Biased T Cell Receptor Usage Directed against Human Leukocyte Antigen DQ8-Restricted Gliadin Peptides Is Associated with Celiac Disease

Broughton, Sophie E.; Petersen, Jan; Theodossis, A.; Scally, S.W.; Loh, Khai Lee; Thompson, Allan; Bergen, Jeroen van; Kooy–Winkelaar, Yvonne; Henderson, Kate; Beddoe, Travis; Tye–Din, Jason A.; Mannering, Stuart I.; Purcell, Anthony W.; McCluskey, James; Anderson, Robert P.; Koning, Frits; Reid, Hugh H.; Rossjohn, Jamie

doi:10.1016/j.immuni.2012.07.013

Cited by 120 publications

(162 citation statements)

References 58 publications

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“…The fact that these clonotypes are not found in all subjects as Ag responsive could be attributable to several factors, including sampling biases (38) and pairing with TCRVa-chains nonpermissive for the specific pHLA complex. Our findings are in keeping with recent in-depth studies of gluten epitope-specific CD4 T cells, which, despite being focused by repeated exposure to the same exogenous antigenic peptides presented by HLA-DQ8 and bearing high-affinity TCRs, show TRBV9*01 bias but very little conservation of residues in the CDR3b region (39). The intense privacy of Ag-specific responses that we observed indicates that the development of clonotypic tracking for biomarker purposes may need to be subject specific.…”

Section: Discussionsupporting

confidence: 91%

A Novel Approach to Tracking Antigen-Experienced CD4 T Cells into Functional Compartments via Tandem Deep and Shallow TCR Clonotyping

Estorninho

Gibson

Kronenberg‐Versteeg

et al. 2013

The Journal of Immunology

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Extensive diversity in the human repertoire of TCRs for Ag is both a cornerstone of effective adaptive immunity that enables host protection against a multiplicity of pathogens and a weakness that gives rise to potential pathological self-reactivity. The complexity arising from diversity makes detection and tracking of single Ag-specific CD4 T cells (ASTs) involved in these immune responses challenging. We report a tandem, multistep process to quantify rare TCRβ-chain variable sequences of ASTs in large polyclonal populations. The approach combines deep high-throughput sequencing (HTS) within functional CD4 T cell compartments, such as naive/memory cells, with shallow, multiple identifier–based HTS of ASTs identified by activation marker upregulation after short-term Ag stimulation in vitro. We find that clonotypes recognizing HLA class II–restricted epitopes of both pathogen-derived Ags and self-Ags are oligoclonal and typically private. Clonotype tracking within an individual reveals private AST clonotypes resident in the memory population, as would be expected, representing clonal expansions (identical nucleotide sequence; “ultraprivate”). Other AST clonotypes share CDR3β amino acid sequences through convergent recombination and are found in memory populations of multiple individuals. Tandem HTS-based clonotyping will facilitate studying AST dynamics, epitope spreading, and repertoire changes that arise postvaccination and following Ag-specific immunotherapies for cancer and autoimmune disease.

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Section: Discussionsupporting

confidence: 91%

A Novel Approach to Tracking Antigen-Experienced CD4 T Cells into Functional Compartments via Tandem Deep and Shallow TCR Clonotyping

Estorninho

Gibson

Kronenberg‐Versteeg

et al. 2013

The Journal of Immunology

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“…Written informed consent was obtained from each subject before enrollment. Patients S, T, vL, LS, and SP have been described previously (9,15). Additional HLA class II genotypes were as follows: patient E, HLA-DQA1*0301-DQB1*0302 homozygous; patient B, HLA-DQA1*0301-DQB1*0302 homozygous; patient Bel, HLA-DQA1*03/03-DQB1*0301/ 0302 heterozygous; patient C, HLA-DQA1*0101/0301-DQB1*0501/0302 heterozygous.…”

Section: Patientsmentioning

confidence: 99%

“…Such observations generally reflect structural and/ or recombinatorial constraints (13,14). Indeed, the first insights into the molecular basis for this biased TRBV usage have been obtained via crystallographic studies (9,10).…”

mentioning

confidence: 99%

“…In particular, T cells specific for the DQ2.5-glia-a2 peptide preferentially express TRBV7-2, whereas those specific for DQ8-glia-a1 typically use TRBV9 (9)(10)(11)(12). Such observations generally reflect structural and/ or recombinatorial constraints (13,14).…”

mentioning

confidence: 99%

“…A single crystal structure of a TRBV9 + TCR-HLA-DQ8-glia-a1 complex shows that two amino acid residues virtually unique to TRBV9 are essential for TCR binding to the HLA-DQ8-glia-a1 complex, thereby providing a potential explanation for TRBV9 bias in HLA-DQ8-mediated CD (9). However, the observed bias toward TRBV9 does not necessarily extend to the affected intestinal tissue of patients because the HLA-DQ8-restricted T cells examined in this study were derived from long-term biopsy cultures.…”

mentioning

confidence: 99%

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Determinants of Gliadin-Specific T Cell Selection in Celiac Disease

Petersen

Bergen

Loh

et al. 2015

The Journal of Immunology

Self Cite

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In HLA-DQ8–associated celiac disease (CD), the pathogenic T cell response is directed toward an immunodominant α-gliadin–derived peptide (DQ8-glia-α1). However, our knowledge of TCR gene usage within the primary intestinal tissue of HLA-DQ8+ CD patients is limited. We identified two populations of HLA-DQ8-glia-α1 tetramer+ CD4+ T cells that were essentially undetectable in biopsy samples from patients on a gluten-free diet but expanded rapidly and specifically after antigenic stimulation. Distinguished by expression of TRBV9, both T cell populations displayed biased clonotypic repertoires and reacted similarly against HLA-DQ8-glia-α1. In particular, TRBV9 paired most often with TRAV26-2, whereas the majority of TRBV9− TCRs used TRBV6-1 with no clear TRAV gene preference. Strikingly, both tetramer+/TRBV9+ and tetramer+/TRBV9− T cells possessed a non–germline-encoded arginine residue in their CDR3α and CDR3β loops, respectively. Comparison of the crystal structures of three TRBV9+ TCRs and a TRBV9− TCR revealed that, as a result of distinct TCR docking modes, the HLA-DQ8-glia-α1 contacts mediated by the CDR3-encoded arginine were almost identical between TRBV9+ and TRBV9− TCRs. In all cases, this interaction centered on two hydrogen bonds with a specific serine residue in the bound peptide. Replacement of serine with alanine at this position abrogated TRBV9+ and TRBV9− clonal T cell proliferation in response to HLA-DQ8-glia-α1. Gluten-specific memory CD4+ T cells with structurally and functionally conserved TCRs therefore predominate in the disease-affected tissue of patients with HLA-DQ8–mediated CD.

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Phenotype‐Based Isolation of Antigen‐Specific CD4⁺ T Cells in Autoimmunity: A Study of Celiac Disease

et al. 2022

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The pathogenic immune response in celiac disease (CeD) is orchestrated by phenotypically distinct CD4 + T cells that recognize gluten epitopes in the context of disease-associated HLA-DQ allotypes. Cells with the same distinct phenotype, but with elusive specificities, are increased across multiple autoimmune conditions. Here, whether sorting of T cells based on their distinct phenotype (Tphe cells) yields gluten-reactive cells in CeD is tested. The method′s efficiency is benchmarked by parallel isolation of gluten-reactive T cells (Ttet cells), using HLA-DQ:gluten peptide tetramers. From gut biopsies of 12 untreated HLA-DQ2.5 + CeD patients, Ttet + /Tphe + , Ttet − /Tphe + , and Ttet − /Tphe − cells are sorted for single-cell T-cell receptor (TCR)-sequencing (n = 8) and T-cell clone (TCC)-generation (n = 5). The generated TCCs are TCR sequenced and tested for their reactivity against deamidated gluten. Gluten-reactivity is observed in 91.2% of Ttet + /Tphe + TCCs, 65.3% of Ttet − /Tphe + TCCs and 0% of Ttet − /Tphe − TCCs. TCR sequencing reveals clonal expansion and sequence sharing across patients, features reflecting antigen-driven responses. The feasibility to isolate antigen-specific CD4 + T cells by the sole use of phenotypic markers in CeD outlines a potential avenue for characterizing disease-driving CD4 + T cells in autoimmune conditions.

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Biased T Cell Receptor Usage Directed against Human Leukocyte Antigen DQ8-Restricted Gliadin Peptides Is Associated with Celiac Disease

Cited by 120 publications

References 58 publications

A Novel Approach to Tracking Antigen-Experienced CD4 T Cells into Functional Compartments via Tandem Deep and Shallow TCR Clonotyping

A Novel Approach to Tracking Antigen-Experienced CD4 T Cells into Functional Compartments via Tandem Deep and Shallow TCR Clonotyping

Determinants of Gliadin-Specific T Cell Selection in Celiac Disease

Phenotype‐Based Isolation of Antigen‐Specific CD4⁺ T Cells in Autoimmunity: A Study of Celiac Disease

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Biased T Cell Receptor Usage Directed against Human Leukocyte Antigen DQ8-Restricted Gliadin Peptides Is Associated with Celiac Disease

Cited by 120 publications

References 58 publications

A Novel Approach to Tracking Antigen-Experienced CD4 T Cells into Functional Compartments via Tandem Deep and Shallow TCR Clonotyping

A Novel Approach to Tracking Antigen-Experienced CD4 T Cells into Functional Compartments via Tandem Deep and Shallow TCR Clonotyping

Determinants of Gliadin-Specific T Cell Selection in Celiac Disease

Phenotype‐Based Isolation of Antigen‐Specific CD4+ T Cells in Autoimmunity: A Study of Celiac Disease

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Phenotype‐Based Isolation of Antigen‐Specific CD4⁺ T Cells in Autoimmunity: A Study of Celiac Disease