Vaccinia Virus H3L Envelope Protein Is a Major Target of Neutralizing Antibodies in Humans and Elicits Protection against Lethal Challenge in Mice

Davies, D. Huw; McCausland, Megan; Valdez, Conrad; Huynh, Devan; Hernandez, Jenny E.; Mu, Yunxiang; Hirst, Siddiqua; Villarreal, Luis P.; Felgner, Philip L.; Crotty, Shane

doi:10.1128/jvi.79.18.11724-11733.2005

Cited by 194 publications

(223 citation statements)

References 67 publications

(90 reference statements)

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“…H3L was strongly recognized by subjects 2 and 10. This protein induces neutralizing Abs (49,72). H3L 229 -237 (ILDNAAKYV) accounted for ϳ7% of reactivity to whole virus (Fig.…”

Section: Discussionmentioning

confidence: 99%

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Dominance and Diversity in the Primary Human CD4 T Cell Response to Replication-Competent Vaccinia Virus

Jing¹,

Chong

Byrd³

et al. 2007

The Journal of Immunology

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Vaccination with replication-competent vaccinia protects against heterologous orthopoxvirus challenge. CD4 T cells have essential roles helping functionally important Ab and CD8 antiviral responses, and contribute to the durability of vaccinia-specific memory. Little is known about the specificity, diversity, or dominance hierarchy of orthopoxvirus-specific CD4 T cell responses. We interrogated vaccinia-reactive CD4 in vitro T cell lines with vaccinia protein fragments expressed from an unbiased genomic library, and also with a panel of membrane proteins. CD4 T cells from three primary vaccinees reacted with 44 separate antigenic regions in 35 vaccinia proteins, recognizing 8 to 20 proteins per person. The integrated responses to the Ags that we defined accounted for 49 to 81% of the CD4 reactivity to whole vaccinia Ag. Individual dominant Ags drove up to 30% of the total response. The gene F11L-encoded protein was immunodominant in two of three subjects and is fragmented in a replication-incompetent vaccine candidate. The presence of protein in virions was strongly associated with CD4 antigenicity. These findings are consistent with models in which exogenous Ag drives CD4 immunodominance, and provides tools to investigate the relationship between Ab and CD4 T cell specificity for complex pathogens.

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“…H3L was strongly recognized by subjects 2 and 10. This protein induces neutralizing Abs (49,72). H3L 229 -237 (ILDNAAKYV) accounted for ϳ7% of reactivity to whole virus (Fig.…”

Section: Discussionmentioning

confidence: 99%

“…Several potent vaccinia neutralizing membrane Ags have been described (38,39,(47)(48)(49). We expressed and purified three proteins (L1R, A33R, B5R) as extracellular domains and one (A27L) as a full-length construct.…”

Section: Cd4 Epitopes In Purified Neutralizing Agsmentioning

confidence: 99%

Dominance and Diversity in the Primary Human CD4 T Cell Response to Replication-Competent Vaccinia Virus

Jing¹,

Chong

Byrd³

et al. 2007

The Journal of Immunology

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“…This study represents, to the best of our knowledge, the first demonstration of the use of transcriptionally active PCR products or any linear PCR fragments as a useful high throughput tool for screening genomic sequence data to identify potential target antigens for vaccine development. Recently, proteinbased approaches have proved promising in this regard [37,38], We further show that transcriptionally active PCR products or linear PCR fragments can be immunogenic in vivo, and are capable of inducing both antibody and cellular immune responses at levels equivalent to those induced by the corresponding supercoiled plasmid DNA. Thus, a TAP-based approach allows for the relative prioritization amongst target antigens included in a high throughput genomic screening strategy on the basis of their immune reactivity.…”

Section: Discussionmentioning

confidence: 75%

Transcriptionally active PCR for antigen identification and vaccine development: In vitro genome-wide screening and in vivo immunogenicity

Regis

Dobaño

Quiñones-Olson

et al. 2008

Molecular and Biochemical Parasitology

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We have evaluated a technology called Transcriptionally Active PCR (TAP) for high throughput identification and prioritization of novel target antigens from genomic sequence data using the Plasmodium parasite, the causative agent of malaria, as a model. First, we adapted the TAP technology for the highly AT-rich Plasmodium genome, using well-characterized P. falciparum and P. yoelii antigens and a small panel of uncharacterized open reading frames from the P. falciparum genome sequence database. We demonstrated that TAP fragments encoding six wellcharacterized P. falciparum antigens and five well-characterized P. yoelii antigens could be amplified in an equivalent manner from both plasmid DNA and genomic DNA templates, and that uncharacterized open reading frames could also be amplified from genomic DNA template. Second, we showed that the in vitro expression of the TAP fragments was equivalent or superior to that of supercoiled plasmid DNA encoding the same antigen. Third, we evaluated the in vivo immunogenicity of TAP fragments encoding a subset of the model P. falciparum and P. yoelii antigens. We found that antigen-specific antibody and cellular immune responses induced by the TAP fragments in mice were equivalent or superior to those induced by the corresponding plasmid DNA vaccines. Finally, we developed and demonstrated proof-of-principle for an in vitro humoral immunoscreening assay for down-selection of novel target antigens. These data support the potential of a TAP approach for rapid high throughput functional screening and identification of potential candidate vaccine antigens from genomic sequence data.

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“…Protein microarray chips were prepared as described [48,51]. Briefly, 15 l purified rGRA1 (2.5 mg/ml) printed onto nitrocellulose-coated FAST TM glass slides (Schleicher & Schuell, Keene, NH) using an OmniGrid 100 microarray printer (Genomics Solutions, Ann Arbor, MI).…”

Section: Measurement Of Humoral Antibody Response Using Protein Micromentioning

confidence: 99%

GRA1 protein vaccine confers better immune response compared to codon-optimized GRA1 DNA vaccine

Döşkaya

Kalantari-Dehaghi

Walsh

et al. 2007

Vaccine

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The present study evaluates immunogenicity and protection potency of a codon-optimized GRA1 DNA vaccine, wild type GRA1 DNA vaccine and an adjuvanted recombinant GRA1 protein vaccine candidate in BALB/c mice against lethal toxoplasmosis. Of the three GRA1 vaccines tested, the recombinant GRA1 protein vaccine results reveal significant increase in immune response and prolonged survival against acute toxoplasmosis compared to DNA vaccinations. Immune response and protection conferred by codon-optimized GRA1 DNA vaccine was slightly better than wild type GRA1 DNA vaccine.

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Vaccinia Virus H3L Envelope Protein Is a Major Target of Neutralizing Antibodies in Humans and Elicits Protection against Lethal Challenge in Mice

Cited by 194 publications

References 67 publications

Dominance and Diversity in the Primary Human CD4 T Cell Response to Replication-Competent Vaccinia Virus

Dominance and Diversity in the Primary Human CD4 T Cell Response to Replication-Competent Vaccinia Virus

Transcriptionally active PCR for antigen identification and vaccine development: In vitro genome-wide screening and in vivo immunogenicity

GRA1 protein vaccine confers better immune response compared to codon-optimized GRA1 DNA vaccine

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