales et possède une activité hélicase à ARN et nucléoside triphosphatase. NS5 a des propriétés enzymatiques importantes : c'est une polymérase ARN-dépendante de l'ARN et une méthyltransférase qui catalyse les méthylations N7 and 2'-0 de l'extrémité 5' de l'ARN viral pour former une structure Cap1 [4]. De plus, NS5 est un antagoniste de la voie

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Novel approaches and challenges to treatment of central nervous system viral infections

Nath

Tyler

2013

Annals of Neurology

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Existing and emerging viral CNS infections are major sources of human morbidity and mortality. Treatments of proven efficacy are currently limited predominantly to herpesviruses and human immunodeficiency virus. Development of new therapies has been hampered by the lack of appropriate animal model systems for some important viruses and by the difficulty in conducting human clinical trials for diseases that may be rare, or in the case of arboviral infections, often have variable seasonal and geographic incidence. Nonetheless, many novel approaches to antiviral therapy are available including candidate thiazolide and purazinecarboxamide derivatives with potential broad-spectrum antiviral efficacy. New herpesvirus drugs include viral helicase-primase and terminase inhibitors. The use of antisense oligonucleotides and other strategies to interfere with viral RNA translation has shown efficacy in experimental models of CNS viral disease. Identifying specific molecular targets within viral replication cycles has led to many existing antivirals and will undoubtedly continue to be the basis of future drug design. A promising new area of research involves therapies based on enhanced understanding of host antiviral immune responses. Toll-like receptor agonists, and drugs that inhibit specific cytokines as well as interferon preparations have all shown potential therapeutic efficacy. Passive transfer of virus-specific cytotoxic T-lymphocytes have been used in humans and may provide an effective therapies for some herpesvirus infections and potentially for progressive multifocal leukoencephalopathy. Humanized monoclonal antibodies directed against specific viral proteins have been developed and in several cases evaluated in humans in settings including West Nile virus and HIV infection and in pre-exposure prophylaxis for rabies.

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Antigen‐specific cytotoxic T lymphocytes protect against lethal West Nile virus encephalitis

Cited by 98 publications

References 47 publications

The relative contribution of antibody and CD8+ T cells to vaccine immunity against West Nile encephalitis virus

The relative contribution of antibody and CD8+ T cells to vaccine immunity against West Nile encephalitis virus

Infection par le virusWest Nilechez l’homme

Novel approaches and challenges to treatment of central nervous system viral infections

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