In vitro evaluation of the sensitization potential of weak contact allergens using langerhans-like dendritic cells and autologous T cells

Contact hypersensitivity is a major public health concern in most industrial countries, which is why predictive tests which could identify potential allergens are needed. We have established an in vitro approach for the detection of primary immune response. This model uses Langerhans-like dendritic...

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Bibliographic Details
Published in:Toxicology (Amsterdam) 2000-04, Vol.145 (1), p.73-82
Main Authors: Rougier, Nathalie, Redziniak, Gérard, Mougin, Danielle, Schmitt, Daniel, Vincent, Claude
Format: Article
Language:English
Subjects:
Allergens - immunology
Allergological tests
Biological and medical sciences
Cells, Cultured
DC maturation
Dendritic cells
Dendritic Cells - immunology
Dermatitis, Contact - etiology
Fetal Blood - immunology
Haptens
Haptens - immunology
Humans
Immunological methods for diagnosis and exploration
Immunopathology
Interleukin-1 - pharmacology
Interleukin-2 - pharmacology
Langerhans cells
Langerhans Cells - immunology
Lymphocyte Activation
Medical sciences
Primary response
T-Lymphocytes - immunology
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Summary:Contact hypersensitivity is a major public health concern in most industrial countries, which is why predictive tests which could identify potential allergens are needed. We have established an in vitro approach for the detection of primary immune response. This model uses Langerhans-like dendritic cells (LLDC) derived from cord blood progenitors and autologous T lymphocytes, isolated from the same blood sample. Treatment of day 12–14 LLDC, with strong haptens trinitrobenzene sulfonic acid (TNP), fluorescein isothiocyanate (FITC) or Bandrowski’s base (BB), results in the proliferation of T lymphocytes, whereas weak allergens and irritants, such as sodium dodecyl sulfate (SDS) are ineffective. The use of immature (day 8) LLDC and the addition of a 48 h stage of incubation after hapten contact, result in phenotypic maturation of LLDC in addition to lymphocyte activation in all the cultures with strong haptens. The 48 h stage of incubation, results in sensitization and in some cases the induction of T cell proliferation to citronellal (1/8), coumarine (1/8) and to a prohapten p-phenylenediamine (pPDA; 2/8). The phenotype of DC after 48 h of contact with a strong hapten, becomes that of mature DC (CD83 +, CD86 + and HLA-DR ++). With fragrance molecules, weak haptens and prohaptens, a comparable phenotype is observed only when T lymphocytes are activated. These data suggest that the unresponsiveness observed with weak haptens, may be the consequence on an incomplete maturation of LLDC.
ISSN:0300-483X
1879-3185
DOI:10.1016/S0300-483X(99)00222-X