Abstract
Red blood cell alloimmunization remains a major complication for transfusion-dependent patients, but immune factors governing risk for alloimmunization are unknown. We hypothesized that CD4+ regulatory T cells (Tregs), which we have shown control the rate and the frequency of red blood cell alloimmunization in mouse models, may dictate responder/nonresponder status. Using a transfusion regimen in which more than 50% of mice develop alloantibodies to human glycophorin A antigen, we found reduced in vitro and in vivo Treg-suppressive activity in responders compared with nonresponders that was the result of impaired Treg suppressor function. Moreover, responders were prone to developing additional alloantibodies to strong immunogens, whereas nonresponders were resistant to alloimmunization. Altogether, our data raise the possibility that Treg activity may be used as a marker for identifying responder/nonresponder status in transfusion recipients.
Introduction
Exposure to red blood cell (RBC) alloantigens through transfusion, pregnancy, or transplantation may result in production of antibodies in the recipient. Alloimmunization may cause several complications, including delay in obtaining matched blood as well as potentially life-threatening delayed hemolytic transfusion reactions, and autoimmunization.1–4 RBC alloimmunization rates are reportedly as low as 0.5% in transfusion recipients but are highest in chronically transfused patients with hemoglobinopathies.5,6 Even nonchronically transfused patients who become alloimmunized are 20 times more likely to form additional antibodies after one or more repeat transfusion events.7
Several factors are predicted to influence the recipient's immune system to react to alloantigens, including the dose and the immunogenicity of the antigen as well as genetic or acquired patient-related factors.8–11 However, possible differences in the immune makeup of transfused patients who make alloantibodies (responders) and those who do not (nonresponders) are not known. By identifying such markers, it may be possible to predict in advance responders and nonresponders, thereby avoiding the use of costly antigen-matched units for nonresponders, and only selecting phenotyped-matched units1,12–15 for responders to reduce alloimmunization-associated morbidity and mortality. CD4+ regulatory T cells (Tregs) characterized by coexpression of Foxp3 and CD25 are key regulators of a wide spectrum of immune responses,16 suppressing activation and proliferation of effector T cells and other immune cells in vivo and/or in vitro.17 We recently found that manipulation of Treg numbers affects the rate and frequency of RBC alloimmunization in mouse models of RBC transfusions.18 Given that Tregs participate in the control of transfusion-associated RBC alloantibody responses,18 we hypothesized that Treg status may differ between responders and nonresponders. In this study, we used a mouse RBC alloimmunization model to test this hypothesis.
Methods
Mouse studies
Male or female 12-week-old C57/BL6 mice were transfused intravenously with 50 μL Ficoll-treated packed RBCs from transgenic human glycophorin A (huGPA)19 or Duffy Fyb mice,20 equivalent to 1 to 2 packed RBC units with 50 μg unmethylated CpG-containing oligonucleotides (CpG-ODN)18,21 for the first week and then on a weekly basis for 2 to 3 additional weeks with RBCs alone. Alloantibody levels in blood samples obtained by retro-orbital sinus bleeding were measured by incubating diluted plasma with GPA transgenic RBCs and analysis by flow cytometry.18 RBC survival studies were performed as previously described.22 Foxp3 expression in splenocytes was measured by intracellular staining with anti-Foxp3 following the manufacturer's instructions (eBioscience, San Diego, CA) and analysis by flow cytometry.
For adoptive transfer experiments, 106 purified sorted splenic CD4+CD25+ cells (> 95% purity; data not shown) were injected in the tail vein, followed by the aforementioned transfusion regimen a day later.18 All animal procedures were performed as approved by the Institutional Animal Care and Use Committee of the New York Blood Center.
Proliferation assay
CD4+CD25− and CD4+CD25+ T cells (5 × 104 cells/well) were cultured in duplicates or triplicates alone or together at various ratios in the presence of anti-CD3 (clone, 1 μg/mL; BD Biosciences, San Jose, CA) together with 5 × 104/well of irradiated splenocytes from responder mice as antigen-presenting cells for 72 hours. The cultures were pulsed with 1 μCi [3H]thymidine for the last 16 hours.
Statistical analysis
The significance of differences between groups of mice was calculated using the Student t test. Relationship between levels of alloanti-huGPA and alloanti-Fyb was determined by the Pearson r correlation.
Results and discussion
Using a weekly transfusion regimen with allogeneic huGPA RBCs in which the administration of CpG-ODN adjuvant is confined to the first week, more than 50% of B6 mice developed alloantibodies after 4 weeks (Figure 1A, 6 separate experiments), indicating minor genetic or environmental variations even within inbred mouse strains. Transfused recipients were grouped as either nonresponders (no alloantibodies with normal transfused allogeneic RBCs survival) or responders (with highest alloanti-huGPA levels plus shortened transfused RBC survival; Figure 1) to explore potential Treg-associated differences between the 2 cohorts. Analysis of Foxp3 expression indicated no differences in the frequency of Tregs between responders and nonresponders (Figure 2A,B).
In vitro suppression of T-cell receptor–stimulated proliferation of other T cells is a commonly used assay for assessing Treg suppressive function.23,24 We examined the immunosuppressive effects of responder and nonresponder Tregs on proliferation of autologous effector CD4+CD25− cells (n = 3, involving 2-4 mice per group). Sorted Tregs from both groups were equally hyporesponsive to polyclonal stimulation with anti-CD3 and antigen-presenting cells (3H incorporation for responders 833 ± 27 cpm and nonresponders 748 ± 65 cpm; P > .3), indicating that Tregs from both cohorts of mice do exhibit the characteristic anergic Treg phenotype. In contrast, sorted CD4+CD25− cells from both responders and nonresponders proliferated (3H incorporation for responders, 14 381 ± 4105 cpm; nonresponders, 10 660 ± 2200 cpm; P > .4). On coculture of autologous CD4+CD25+ and CD4+CD25− cells at different ratios, Tregs from nonresponders and responders suppressed proliferation of effector T cells at 1:1 and 1:2 ratios in a dose-dependent manner (Figure 2C). However, Tregs from nonresponders were better suppressors as indicated by lower proliferation rates at low Treg to CD4+CD25− ratios (at 1:4 ratio, 18% vs 29%; at 1:8 ratio, 25% vs 43%; and at 1:16 ratio, 38% vs 60%, all P < .05, Figure 2C).
The reduced regulatory function in responders could be the result of a decrease in their Treg function or to refractoriness of their CD4+CD25− cells to suppression. Cross-mixing experiments were performed in which responder and nonresponder Tregs were cocultured with the autologous and the converse CD4+CD25− cells from either nonresponders or responders. At 1:16 CD4+CD25+/CD4+CD25− ratios, responder Tregs could not effectively inhibit proliferation of nonresponder or responder CD4+CD25− cells (Figure 2D), indicating an inherent impaired suppressor function in responder Tregs. In contrast, Tregs from nonresponders suppressed the proliferation of CD4+CD25− cells from both responders and nonresponders to a similar degree (Figure 2D), indicating normal responsiveness of responder effector cells to suppression. We next examined whether the demonstrated differential in vitro Treg activity affected alloimmunization rates in vivo. Naive B6 mice were adoptively transferred with sorted splenic Tregs from responders and nonresponders before initiation of the transfusion regimen with huGPA RBCs. We found that, although adoptive transfer of responders and nonresponder Tregs suppressed the levels of alloantibodies in transfusion recipients, suppression was more effective in mice treated with Tregs from nonresponders (Figure 2E, P = .004), consistent with the in vitro data.
We also tested whether responders with less suppressive Treg activity are more susceptible to developing additional alloantibodies if challenged, and conversely, whether nonresponders with better Treg suppressors are resistant to development of additional alloantibodies. We used RBCs from transgenic mice expressing human Duffy Fyb antigen.20 We found that mice mounted a weaker alloanti-Fyb response compared with alloanti-huGPA responses using our standard transfusion regimen (data not shown), indicating that huFyb is less immunogenic than huGPA. When mice were transfused with huGPA RBCs followed by huFyb RBCs, 17 of 29 mice produced alloanti-huGPA, but none of the mice developed detectable alloanti-Fyb. In the reverse transfusion experiment using huFyb RBCs first and then huGPA RBCs, the levels of alloanti-huGPA production correlated with those of alloanti-Fyb (Figure 2F, Pearson r = 0.66 and P = .002). These data suggest that, despite a reduced Treg activity in responder mice, the immunogenicity of the second alloantigen is an important factor in eliciting an immune response.25 Nevertheless, nonresponders with the demonstrated potent Treg suppressor function are resistant to making subsequent alloantibodies, whereas responders are more susceptible, raising the possibility that Treg activity may be used as a marker for evaluating responder/nonresponder status in transfusion recipients.
The online version of this article contains a data supplement.
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Acknowledgments
The authors thank Dr Petra Hoffmann (University Hospital Regensburg, Regensburg, Germany) for helpful discussions.
Authorship
Contribution: W.B., S.H., and J.Y. designed and performed research and analyzed data; and K.Y. designed research, analyzed data, and wrote the paper.
Conflict-of-interest disclosure: The authors declare no competing financial interests.
Correspondence: Karina Yazdanbakhsh, Laboratory of Complement Biology, New York Blood Center, 310 E 67th St, New York, NY 10021; e-mail: kyazdanbakhsh@nybloodcenter.org.
References
Author notes
*W.B., J.Y., and S.H. contributed equally to this work.