Antigen-driven clonal selection shapes the persistence of HIV-1–infected CD4+ T cells in vivo
Francesco R. Simonetti, … , Janet D. Siliciano, Robert F. Siliciano
Francesco R. Simonetti, … , Janet D. Siliciano, Robert F. Siliciano
Published December 10, 2020
Citation Information: J Clin Invest. 2021;131(3):e145254. https://doi.org/10.1172/JCI145254.
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Research Article AIDS/HIV Immunology

Antigen-driven clonal selection shapes the persistence of HIV-1–infected CD4+ T cells in vivo

Abstract

Clonal expansion of infected CD4+ T cells is a major mechanism of HIV-1 persistence and a barrier to achieving a cure. Potential causes are homeostatic proliferation, effects of HIV-1 integration, and interaction with antigens. Here, we show that it is possible to link antigen responsiveness, the full proviral sequence, the integration site, and the T cell receptor β-chain (TCRβ) sequence to examine the role of recurrent antigenic exposure in maintaining the HIV-1 reservoir. We isolated CMV- and Gag-responding CD4+ T cells from 10 treated individuals. Proviral populations in CMV-responding cells were dominated by large clones, including clones harboring replication-competent proviruses. TCRβ repertoires showed high clonality driven by converging adaptive responses. Although some proviruses were in genes linked to HIV-1 persistence (BACH2, STAT5B, MKL1), the proliferation of infected cells under antigenic stimulation occurred regardless of the site of integration. Paired TCRβ and integration site analysis showed that infection could occur early or late in the course of a clone’s response to antigen and could generate infected cell populations too large to be explained solely by homeostatic proliferation. Together, these findings implicate antigen-driven clonal selection as a major factor in HIV-1 persistence, a finding that will be a difficult challenge to eradication efforts.

Authors

Francesco R. Simonetti, Hao Zhang, Garshasb P. Soroosh, Jiayi Duan, Kyle Rhodehouse, Alison L. Hill, Subul A. Beg, Kevin McCormick, Hayley E. Raymond, Christopher L. Nobles, John K. Everett, Kyungyoon J. Kwon, Jennifer A. White, Jun Lai, Joseph B. Margolick, Rebecca Hoh, Steven G. Deeks, Frederic D. Bushman, Janet D. Siliciano, Robert F. Siliciano

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Figure 5

Analysis of VDJ and provirus pairs belonging to the same antigen-responding clone.

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Analysis of VDJ and provirus pairs belonging to the same antigen-respond...
(A) ddPCR design for duplex quantification of VDJ and proviral copies from gDNA of sorted cells. (B) Representative ddPCR 2D plot of duplex amplification of CASIGSSAAFF and cognate provirus integrated into the MKL1 gene. (C) Quantification of clonotypes by VDJ-specific ddPCR strongly correlated with TCRβ ImmunoSeq. Five CMV-responding clonotypes (described in D) were quantified in sorted cells responding to CMV or anti-CD3/anti-CD28 stimulation; axes represent log10 abundance. (D) log10-ranked abundance plots of CMV- of Gag-responding cells showing HIV-1–infected clonotypes for which both the VDJ rearrangement and the integration site were identified (highlighted in orange). For each pair, bar graphs show the frequency of provirus (orange) and VDJ (blue) copies in CMV-responding and nonresponding memory cells. Provirus-to-VDJ ratios were used to calculate the percentage of a given clone that was HIV-1 infected.