Expression and reactivation of HIV in a chemokine induced model of HIV latency in primary resting CD4+ T cells

BACKGROUND: We recently described that HIV latent infection can be established in vitro following incubation of resting CD4+ T-cells with chemokines that bind to CCR7. The main aim of this study was to fully define the post-integration blocks to virus replication in this model of CCL19-induced HIV l...

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Autores principales: Saleh, Suha, Wightman, Fiona, Ramanayake, Saumya, Alexander, Marina, Kumar, Nitasha, Khoury, Gabriela, Pereira, Cândida, Purcell, Damian, Cameron, Paul U, Lewin, Sharon R
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2011
Materias:
Research
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3215964/
https://www.ncbi.nlm.nih.gov/pubmed/21992606
http://dx.doi.org/10.1186/1742-4690-8-80
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author Saleh, Suha
Wightman, Fiona
Ramanayake, Saumya
Alexander, Marina
Kumar, Nitasha
Khoury, Gabriela
Pereira, Cândida
Purcell, Damian
Cameron, Paul U
Lewin, Sharon R
author_facet Saleh, Suha
Wightman, Fiona
Ramanayake, Saumya
Alexander, Marina
Kumar, Nitasha
Khoury, Gabriela
Pereira, Cândida
Purcell, Damian
Cameron, Paul U
Lewin, Sharon R
author_sort Saleh, Suha
collection PubMed
description BACKGROUND: We recently described that HIV latent infection can be established in vitro following incubation of resting CD4+ T-cells with chemokines that bind to CCR7. The main aim of this study was to fully define the post-integration blocks to virus replication in this model of CCL19-induced HIV latency. RESULTS: High levels of integrated HIV DNA but low production of reverse transcriptase (RT) was found in CCL19-treated CD4+ T-cells infected with either wild type (WT) NL4.3 or single round envelope deleted NL4.3 pseudotyped virus (NL4.3- Δenv). Supernatants from CCL19-treated cells infected with either WT NL4.3 or NL4.3- Δenv did not induce luciferase expression in TZM-bl cells, and there was no expression of intracellular p24. Following infection of CCL19-treated CD4+ T-cells with NL4.3 with enhanced green fluorescent protein (EGFP) inserted into the nef open reading frame (NL4.3- Δnef-EGFP), there was no EGFP expression detected. These data are consistent with non-productive latent infection of CCL19-treated infected CD4+ T-cells. Treatment of cells with phytohemagluttinin (PHA)/IL-2 or CCL19, prior to infection with WT NL4.3, resulted in a mean fold change in unspliced (US) RNA at day 4 compared to day 0 of 21.2 and 1.1 respectively (p = 0.01; n = 5), and the mean expression of multiply spliced (MS) RNA was 56,000, and 5,000 copies/million cells respectively (p = 0.01; n = 5). In CCL19-treated infected CD4+ T-cells, MS-RNA was detected in the nucleus and not in the cytoplasm; in contrast to PHA/IL-2 activated infected cells where MS RNA was detected in both. Virus could be recovered from CCL19-treated infected CD4+ T-cells following mitogen stimulation (with PHA and phorbyl myristate acetate (PMA)) as well as TNFα, IL-7, prostratin and vorinostat. CONCLUSIONS: In this model of CCL19-induced HIV latency, we demonstrate HIV integration without spontaneous production of infectious virus, detection of MS RNA in the nucleus only, and the induction of virus production with multiple activating stimuli. These data are consistent with ex vivo findings from latently infected CD4+ T-cells from patients on combination antiretroviral therapy, and therefore provide further support of this model as an excellent in vitro model of HIV latency.
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spelling pubmed-32159642011-11-16 Expression and reactivation of HIV in a chemokine induced model of HIV latency in primary resting CD4+ T cells Saleh, Suha Wightman, Fiona Ramanayake, Saumya Alexander, Marina Kumar, Nitasha Khoury, Gabriela Pereira, Cândida Purcell, Damian Cameron, Paul U Lewin, Sharon R Retrovirology Research BACKGROUND: We recently described that HIV latent infection can be established in vitro following incubation of resting CD4+ T-cells with chemokines that bind to CCR7. The main aim of this study was to fully define the post-integration blocks to virus replication in this model of CCL19-induced HIV latency. RESULTS: High levels of integrated HIV DNA but low production of reverse transcriptase (RT) was found in CCL19-treated CD4+ T-cells infected with either wild type (WT) NL4.3 or single round envelope deleted NL4.3 pseudotyped virus (NL4.3- Δenv). Supernatants from CCL19-treated cells infected with either WT NL4.3 or NL4.3- Δenv did not induce luciferase expression in TZM-bl cells, and there was no expression of intracellular p24. Following infection of CCL19-treated CD4+ T-cells with NL4.3 with enhanced green fluorescent protein (EGFP) inserted into the nef open reading frame (NL4.3- Δnef-EGFP), there was no EGFP expression detected. These data are consistent with non-productive latent infection of CCL19-treated infected CD4+ T-cells. Treatment of cells with phytohemagluttinin (PHA)/IL-2 or CCL19, prior to infection with WT NL4.3, resulted in a mean fold change in unspliced (US) RNA at day 4 compared to day 0 of 21.2 and 1.1 respectively (p = 0.01; n = 5), and the mean expression of multiply spliced (MS) RNA was 56,000, and 5,000 copies/million cells respectively (p = 0.01; n = 5). In CCL19-treated infected CD4+ T-cells, MS-RNA was detected in the nucleus and not in the cytoplasm; in contrast to PHA/IL-2 activated infected cells where MS RNA was detected in both. Virus could be recovered from CCL19-treated infected CD4+ T-cells following mitogen stimulation (with PHA and phorbyl myristate acetate (PMA)) as well as TNFα, IL-7, prostratin and vorinostat. CONCLUSIONS: In this model of CCL19-induced HIV latency, we demonstrate HIV integration without spontaneous production of infectious virus, detection of MS RNA in the nucleus only, and the induction of virus production with multiple activating stimuli. These data are consistent with ex vivo findings from latently infected CD4+ T-cells from patients on combination antiretroviral therapy, and therefore provide further support of this model as an excellent in vitro model of HIV latency. BioMed Central 2011-10-12 /pmc/articles/PMC3215964/ /pubmed/21992606 http://dx.doi.org/10.1186/1742-4690-8-80 Text en Copyright ©2011 Saleh et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research
Saleh, Suha
Wightman, Fiona
Ramanayake, Saumya
Alexander, Marina
Kumar, Nitasha
Khoury, Gabriela
Pereira, Cândida
Purcell, Damian
Cameron, Paul U
Lewin, Sharon R
Expression and reactivation of HIV in a chemokine induced model of HIV latency in primary resting CD4+ T cells
title Expression and reactivation of HIV in a chemokine induced model of HIV latency in primary resting CD4+ T cells
title_full Expression and reactivation of HIV in a chemokine induced model of HIV latency in primary resting CD4+ T cells
title_fullStr Expression and reactivation of HIV in a chemokine induced model of HIV latency in primary resting CD4+ T cells
title_full_unstemmed Expression and reactivation of HIV in a chemokine induced model of HIV latency in primary resting CD4+ T cells
title_short Expression and reactivation of HIV in a chemokine induced model of HIV latency in primary resting CD4+ T cells
title_sort expression and reactivation of hiv in a chemokine induced model of hiv latency in primary resting cd4+ t cells
topic Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3215964/
https://www.ncbi.nlm.nih.gov/pubmed/21992606
http://dx.doi.org/10.1186/1742-4690-8-80
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