AI Article Synopsis

  • Identification of regulatory T cells (Treg cells) in human blood is crucial for diagnosis and therapy, but their low frequency can lead to the underestimation of their presence.
  • Transient downregulation of the Foxp3 protein in these cells can occur when they are not exposed to certain cytokines, making them difficult to detect.
  • Incubating certain T cells with IL-2, -7, or -15 significantly increases detectable Treg cell frequencies not through division but by enhancing the expression of key proteins like CD25, thus revealing previously hidden "latent" Treg cells in clinical settings.

Article Abstract

The identification of regulatory T cells (Treg cells) in human peripheral blood is an important tool in diagnosis, research, and therapeutic intervention. As compared to lymphoid tissues, the frequencies of circulating Treg cells identified as CD4 CD25 Foxp3 are, however, low. We here show that many of these cells remain undetected due to transient down regulation of Foxp3, which rapidly decays in the absence of cytokine-mediated STAT5 signals. Short-term incubation of PBMCs or isolated CD4 T cells, but not of lymph node cells, with IL-2, -7, or -15 more than doubles the frequency of Foxp3 CD25 among CD4 T cells detectable by flow cytometry. This increase is not due to cell division but to upregulation of both proteins. At the same time, the uncovered Treg cells up-regulate CD25 and down-regulate CD127, making them accessible to viable cell sorting. "Latent" Treg cells have a demethylated FOXP3 TSDR sequence, are enriched in naïve, non-cycling cells, and are functional. The confirmation of our findings in RA and SLE patients shows the feasibility of uncovering latent Treg cells for immune monitoring in clinical settings. Finally, our results suggest that unmasking of latent Treg cells contributes to the increase in circulating CD4 CD25 Foxp3 cells reported in IL-2 treated patients.

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http://dx.doi.org/10.1002/eji.201747244DOI Listing

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