Exposure of cinnamyl alcohol in co‐culture of BEAS‐2B and dendritic cells: Interaction between CYP450 and cytokines

Author:

Yoshizaki Kelly1ORCID,Frias Daniela Perroni1ORCID,Maier Kevin1ORCID,Smelan Juliana1ORCID,Correia Aristides Tadeu2ORCID,Oliveira Luanda Mara da Silva3ORCID,Amato‐Lourenço Luís Fernando14ORCID,Santillo Bruna Tereso3ORCID,Prado Carla Máximo5ORCID,Oshiro Telma Miyuki3ORCID,Barbuto Jose Alexandre M.6ORCID,Mauad Thais1ORCID,Macchione Mariangela1ORCID

Affiliation:

1. Laboratory of Experimental Environmental Pathology, Department of Pathology São Paulo University Medical School São Paulo Brazil

2. Thoracic Surgery Division, Department of Cardiopneumology, InCor, Clinics Hospital, School of Medicine University of São Paulo São Paulo Brazil

3. Laboratory of Medical Investigation in Dermatology and Immunodeficiences, Hospital das Clínicas HCFMUSP, Faculdade de Medicina Universidade de São Paulo São Paulo Brazil

4. Institute of Advanced Studies (IEA) Global Cities Program University of São Paulo São Paulo Brazil

5. Federal University of São Paulo Santos Brazil

6. Department of Immunology, Institute of Biomedical Sciences University of São Paulo São Paulo Brazil

Abstract

AbstractThe prevalence of fragrances in various hygiene products contributes to their sensorial allure. However, fragrances can induce sensitization in the skin or respiratory system, and the mechanisms involved in this process are incompletely understood. This study investigated the intricate mechanisms underlying the fragrance's effects on sensitization response, focusing on the interplay between CYP450 enzymes, a class of drug‐metabolizing enzymes, and the adaptive immune system. Specifically, we assessed the expression of CYP450 enzymes and cytokine profiles in culture of BEAS‐2B and mature dendritic cells (mDC) alone or in co‐culture stimulated with 2 mM of a common fragrance, cinnamyl alcohol (CA) for 20 h. CYP1A1, CYP1A2, CYP1B1, CYP2A6, and CYP2A13 were analyzed by RT‐PCR and IL‐10, IL‐12p70, IL‐18, IL‐33, and thymic stromal lymphopoietin (TSLP) by Cytometric Bead Array (CBA). Through RT–PCR analysis, we observed that CA increased CYP1A2 and CYP1B1 expression in BEAS‐2B, with a further increased in BEAS‐2B‐mDC co‐culture. Additionally, exposure to CA increased IL‐12p70 levels in mDC rather than in BEAS‐2B‐mDC co‐culture. In regards to IL‐18, level was higher in BEAS‐2B than in BEAS‐2B‐mDC co‐culture. A positive correlation between the levels of IL‐10 and CYP1B1 was found in mDC‐CA‐exposed and between IL‐12p70 and CYP1A1 was found in BEAS‐2B after CA exposure. However, IL‐12p70 and CYP1A2 as well as IL‐18, IL‐33, and CYP1A1 levels were negative, correlated mainly in co‐culture control. These correlations highlight potential immunomodulatory interactions and complex regulatory relationships. Overall, exposure to CA enhances CYP450 expression, suggesting that CA can influence immune responses by degrading ligands on xenosensitive transcription factors.

Publisher

Wiley

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