A total of 96 specific pathogen-free male BALB/c mice (age, 6–8 weeks; weight, 18±2 g) were purchased from the Laboratory Animal Center of Yangzhou University (Yangzhou, China) and housed in plastic cages in a laminar flow cabinet with sterilized wood-chip bedding. The room temperature was maintained at 23±2°C and a relative humidity of 55±10% with a 12-h light-dark cycle. All mice were provided with free access to food and water. All animal experiments were approved by the Animal Care and Ethics Committee of Jiangsu University (Jiangsu, China).

As described by Wang et al (22), 50 mice were sensitized intraperitoneally on days 1 and 11 with 50 µg ovalbumin (OVA; Sigma-Aldrich; Merck KGaA, Darmstadt, Germany) and 2 mg aluminum hydroxide gel in 0.1 ml PBS. Sensitized mice were subsequently exposed to OVA (10 mg/ml in PBS) inhalation challenges for 30 min every day between days 22 and 26. Control animals received PBS. The mice were assessed for allergic inflammation of the lungs 24 h after the final lung challenge, the peripheral blood and lung tissue specimens were collected (Fig. 1A). Asthmatic mice were confirmed by the presence of lung inflammation with HE staining (Fig. 1B) and increased IgE in serum, measured by ELISA (Mouse IgE ELISA kit; AKRIE-010; Shibayagi, Shibukawa, Japan), according to the manufacturer's protocol (Fig. 1C). Lung tissue was initially perfused with PBS and mechanically crushed, followed by digestion at 37°C for 2 h in RPMI medium with 10% fetal bovine serum (Gibco; Thermo Fisher Scientific, Inc., Waltham, MA, USA) and collagenase I (0.25%), to acquire a single cell suspension. The cell suspension was filtrated through 40 mm filters for flow cytometry analysis.

Single-cell suspensions (2×10⁶ cells) from lung tissues were incubated with fluorescein isothiocyanate-labeled Lin (22–7770-72; 1:100; eBioscience, Inc., San Diego, CA, USA), PerCP/Cy5.5-labeled ICOS (107705; 1:100; BioLegend, Inc., San Diego, CA, USA) and PE-labeled T1/ST2 (145303; 1:100; BioLegend, Inc.) antibodies at 4°Cfor 30 min, and fixed with 4% paraformaldehyde for flow cytometry analysis. The FITC-IgG1 (401913; 1:200, BioLegend, Inc.), PerCP/Cy5.5-IgG1 (402027, 1:200, BioLegend, Inc.) and PE-IgG1 (12–4301, 1:200; eBioscience, Inc.) served as the isotype controls. Stained cells were analyzed with an Accuri™ C6 flow cytometer (BD Biosciences, Franklin Lakes, NJ, USA) using FlowJo software 7.6 (TreeStar, Inc., Ashland, OR, USA). ILC2s were identified as Lin-ICOS+ST2+. GITR+ cells were characterized with anallophycocyanin-labeled GITR antibody (109101; 1:200; eBioscience, Inc.) and GITRL+ cells were stained with a phycoerythrin (PE)-GITRL antibody (120305; 1:200; BioLegend, Inc.). Mouse spleen cells for flow cytometry analysis were obtained as previously described (22).

Freshly obtained lung tissue of asthmatic mice was fixed in 4% paraformaldehyde for 24 h and embedded in paraffin. Paraffin-embedded lungs were sectioned (4–6 µm) and stained with H&E for morphometric analysis. GITRs in the lungs were identified by immunofluorescence staining. As described previously (23), sections for immunofluorescence staining were heated for 3 h in a 37°C incubator and dewaxed followed by antigen unmasking. Sections were subsequently blocked with 1% (weight/volume) bovine serum albumin (Sigma-Aldrich; Merck KGaA) at 37°C for 30 min, stained with a primary antibody against mouse GITR (14–5874-80; 1:200; eBioscience, Inc.) and visualized with a goat-anti-rat PE-conjugated secondary antibody (sc-3738; 1:200, Santa Cruz Biotechnology, Inc., Dallas, Texas, USA). Finally, slides were stained in Hoechst 33342 for 10 min. All sections were coverslipped with neutral resin medium, visualized under an Olympus fluorescence microscope and analyzed using ImageJ software v2.1.4.7 (https://imagej.nih.gov/ij/).

Total RNA was isolated from frozen tissues or fresh lung cells using TRIzol^® (Invitrogen; Thermo Fisher Scientific, Inc.) and 500 ng total RNA was reverse transcribed using a PrimeScript RT reagent kit (Takara Bio, Inc., Otsu, Japan) according to the manufacturer's protocol. Based on GenBank sequences, the primers used in this study were designed by Primer Premier 5.0 software (Premier Biosoft International, Palo Alto, CA, USA) and synthesized by Invitrogen (Thermo Fisher Scientific, Inc.). Primer sequences are presented in Table I. Gene-specific PCR products were amplified with SYBR^® Premix Ex Taq (Takara Biotechnology Co., Ltd., Dalian, China) according to the manufacturer's protocol. Briefly, 95°C pre-denaturation for 3 min (1 cycle); 95°C denaturation for 10 sec, 60°C annealing for 30 sec, 72°C extension for 1 min (30 cycles). The levels of target gene expression were normalized to β-actin expression using the 2^−∆∆Cq method (24). All samples were performed in triplicate.

The murine GITRL fusion protein and control protein were expressed in E. coli BL-21 with mGITRL-Pet-32a and eGFP-Pet-32a as previously described (25,26), respectively. Expression was performed at 30°C, and induced with 1 mmol/lisopropyl β-D-1-thiogalacto-pyranoside (Sigma-Aldrich; Merck KGaA) for 6 h, fusion proteins were purified by an immobilized affinity chromatography nickel column (Bio-Rad Laboratories, Inc., Hercules, CA, USA). The endotoxin was removed using a ToxinEraser^™ Endotoxin Removal kit (Genscript, Piscataway, NJ, USA). A total of 1–5 days prior to the first OVA challenge, the asthmatic mice were treated intravenously with 20 µg purified recombinant mGITRL protein and control protein per mice per day.

Plasma IL-5 and IL-13 were measured by ELISA, according to the manufacturer's protocols (IL-5, LS-F262; eBioscience, Inc; and IL-13, EM016; Shanghai ExCell Biology, Shanghai, China). All samples were measured in triplicate using a microplate reader, and the mean concentration was calculated from the standard curve.

All statistical analyses were performed using GraphPad Prism Version 5.0 software (GraphPad Software, Inc., La Jolla, CA, USA). Data are presented as the mean ± standard deviation. Comparisons between two groups were performed using independent-samples t-test. Pearson's correlation was used to detect the correlation between two continuous variables. P<0.05 was considered to indicate a statistically significant difference.

Flow cytometry analysis demonstrated that the percentage of GITR-positive cells in the spleen (Fig. 2A) and lung tissue (Fig. 2B) were significantly increased in asthmatic mice. Immunofluorescence staining indicated that increased GITR-positive cells were present in inflammatory lung tissue (Fig. 2C). Additionally, GITR mRNA expression in lung tissues of asthmatic mice was determined by RT-qPCR, and was demonstrated to be increased 2-fold compared with control mice (Fig. 2D). GITR and its ligand, GITRL, have been previously demonstrated to regulate the reactivity of various different cell types and to influence a variety of immunological conditions (11). Therefore, the present study detected the expression level of GITRL in the lung tissue of asthmatic mice and observed that its expression was additionally increased compared with control mice (Fig. 2E). The results indicated that GITR/GITRL signaling may be enhanced in asthmatic mice.

ILC2s were identified as Lin-ICOS+ST2+. The frequency of ILC2s in lung tissue from asthmatic mice was significantly increased compared with controls (Fig. 3A). RORα has been previously demonstrated to have a crucial function in ILC2 development and function, and ST2 is a surface marker that is expressed by and is relatively specific to ILC2s. The present study additionally detected the expression levels of RORα, ICOS and ST2 mRNA by using RT-qPCR. mRNA expression levels of ICOS (Fig. 3B), ST2 (Fig. 3C) and RORα (Fig. 3D) were significantly increased in the lung tissues of asthmatic mice compared with control mice. The results indicated that ILC2s and ILC2-associated molecules were upregulated in the lung tissue of asthmatic mice.

It has previously been demonstrated that IL-25 and IL-33-responsive ILC2s infiltrate the lung from peripheral blood and become a primary innate source of IL-13, and additionally produce large amounts of IL-5 (27). The present study compared gene expression levels in lung tissues from the asthmatic model and control mice by RT-qPCR, and demonstrated that the mRNA expression levels of IL-13 (Fig. 4A) and IL-5 (Fig. 4B) were significantly increased in asthmatic mice, which was consistent with the results of serum testing (Fig. 4C and D, respectively).

GITR/GITRL has an important role in regulating immune polarization conditions. To understand the association between GITR and ILC2-associated molecules and cytokines in asthmatic mice, the present study analyzed the correlation between mRNA expression levels of GITR/GITRL and RORα, T1/ST2, IL-13, and IL-5. The results indicated that there was a significant, positive correlation between GITR and ILC2-associated molecules or signature cytokines in asthmatic mice (Fig. 5).

As presented in Fig. 3, ILC2s were located in the native lung tissue of mice and were induced by intranasal OVA administration. Once lung cells from PBS-and OVA-treated mice had been obtained, lung ILC2s were identified as Lin-ICOS+ST2+ cells and the expression of GITR and GITRL expression on resting and activated lung ILC2s was investigated by flow cytometry. As presented in Fig. 6A, different expression levels of GITR amongst control, PBS-treated and OVA-treated groups was observed; however, GITRL expression levels were more consistent in the three groups.

To determine the effect of GITRL on AHR, sensitized mice were treated intravenously with 20 µg GITRL or control protein prior to the first OVA challenge, and lung ILC2s were subsequently analyzed by flow cytometry. Compared with the controls, GITRL administration induced a significant increase in the frequency of GITR+ cells (Fig. 6B) and ILC2s (Fig. 6C) in lung tissue.