[HTML][HTML] Prospective tracking of donor-reactive T-cell clones in the circulation and rejecting human kidney allografts
C Aschauer, K Jelencsics, K Hu, A Heinzel… - Frontiers in …, 2021 - frontiersin.org
C Aschauer, K Jelencsics, K Hu, A Heinzel, MG Gregorich, J Vetter, S Schaller, SM Winkler…
Frontiers in immunology, 2021•frontiersin.orgBackground Antigen recognition of allo-peptides and HLA molecules leads to the activation
of donor-reactive T-cells following transplantation, potentially causing T-cell-mediated
rejection (TCMR). Sequencing of the T-cell receptor (TCR) repertoire can be used to track
the donor-reactive repertoire in blood and tissue of patients after kidney transplantation.
Methods/Design In this prospective cohort study, 117 non-sensitized kidney transplant
recipients with anti-CD25 induction were included. Peripheral mononuclear cells (PBMCs) …
of donor-reactive T-cells following transplantation, potentially causing T-cell-mediated
rejection (TCMR). Sequencing of the T-cell receptor (TCR) repertoire can be used to track
the donor-reactive repertoire in blood and tissue of patients after kidney transplantation.
Methods/Design In this prospective cohort study, 117 non-sensitized kidney transplant
recipients with anti-CD25 induction were included. Peripheral mononuclear cells (PBMCs) …
Background
Antigen recognition of allo-peptides and HLA molecules leads to the activation of donor-reactive T-cells following transplantation, potentially causing T-cell-mediated rejection (TCMR). Sequencing of the T-cell receptor (TCR) repertoire can be used to track the donor-reactive repertoire in blood and tissue of patients after kidney transplantation.
Methods/Design
In this prospective cohort study, 117 non-sensitized kidney transplant recipients with anti-CD25 induction were included. Peripheral mononuclear cells (PBMCs) were sampled pre-transplant and at the time of protocol or indication biopsies together with graft tissue. Next-generation sequencing (NGS) of the CDR3 region of the TCRbeta chain was performed after donor stimulation in mixed lymphocyte reactions to define the donor-reactive TCR repertoire. Blood and tissue of six patients experiencing a TCMR and six patients without rejection on protocol biopsies were interrogated for these TCRs. To elucidate common features of T-cell clonotypes, a network analysis of the TCR repertoires was performed.
Results
After transplantation, the frequency of circulating donor-reactive CD4 T-cells increased significantly from 0.86 ± 0.40% to 2.06 ± 0.40% of all CD4 cells (p < 0.001, mean dif.: -1.197, CI: -1.802, -0.593). The number of circulating donor-reactive CD4 clonotypes increased from 0.72 ± 0.33% to 1.89 ± 0.33% (p < 0.001, mean dif.: -1.168, CI: -1.724, -0.612). No difference in the percentage of donor-reactive T-cells in the circulation at transplant biopsy was found between subjects experiencing a TCMR and the control group [p = 0.64 (CD4+), p = 0.52 (CD8+)]. Graft-infiltrating T-cells showed an up to six-fold increase of donor-reactive T-cell clonotypes compared to the blood at the same time (3.7 vs. 0.6% and 2.4 vs. 1.5%), but the infiltrating TCR repertoire was not reflected by the composition of the circulating TCR repertoire despite some overlap. Network analysis showed a distinct segregation of the donor-reactive repertoire with higher modularity than the overall TCR repertoire in the blood. These findings indicate an unchoreographed process of diverse T-cell clones directed against numerous non-self antigens found in the allograft.
Conclusion
Donor-reactive T-cells are enriched in the kidney allograft during a TCMR episode, and dominant tissue clones are also found in the blood.
Trial Registration
Clinicaltrials.gov: NCT: 03422224 (https://clinicaltrials.gov/ct2/show/NCT03422224).
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