![T-cell compartments and T-cell cytokine production are restored after hematopoietic stem cell transplant. (A) T-cell subsets evaluated before transplant show a decreased proportion of CD8+ T cells and increased proportion of CD4+ T cells compared with control that increase and decrease, respectively, posttransplant to proportions that are comparable to control T cells. The figure is representative of 3 independent repeats pre- and posttransplant. (B) T-cell memory subsets before transplant show an increased proportion of naive T cells (CCR7hi/CD45ROLo) and a reduced proportion of effector and effector memory T cells (CCR7lo/CD45ROhi and CCR7lo/CD45ROlo). (C) Cytokine secretion (interferon-γ [IFN-γ], interleukin-2 [IL-2], and tumor necrosis factor-α [TNF-α]) in pre- and posttransplant CD8+ T cells. Graphs show percent of positive cells after staphylococcal enterotoxin B stimulation, normalized to control for each cytokine. Cells were gated on live cells, CD3+, CD4+, and CD8+ T cells, and percentage of cytokine secreting cells was determined against side scatter for each subset. Cytokine secretion was measured on 3 separate time points before transplant and at least twice posttransplant. (D) Cytokine secretion in CD4+ T cells pre- and posttransplant. Graphs show percent of positive cells after staphylococcal enterotoxin B stimulation normalized to control for each cytokine. Cells were gated on live cells, CD3+, CD4+, and CD8+ T cells, and percentage of cytokine-secreting cells was determined against side scatter for each subset. Cytokine secretion was measured on 3 separate timepoints before transplant and at least twice posttransplant. (E) TCRb repertoire was determined by high-throughput sequencing of sorted T-cell subsets (T conventional, CD8+ T cells, Treg, T follicular helper cells). Representative hierarchical tree maps show TRB repertoire diversity in patient PBMC samples after transplant. Each dot represents a unique CDR-3, and the size of each dot corresponds to the frequency of that CDR-3 in the total population of sequences obtained. Shannon’s H entropy index measures the diversity of the repertoire, taking into account the clonal size distribution in the overall repertoire, and is indicated below each tree map.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/138/19/10.1182_blood.2021011005/4/bloodbld2021011005f2.png?Expires=1724818989&Signature=rKQRQYwNR6yy97F7CieJSPWrBZu9EbhqESpHrn6Uy2kFgF5UBN9UKqKMXJT6gG6LEvt9U~bPHDboAND7nqiWao76ITg2aMdTk4cpC7fx2ti01l2GOKTRKxCgQQEfjRTm6l4jOkGgvnkqXbO4tWvf8XbGPE4WMbJmrjdsimTvZ2U6CJ8cBRZFOgZi6ww7tYezzdTdquwTIjuDhwmPwDizoVIm1a4~WGYspjt0jVHrAF9WHCwRvEIpnX~1GpSQqpeuRdIvTyHGJLXCtkhMoLDlNdmVh4R388t0CGyAXOTcQmaED3bW3~Bww6J9jCNlrH17ng4QxV7rEot~U34f6Ro7TQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
T-cell compartments and T-cell cytokine production are restored after hematopoietic stem cell transplant. (A) T-cell subsets evaluated before transplant show a decreased proportion of CD8+ T cells and increased proportion of CD4+ T cells compared with control that increase and decrease, respectively, posttransplant to proportions that are comparable to control T cells. The figure is representative of 3 independent repeats pre- and posttransplant. (B) T-cell memory subsets before transplant show an increased proportion of naive T cells (CCR7hi/CD45ROLo) and a reduced proportion of effector and effector memory T cells (CCR7lo/CD45ROhi and CCR7lo/CD45ROlo). (C) Cytokine secretion (interferon-γ [IFN-γ], interleukin-2 [IL-2], and tumor necrosis factor-α [TNF-α]) in pre- and posttransplant CD8+ T cells. Graphs show percent of positive cells after staphylococcal enterotoxin B stimulation, normalized to control for each cytokine. Cells were gated on live cells, CD3+, CD4+, and CD8+ T cells, and percentage of cytokine secreting cells was determined against side scatter for each subset. Cytokine secretion was measured on 3 separate time points before transplant and at least twice posttransplant. (D) Cytokine secretion in CD4+ T cells pre- and posttransplant. Graphs show percent of positive cells after staphylococcal enterotoxin B stimulation normalized to control for each cytokine. Cells were gated on live cells, CD3+, CD4+, and CD8+ T cells, and percentage of cytokine-secreting cells was determined against side scatter for each subset. Cytokine secretion was measured on 3 separate timepoints before transplant and at least twice posttransplant. (E) TCRb repertoire was determined by high-throughput sequencing of sorted T-cell subsets (T conventional, CD8+ T cells, Treg, T follicular helper cells). Representative hierarchical tree maps show TRB repertoire diversity in patient PBMC samples after transplant. Each dot represents a unique CDR-3, and the size of each dot corresponds to the frequency of that CDR-3 in the total population of sequences obtained. Shannon’s H entropy index measures the diversity of the repertoire, taking into account the clonal size distribution in the overall repertoire, and is indicated below each tree map.