Indoleamine 2,3-dioxygenase expression in patients with allergic rhinitis: a case-control study

This study is a case-control study. It was carried out at the Department of Otorhinolaryngology, Tampere University Hospital, Finland and has been approved by the Hospital's Ethical committee. Written informed consent was obtained from all patients. The subjects were Caucasian. Patients were either atopic with allergic rhinoconjunctivitis symptoms, or non-atopic. Moreover, the patients did not have other diseases such as asthma. The diagnosis of birch pollen-induced allergic rhinitis was based on a history of seasonal allergic rhinitis during spring, clinical examination, and skin prick test positivity. Characteristics of the subject groups are shown in table 1. Specimens were taken from the nasal cavity. Biopsies from the anterior edge of the inferior turbinate were obtained with Fokkens' forceps under local anaesthesia. Specimens were taken during both winter (off season) and during peak allergen exposure in spring (in season, natural allergen exposure). Patients were not allowed to use their medication (antihistamine and/or nasal corticosteroids) for a minimum of 5 days before nasal biopsies were taken.

Nasal specimens were immediately snap-frozen in liquid nitrogen and stored at -80°C until analysis. Tissue samples were stained with hemalaun-eosin to calculate the number of mucosal leukocytes and eosinophils/mm² and to evaluate the inflammation score (0 = no inflammation, 1 = mild, 2 = moderate, 3 = severe inflammation) For light microscope evaluation, immunoperoxidase staining was used and specimens were cut into 3-5 μm thick frozen sections on Superfrost Plus microscope slides. (Menzel-Gläser, Braunschweig, Germany). Frozen sections were fixed with formalin during 45 minutes. Fully automated immunostaining was performed by Ventana BenchMark LT Automated IHC Stainer (Ventana Medical System, Arizona, USA). Ultraview Universal DAB detection kit (catalogue No. 760-500, Ventana Medical System, Arizona, USA) was used. For epitope retrieval CC1: Tris -EDTA buffer pH 8.0 (catalogue No 950-124, Ventana) was used at 95°C to 100°C for 8 minutes. Endogenous peroxidase was blocked with UV-Inhibitor 3% H202 (Ventana) for 4 minutes at 37°C. Tissue slides were rinsed between steps with Ventana Tris-based Reaction buffer (catalogue No. 950-300, Ventana). Slides were incubated at 37°C for 32 minutes with mAb anti-Indoleamine 2,3 dioxygenase (1:200, clone MAB5412, Chemicon International Inc., USA) followed by application of Ventana Ultraview HRP Universal Multimer (8 minutes at 37°C). Diaminobenzidine (DAB) was used as a chromogen and haematoxylin as a nuclear stain. Known positive tissue samples (from coeliac or inflammatory bowel disease) were also used to confirm the staining reliability of all separate staining patches [17, 18]. The specificity of immunohistochemistry was controlled by omitting the primary antibodies or replacing them with irrelevant antisera.

Sections were examined with a Leica DM 2000 light microscope (Leica Microsystems GmbH, Wetzlar, Germany) by two independent observers blinded to the experimental conditions. In a sample, there was either moderate or strong immunoreactivity of all epithelial cells or no epithelial positivity at all. Thus, the results were expressed as IDO positive epithelium or IDO negative epithelium. The percentage of IDO positive mucosal leukocytes was counted.

Statistical analysis was carried out by SPSS Base 15.0 Statistical Software Package (SPSS Inc., Chicago, IL, USA). Data is expressed as medians or means. For comparisons, the results were analysed by, Fisher's exact (discrete) or Kruskal Wallis and Mann Whitney U tests (continuous). For pair-wise comparisons McNemar's and Wilcoxon tests were used. Two-tailed P-values of < 0.05 were considered statistically significant.