Latency reversal agents affect differently the latent reservoir present in distinct CD4+ t subpopulations

Latency reversal agents (LRAs) have proven to induce HIV-1 transcription in vivo but are ineffective at decreasing the size of the latent reservoir in antiretroviral treated patients. The capacity of the LRAs to perturb the viral reservoir present in distinct subpopulations of cells is currently unk...

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Detalles Bibliográficos
Autores: Grau Expósito, Judith|||0000-0001-9350-2429, Luque-Ballesteros, Laura|||0000-0001-9515-5889, Navarro, Jordi|||0000-0002-7187-0367, Curran, Adrian|||0000-0002-1263-0814, Burgos, Joaquín|||0000-0001-8445-3047, Ribera, Esteban|||0000-0002-3752-8808, Torrella Domingo, Adriana|||0000-0003-1848-5096, Planas, Bibiana|||0000-0002-1490-7127, Badía, Rosa|||0000-0002-8222-5697, Martin-Castillo, Mario, Fernández-Sojo, Jesús, Genescà Ferrer, Meritxell|||0000-0001-6413-3812, Falcó, Vicenç|||0000-0001-9626-0023, Buzón, Maria José|||0000-0003-4427-9413
Tipo de recurso: artículo
Fecha de publicación:2019
País:España
Institución:Universitat Autònoma de Barcelona
Repositorio:Dipòsit Digital de Documents de la UAB
Idioma:inglés
OAI Identifier:oai:ddd.uab.cat:223700
Acceso en línea:https://ddd.uab.cat/record/223700
https://dx.doi.org/urn:doi:10.1371/journal.ppat.1007991
Access Level:acceso abierto
Palabra clave:Anti-HIV Agents
CD4-Positive T-Lymphocytes
Depsipeptides
Diterpenes
HIV Infections
HIV-1
Humans
Viral Load
Virus Activation
Virus Latency
Descripción
Sumario:Latency reversal agents (LRAs) have proven to induce HIV-1 transcription in vivo but are ineffective at decreasing the size of the latent reservoir in antiretroviral treated patients. The capacity of the LRAs to perturb the viral reservoir present in distinct subpopulations of cells is currently unknown. Here, using a new RNA FISH/flow ex vivo viral reactivation assay, we performed a comprehensive assessment of the viral reactivation capacity of different families of LRAs, and their combinations, in different CD4 T cell subsets. We observed that a median of 16.28% of the whole HIV-reservoir induced HIV-1 transcripts after viral reactivation, but only 10.10% of these HIV-1 RNA cells produced the viral protein p24. Moreover, none of the LRAs were powerful enough to reactivate HIV-1 transcription in all CD4 T cell subpopulations. For instance, the combination of Romidepsin and Ingenol was identified as the best combination of drugs at increasing the proportion of HIV-1 RNA cells, in most, but not all, CD4 T cell subsets. Importantly, memory stem cells were identified as highly resistant to HIV-1 reactivation, and only the combination of Panobinostat and Bryostatin-1 significantly increased the number of cells transcribing HIV within this subset. Overall, our results validate the use of the RNA FISH/flow technique to assess the potency of LRAs among different CD4 T cell subsets, manifest the intrinsic differences between cells that encompass the latent HIV reservoir, and highlight the difficulty to significantly impact the latent infection with the currently available drugs. Thus, our results have important implications for the rational design of therapies aimed at reversing HIV latency from diverse cellular reservoirs.