key: cord-0004214-iwvjz3bf authors: Hebert, K. D.; Mclaughlin, N.; Galeas-Pena, M.; Zhang, Z.; Eddens, T.; Govero, A.; Pilewski, J. M.; Kolls, J. K.; Pociask, D. A. title: Targeting the IL-22/IL-22BP axis enhances tight junctions and reduces inflammation during influenza infection date: 2019-10-09 journal: Mucosal Immunol DOI: 10.1038/s41385-019-0206-9 sha: 3b39a84673e9b497f2592d45ec63bccdebb63acf doc_id: 4214 cord_uid: iwvjz3bf The seasonal burden of influenza coupled with the pandemic outbreaks of more pathogenic strains underscore a critical need to understand the pathophysiology of influenza injury in the lung. Interleukin-22 (IL-22) is a promising cytokine that is critical in protecting the lung during infection. This cytokine is strongly regulated by the soluble receptor IL-22-binding protein (IL-22BP), which is constitutively expressed in the lungs where it inhibits IL-22 activity. The IL-22/IL-22BP axis is thought to prevent chronic exposure of epithelial cells to IL-22. However, the importance of this axis is not understood during an infection such as influenza. Here we demonstrate through the use of IL-22BP-knockout mice (il-22ra2(−/−)) that a pro-IL-22 environment reduces pulmonary inflammation during H1N1 (PR8/34 H1N1) infection and protects the lung by promoting tight junction formation. We confirmed these results in normal human bronchial epithelial cells in vitro demonstrating improved membrane resistance and induction of the tight junction proteins Cldn4, Tjp1, and Tjp2. Importantly, we show that administering recombinant IL-22 in vivo reduces inflammation and fluid leak into the lung. Taken together, our results demonstrate the IL-22/IL-22BP axis is a potential targetable pathway for reducing influenza-induced pneumonia. The seasonal burden of influenza, coupled with the potential catastrophe of pandemic outbreaks, underscores the critical need for understanding the pathophysiology of influenza injury. Vaccination remains a cornerstone in the prevention of infection. However, vaccine efficacy can vary from 50 to 80% in a healthy population 1 and is significantly decreased in groups such as the immune compromised, 2 very young children and the elderly. 1 Thus, while much of the focus is on prevention, there are significant populations that remain at risk of infection. With the recent emergence of more pathogenic strains such as the 2009 and 2014 H1N1, infection can have more devastating consequences. During the 2013-2014 influenza season alone, it was reported that a very high number of young, otherwise healthy individuals required critical care in the intensive care unit, with a high percentage (72%) of these patients developing acute respiratory distress syndrome (ARDS) and respiratory failure requiring ventilator therapy. 3 The current course of treatment for these patients consists of anti-viral therapies (Oseltamvir or Zanamivir), which are most effective when given within 48 hours of the onset of symptoms. This is often well outside the window in which individuals seek medical attention. Given the tremendous inflammation and injury that occurs in the lung after influenza infection, effective therapeutic regimens should be focused on reducing viral burden, while decreasing inflammation and at the same time promoting lung/epithelial repair. The host response to influenza infection has been the subject of intense research to determine whether aspects of this response can be exploited therapeutically. It is important to understand that cytokines play critical roles in both regulating protective and reparative processes as well as causing injury. Interleukin-22 has great potential in reducing pulmonary injury and promoting epithelial repair. Its limited receptor distribution allows IL-22 to have a focused effect on the epithelium. Through the IL-22Ra1/IL-10Rb receptor complex, IL-22 activates signal transducer and activator of transcription 3 (STAT3) in the lung epithelium, thereby augmenting barrier function, epithelial repair, and the induction of anti-microbial genes. 4 Our lab 5 and others [6] [7] [8] have shown that IL-22 is important for recovery during influenza infection, as Il22 −/− mice have more severe injury. Moreover, we showed IL-22 receptor distribution in the lung and its importance in reducing lung pathology in both the airways and lung parenchyma after influenza challenge. We also found that Il22 −/− mice infected with H1N1 PR/834 have enhanced structural lung pathology, defective expression of genes that control epithelial repopulation, and increased evidence of fibrosis. 5 Generally, IL-22 is not found in the naive lung and is produced by activated T cells following infection. In the case of influenza, IL-22 is produced by both natural killer (NK) and natural killer T (NKT) cells. 7, 9 Once it is produced, it can be post-translationally regulated through interactions with IL-22-binding protein (IL-22BP). This soluble receptor is a naturally occurring antagonist that has a 20-1000-fold higher affinity for IL-22 than the membranebound IL-22Ra1. [10] [11] [12] IL-22BP binds IL-22 at a site that is directly adjacent to and interferes with the binding of both its membranebound receptors, IL-22Ra1 and IL-10Rb. 11 When bound to IL-22BP, IL-22 is unable to signal through STAT3. [10] [11] [12] There are currently three isoforms that have been identified in humans. 9 Isoform 1 is retained intracellularly and does not bind IL-22. Human isoform 1 has been found to interact with components of the unfolded protein response. 13 Human isoform 2 is most closely related to the single murine isoform of IL-22BP and is induced under inflammatory conditions. Human isoform three binds IL-22 with less affinity than human isoform two and is present at high levels during homeostatic conditions. 10 In the intestine, IL-22BP is made by dendritic cells 14, 15 and is regulated by the inflammasome. 15 Neutralizing IL-22BP in the lung significantly increases survival and decreases neutrophilia in a mouse model of Pseudomonas aeruginosa. 16 Under naive conditions in the lung, alveolar epithelial cells and alveolar macrophages (AMs) have been identified as sources of IL-22BP, 17, 18 and neutrophils are a source during catastrophic lung injury. 18 In the current study, we demonstrate that shifting the balance of the IL-22/IL-22BP axis in favor of IL-22 promotes recovery during influenza infection by promoting tight junction formation. We demonstrate that NK and CD45 − cells and macrophages are main cellular sources of IL-22BP under naive conditions. However, following influenza infection, these cellular sources decrease production, whereas production by dendritic cells is upregulated. Using Il22ra2 −/− mice we demonstrate that a pro-IL-22 environment significantly reduces pulmonary inflammation and vascular leak into the lung as well as lung pathology. We further reveal that this reduction in lung leak may be due to increases in tight junctions (CLDN4, TJP1, and TJP2), which was confirmed both in vitro and in vivo. More importantly, we demonstrate that the therapeutic nature of IL-22 as oropharyngeal administration of IL-22:Fc during infection improved the epithelial barrier and reduced inflammation. Six-to 8-week-old wild-type (WT) mice (C57Bl/6) were acquired from Jackson labs. Il22ra1 fl/fl mice on a C57BL/6 (B6) background have been previously described. 19 To knock out the receptor, these mice were crossed to eIIa-cre mice. To determine functional recombination, DNA was extracted and subjected to PCR using primers spanning exon 3. To determine functional deletion of IL-22RA1, lungs were removed, and real-time PCR was performed for the Il22ra1. Il22ra2 −/− mice have been previously described and were backcrossed 12 times on a C57Bl/6 background to generate full knockouts. 15 Male mice were used for all experiments and housed in pathogen-free conditions in accordance with Tulane University's Institutional Animal Care and Use Committee. Oropharyngeal administration of influenza and IL-22:Fc All treatments were performed via oropharyngeal aspiration while mice were under isofluorane anesthesia. H1N1 (Pr8) was administered at 100 PFU (pore-forming unit) in 100 μl of sterile phosphate-buffered saline (PBS). Five micrograms of IL-22:Fc (Generon, Shanghai, China) was administered in 50 μl of sterile PBS. Cell sorting Lungs from WT mice were harvested after 5 days post infection with H1N1 (Pr8) at 100 PFU in 100 μl of sterile PBS. Lungs were placed in 2 ml of Advanced RPMI media supplemented with 10% fetal bovine serum (FBS), 1% penicillin/streptomycin, heparin (100 U/ml), and DNAse I (100 U/ml). After mincing the lungs, Liberase TH at 75 μg/ml was added. The tissue was incubated for 25 min at 37°C in an elliptical shaker. After incubation, cells passed through a 70 μM filter and incubated in red blood cell lysis buffer prior final resuspension in flow buffer. The following surface markers were used for fluorescence-activated cell sorting (FACS): CD45 (Tonbo Biosciences, San Diego, CA), CD11b, CD11c, anti-γδ, CD3, CD4, NK1.1 (all from BioLegend, San Diego, CA), and Siglec F (BD Biosciences, San Jose, CA). Cells were sorted using a FACSAria II instrument (BD Biosciences). Cells from naive mice were isolated and sorted as described above as controls. For flow sorting, single cells (based on forward and side scatter) were gated as follows: (1) γδ T cells = CD45 + , CD3 + , γδ + ; (2) NK cells = CD45 + , NK1.1 + ; (3) interstitial macrophages (IMs) = CD45 + , F4/80 + , CD11b + , Siglec F − ; (4) AMs = CD45 + , F4/80 + , CD11b + , Siglec F + ; and (5) dendritic cells = CD45 + , F4/80 + , CD11c + ,CD103 + . An aliquot of each sorted population was resorted post collection to verify purity, which was >97% for all populations. Analysis of lung inflammation and injury Mouse lungs were lavaged with 1 ml of sterile PBS. Bronchoalveolar lavage 20 was then used for evaluation of inflammatory cells by differential cell counting. To measure lung injury, total protein in the first milliliter of bronchoalveolar lavage (BAL) fluid was measured using the BCA Protein Assay Kit (Pierce Chemical, Rockford, IL). Lactate dehydrogenase (LDH) activity was measured using the LDH assay (Sigma-Aldrich, St. Louis, MO). Both assays were performed in a 96-well plate for 30 min according to the manufacturer's instructions and analyzed using the Benchmark Plus plate reader (Bio-Rad, Hercules, CA). To measure lung leak, the Evan's blue assay was used. Briefly, mice were injected intravenously (i.v.) with a 0.1% sterile solution of Evan's blue dye 30 min prior to sacrifice. The mouse paws and nose turning blue after injection verified dissemination of the dye visually. Evan's blue was measured in the BAL by measuring absorbance at 620 nm on a spectrophotometer. Right lung lobe from a separate cohort of mice was used to measure differences in inflammatory cells in the lung by flow cytometry. Briefly, CD45 + cells differentiated total inflammatory cells. F4/80 was used to differentiate total macrophages. M2 macrophages were differentiated by double-positive MHCII + and CD206 + cells. M1 macrophages were differentiated by MHCII + CD206 − cells. For histopathology, the left lung was fixed with 10% neutral-buffered formalin before dehydration and paraffin embedding. Paraffin blocks were sectioned at 5 μm and stained with hematoxylin and eosin. To score the pathology, slides were blinded and full-field low magnification (×2) images were taken from three sections per mouse. Total inflammation was scored by outlining and measuring the inflamed area using ImageJ and dividing by the total outlined area of the lung section. Numerical scoring was performed as previously described. 5 Briefly, airway pathology was scored on a scale of 1-4 as follows: 0 = no obvious signs of infection; 1 = mild peribronchiolar inflammation; 2 = mild mucus cell metaplasia; 3 = mucus cell metaplasia with obvious inflammation; 4 = severe mucus cell metaplasia, epithelial piling, and severe inflammation. Alveolitis was scored on a 1-4 scale as well. This scale was: 0 = no obvious inflammation; 1 = minimal focal inflammation; 2 = multifocal, mild inflammation; 3 = diffuse, conspicuous coalescing inflammation; and 4 = severe parenchymal inflammation with no obvious airspaces. Cytokine analysis Cytokine analysis was performed on whole lung supernatants from single-cell suspensions using the Bio-Rad BioPlex Pro Mouse Cytokine 23-Plex Kit as per the manufacturer's instructions and luminescence detected using the Bio-Rad BioPlex 200 (Bio-Rad, Hercules, CA). Bronchial brushings Mice were euthanized by CO 2 inhalation and cervical dislocation was performed. The rib cage was removed to visualize the lungs. The trachea was exposed, and an incision was made to remove the viscera and muscle around it. Carefully, a small incision was made into the trachea and an abraded PE-10 polyethylene tubing (BD Biosciences, San Jose, CA) was then used to brush inside each branch of the right and left side of the upper airways. One piece of tubing was used to brush each side, respectively. Tubing from each bronchial brushing was transferred into 200 μl Trizol (Life Technologies, Carlsbad, CA) and then flash frozen until RNA isolation as described in quantitative reverse transcription PCR (RT-qPCR) section. The presence of upper airway cells were confirmed via RT-qPCR for Scgb1a1. Cell culture For air-liquid interface (ALI) cultures, fully differentiated HBE cell cultures were derived from the Center for Organ Recovery and Education. Cells were prepared using previously described methods 21 approved by the University of Pittsburgh IRB. Briefly, bronchi from the second to sixth generations were collected, rinsed, and incubated overnight in Eagle's minimum essential medium at 4°C. The bronchi were then digested in MEM containing protease XIV and DNase. The epithelial cells were removed and collected by centrifugation and then resuspended in bronchial epithelial growth medium and plated onto collagentreated tissue culture flasks. When 80-90% confluence was reached, the passage 0 cells were trypsinized and seeded onto collagen-coated transwell filters. Upon reaching confluence, the cultures were maintained at an ALI and media were changed basolaterally twice weekly. Individual experiments were performed on cells grown from a single donor. There were four total donors for the experiments performed here. BEAS-2B and primary normal human bronchial epithelial (NHBE) cells (Lonza, Allendale, NJ) were cultivated in bronchial epithelial cell basal medium (BEBM) with BEGM SingleQuots (Lonza, Allendale, NJ) and 1% penicillin/streptomycin. For primary cell lines, all plates were coated with 0.01 mg/ml human fibronectin (Corning, Oneonto, NY), 0.03 mg/ml bovine collagen type I (Advanced Biomatrix, Carlsbad, CA), and 0.01 mg/ml bovine serum albumin (Fisher Bioreagents, Waltham, MA) in serum-free BEBM. A549 cells were cultivated in Dulbecco's modified Eagle's medium (DMEM) with 10% FBS and 1% penicillin/streptomycin. For maintenance of all stock cultures, cells were grown to~70% confluence, and then dissociated using 0.25% Trypsin-EDTA (Gibco, Waltham, MA). For primary cell lines, after dissociation cells were transferred to a 50 ml conical then spun down at 500 × g for 5 min. Trypsin was then aspirated and fresh BEBM growth media were added before plating cells. H1N1 infection of cell culture Cells grown at ALI were infected apically with 2009 H1N1 (multiplicity of infection (MOI) 100) in 50 μl of media. Media were removed after 4 h. Transepithelial resistance was measured using a voltmeter (Evom2 Epithelial Voltohmmeter, World Precision Instruments). IL-22:Fc was added to the basal media. For non-ALI cultures, cells were seeded in 6-well plates at 3.0 × 10 5 cells/well and allowed to grow near 70% confluency in their respective growth media (DMEM or BEBM). A549 cells were then serum starved in DMEM with 1% FBS. After 24 h, cells were then infected with Pr8 (MOI 50). Following infection cells were treated with 30 ng/ml of IL-22 (R&D Systems, Minneapolis, MN) for an additional 24 h. Cells were then harvested in Trizol (Life Technologies, Carlsbad, CA) for RNA extraction or fixed in 4% paraformaldehyde (PFA) for immunofluorescence analysis after 48 h. Immunofluorescence NHBE cells were seeded at 0.05 × 10 5 cells/well on glass bottom 24-well plates and grown to near 70% confluency. Once 70% confluent, cells were serum starved in DMEM with 1% FBS. Cells were then infected for 24 h at MOI 50 (Pr8). Followed by treatment with 30 ng/ml of IL-22 (R&D Systems, Minneapolis, MN) for an additional 48 h. At the end of the treatment time period, cells were then fixed in 4% PFA and permeabilized in 0.2% Triton X-100. Cells were washed with PBS and blocked in 5% normal goat serum and then stained for ZO-1 (Invitrogen, Carlsbad, CA) at 10 μg/ml for 1 h each, respectively. Goat anti-rabbit 488 (Invitrogen, Carlsbad, CA) was then used as a secondary antibody and samples were counterstained with DAPI (4′,6-diamidino-2-phenylindole). EVOS FL Auto Imaging System (Thermo Fisher Scientific Inc., Carlsbad, CA) was used for analysis. RT-qPCR RNA isolation was performed on cells and bronchial brushings using the Trizol method (Life Technologies, Carlsbad, CA). Briefly, 200 μl of chloroform and 200 μl of sterile PBS was added to each sample and shaken vigorously for 30 s. Samples were incubated for 10 min and then spun down at 12,000 × g for 15 min at 4°C. The aqueous phase was then placed into 500 μl isopropanol, mixed lightly, and incubated for 5 min. Samples were then spun down at 12,000 × g for 10 min at 4°C. Supernatant was decanted and then 1 ml of 75% ethanol was added to each sample and spun down at 7600 × g for 5 min. This step was repeated twice and then RNA pellet was allowed to air dry before adding 30 μl of nuclease-free water. RNA was quantified by NanoDrop and quality was determined by a 260/280 verification of~2. One microgram of RNA was reverse transcribed using iScript (Bio-Rad, Hercules, CA) and verified by RT-PCR amplification of the glyceraldehyde 3phosphate dehydrogenase (GAPDH) housekeeping gene. TaqMan Gene Expression primers (Applied Biosystems) were used to determine levels of: GAPDH (Hs02758991_g1), CLDN2 (Hs00252666_s1), CLDN4 (Hs00976831_s1), TJP2 (Hs00910543_m1), Gapdh (Mm99999915_g1), Cldn4 (Mm00515514_s1), Ocln (Mm005 00912_m1), Tjp1 (Mm00493699_m1), IL-22Ra2 (Mm01192969_m1), and Tjp2 (Mm00495620_m1). Statistical analysis All data are represented as the mean ± SEM. Significance was determined using either an unpaired two-tailed t test when comparing two groups or a one-way analysis of variance (ANOVA) with Tukey's adjustment when comparing multiple groups. All statistics were calculated using GraphPad Prism 6. Il22ra2 −/− mice have rapid recovery from influenza infection IL-22 is beneficial at the epithelial surface during infection. 5, 7, 8, 22 Under naive circumstances, Il22 transcripts are not measured in the lung, while Il22ra2 transcripts can be found at relatively abundant levels (Fig. 1a) . During influenza infection, Il22 transcript can be measured starting 4 days after infection and peaking around day 6. This is accompanied by a reduction in il22ra2 starting at day 4 and not returning until day 12 (Fig. 1b) . We have had difficulty finding reliable antibodies to measure mouse IL-22BP. Therefore, to determine the source of IL-22BP following influenza infection, cells were FACS sorted from whole lung digests of naive mice or mice 5 days post infection. Under naive conditions, Il22ra2 was produced by CD45 − cells, NK cells, and both IMs and AMs macrophages. Within 5 days of influenza infection, expression of Il22ra2 was lost in these cells, while expression of Il22ra2 was increased in dendritic cells (Fig. 1c) . While loss of IL-22 during influenza infection is associated with epithelial disrepair, [5] [6] [7] to date there are no publications investigating the impact of IL-22BP in the lung during influenza infection. To determine the importance of IL-22BP during influenza infection, Il22ra2 −/− mice were infected with a sub-lethal concentration (100 PFU) of influenza (A/PR8) and followed for 10 days. Over this time period, the Il22ra2 −/− mice lost significantly less weight and began recovering more rapidly than WT controls (Fig. 2a) . While IL-22 can have anti-microbial properties in the lung, it was not known if IL-22 would promote anti-viral response. As such, we measured influenza burden by real-time qPCR for the viral M1 gene as we have previously described. 5, 23 We found that despite the differences in weight loss, there were no significant differences in viral burden between Il22ra2 −/− and WT mice at 6 dpi (days post infection) and both groups cleared the virus by day 10 (Fig. 2b) . The viral burden findings were not that surprising, as Il22 −/− mice do not have any differences in viral clearance with the major phenotype in the Il22 −/− mice being decreased epithelial repair. [5] [6] [7] Therefore, we next examined histopathology. PR8 infection commonly induces severe airway and parenchymal inflammation at day 10, as seen in Fig. 2c . Il22ra2 −/− mice had decreased parenchymal inflammation (Fig. 2c-f) , with mild inflammation around the airways (Fig. 2c, d) . Moreover, we did not see a difference in the number of affected airways (as seen by surrounding inflammation and mucous cell metaplasia) or amount of airway metaplasia (Fig. 2e) , suggesting that there was equal distribution of virus. We did, however, observe less alveolitis (Fig. 2f) . Il22ra2 −/− mice have decreased inflammation The differences in the inflammatory dissemination observed from the histopathology were somewhat surprising as IL-22 has not been found to have a profound impact on inflammation during influenza infection. [5] [6] [7] To better understand the changes occurring in the inflammatory compartment, bronchoalveolar lavage 20 fluid was collected and total inflammatory cells were counted. There were no differences in the BAL of mock-infected WT and Il22ra2 −/− mice (Fig. 3a, b) with >98% of the cells being macrophages (data not shown). In conjunction with the histopathology data, Il22ra2 −/− mice had decreases in inflammation. At day 5, where the weight loss curves began to diverge, there was a decrease in total inflammation (Fig. 3a) as well as a reduction in the total number of T cells (Fig. 3c) . These data corresponded with decreased cytokine levels of IL-6, IL-17, interferon-γ (IFN-γ), and RANTES (regulated on activation, normal T cell expressed and secreted) (Fig. 3f) . Inflammatory changes persisted through day 10, where Il22ra2 −/− mice had significant decreases in total inflammatory cells (Fig. 3b) . In comparison to day 5, both groups had decreases in total neutrophils and lymphocytes with an increase in macrophage numbers. This increase was significantly abrogated (p < 0.0001) in the Il22ra2 −/− mice however (Fig. 3d) . Differences in types of macrophages were investigated as they were the most robustly altered between the WT and il22ra2 −/− groups at day 10. Despite significant differences in total numbers of macrophages between the groups, the ratio of M2 (CD45 + F4/80 + MHCII + CD206 + )/M1 (CD45 + F4/80 + MHCII + CD206 − ) macrophages remained unchanged (Fig. 3e) . Il22ra2 −/− mice have decreased pulmonary injury and pulmonary edema Previous work from our lab has shown Il22-knockout mice have severe epithelial injury and reduced epithelial repair during influenza infection. 5 We therefore hypothesized that a pro-IL-22 signaling environment would lessen the pulmonary injury seen during influenza infection. To test this Il22ra2 −/− , mice were sacrificed 5 dpi, during optimal IL-22 expression. We found that Il22ra2 −/− mice had significantly less injury as measured by LDH Fig. 4a) . Further, they had significantly less leak into the lung as measured by total protein in the BAL (Fig. 4b) . To confirm these data, a subset of influenza-infected mice were injected (i.v.) with Evan's blue dye 30 min prior to sacrifice. Similar to the total protein data, Il22ra2 −/− mice had significantly less dye in the BAL (Fig. 4c) , demonstrating less pulmonary edema during influenza infection. Loss of barrier function from influenza infection has been attributed to reduced claudin expression in epithelial cells leading to reduced tight junction formation. 24 To understand if our observed differences in lung leak were associated with changes in tight junction proteins, we analyzed gene expression of claudins and tight junction proteins. RNA was collected from mouse bronchial brushings (5 dpi), allowing us to focus primarily on epithelial gene expression. In agreement with the pulmonary leak data, we found Il22ra2 −/− mice had significantly higher expression of Tjp1,Tjp2, Cldn4, and Ocln during infection (Fig. 4d) . The in vivo findings suggest that a pro-IL-22 signaling environment (decreased IL-22BP and increased IL-22) protects the epithelial barrier by promoting tight junction formation. To verify these findings, we next took an in vitro approach. Human lung airway epithelial cells grown at ALI were infected with influenza (2009 H1N1 MOI 100). Cells were treated with human IL-22:Fc one day after infection and barrier integrity was monitored by measuring resistance across the monolayer (transepithelial/endothelial electrical resistance (TEER)). Interestingly, treatment with IL-22 was not protective, as membrane resistance was lost in both groups. However, IL-22 treatment did promote a faster recovery in membrane resistance by day 3 (Fig. 5a) . In conjunction with these data, we found IL-22 treatment of NHBE cells grown in collagen induced TJP1 (Fig. 5b) and a significant increase in CLDN4 (Fig. 5c) . We also found that IL-22 promoted restoration of ZO-1 in influenza-infected A549 cells (MOI 50) (Fig. 5d, e) . The ability to reduce leak into lung has promise in preventing severe influenza-induced pneumonia and the resultant ARDS that occurs. To test the impact of IL-22 administration, we used a human recombinant (r)IL-22:Fc, 25 which is capable of signaling on mouse cells (Fig. 6a) . Mice were treated with IL-22:Fc or Fc control 6 days after infection, when the expression of Il22ra2 significantly wanes (Fig. 1b) . Measurement of vascular leak into the lung revealed a significant decrease 24 hours after IL-22:Fc treatment (Fig. 6b) . To confirm these results were not due to off-target effects of the human IL-22 or the Fc, we performed experiments in mice lacking the IL-22 receptor. Il22ra1 −/− mice 19, 26 were crossed with eIIa-cre +/+ (eIIa cre ) mice. This cre is expressed in the early mouse embryo and thus causes recombination and excision of Il22ra1 globally. eIIa cre × Il22ra1 fl/fl or eIIa cre controls were infected and treated at days 6 and 8 after infection. Although not significant, IL-22R-competent mice, but not IL-22R-deficient mice, recover weight after IL-22 treatment. Moreover, results showed that IL-22:Fc treatment significantly reduced the influx of inflammatory cells in the BAL of eIIa cre mice, but not the mice lacking the IL-22 receptor (eIIacre +/+ × Il22ra1 fl/fl ) (Fig. 6d) or in control-treated mice. These data demonstrate that IL-22 signaling through the IL-22 receptor can significantly restore lung tight junctions and reduce inflammation. 8 as expression of Il22 increase in response to influenza infection, there is a reduction of Il22ra2. This is during the same time that the IL-22Ra1 is increased on epithelial cells. 5, 28 These changes allow the lung to become a more permissive environment for IL-22 activity. This has been confirmed by microarray studies in which only 431 genes were differentially regulated after IL-22 treatment in naive mice as opposed to 1231 genes after IL-22 treatment in influenza-infected mice. 22 With the exception of rotavirus, 29 IL-22 does not alter viral load in other organ systems. 30, 31 We confirm these observations, as a pro-IL-22 signaling environment in il-22ra2 −/− mice had no bearing on influenza burden. Our studies are further supported by findings in the Il22 −/− mice, which also had no differences in viral burden. [5] [6] [7] Interestingly, our findings in the Il22ra2 −/− mice demonstrate that pulmonary recovery is independent of the viral load of the animal. The decreased inflammation in the Il22ra2 −/− mice was somewhat surprising, as Il22 −/− mice have no inflammatory phenotype during influenza infection. [5] [6] [7] The effects of IL-22 are dependent on the inflammatory milieu and it has been hypothesized that the evolutionary function of IL-22BP is to act e Comparative quantification of ZO-1 mean fluorescent intensity by group. Statistical analysis was performed using one-way ANOVA with Tukey's post hoc test. n = 5 and is representative of three experiments. *p < 0.05, **p < 0.01, ***p < 0.001, and ****p < 0.0001 as a rheostat controlling the concentration of IL-22 in the milieu and thus its function. 10 We found significantly enhanced expression of IL-6, IL-17, IFNγ, and RANTES in WT mice when compared to Il22ra2 −/− mice. Both IL-6 and IL-17 have negative implications in influenza infection. IL-6 is associated with more severe infection 32 and clinically worse outcomes. 33 Similarly, IL-17 is associated with exacerbated influenza associated pathology [34] [35] [36] While it is unclear if IL-22 reduces IL-17 or IL-6 directly or through a general reduction of inflammation, it is likely that the reduction of these two cytokines is associated with the improved recovery observed in the Il22ra2 −/− mice. We found that IL-22 promotes tight junction formation during influenza infection, reducing fluid buildup in the lung and induces claudin-4 both in vivo and in vitro. This tight junction transmembrane protein is found on epithelium throughout the lung. 37 It functions to promote fluid clearance through paracellular chloride efflux. 38 It is induced during mechanical trauma [39] [40] [41] and induction is considered protective in lung injury in both mice and humans. [39] [40] [41] [42] During influenza, claudin-4 is the primary tight junction protein that is decreased. 24 The increased claudin-4, as well as other scaffold proteins (zo-1 and zo-2) likely account for the reduced fluid buildup seen in pro-IL-22 conditions. These data not only have implications for influenza, they are also promising for other injurious or infectious situations that induce acute lung injury. Admittedly, a caveat to these studies is that mice have only one isoform of IL-22BP as opposed to humans who have three. 10, 17, 43 The different isoforms have varied distribution throughout the body as well as varying affinity for IL-22. 10, 17, 43 The mouse Il-22ra2 is homologous to the human isoform 2 (IL-22Ra2v2), which has the highest affinity for IL-22. 10, 44 This isoform was initially thought to be the predominant isoform. 17, 43 However, it has been recently shown that the third isoform (IL-22Ra2v3) is the most highly expressed isoform in most healthy organs, including the lung. 10 Isoform 2, on the other hand, has been found to be induced during inflammatory triggers such as TLR2 activation 10 and retinoic acid 45 in vitro. While it is unclear what happens to the balance of these isoforms in vivo during infection, it is likely our findings presented here are representative of the IL-22/IL-22BP (isoform 2) axis during infection. Our studies demonstrate that tipping the IL-22/IL-22BP axis in favor of IL-22 is beneficial during influenza infection. Furthermore, targeting this axis has also proven useful in lung bacterial infections 4, 19 and fungal infections, 46 as well as bacterial co-infections. 8, 22 The question remains though-If IL-22 is so important in resolving infection, why is it so tightly controlled and is it safe to target? The answers to this can be found at other epithelial surfaces. In the skin, overabundance of IL-22 is associated with increased inflammation and psoriasis [for a review see ref. 47 ] and reduced expression of IL-22BP only exacerbates this process. 48, 49 In the intestine, where IL-22 is constitutively expressed to protect the mucosal surface, 50 Il22ra2 −/− mice develop greater number of tumors in a colitis cancer model. 15 Therefore, too much IL-22 can have negative consequences. This does not preclude the positive, potentially therapeutic data we present here. Our studies examine very acute responses to IL-22/ IL-22BP imbalance and therefore not likely to induce pathology that is seen in diseases of chronic IL-22/IL-22BP imbalance. The IL-22/IL-22BP axis has likely evolved to protect organs from the potentially inflammatory and proliferative effects of chronic IL-22 exposure. The balance between the two proteins naturally shifts during influenza infection, to allow the lung to be more pro-IL-22. While knocking out Il22ra2 has a profound benefit on recovery during influenza infection, there are currently not any known therapeutic approaches designed to do this. Administration of IL-22:Fc may prove to be more beneficial. IL-22:Fc is currently in clinical trials for intestinal graftversus-host disease (NCT02406651) and alcoholic hepatitis (NCT02655510) and may prove to be a useful therapy during influenza-induced pneumonia. 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