Early treatment and PD1 inhibition enhance HIV-specific functionality of follicular CD8+ T cells
Susanne Rueger, Eva Gruener, Danni Wang, Faiaz Shaik Abdool, Veronica Ober, Theresa Vallée, Renate Stirner, Raffaele Conca, Immanuel Andrä, Lisa Rogers, Robert Zahn, Elke Gersbacher, Joanna Eger, Ramona Pauli, Nils Postel, Christoph D. Spinner, Jörg J. Vehreschild, Melanie Stecher, Hans Nitschko, Josef Eberle, Johannes R. Bogner, Ulrich Seybold, Rika Draenert, Al Leslie, Henrik N. Kløverpris, Christof Geldmacher, Maximilian Muenchhoff, Kathrin Held, Julia Roider
Susanne Rueger, Eva Gruener, Danni Wang, Faiaz Shaik Abdool, Veronica Ober, Theresa Vallée, Renate Stirner, Raffaele Conca, Immanuel Andrä, Lisa Rogers, Robert Zahn, Elke Gersbacher, Joanna Eger, Ramona Pauli, Nils Postel, Christoph D. Spinner, Jörg J. Vehreschild, Melanie Stecher, Hans Nitschko, Josef Eberle, Johannes R. Bogner, Ulrich Seybold, Rika Draenert, Al Leslie, Henrik N. Kløverpris, Christof Geldmacher, Maximilian Muenchhoff, Kathrin Held, Julia Roider
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Research Article AIDS/HIV Immunology

Early treatment and PD1 inhibition enhance HIV-specific functionality of follicular CD8+ T cells

Abstract

People living with HIV treated during acute infection are the group for whom achieving functional cure appears most viable. Follicular CD8+ T cells could contribute to HIV reservoir clearance by accessing B cell follicles through CXCR5 expression. This study examines peripheral follicular CD8+ T cells using flow cytometry, transcriptome analyses, and functional assays in people treated during acute (n = 37) and chronic (n = 18) infection, as well as in individuals naturally controlling HIV (n = 20) and living without HIV (n = 10). Our results reveal that early, as opposed to late, treatment initiation preserves antiviral effector functions of follicular CD8+ T cells, which are further enhanced by PD1 inhibition. We also identify a correlation between follicular CD8+ T cells and intact proviral HIV DNA levels in acute, but not chronic, infection. Longitudinal transcriptomic analysis of peripheral effector cells after 48 weeks of suppressive therapy indicated traits of recent antigen exposure, suggesting potential recirculation into lymphoid tissue. These findings underscore the pivotal role of follicular CD8+ T cells in anti-HIV responses and support investigating targeted cure strategies, such as anti-PD1 therapy, especially in individuals initiating treatment during acute infection.

Authors

Susanne Rueger, Eva Gruener, Danni Wang, Faiaz Shaik Abdool, Veronica Ober, Theresa Vallée, Renate Stirner, Raffaele Conca, Immanuel Andrä, Lisa Rogers, Robert Zahn, Elke Gersbacher, Joanna Eger, Ramona Pauli, Nils Postel, Christoph D. Spinner, Jörg J. Vehreschild, Melanie Stecher, Hans Nitschko, Josef Eberle, Johannes R. Bogner, Ulrich Seybold, Rika Draenert, Al Leslie, Henrik N. Kløverpris, Christof Geldmacher, Maximilian Muenchhoff, Kathrin Held, Julia Roider

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Figure 3

CXCR5+CD8+ T cell localization in tonsils and their distinct transcriptomic profile in circulation compared with CXCR5CD8+ T cells.

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CXCR5+CD8+ T cell localization in tonsils and their distinct transcripto...
(AC) Immunofluorescence microscopy of tonsil tissue from participants LWH: viremic (A) and aviremic participant on ART (B) and an individual naturally controlling HIV (C). VL, viral load; cp, copies. Whole tonsil tissue sections were stained, and GCs identified (white dotted circles). Inserts represent zoomed into areas of GCs (white rectangles). Orange, CXCR5; pink, CD8; green, HIV p24; blue, DAPI/nuclear counterstain. Original magnification, ×40. Scale bars: 100 μm, 10 μm (insets), and 5 μm (zoomed-in insets). See Supplemental Figure 3C for the isotype control staining. (D) Heatmap of selected differentially expressed genes (DEGs) in CXCR5+CD8+ versus CXCR5CD8+ T cells from people LWH (n = 13; max 4 weeks on ART) categorized in functional gene groups. Relative changes in gene expression between CXCR5+CD8+ and CXCR5CD8+ T cells are depicted. Normalized read counts, calculated with DESeq2, were converted into z scores and mean z scores of all analyzed individuals per gene per CXCR5+ and CXCR5 cell types are plotted. Plotted DEGs were selected based on their function. Red indicates higher and blue lower expression. (E) Enriched GO terms (biological process) from significantly DEGs that are downregulated (left, blue background) and upregulated (right, red background) in CXCR5+CD8+ T cells compared with their CXCR5 counterparts (BH-adjusted P values < 1 × 10–4). The line length represents the ratio of the number of genes that are part of the pathway differentially expressed between cell types to the total number of genes differentially expressed between cell types. Dot size represents the absolute observed number of DEGs in CXCR5+CD8+ versus CXCR5CD8+ T cells per pathway. Line and dot color code is according to the adjusted P value.