To treat patients with refractory cytomegalovirus (CMV) reactivation after allogeneic stem cell transplantation, a phase I/II clinical study on adoptive transfer of in vitro-generated donor-derived or patient-derived CMV pp65-specific CD8+ T-cell lines was performed. Peripheral blood mononuclear cells from CMV seropositive donors or patients were stimulated with HLA-A*0201-restricted and/or HLA-B*0702-restricted CMV pp65 peptides (NLV/TPR) and 1 day after stimulation interferon-γ)-producing cells were enriched using the CliniMACS Cytokine Capture System (interferon-γ), and cultured with autologous feeders and low-dose interluekin-2. After 7–14 days of culture, quality controls were performed and the CMV-specific T-cell lines were administered or cryopreserved. The T-cell lines generated contained 0.6–17×106 cells, comprising 54%–96% CMV pp65-specific CD8+ T cells, and showed CMV-specific lysis of target cells. Fifteen CMV-specific T-cell lines were generated of which 8 were administered to patients with refractory CMV reactivation. After administration, no acute adverse events and no graft versus host disease were observed and CMV load disappeared. In several patients, a direct relation between administration of the T-cell line and the in vivo appearance of CMV pp65-specific T cells could be documented. In conclusion, administration of CMV pp65-specific CD8+ T-cell lines was found to be feasible and safe, and enduring efficacy of administered CMV pp65-specific CD8+ T-cell lines could be demonstrated.
To the Editor: SARS-CoV-2 vaccine immunogenicity is commonly evaluated by measuring antibody titers against the SARS-CoV-2 Spike (S) protein. Previously, inferior humoral vaccination responses in patients with lymphoid malignancies have been shown.1 This can be attributed to immune defects caused by disease or treatment. NHL and CLL treated with CD20- and MM with CD38-directed therapies, leads to long-lasting B- or plasma-cell depletion, respectively. CLL and MM are associated with hypogammaglobulinemia and aberrations in T-cell function. T-cell immunity is vital for viral clearance and long-lasting protection against COVID-19 after vaccination.2 Moreover, high CD8+ T-cells contribute to COVID-19 survival in hematological patients.3 Studies investigating T-cell responses after vaccination in patients with lymphoid malignancies are, however, scarce and results are conflicting. This leaves a knowledge gap, underlining the urgency of an in-depth and reproducible analysis of functional SARS-CoV-2 specific T-cell responses following vaccination in hematological patients. Patients. Adult patients diagnosed with CLL, NHL, or MM at two tertiary care centers in the Netherlands undergoing SARS-CoV-2 vaccination were included in the study. Serological and T-cell responses were evaluated pre-vaccination and 2 weeks, 3- and 6-months post-vaccination. Patients were included between March and June 2021. All participants gave written informed consent and all procedures performed were in accordance with the ethical standards of the national research committee and the 1964 Helsinki declaration (NL76863.068.21/METC 21-014). Vaccination responses. Antibody levels were measured with an anti-SARS-CoV-2 S immunoassay (Elecsys, Roche Diagnostics International Ltd). Adequate seroconversion was defined as an Ig serum concentration ≥250 BAU/ml. CD4+ and CD8+ T-cell responses were evaluated by stimulation of PBMCs using a 15-mer with 11 amino acid overlapping SARS-CoV-2 spike peptide pool (SB-peptide). T-cell activation and phenotype were measured by flow cytometry: CD154, CD137, CD69, IFN-γ, TNF-α, IL-2, IL-4, PD-1, IL-17, CXCR5, and FOXP3. In parallel, SARS-CoV-2-specific CD8+ T-cells were detected using spike peptide-HLA tetramer (spike/HLA-tetramer) staining combined with differentiation markers (CD45RA and CCR7). Stimulation with CEFX peptide pool (JPT/LUMC), containing peptides of CMV and other common pathogens, was used as a positive control. A response was considered to be positive if ≥0.05% of all CD4+ T-cells are spike reactive and if ≥0.005% of all CD8+ T-cells are spike reactive or binding spike-specific human leukocyte antigen (HLA)-peptide tetramers. These thresholds were based on the CD4 and CD8 T-cell responses measured in nine healthy individuals (data not shown). Additional information is provided in Supplemental Methods. Statistics. Continuous variables are described as median (IQR) and categorical variables as number and percentage of total. Antibody and T-cell responses of diagnostic subgroups were compared to population proportions using one-sample binomial testing. Missing data varied across timepoints; therefore, the number of included measurements is mentioned in the figures and confidence intervals are provided. To evaluate factors associated with humoral and cellular responses, univariable logistic regression was performed. To compare groups Chi square, Wilcoxon or Mann–Whitney U tests were used when applicable. All tests were two-sided with an α of 0.05. Analyses were performed using IBM SPSS Statistics (version 25.0.0.2) and Graphpad Prism (version 9.3.1). One hundred and sixty patients diagnosed with CLL (n = 31), aggressive NHL (n = 39), indolent NHL (n = 57), MM (n = 30), and other (acute lymphoblastic leukemia n = 2, autoimmune pancytopenia n = 1) were included (Table S1). All patients received two doses of an mRNA vaccine. Eight patients with pre-vaccination positive anti-SARS-CoV-2 S Ig were excluded from the analysis. Adequate seroconversion rates 2 weeks post-vaccination were 31% in CLL, 62% in aggressive NHL, 60% in indolent NHL, and 93% in MM patients (Figure 1A). Compared to an age-adjusted population proportion of 99%, this was significantly lower in patients with all disease categories, except MM. Recent treatment with anti-CD20 containing regimens significantly reduces adequate seroconversion rate (Figure S1A). However, when treatment was >12 months before vaccination, this seroconversion rate increased significantly to 87% (Figure S1B), indicating that sufficient B-cell recovery to elicit seroconversion takes at least 12 months after B-cell depleting therapy. Next to disease and treatment, univariable logistic regression analysis showed that only a lymphocyte count below 1*109/L was a significant predictor of humoral outcome (Figure S2A), which is related to B-cell-depleting therapy. These findings are in line with previous studies.1 T-cell responses were measured in 49 patients lacking and 14 patients with adequate seroconversion (Table S2). Spike-specific CD4+ T-cell responses significantly increased in all disease cohorts 2 weeks after mRNA vaccination, whilst control CEFX-specific T-cells remained stable pre- and post-vaccination (Figures 1B and S3A). Spike-specific CD8+ T-cell responses based on reactivation with Spike peptides (Figure 1C) and spike/HLA-tetramer staining (Figure 1D) were increased in CLL and both NHL cohorts 2 weeks after vaccination. Most spike-specific CD4+ and CD8+ T-cell responses remained present over time with fluctuations (Figure 1B–D) and demonstrated to exhibit a type 1 cytokine profile (Figure S4). No clear effect of a third vaccination was seen at 6 months post-initial vaccination; however, only 62% of patients received a third vaccination and this was at various time points before the 6-month time point (median: 46 days, range: 1–70). Expression of PD-1, an early T-cell activation marker, was most prominent 2 weeks after vaccination (Figure S4D,K). In the subset of Spike-specific CD4+ T-cells, both T follicular helper cells and regulatory T-cells were present, though low in number (Figure S4G–H). Spike-specific CD8+ T-cells were mostly effector memory phenotype (Figure S4L). These results were in line with the phenotype observed in a healthy control cohort (n = 9) and previous studies in healthy cohorts (data not shown).4 Our in-depth T-cell analysis demonstrated induction of Spike-specific CD4+ responses in 75%, 92%, 81%, and 60% of CLL, aggressive NHL, indolent NHL, and MM, respectively (Figure 1A). Induction of Spike-specific CD8+ responses (presence of Spike-specific and/or Spike/HLA-tetramer+ CD8+ T-cells) were 77%, 82%, 71%, and 50%, respectively (Figure 1A). These data collectively indicate that induction of T-cell responses does not seem to be affected by disease. However, it is important to note that, though low in number of patients analyzed, T-cell responses seem to be hampered in MM. Possible explanation is the use of dexamethasone and/or anti-CD38 therapy, which are known to negatively affect T-cells and their function. When comparing the Spike-specific T-cell responses between patients with and without adequate seroconversion, no significant differences were observed in the percentage of patients that generated a CD4+ T-cell response nor the percentage of Spike-specific CD4+ T-cells in individual patients (Figures 1E,F and S2B), indicating that the lack of humoral responses was not caused by lack of CD4+ T-cell help (Figure 1A). Furthermore, no difference was observed in the percentage of patients that generated a CD8+ T-cell response (Figures 1E and S2C); however, the frequency of Spike-specific CD8+ T-cells was significantly higher in patients lacking serological response (Figure 1F) 2 weeks post-vaccination, which could represent an immune compensation mechanism that might contribute to a survival advantage in case of severe COVID-19.3 T-cell immunity is known to decline with advanced age. In this study, age was the only significant predictor of Spike-specific T-cell responses (CD4+ OR: 0.18, CD8+ OR: 0.05). (Figure S2B,C), both Spike-specific CD4+ and CD8+ T-cell responses decline significantly for patients aged over 68 years (Figure 1G). Though cellular responses after SARS-COV-2 vaccination in patients with lymphoid malignancies have been suggested,5 we for the first time show with a highly specific and reproducible technique that nearly all lymphoid malignancy patients exhibit a good Spike-specific CD4+ and CD8+ T-cell response 2 weeks to 3 months after vaccination (Figure 1H). Limitations of this study include a limited sample size, making it difficult to perform subgroup analysis especially within disease cohorts. Therefore, analyzing specific treatment-related effects is not possible. However, this cohort does represent a real-world situation for patients in two secondary-/tertiary-care centers in the Netherlands. In addition, the peptide pools used in the T-cell assays were based on the ancestral Wuhan strain sequence which is not the current circulating variant. However, it is important to note that it has been shown that T-cell responses induced by mRNA-1273 and BNT162b2 are minimally affected by the mutations found in omicron.6 In conclusion, this study demonstrates that the majority of patients lacking adequate seroconversion following SARS-CoV-2 mRNA vaccination were able to generate a cellular immune response. Moreover, a hampered humoral response is compensated by a stronger cellular response, which indicates that vaccination is of significance also in patients lacking seroconversion. Lara S. Boerenkamp and Cilia R. Pothast contributed equally to this manuscript. Mirjam H. M. Heemskerk and Catharina H. M. J. Van Elssen contributed equally to this manuscript. Mirjam H. M. Heemskerk, Inge H. M. van Loo, and Catharina H. M. J. Van Elssen designed the study. Lara S. Boerenkamp collected data, performed data management, analyzed the data, made figures, and wrote the manuscript. Cilia R. Pothast designed experimental set-up, performed experiments, analyzed the data, made figures, and wrote the manuscript. Romy C. Dijkland and Kayleigh van Dijk performed experiments. Gwendolyn N. Y. van Gorkom assisted with statistical data analysis. Lotte Wieten collected samples. All authors critically revised the manuscript and reviewed and approved the final manuscript. The authors would like to thank all patients and colleagues from Maastricht University Medical Center and Leiden University Medical Center who made this study possible. Flow cytometry was performed at the Flow cytometry Core Facility (FCF) of Leiden University Medical Center (LUMC) in Leiden, Netherlands (https://www.lumc.nl/research/facilities/fcf). The authors declare no conflicts of interest. The data that support the findings of this study are available from the corresponding author, Lara S. Boerenkamp, upon reasonable request. Figure S1. Serological response rates 2 weeks after SARS-CoV-2 mRNA vaccination. Figure S2. Potential predictive factors for serological CD4+ or CD8+ T-cell response. Figure S3. CD4+ and CD8+ T-cell responses after stimulation with CEFX peptide pool. Figure S4. Cytokine production and marker expression of spike-specific CD4+ and CD8+ T-cells. Figure S5. Flow cytometry gating example for peptide stimulation assays and tetramer staining. Appendix S1. Supporting Information. Please note: The publisher is not responsible for the content or functionality of any supporting information supplied by the authors. Any queries (other than missing content) should be directed to the corresponding author for the article.
Allogeneic stem cell transplantation (alloSCT) provides a curative treatment option for hematological malignancies. After HLA-matched alloSCT, donor-derived T cells recognize minor histocompatibility antigens (MiHAs), which are polymorphic peptides presented by HLA on patient cells. MiHAs are absent on donor cells due to genetic differences between patient and donor. T cells targeting broadly expressed MiHAs induce graft-versus-leukemia (GvL) reactivity as well as graft-versus-host disease (GvHD), while T cells for MiHAs with restricted or preferential expression on hematopoietic or non-hematopoietic cells may skew responses toward GvL or GvHD, respectively. Besides tissue expression, overall strength of GvL and GvHD is also determined by T-cell frequencies against MiHAs. Here, we explored the use of DNA barcode-labeled peptide-MHC multimers to detect and monitor antigen-specific T cells for the recently expanded repertoire of HLA-I-restricted MiHAs. In 16 patients who experienced an immune response after donor lymphocyte infusion, variable T-cell frequencies up to 30.5% of CD8 + T cells were measured for 49 MiHAs. High T-cell frequencies above 1% were measured in 12 patients for 19 MiHAs, with the majority directed against mismatched MiHAs, typically 6–8 weeks after donor lymphocyte infusion and at the onset of GvHD. The 12 patients included 9 of 10 patients with severe GvHD, 2 of 3 patients with limited GvHD and 1 of 3 patients without GvHD. In conclusion, we demonstrated that barcoded peptide-MHC multimers reliably detect and allow monitoring for MiHA-specific T cells during treatment to investigate the kinetics of immune responses and their impact on development of GvL and GvHD after HLA-matched alloSCT.
