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Biodistribution and immunity of adenovirus 5/35 and modified vaccinia Ankara vector vaccines against human immunodeficiency virus 1 clade C
in
Adenoviruses
/ Alanine transaminase
/ Animal models
/ Aspartate aminotransferase
/ Biodistribution
/ Dendritic cells
/ Gag protein
/ HIV
/ Human immunodeficiency virus
/ Immune system
/ Immunity
/ Tropism
/ Vaccines
/ Vaccinia
/ γ-Interferon
2022
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Biodistribution and immunity of adenovirus 5/35 and modified vaccinia Ankara vector vaccines against human immunodeficiency virus 1 clade C
by
in
Adenoviruses
/ Alanine transaminase
/ Animal models
/ Aspartate aminotransferase
/ Biodistribution
/ Dendritic cells
/ Gag protein
/ HIV
/ Human immunodeficiency virus
/ Immune system
/ Immunity
/ Tropism
/ Vaccines
/ Vaccinia
/ γ-Interferon
2022
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While trying to remove the title from your shelf something went wrong :( Kindly try again later!
Do you wish to request the book?
Biodistribution and immunity of adenovirus 5/35 and modified vaccinia Ankara vector vaccines against human immunodeficiency virus 1 clade C
in
Adenoviruses
/ Alanine transaminase
/ Animal models
/ Aspartate aminotransferase
/ Biodistribution
/ Dendritic cells
/ Gag protein
/ HIV
/ Human immunodeficiency virus
/ Immune system
/ Immunity
/ Tropism
/ Vaccines
/ Vaccinia
/ γ-Interferon
2022
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Biodistribution and immunity of adenovirus 5/35 and modified vaccinia Ankara vector vaccines against human immunodeficiency virus 1 clade C
Journal Article
Biodistribution and immunity of adenovirus 5/35 and modified vaccinia Ankara vector vaccines against human immunodeficiency virus 1 clade C
2022
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Overview
Previously, we developed a chimeric adenovirus type 5 with type 35 fiber (Ad5/35), which has high tropism to dendritic cells and low hepatoxicity. For further clinical use, we constructed two recombinant vectors expressing human immunodeficiency virus 1 (HIV-1) clade C gag (Ad5/35-Cgag and MVA-Cgag). The biodistribution of the two viral vectors in a mouse model and immunity in monkeys were assessed. The mice received a single intramuscular injection with the vectors alone. The gag gene in the tissues were periodically detected using a real-time quantitative polymerase chain reaction. The distribution of Ad5/35 was also detected using an in vivo imaging system, followed by luciferase-expressing Ad5/35 administration. We found that Ad5/35-Cgag DNA and luciferase activity were detectable until 8 weeks post-administration, whereas MVA-Cgag was undetectable 72 h post-administration. Furthermore, viral administration did not increase serum aspartate aminotransferase and alanine aminotransferase levels in either mouse or monkey models. Moreover, intramuscular administration of Ad5/35-Cgag induced the gag-specific antibody level and IFNγ-secreting PBMCs, the boost with MVA-Cgag further increased the responses and lasted more than 20 weeks from the initial administration. These data demonstrate that Ad5/35 and MVA vectors are safe for in vivo use, and prime-boost with Ad5/35-MVA vaccines is suitable for clinical use against HIV-1 clade C.
Publisher
Nature Publishing Group
Subject
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