Frontiers in Immunology (Apr 2025)

Repertoire-based mapping and time-tracking of T helper cell subsets in scRNA-Seq

  • Daniil K. Lukyanov,
  • Daniil K. Lukyanov,
  • Valeriia V. Kriukova,
  • Kristin Ladell,
  • Irina A. Shagina,
  • Irina A. Shagina,
  • Dmitry B. Staroverov,
  • Dmitry B. Staroverov,
  • Bella E. Minasian,
  • Anna S. Fedosova,
  • Pavel Shelyakin,
  • Oleg N. Suchalko,
  • Alexander Y. Komkov,
  • Konstantin A. Blagodatskikh,
  • Kelly L. Miners,
  • Olga V. Britanova,
  • Olga V. Britanova,
  • Olga V. Britanova,
  • Andre Franke,
  • David A. Price,
  • David A. Price,
  • Dmitry M. Chudakov,
  • Dmitry M. Chudakov,
  • Dmitry M. Chudakov,
  • Dmitry M. Chudakov,
  • Dmitry M. Chudakov

DOI
https://doi.org/10.3389/fimmu.2025.1536302
Journal volume & issue
Vol. 16

Abstract

Read online

IntroductionThe functional programs of CD4+ T helper (Th) cell clones play a central role in shaping immune responses to different challenges. While advances in single-cell RNA sequencing (scRNA-Seq) have significantly improved our understanding of the diversity of Th cells, the relationship between scRNA-Seq clusters and the traditionally characterized Th subsets remains ambiguous.MethodsIn this study, we introduce TCR-Track, a method leveraging immune repertoire data to map phenotypically sorted Th subsets onto scRNA-Seq profiles.Results and discussionThis approach accurately positions the Th1, Th1-17, Th17, Th22, Th2a, Th2, T follicular helper (Tfh), and regulatory T-cell (Treg) subsets, outperforming mapping based on CITE-Seq. Remarkably, the mapping is tightly focused on specific scRNA-Seq clusters, despite 4-year interval between subset sorting and the effector CD4+ scRNA-Seq experiment. These findings highlight the intrinsic program stability of Th clones circulating in peripheral blood. Repertoire overlap analysis at the scRNA-Seq level confirms that the circulating Th1, Th2, Th2a, Th17, Th22, and Treg subsets are clonally independent. However, a significant clonal overlap between the Th1 and cytotoxic CD4+ T-cell clusters suggests that cytotoxic CD4+ T cells differentiate from Th1 clones. In addition, this study resolves a longstanding ambiguity: we demonstrate that, while CCR10+ Th cells align with a specific Th22 scRNA-Seq cluster, CCR10−CCR6+CXCR3−CCR4+ cells, typically classified as Th17, represent a mixture of bona fide Th17 cells and clonally unrelated CCR10low Th22 cells. The clear distinction between the Th17 and Th22 subsets should influence the development of vaccine- and T-cell-based therapies. Furthermore, we show that severe acute SARS-CoV-2 infection induces systemic type 1 interferon (IFN) activation of naive Th cells. An increased proportion of effector IFN-induced Th cells is associated with a moderate course of the disease but remains low in critical COVID-19 cases. Using integrated scRNA-Seq, TCR-Track, and CITE-Seq data from 122 donors, we provide a comprehensive Th scRNA-Seq reference that should facilitate further investigation of Th subsets in fundamental and clinical studies.

Keywords