T cell responses to human platelet antigen–1a involve a unique form of indirect allorecognition
Maria Therese Ahlen, Anne Husebekk, Ida Løken Killie, Bjørn Skogen, Tor Brynjar Stuge
Maria Therese Ahlen, Anne Husebekk, Ida Løken Killie, Bjørn Skogen, Tor Brynjar Stuge
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Research Article Immunology

T cell responses to human platelet antigen–1a involve a unique form of indirect allorecognition

Abstract

Fetal and neonatal alloimmune thrombocytopenia (FNAIT) is a pregnancy-related condition caused by maternal antibodies binding an alloantigen on fetal platelets. In most cases the alloantigen is formed by a single amino acid, integrin β3 Leu33, referred to as human platelet antigen–1a (HPA-1a). Production of anti–HPA-1a antibodies likely depends on CD4+ T cells that recognize the same alloantigen in complex with the HLA-DRA/DRB3*01:01 molecule. While this complex is well characterized, T cell recognition of it is not. Here, to examine the nature of antigen recognition by HPA-1a–specific T cells, we assayed native and synthetic variants of the integrin β3 peptide antigen for binding to DRA/DRB3*01:01-positive antigen-presenting cells and for T cell activation. We found that HPA-1a–specific T cells recognize non-allogeneic integrin β3 residues anchored to DRA/DRB3*01:01 by the allogeneic Leu33, which itself is not directly recognized by these T cells. Furthermore, these T cell responses are diverse, with different T cells depending on different residues for recognition. This represents a unique form of indirect allorecognition in which a non-allogeneic peptide sequence becomes immunogenic by stable anchoring to MHC by an allogeneic residue.

Authors

Maria Therese Ahlen, Anne Husebekk, Ida Løken Killie, Bjørn Skogen, Tor Brynjar Stuge

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Figure 1

Peptide binding to cell lines.

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Peptide binding to cell lines. Binding of control 12-mer peptides (L33 a...
Binding of control 12-mer peptides (L33 and P33) extended with a biotinylated linker peptide were incubated with DRB3*01:01-positive cell lines (STEINLIN and D4BL4) or control cell lines (DUCAF, EMJ) at 5 μM peptide in the presence of 2.5 μM AdEtOH. The efficiency of binding to APCs was assessed by flow cytometry with streptavidin-conjugated R-PE. (A) Representative raw data of one of 3 independent peptide binding assays (1 of 2 replicates shown). (B) Comparison of percent specific binding. Data points from independent experiments are presented as dots, with bars representing mean ± SEM of at least 3 experiments. Raw data values were median R-PE fluorescence intensity on B-LCLs (gated by light scatter cytogram). Background intensity (cells only, no peptide) was subtracted before calculating the specific binding within each experiment (L33 peptide on STEINLIN defined as 100%). AdEtOH, adamantane ethanol; APC, antigen presenting cell; R-PE, R-phycoerythrin; B-LCL, B-lymphoblastoid cell lines.