The intensity of T cell receptor engagement determines the cytokine pattern of human allergen‐specific T helper cells

Carballido, José M.; Faith, A.; Carballido‐Perrig, Nicole; Blaser, Kurt

doi:10.1002/eji.1830270224

Cited by 57 publications

(65 citation statements)

References 57 publications

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“…These T cells clones were selected for this study because they all recognize the same T cell epitope in Der p 2 (residues 28 -40) in association with the HLA class II molecule DRB1*1101. Although variation was observed in the pattern of response elicited by individual T cell clones following recognition of the analogue peptide (p 2, 28 -40A 34,36 ), the overlying trend was for a shift in effector function from the Th2 to Th1 pathway. Stimulation of AC1.1, AC34.11, and AC34.26 cells with p 2, 28 -40A 34,36 enhanced IFN-␥ secretion as compared with the native peptide at equimolar concentrations, whereas proliferation and IL-5 production induced by either peptide were similar in magnitude (Table I).…”

Section: Measurement Of Ifn-␥ Il-4 Il-5 Il-10 and Tgf-␤ In Cell Cmentioning

confidence: 99%

“…The Der p 2 peptides, p 2, 28 -40 (IIHRGKPFQLEAV) and p 2, 28 -40A 34,36 (IIHRGKAFALEAV) were purchased from Genosys (Cambridge, U.K.). The peptides were tested for nonspecific immunosuppressive and mitogenic activity on cloned T cells reactive with influenza virus hemagglutinin.…”

Section: Antigensmentioning

confidence: 99%

“…Thus, the biological activity displayed by the analogue peptide is not the result of a contaminant. Biotinylated peptides p 2, 28 -40 and p 2, 28 -40A 34,36 were purchased from Advanced Biotechnology Centre (Imperial College School of Medicine at Charing Cross Hospital, London, U.K.).…”

Section: Antigensmentioning

confidence: 99%

“…Binding affinity of peptides p 2, 28 -40 and its analogue p 2, 28 -40A 34,36 to HLA-DRB1*1101 was determined as follows: biotinylated versions of both peptides were incubated with live L-1101 cells (3 ϫ 10 5 cells/well of a 96-well round-bottom tissue culture plate), over a range of concentrations, in a total volume of 200 l RPMI 1640/1% FCS for 4 h. Cells were washed and incubated with 10 g/ml avidin D FITC (Vector Laboratories, Peterborough, U.K.) for 30 min at 4°C and washed. Dead cells were excluded from the analysis by staining with 10 g/ml propidium iodide.…”

Section: Peptide Binding To Hla-drb1*1101mentioning

confidence: 99%

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Threshold Signaling of Human Th0 Cells in Activation and Anergy: Modulation of Effector Function by Altered TCR Ligand

Verhoef

Lamb

2000

The Journal of Immunology

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Molecular interactions between TCR and its natural ligand, in the presence of costimulatory signals, elicit T cell effector functions, whereas subtle changes in the structure of antigenic peptides may induce only selected T cell effector function including anergy. In this study, we have investigated the immunological activity of an altered TCR ligand (p 2, 28–40A34,36) derived from the immunodominant T cell epitope of the group 2 allergen of house dust mite, in which residues at positions 34 and 36 were substituted by alanine. Elevated IFN-γ synthesis was induced by equimolar concentrations of the analogue compared with native peptide (p 2, 28–40) and was paralleled by increased down-regulation of cell surface CD3. IL-5 and IL-10 production exhibit the same sensitivity to both peptides, implying that the induction of T cell effector functions are not all proportional to TCR occupancy. Both native peptide and the analogue bound to MHC class II (DRB1*1101) molecules with similar affinities. Furthermore, p 2, 28–40A34,36 induced T cell anergy at lower concentrations than native peptide. During the induction of anergy, TGF-β production was comparable for both peptides, whereas IL-10 secretion was markedly increased but more so in response to p 2, 28–40A34,36. Membrane expression of costimulatory ligands CD80 and CD86 was similar for native peptide and p 2, 28–40A34,36 and increased in activation, whereas only CD86 was elevated during anergy. The modulation of T cell effector function with altered TCR ligands may have practical applications in reprogramming allergic inflammatory responses through the induction of T cell anergy and/or the promotion of Th1 cytokines.

show abstract

Section: Measurement Of Ifn-␥ Il-4 Il-5 Il-10 and Tgf-␤ In Cell Cmentioning

confidence: 99%

Section: Antigensmentioning

confidence: 99%

Section: Antigensmentioning

confidence: 99%

Section: Peptide Binding To Hla-drb1*1101mentioning

confidence: 99%

See 2 more Smart Citations

Threshold Signaling of Human Th0 Cells in Activation and Anergy: Modulation of Effector Function by Altered TCR Ligand

Verhoef

Lamb

2000

The Journal of Immunology

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“…1). However, T-cell unresponsiveness (anergy) can also be induced in vitro, when pure antigen-specific T cells are incubated with peptides in the absence of antigen presenting cells (APCs) (25). Under these conditions, T cells are possibly presenting the antigens themselves, but fail to costimulate each other and therefore, receive only one T-cell activation signal.…”

Section: Two Signal Hypothesismentioning

confidence: 99%

T‐cell tolerance in allergic response

Schmidt‐Weber¹,

Blaser²

2002

Allergy

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Differential regulation of human T cell cytokine patterns and IgE and IgG4 responses by conformational antigen variants

Akdiş¹,

Blesken²,

Wymann³

et al. 1998

Eur. J. Immunol.

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Bee venom phospholipase A2 (PLA) represents the major allergen and antigen in allergic and non-allergic individuals sensitized to bee sting. We have studied specific activation of peripheral T cells by different structural and conformational variants of PLA and secretion of cytokines regulating IgE and IgG4 antibody (Ab) formation. PLA molecules expressing the correctly folded tertiary structure, which show high affinity to membrane phospholipids and were recognized by Ab from bee sting allergic patients, induced high IL-4, IL-5 and IL-13 production in peripheral blood mononuclear cell cultures. In contrast, non-refolded recombinant PLA (rPLA) and reduced and alkylated native PLA (nPLA) induced more IFN-gamma and IL-2 and higher proliferative responses. Differences in proliferation and cytokine patterns among correctly folded and non-refolded PLA resulted from conformation-dependent involvement of different antigen-presenting cell (APC) types. Antigen (Ag)-presenting B cells recognized PLA only in its natural conformation, stimulated Th2 type cytokines and induced IgE Ab. Non-refolded PLA was recognized, processed and presented exclusively by monocytes and induced a Th1 dominant cytokine profile leading to IgG4 production by B cells. The possibility that production of particular cytokine patterns and Ig isotype was influenced by the enzymatic activity of PLA was excluded by using enzymatically inactive H34Q point-mutated, refolded rPLA. These findings demonstrate the decisive role of specific Ag recognition by different APC, depending on structural features, membrane phospholipid binding property and the existence of conformational B cell epitopes, in the differential regulation of memory IgE and IgG4 Ab. Furthermore, they show that a change from IgE-mediated allergy to normal immunity against a major allergen can be induced by rPLA variants that are not recognized by specific Ab and B cells but still carry the T cell epitopes. These features may enable new applications for safer immunotherapy.

show abstract

The intensity of T cell receptor engagement determines the cytokine pattern of human allergen‐specific T helper cells

Cited by 57 publications

References 57 publications

Threshold Signaling of Human Th0 Cells in Activation and Anergy: Modulation of Effector Function by Altered TCR Ligand

Threshold Signaling of Human Th0 Cells in Activation and Anergy: Modulation of Effector Function by Altered TCR Ligand

T‐cell tolerance in allergic response

Differential regulation of human T cell cytokine patterns and IgE and IgG4 responses by conformational antigen variants

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