Exosomal Tat protein activates latent HIV-1 in primary, resting CD4+ T lymphocytes
Xiaoli Tang, Huafei Lu, Mark Dooner, Stacey Chapman, Peter J. Quesenberry, Bharat Ramratnam
Xiaoli Tang, Huafei Lu, Mark Dooner, Stacey Chapman, Peter J. Quesenberry, Bharat Ramratnam
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Research Article AIDS/HIV Infectious disease

Exosomal Tat protein activates latent HIV-1 in primary, resting CD4+ T lymphocytes

Abstract

Replication competent HIV-1 persists in a subpopulation of CD4+ T lymphocytes despite prolonged antiretroviral treatment. This residual reservoir of infected cells harbors transcriptionally silent provirus capable of reigniting productive infection upon discontinuation of antiretroviral therapy. Certain classes of drugs can activate latent virus but not at levels that lead to reductions in HIV-1 reservoir size in vivo. Here, we show the utility of CD4+ receptor targeting exosomes as an HIV-1 latency reversal agent (LRA). We engineered human cellular exosomes to express HIV-1 Tat, a protein that is a potent transactivator of viral transcription. Preparations of exosomal Tat-activated HIV-1 in primary, resting CD4+ T lymphocytes isolated from antiretroviral-treated individuals with prolonged periods of viral suppression and led to the production of replication competent HIV-1. Furthermore, exosomal Tat increased the potency of selected LRA by over 30-fold in terms of HIV-1 mRNA expression, thereby establishing it as a potentially new class of biologic product with possible combinatorial utility in targeting latent HIV-1.

Authors

Xiaoli Tang, Huafei Lu, Mark Dooner, Stacey Chapman, Peter J. Quesenberry, Bharat Ramratnam

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Figure 5

EXO-Tat exosomes reactivate latent HIV-1 ex vivo in resting CD4+ (rCD4+) T cells.

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EXO-Tat exosomes reactivate latent HIV-1 ex vivo in resting CD4+ (rCD4+)...
rCD4+ T cells were isolated from the PBMCs of ART-treated patient blood. Two million rCD4+ T cells were treated with control exosomes (Exo-C), EXO-Tat exosomes (EXO-Tat), panobinostat (Pan), disulfiram (Dis), or PMA/I as indicated for 4 days. The cells and supernatants were separated by centrifugation. HIV-1 mRNA was determined by qPCR. P24 concentration in the supernatants was measured by ELISA. (A) EXO-Tat exosomes reactivated latent HIV-1 and increased its mRNA expression in cells. (B) EXO-Tat exosomes increased the release of HIV-1 mRNA into culture medium as detected by qPCR. (C and D) Comparison of the latency reversing potency of EXO-Tat exosomes with Pan or Dis. EXO-Tat exosomes synergistic effect with Pan or Dis, increasing HIV-1 mRNA expression in cells (C) or in supernatants (D). (E) EXO-Tat reactivated replication competent HIV-1 as measured by p24 concentration in the supernatants of 3/6 patient samples. The lowest limit of p24 quantification is 0.0075 pg/ml. Quantitative data was analyzed by ANOVA with between-group comparisons evaluated with post-hoc Tukey-Kramer HSD tests, which correct for multiple comparison. Data are expressed as mean ± SEM. P < 0.05 indicates statistical significance.