Abstract

Immunological memory is characterized by the ability of the immune system to respond specifically and more rapidly upon a subsequent encounter with a pathogen or antigen. This specific and rapid recall response defines the basis for vaccination whose goal it is to induce long-term protective immunity. The memory T cell population is very heterogeneous, and whose number, tissue location, and fitness can greatly impacttheir ability to protect against re-infection. It is clear that multiple factors are important for the initial T cell priming but what are less clear are the effects different vaccine vectors and routes of immunization have on the development of T cell memory. To address this we have compared CD8 T cell memory generated after DNA vaccination or influenza infection with LCMV viral infection. We previously have found that DNA vaccine vectors delivered via intramuscular injection produce lesser quality memory CD8 T cells compared to LCMV infection. We have extended our study address if different DNA delivery mechanisms, in this case electroporation combined with intramuscular injection, can have a greater impact on the quality of the resulting CD8 T cell memory. Compared to intramuscular injection alone electroporation resulted in a 2-fold higher number of antigen-specific memory CD8 T cells. However our preliminary results suggest thatanalogous to our previous studies the DNA memory CD8 T cells were suboptimal compared to those generated after LCMV infection. Influenza viruses remain one of the most medically important pathogens, which cause significant morbidity and mortality annually. Using DNA microarrays we compared the gene expression profiles of memory CD8 T cells generated after intranasal influenza infection with those generated after a systemic LCMV infection. Interestingly we found very little differences in the geneexpression profiles. The influenza memory cells showed a decrease in IFN-? and IL-2 gene expression, and an increase in a number of genes involved in the negative regulation of cell cycle. These findings may partially explain why influenza memory cells are suboptimal compared to LCMV memory cells. Our data demonstrates that the programming of memory CD8 T cells by both DNA and influenza may not be optimaland importantly for vaccine development clearly demonstrates that different vaccine vectors can generate different quality memory cells.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Specialized Center--Cooperative Agreements (U54)
Project #
3U54AI057157-06S1
Application #
7652151
Study Section
Special Emphasis Panel (ZAI1-NBS-M (M2))
Project Start
2008-03-15
Project End
2009-02-28
Budget Start
2008-03-15
Budget End
2009-02-28
Support Year
6
Fiscal Year
2008
Total Cost
$328,259
Indirect Cost

  Institution

Name
University of North Carolina Chapel Hill
Department
Type
DUNS #
608195277
City
Chapel Hill
State
NC
Country
United States
Zip Code
27599

  Publications

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Graham, Rachel L; Deming, Damon J; Deming, Meagan E et al. (2018) Evaluation of a recombination-resistant coronavirus as a broadly applicable, rapidly implementable vaccine platform. Commun Biol 1:179
Qi, Xiaoxuan; Wang, Wenjian; Dong, Haohao et al. (2018) Expression and X-Ray Structural Determination of the Nucleoprotein of Lassa Fever Virus. Methods Mol Biol 1604:179-188
Kocher, Jacob F; Lindesmith, Lisa C; Debbink, Kari et al. (2018) Bat Caliciviruses and Human Noroviruses Are Antigenically Similar and Have Overlapping Histo-Blood Group Antigen Binding Profiles. MBio 9:
Dhanwani, Rekha; Huang, Qinfeng; Lan, Shuiyun et al. (2018) Establishment of Bisegmented and Trisegmented Reverse Genetics Systems to Generate Recombinant Pichindé Viruses. Methods Mol Biol 1604:247-253
Shao, Junjie; Liu, Xiaoying; Liang, Yuying et al. (2018) Assays to Assess Arenaviral Glycoprotein Function. Methods Mol Biol 1604:169-178
Huang, Qinfeng; Shao, Junjie; Liang, Yuying et al. (2018) Assays to Demonstrate the Roles of Arenaviral Nucleoproteins (NPs) in Viral RNA Synthesis and in Suppressing Type I Interferon. Methods Mol Biol 1604:189-200
Gunn, Bronwyn M; Jones, Jennifer E; Shabman, Reed S et al. (2018) Ross River virus envelope glycans contribute to disease through activation of the host complement system. Virology 515:250-260
Shao, Junjie; Liang, Yuying; Ly, Hinh (2018) Roles of Arenavirus Z Protein in Mediating Virion Budding, Viral Transcription-Inhibition and Interferon-Beta Suppression. Methods Mol Biol 1604:217-227
Wirawan, Melissa; Fibriansah, Guntur; Marzinek, Jan K et al. (2018) Mechanism of Enhanced Immature Dengue Virus Attachment to Endosomal Membrane Induced by prM Antibody. Structure :

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