Your search keyword '"S. Wyatt"' showing total 7 results

1. Immunogenicity in Macaques of the Clinical Product for a Clade B DNA/MVA HIV Vaccine: Elicitation of IFN-γ, IL-2, and TNF-α Coproducing CD4 and CD8 T Cells

Author

Tianwei Yu, Linda S. Wyatt, Lakshmi Chennareddi, Bernard Moss, Harriet L. Robinson, David C. Montefiori, Sunita Sharma, Sunil Kannanganat, Rama Rao Amara, Lilin Lai, and Jun Zhao

Subjects

CD4-Positive T-Lymphocytes, Interleukin 2, Modified vaccinia Ankara, viruses, medicine.medical_treatment, Immunology, Priming (immunology), CD8-Positive T-Lymphocytes, Biology, Interferon-gamma, Virology, Vaccines, DNA, medicine, Animals, Cytotoxic T cell, Interferon gamma, HIV vaccine, AIDS Vaccines, Tumor Necrosis Factor-alpha, Immunogenicity, Infectious Diseases, Cytokine, Cytokines, Interleukin-2, Macaca, medicine.drug

Abstract

The clinical product for a clade B HIV DNA/MVA vaccine expressing Gag, Pol, and Env has been tested for immunogenicity in macaques. Responding T cells were at the threshold for detection following DNA priming at weeks 0 and 8 but underwent sharp expansions and contractions following MVA boosting at weeks 16 and 24. Both CD4 and CD8 T cell responses had high frequencies of cytokine coproducing cells with >50% of the memory cells coproducing multiple cytokines including IL-2. The highest responses were elicited to Gag, followed by Env and then Pol. In two of six macaques, the vaccine also elicited low levels of neutralizing Ab for easy to neutralize clade B isolates.

Published

2007

2. Short Communication: Studies in Macaques on Cross-Clade T Cell Responses Elicited by a DNA/MVA AIDS Vaccine, Better Conservation of CD8 Than CD4 T Cell Responses

Author

Harold M. McClure, Bernard Moss, Linda S. Wyatt, Harriet L. Robinson, Sunita Sharma, Lakshmi Chennareddi, Sal Butera, Janet M. McNicholl, James M. Smith, James G. Herndon, Dennis Ellenberger, Bin Li, Milloni Patel, and Rama Rao Amara

Subjects

Modified vaccinia Ankara, Cellular immunity, T cell, Immunology, Priming (immunology), Biology, Virology, Virus, law.invention, Infectious Diseases, medicine.anatomical_structure, law, Recombinant DNA, medicine, HIV vaccine, CD8

Abstract

One of the unknowns faced by an HIV/AIDS vaccine is the ability of a single clade vaccine to protect against the multiple genetic subtypes and recombinant forms of HIV-1 present in the current pandemic. Here, we use a macaque model to investigate the ability of our clade B vaccine that consists of DNA priming and modified vaccinia Ankara (MVA) virus boosting to elicit T cell responses that recognize an A/G recombinant of HIV- 1. To test for cross-reactive T cells, intracellular cytokine staining was conducted using five pools of Gag and six pools of Env peptides representing B or A/G sequences. Studies using the peptide pools revealed essentially complete conservation of the CD8 response but only ∼50% conservation of the CD4 response. Thus, the ability of an HIV vaccine for one clade to protect against other clades may be more limited by the ability to provide CD4 T cell help than the ability to elicit CD8 effector functions.

Published

2005

3. DNA/MVA Vaccine for HIV Type 1: Effects of Codon-Optimization and the Expression of Aggregates or Virus-Like Particles on the Immunogenicity of the DNA Prime

Author

Lakshmi Chennareddi, Milloni Patel, Harriet L. Robinson, Sunita Sharma, Bernard Moss, Yan Xu, James M. Smith, David Campbell, Dennis Ellenberger, Harold M. McClure, Linda S. Wyatt, Salvatore T. Butera, Hong Yi, James G. Herndon, David C. Montefiori, and Rama Rao Amara

Subjects

Modified vaccinia Ankara, viruses, Immunology, HIV Infections, Booster dose, Genes, env, complex mixtures, Virus, chemistry.chemical_compound, Virus-like particle, Virology, Vaccines, DNA, Animals, HIV vaccine, Codon, AIDS Vaccines, biology, Immunogenicity, Vaccination, virus diseases, biology.organism_classification, Genes, gag, Genes, pol, Macaca mulatta, Infectious Diseases, chemistry, Lentivirus, HIV-1, DNA

Abstract

Recently, a vaccine consisting of DNA priming followed by boosting with modified vaccinia Ankara (MVA) has provided long-term protection of rhesus macaques against a virulent challenge with a chimera of simian and human immunodeficiency viruses. Here, we report studies on the development of the DNA component for a DNA/MVA HIV vaccine for humans. Specifically, we assess the ability of a codon-optimized Gag-expressing DNA and two noncodon-optimized Gag-Pol-Env-expressing DNAs to prime the MVA booster dose. The codon-optimized DNA expressed virus-like particles (VLPs), whereas one of the noncodon-optimized DNAs expressed VLPs and the other expressed aggregates of HIV proteins. The MVA boost expressed Gag-Pol and Env and produced VLPs. Immunogenicity studies in macaques used one intramuscular prime with 600 microg of DNA and two intramuscular boosts with 1 x 10(8) pfu of MVA at weeks 8 and 30. The codon-optimized and noncodon-optimized DNAs proved similar in their ability to prime anti-Gag T cell responses. The aggregate and VLP-expressing Gag-Pol-Env DNAs also showed no significant differences in their ability to prime anti-Env Ab responses. The second MVA booster dose did not increase the peak CD4 and CD8 T cell responses, but increased anti-Env Ab titers by 40- to 90-fold. MVA-only immunizations elicited 10-100 times lower frequencies of T cells and 2-4 lower titers of anti-Env Ab than the Gag-Pol-Env DNA/MVA immunizations. Based on the breadth of the T cell response and a trend toward higher titers of anti-Env Ab, we are moving forward with human trials of the noncodon-optimized VLP-expressing DNA.

Published

2004

4. Multiprotein HIV Type 1 Clade B DNA and MVA Vaccines: Construction, Expression, and Immunogenicity in Rodents of the MVA Component

Author

Harriet L. Robinson, Jin Yan Liu, Linda S. Wyatt, Patricia L. Earl, David C. Montefiori, James M. Smith, and Bernard Moss

Subjects

Genes, Viral, viruses, Immunoelectron microscopy, Guinea Pigs, Immunology, Enzyme-Linked Immunosorbent Assay, CD8-Positive T-Lymphocytes, HIV Antibodies, Genes, env, complex mixtures, Virus, DNA vaccination, law.invention, Mice, chemistry.chemical_compound, Genes, Reporter, Neutralization Tests, law, Virology, Vaccines, DNA, Animals, Point Mutation, AIDS Vaccines, Recombination, Genetic, Mice, Inbred BALB C, Vaccines, Synthetic, Integrases, biology, Immunogenicity, HIV, virus diseases, RNA-Directed DNA Polymerase, biology.organism_classification, Genes, gag, Genes, pol, Protein Structure, Tertiary, Integrase, Infectious Diseases, chemistry, Lentivirus, biology.protein, Recombinant DNA, Simian Immunodeficiency Virus, Vaccinia, Gene Deletion

Abstract

Recombinant modified vaccinia virus Ankara (MVA) expressing SIV or SHIV Gag-Pol and Env, alone or in conjunction with a related DNA vaccine, effectively controls immunodeficiency virus infections in nonhuman primates. Here we describe the construction, characterization, and immunogenicity of MVA/HIV 48, a candidate HIV-1 clade B Gag-Pol-Env vaccine. A novel transfer vector was designed to allow the incorporation of HIV genes regulated by vaccinia virus promoters together with a reporter gene into a single site in the MVA genome and to automatically delete the reporter after the initial isolation of the recombinant MVA. MVA/HIV 48 contains chimeric HIV-1 HXB-2/BH10 gag-pol sequences, a deletion of integrase, inactivating point mutations in reverse transcriptase, and HIV-1 ADA env sequences with a truncation of most of the cytoplasmic domain to enhance expression on the plasma membrane. Cells infected with MVA/HIV 48 expressed HIV proteins, which were processed to the expected size. The Env was inserted into the plasma membrane and was functional in a CCR5 coreceptor-dependent cell fusion assay. Moreover, virus-like particles were released into the medium and budding particles containing Env were visualized by immunoelectron microscopy. Rodents that were immunized with MVA/HIV 48 produced antibodies, which neutralized a heterologous HIV-MN strain, and Gag-specific CD8 T cells. In the accompanying paper, we show that MVA/HIV 48 provided efficient boosting of an HIV DNA vaccine.

Published

2004

5. Multiprotein HIV Type 1 Clade B DNA/MVA Vaccine: Construction, Safety, and Immunogenicity in Macaques

Author

Harold M. McClure, Linda S. Wyatt, Walid Heneine, Bernard Moss, Lakshmi Chennareddi, James G. Herndon, Milloni Patel, Bharat Parekh, Patricia L. Earl, James M. Smith, Dennis Ellenberger, Salvatore T. Butera, Harriet L. Robinson, Sunita Sharma, Hong Yi, and Rama Rao Amara

Subjects

CD4-Positive T-Lymphocytes, Modified vaccinia Ankara, viruses, Immunology, Immunization, Secondary, Gene Products, gag, Priming (immunology), HIV Infections, CD8-Positive T-Lymphocytes, HIV Antibodies, Biology, Genes, env, complex mixtures, Epitope, Virus, law.invention, DNA vaccination, law, Virology, Vaccines, DNA, Animals, Point Mutation, AIDS Vaccines, Recombination, Genetic, Immunogenicity, Vaccination, Gene Products, env, virus diseases, Genes, gag, Genes, pol, Macaca mulatta, HIV Reverse Transcriptase, Reverse transcriptase, Protein Structure, Tertiary, Infectious Diseases, HIV-1, Recombinant DNA, Cytokines, Simian Immunodeficiency Virus, Gene Deletion

Abstract

Recently, a simian/human immunodeficiency virus (SHIV) vaccine consisting of priming with a Gag-Pol-Env-expressing DNA and boosting with a Gag-Pol-Env-expressing recombinant modified vaccinia Ankara (rMVA) has successfully controlled a virulent SHIV challenge in a macaque model. In this, and the accompanying paper, we report on the construction and testing of a Gag-Pol-Env DNA/MVA vaccine for HIV-1/AIDS. The DNA vaccine, pGA2/JS2, expresses aggregates of Gag proteins and includes safety mutations that render it integration, reverse transcription, and packaging defective. The rMVA vaccine, MVA/HIV 48, is integration and reverse transcription defective and has a truncated Env to enhance expression on the plasma membrane. In a study in rhesus macaques, priming with pGA2/JS2 and boosting with MVA/HIV 48 raised high frequencies of T cells for Gag and Env and lower frequencies of T cells for PR, RT, and Tat. Stimulations with five peptide pools for Gag and seven peptide pools for Env revealed epitopes for cellular immune responses throughout Gag and Env. On average, CD4 T cells from the vaccinated animals recognized 7.1 peptide pools and CD8 T cells, 3.2 peptide pools. Both the height and the breadth of the elicited cellular response provide hope that this multiprotein DNA/MVA vaccine will successfully control clade B isolates of HIV-1, as well as contribute to the control of other clades and recombinant forms of HIV-1/AIDS.

Published

2004

6. Gp120-Alum Boosting of a Gag-Pol-Env DNA/MVA AIDS Vaccine: Poorer Control of a Pathogenic Viral Challenge

Author

Bernard Moss, Linda S. Wyatt, Francois Villinger, Suzan L. Buge, Hak-Ling Ma, Silvija I. Staprans, James G. Herndon, Janet M. McNicholl, Patricia L. Earl, Shawn P. O'Neil, Eddye Carter, Harriet L. Robinson, Yan Xu, David C. Montefiori, Elizabeth G. Hill, and Rama Rao Amara

Subjects

Modified vaccinia Ankara, viruses, Immunology, Simian Acquired Immunodeficiency Syndrome, Vaccinia virus, Viremia, HIV Envelope Protein gp120, Virus, law.invention, law, Virology, Vaccines, DNA, medicine, Animals, Neutralizing antibody, AIDS Vaccines, biology, Gene Products, env, virus diseases, medicine.disease, Macaca mulatta, Fusion Proteins, gag-pol, Vaccination, Infectious Diseases, Recombinant DNA, biology.protein, Simian Immunodeficiency Virus, Viral disease, Antibody

Abstract

Envelope protein immunogens may improve DNA or live-vectored HIV vaccines by complementing antiviral cellular responses with Env antibodies. We tested this concept by administering two immunizations of alum-adjuvanted HIV-1 89.6 gp120 to macaques being primed at weeks 0 and 8 with SHIV 89.6 Gag-Pol-Env DNA and boosted at week 24 with SHIV-89.6 Gag-Pol-Env recombinant modified vaccinia Ankara (MVA). Three hundred micrograms of gp120 was delivered with the second DNA prime and the MVA booster. Eight months after vaccination, all animals were challenged intrarectally with the related, yet serologically distinct, SHIV-89.6P. The gp120 immunizations raised binding, but not neutralizing antibody for the challenge virus, and allowed testing of whether gp120 vaccines that fail to raise neutralizing antibody can improve protection. Following the second gp120 immunization, the plus-gp120 group showed >10 times higher levels of binding antibody than the minus-gp120 group. These levels fell and were overall similar in both groups at the time of challenge. Following the second challenge, both groups had similar temporal patterns and heights of binding and neutralizing antibodies. However, the plus-gp120 group had less consistent control of viremia and higher levels of plasma viral RNA for the first year postchallenge. Assays for complement-dependent enhancing antibody revealed a trend toward higher levels of activity in the plus-gp120 group. This trend did not reach significance in our animal groups of 8. We conclude that gp120 inoculations that fail to raise neutralizing antibody do not improve the efficacy of Gag-Pol-Env DNA/MVA vaccines.

Published

2003

7. Studies in macaques on cross-clade T cell responses elicited by a DNA/MVA AIDS vaccine, better conservation of CD8 than CD4 T cell responses

Author

James M, Smith, Rama Rao, Amara, Linda S, Wyatt, Dennis L, Ellenberger, Bin, Li, James G, Herndon, Milloni, Patel, Sunita, Sharma, Lakshmi, Chennareddi, Sal, Butera, Janet, McNicholl, Harold M, McClure, Bernard, Moss, and Harriet L, Robinson

Subjects

AIDS Vaccines, CD4-Positive T-Lymphocytes, Vaccines, Synthetic, HIV-1, Vaccines, DNA, Animals, Macaca, Vaccinia virus, CD8-Positive T-Lymphocytes, Cross Reactions

Abstract

One of the unknowns faced by an HIV/AIDS vaccine is the ability of a single clade vaccine to protect against the multiple genetic subtypes and recombinant forms of HIV-1 present in the current pandemic. Here, we use a macaque model to investigate the ability of our clade B vaccine that consists of DNA priming and modified vaccinia Ankara (MVA) virus boosting to elicit T cell responses that recognize an A/G recombinant of HIV-1. To test for cross-reactive T cells, intracellular cytokine staining was conducted using five pools of Gag and six pools of Env peptides representing B or A/G sequences. Studies using the peptide pools revealed essentially complete conservation of the CD8 response but only approximately 50% conservation of the CD4 response. Thus, the ability of an HIV vaccine for one clade to protect against other clades may be more limited by the ability to provide CD4 T cell help than the ability to elicit CD8 effector functions.

Published

2005