HIV-1 latency reversal agent boosting is not limited by opioid use
Tyler Lilie, … , Nina Lin, Athe Tsibris
Tyler Lilie, … , Nina Lin, Athe Tsibris
Published October 29, 2024
Citation Information: JCI Insight. 2024;9(22):e185480. https://doi.org/10.1172/jci.insight.185480.
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Research Article AIDS/HIV Immunology

HIV-1 latency reversal agent boosting is not limited by opioid use

Abstract

Opioid use may affect the HIV-1 reservoir and its reversal from latency. We studied 47 virally suppressed people with HIV (PWH) and observed that lower concentration of HIV-1 latency reversal agents (LRAs), used with small molecules that did not reverse latency, synergistically increased the magnitude of HIV-1 reactivation ex vivo, regardless of opioid use. This LRA boosting, which combined a second mitochondria-derived activator of caspases mimetic or low-dose PKC agonist with histone deacetylase inhibitors, generated more unspliced HIV-1 transcription than PMA with ionomycin (PMAi), the maximal known HIV-1 reactivator. LRA boosting associated with greater histone acetylation, modulated surface activation-induced markers, and altered T cell production of TNF-α, IL-2, and IFN-γ. HIV-1 reservoirs in PWH contained unspliced and polyadenylated virus mRNA, the ratios of which were greater in resting than total CD4+ T cells and corrected to 1:1 with PMAi exposure. We characterized treated suppressed HIV-1 infection as a period of inefficient, not absent, virus transcription. Multiply spliced HIV-1 transcripts and virion production did not consistently increase with LRA boosting, suggesting the presence of a persistent posttranscriptional block. LRA boosting can be leveraged to probe mechanisms of an effective cellular HIV-1 latency reversal program.

Authors

Tyler Lilie, Jennifer Bouzy, Archana Asundi, Jessica Taylor, Samantha Roche, Alex Olson, Kendyll Coxen, Heather Corry, Hannah Jordan, Kiera Clayton, Nina Lin, Athe Tsibris

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Figure 5

Comparative analysis of LRA boosting effects in PBMCs and CD4+ T cells.

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Comparative analysis of LRA boosting effects in PBMCs and CD4+ T cells. ...
HIV-1 unspliced caRNA levels were assessed in HEAL cohort participant samples (n = 11) during (A) low-dose bryostatin-based and (B) AZD5582-based LRA boosting combinations in PBMCs, when compared with PMAi. Data are presented as means ± SEM. Circle color denotes a given HEAL participant across figure panels. (C) Absolute HIV-1 unspliced caRNA levels in parallel PBMC and CD4+ T cell LRA exposures. PBMC and CD4 results are separated by a vertical dotted line. (D) Representation of data in C as fold-change in HIV-1 caRNA levels. (E) Corresponding HIV-1 RNA levels from culture supernatants. (F) Multiply spliced HIV-1 RNA levels as determined in a modified TILDA, comparing RMD-bryostatin combinations at 2 bryostatin concentrations and PMAi. (G) Combined OPHION and HEAL participant results (n = 47) that summarize PBMC LRA boosting responses, for LRA conditions common to both datasets. Results from OPHION participant samples, carried over from Figure 2A, are shown in gray circles. HEAL participant results are shown in color. *P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001 for Kruskal-Wallis, corrected with Dunn’s multiple-comparison test. NDC, no-drug control, contains 0.2% DMSO; R, RMD 20 nM; P, PNB 30 nM; B, bryostatin 1 nM; A, AZD5582 100 nM.