Sinonasal and polyp tissues were obtained from patients with bilateral CRS during routine functional endoscopic sinus surgery. All subjects provided written informed consent for study participation, and the study was approved by the internal review board of Seoul National University Hospital, Boramae Medical Center. The diagnosis of CRS was based on personal history, physical examination, nasal endoscopy and computed tomography findings of the sinuses according to the 2012 European position paper on rhinosinusitis and nasal polyps (EPOS) guidelines.1 Exclusion criteria were as follows: 1) younger than 18 years of age; 2) prior treatment with antibiotics, systemic or topical corticosteroids, or other immune-modulating drugs for 4 weeks before surgery; and 3) unilateral rhinosinusitis, antrochoanal polyp, allergic fungal sinusitis, cystic fibrosis, or immotile ciliary disease. Control tissues were obtained during other rhinologic surgeries, such as skull base, lacrimal duct or orbital decompression surgery, from patients without any sinonasal diseases. UP tissue was obtained from control subjects and those with CRSsNP or CRSwNP. NP tissue was also obtained from CRSwNP patients. All samples were homogenized with a mechanical homogenizer at 1,000 rpm for 5 minutes on ice. After homogenization, the suspensions were centrifuged at 3,000 rpm for 10 minutes at 4ºC, and the supernatants were separated and stored at −80ºC for further analysis of cytokines and other inflammatory mediators. The atopic status of study subjects was evaluated using the ImmunoCAP^® assay (Phadia, Uppsala, Sweden) to detect immunoglobulin E (IgE) antibodies against 6 mixtures of common aeroallergens (house dust mites, molds, trees, weeds and grass pollen, and animal dander). Subjects were considered atopic if the allergen-specific IgE level was greater than 0.35 kU/L to any 1 or more of the allergens. A diagnosis of asthma was based on the medical history and lung function analysis, including methacholine challenge test by an allergist. In this study, CRSwNP were classified as eosinophilic CRSwNP (E-CRSwNP) if eosinophils comprised more than 10% of the inflammatory cell population and as non-eosinophilic CRSwNPs (NE-CRSwNP) if eosinophils comprised less than 10% of the inflammatory cells.1120 Additional information and details of the subjects' characteristics are listed in Table 1.

The protein concentrations for tissue extracts were determined using the Pierce 660 nm Protein Assay Kit (Thermo Scientific Inc., New York, NY, USA). All the protein levels in the tissue homogenate were normalized to the concentration of total protein (mg/mL). Samples were thawed at room temperature and vortexed to ensure well-mixed samples. In the present study, multiplex cytokine analysis kits (IL-1α, IL-1β, IL-2Rα, IL-4, IL-5, IL-6, IL-10, IL-13, IL-17A, IL-22, IL-23, interferon [IFN]-γ, tumor necrosis factor [TNF]-α, C-C motif chemokine ligand [CCL]-11, CCL-24, RANTES, CXCL-1, CXCL-2, CXCL-8, myeloperoxidase [MPO], monocyte chemoattractant protein [MCP]-4, vascular cell adhesion molecule [VCAM]-1, intercellular adhesion molecule [ICAM]-1, matrix metallopeptidase [MMP]-1, MMP-2, MMP-3, MMP-9, tissue inhibitor of metalloproteinase [TIMP]-1 were obtained from R&D systems (Cat. No. LMSAHM), and data were collected using Luminex 100 (Luminex, Austin, TX, USA). Data analysis was performed using the MasterPlex QT version 2.0 (MiraiBio, Alameda, CA, USA). Sensitivity of each cytokine is as follows: IL-1α (0.9 pg/mL), IL-1β (0.8 pg/mL), IL-2Rα (1.3 pg/mL), IL-4 (9.3 pg/mL), IL-5 (0.5 pg/mL), IL-6 (1.7 pg/mL), IL-10 (1.6 pg/mL), IL-13 (32.4 pg/mL), IL-17A (1.8 pg/mL), IL-22 (11.7 pg/mL), IL-23 (11.4 pg/mL), IL-33 (1.8 pg/mL), IFN-γ (0.4 pg/mL), TNF-α (1.2 pg/mL), CCL-11 (14.6 pg/mL), CCL-24 (1.34 pg/mL), RANTES (1.8 pg/mL), CXCL-1 (5.3 pg/mL), CXCL-2 (7.86 pg/mL), CXCL-8 (1.82 pg/mL), MPO (20.4 pg/mL), MCP-4 (0.42 pg/mL), VCAM-1 (238 pg/mL), ICAM-1 (87.9 pg/mL), MMP-1 (2.7 pg/mL), MMP-2 (108 pg/mL), MMP-3 (5.3 pg/mL), MMP-9 (13.6 pg/mL) and TIMP-1 (3.42 pg/mL). All assays were run in duplicate according to the manufacturers' protocol.

Statistical analyses were performed using IBM SPSS 21 (SPSS, Inc., Chicago, IL, USA) and GraphPad Prism software 6.0 (GraphPad Software Inc, La Jolla, CA, USA). Descriptive statistics were performed, and values are described as a median ± interquartile range. For comparisons among multiple groups, the Kruskal-Wallis test was first used to establish the significant difference and then, if the significance was found, the Mann-Whitney U test was secondarily performed between 2 groups and Bonferroni correction was used to adjust the significance level for each comparison. Specific differences between 2 groups were determined by the Mann-Whitney test. Correlations were assessed by Spearman rank. The significance level was set at α value of 0.05. A multivariate analysis of multiplex or enzyme-linked immunosorbent assay (ELISA) protein data was performed using principal component analysis (PCA) on correlation matrices of protein levels of all measured mediators of inflammation.

To characterize the profile of cytokines and inflammatory mediators according to the CRS phenotype, we performed ELISA and multiplex bead-based immunoassay for key inflammatory mediators in UP tissues from controls, CRSsNP and CRSwNP, and in NP tissues from CRSwNP (Tables 2 and 3).

NP tissues from NE-CRSwNP showed higher expression levels of Th2-associated mediators (IL-4, IL-5, IL-13, CCL-11, CCL-24, MCP-4, and RANTES), Th17-associated mediators (IL-17A, IL-23, CXCL-1, CXCL-2 and CXCL-8), IFN-γ as a Th1 cytokine, pro-inflammatory cytokines (IL-1α, IL-1β, IL-2Rα and IL-6), and adhesion molecule (ICAM-1) than UP tissues from controls. These results are consistent with those of previous reports demonstrating a mixed inflammation pattern of NE-CRSwNP.111213 In the analysis of remodeling markers, the increased expression of MMP-1 and MMP-9 was observed in NP tissues from NE-CRSwNP, whereas TIMP-1 was down-regulated. Among them, the signature inflammatory markers which were at the highest level among all the groups in NE-CRSwNP were IL-17A, IL-1β, and MMP-9. Interestingly, MMP-9 has been reported to be associated with neutrophilic inflammation.2122

Meanwhile, we found that the levels of Th2-associated mediators (IL-4, IL-5, IL-13, CCL-11, CCL-2,4 and MCP-4), pro-inflammatory cytokines (IL-1α, IL-1β, IL-2Rα, and IL-6), adhesion molecule (VCAM-1 and ICAM-1) and IL-23 were increased in NP tissues from E-CRSwNP, compared with UP tissues from controls. These results were in accordance with those of previous reports demonstrating Th2-deviated inflammation in E-CRSwNP.456 In the analysis of remodeling markers, the increased expression of MMP-1, MMP-3, and MMP-9 was observed in NP tissues from E-CRSwNP. Among them, the signature inflammatory markers of E-CRSwNP are IL-5, CCL-11, MCP-4, and VCAM-1.

On the analysis of UP tissues from CRSsNP, Th2 cytokines (IL-5 and IL-13) and Th17-associated mediators (IL-17A, IL-22, IL-23, CXCL-2, and ICAM-1) and MMP-9 were significantly up-regulated, compared with controls. These results mean that CRSsNP is characterized by mixed inflammation and their immunologic characteristics are similar to those of NE-CRSwNP. However, there are no signature inflammatory markers in CRSsNP, compared with UP or NP tissues of other subtypes of CRS (Supplementary Tables S1 and S2).

To evaluate the difference in cytokines, inflammatory mediators, and remodeling markers related to the evolution of NPs, we compared levels of expression between UP and NP tissues within the same patients (Tables 4 and 5). Although NP tissues from NE-CRSwNP and E-CRSwNP showed different signature inflammatory profiles in Tables 2 and 3, both groups showed common changes in several immunologic profiles on the comparison between UP and NP tissues. We found that up-regulation of Th2-associated mediators (IL-5 and CCL-11), IL-23, IL-2Rα, VCAM-1, and remodeling markers such as MMP-3, MMP-9 were observed in both NP tissues from NE-CRSwNP and E-CRSwNP groups. However, the expression of CCL-24, MCP-4, IL-1α, and IL-6 was only increased in NP tissues from patients with E-CRSwNP, but IFN-γ expression as a Th1 cytokine was decreased in those.

To investigate whether the overall profile of multiple mediators could discriminate CRS subtypes and sinonasal tissue types, we performed the PCA using the interpretation of multivariate immunoplex data (Fig. 1). The PCA retained 4 components and it presented in Supplementary Table S3. The first component (PC1) accounted for 23.1% of the variance in the dataset and its greater discriminators were IL-1β, IFN-γ, IL-6, MMP-9, and IL-1α (in order). The second component (PC2) accounted for 14.8% of the variance in the dataset and its greater discriminators included MMP3, CCL-24, VCAM-1, MMP-1, and IL-5 (in order). Thus, PC1 represented a predominant Th1 or proinflammatory profile, whereas PC2 indicated a relative Th2 profile. In this analysis, we observed that both PC1 and PC2 were helpful in discriminating between controls and subtypes of CRS. Additionally, the Th2 profile on PC2 could help distinctly discriminate the different tissues of CRS (UP vs. NP) but were not helpful in clearly defining for subtypes of NP (NE-CRSwNP-NP vs. E-CRSwNP-NP).