Michelle L Manni1, Sivanarayana Mandalapu1, Andres Salmeron2, Jose M Lora2, Jay K Kolls3, John F Alcorn1. 1. Department of Pediatrics, Children's Hospital of Pittsburgh of UPMC, Pittsburgh, PA USA. 2. Constellation Pharmaceuticals, Inc., Cambridge, MA USA. 3. Richard King Mellon Foundation Institute for Pediatric Research, Children's Hospital of Pittsburgh of UPMC, Pittsburgh, PA USA.
Abstract
Atopic asthma is a prevalent respiratory disease that is characterized by inflammation, mucus hypersecretion, and airway hyperresponsiveness. The complexity of this heterogeneous disorder has commanded the need to better define asthma phenotypes based on underlying molecular mechanisms of disease. Although classically viewed as a type 2-regulated disease, type 17 helper T (Th17) cells are known to be influential in asthma pathogenesis, predominantly in asthmatics with neutrophilia and severe refractory disease. Bromodomain and extra-terminal domain (BET) chromatin adaptors serve as immunomodulators by directly regulating Th17 responses and Th17-mediated pathology in murine models of autoimmunity and infection. Based on this, we hypothesized that BET proteins may also play an essential role in neutrophil-dominant allergic airway disease. Using a murine model of neutrophil-dominant allergic airway disease, we demonstrate that BET inhibition limits pulmonary inflammation and alters the Th17-related inflammatory milieu in the lungs. In addition, inhibition of BET proteins improved lung function (specifically quasi-static lung compliance and tissue elastance) and reduced mucus production in airways. Overall, these studies show that BET proteins may have a critical role in asthma pathogenesis by altering type 17 inflammation, and thus interfering with BET-dependent chromatin signaling may provide clinical benefits to patients suffering from asthma.
Atopic asthma is a prevalent respiratory disease that is characterized by inflammation, mucus hypersecretion, and airway hyperresponsiveness. The complexity of this heterogeneous disorder has commanded the need to better define asthma phenotypes based on underlying molecular mechanisms of disease. Although classically viewed as a type 2-regulated disease, type 17 helper T (Th17) cells are known to be influential in asthma pathogenesis, predominantly in asthmatics with neutrophilia and severe refractory disease. Bromodomain and extra-terminal domain (BET) chromatin adaptors serve as immunomodulators by directly regulating Th17 responses and Th17-mediated pathology in murine models of autoimmunity and infection. Based on this, we hypothesized that BET proteins may also play an essential role in neutrophil-dominant allergic airway disease. Using a murine model of neutrophil-dominant allergic airway disease, we demonstrate that BET inhibition limits pulmonary inflammation and alters the Th17-related inflammatory milieu in the lungs. In addition, inhibition of BET proteins improved lung function (specifically quasi-static lung compliance and tissue elastance) and reduced mucus production in airways. Overall, these studies show that BET proteins may have a critical role in asthma pathogenesis by altering type 17 inflammation, and thus interfering with BET-dependent chromatin signaling may provide clinical benefits to patients suffering from asthma.
Asthma is a chronic inflammatory disease of the airways and represents a significant health burden worldwide12. Allergen-specific CD4+ T helper (Th) cells drive atopic asthma pathogenesis, which is characterized by pulmonary inflammation, mucus cell metaplasia, airway remodeling, and airway hyperresponsiveness (AHR). Although once viewed as a predominantly Th2 cell-dominant disorder, it is now recognized that asthma is a clinically heterogeneous disease. In severe refractory asthma, Th2 and/or Th17 cells are thought to contribute to disease pathogenesis. Specifically, Th17 cells, which produce IL-17 and IL-22, are known to mediate neutrophilia and influence asthma severity3456. Our recent work has recognized this Th17-related phenotype in asthmatics with severe refractory disease, and has shown that different molecular mechanisms likely contribute to each of the observed asthma pathologies (inflammation, AHR, and mucus production)7. Although Th2-related disease is well studied, the complexity and diversity of the clinical presentation of asthma warrants further study to elucidate and clarify the molecular mechanisms underlying disease and ultimately establish more effective therapies.Acetylation of histones promotes the recruitment of effector proteins, alters the confirmation of chromatin, and regulates transcription of inflammatory and immunoregulatory genes8. Bromodomain and extra-terminal (BET) proteins possess bromodomain motifs that bind acetylated lysine residues in histones, thereby regulating transcription of genes involved in cellular proliferation, cell cycle progression and apoptosis9. The BET family of adaptor proteins is composed of Brd2, Brd3, Brd4, and testis-specific Brdt. Selective, small molecule inhibitors of BET proteins displace BET bromodomains from chromatin by competitively binding to the aceyl-lysine recognition pocket. This disruption of the interaction between BET proteins and acetylated histones has been shown to impede transcription of genes that mediate cellular growth and survival in cancers91011121314, control inflammatory responses15, and regulate cell function of innate and adaptive immune cells16171819.Based on the fundamental role of BET bromodomains in cell growth and proliferation, recent studies have focused on establishing a link between BET proteins and inflammatory responses in disease. Mele and colleagues have shown that BET proteins are critical for controlling both human and murine Th17 differentiation and activation as well as for regulating Th17-associated cytokine production (IL-17, IL-21, and GM-CSF)16. More importantly, their work showed that the BET family members Brd2 and Brd4 critically modulate Th17 biology by associating with the Il17 locus in a bromodomain-dependent manner, thereby directly controlling the transcription of IL-1716. A study by Chen et al. also showed BET inhibition repressed Th17 cell responses in explanted tissues from cystic fibrosis patients20. Aside from circulating immune cells, BET proteins have been shown to influence cell function and response of airway epithelial cells2021, airway smooth muscle2223, and lung fibroblasts24. Further, pharmacological inhibition of BET bromodomains was protective in murine models of autoimmunity16, bleomycin-induced pulmonary fibrosis24, LPS-induced shock18, and Pseudomonas aeruginosa lung infection20.Although the role of epigenetic regulation in asthma pathogenesis remains unclear, evidence of altered histone acetylation, aberrant histone acetyltransferases and histone deacetylases expression, as well as abnormal expression of genes involved in pulmonary repair and inflammation has been reported in the airways of asthmatics2122232526272829. Additionally, mimics of BET bromodomains have been shown to inhibit airway smooth muscle cell proliferation and cytokine release from patients with asthma2223. Based on these findings and the role of BET proteins in Th17 cell function, we hypothesize that the BET inhibitor CPI-203 would limit asthma pathogenesis in a Th17-induced murine model of severe refractory asthma. Overall, this work establishes a role for BET proteins in Th17-mediated allergic airway disease and suggests that interfering with BET-dependent chromatin signaling may provide clinical benefits to patients suffering from asthma.
Materials and Methods
Mice
6–8 week old, female BALB/c SCID and DO11.10 TCR-transgenic mice were purchased from Taconic. All mice were housed in a pathogen-free environment at the Children’s Hospital of Pittsburgh of UPMC and were given food and water ad libitum. All animal experiments were reviewed and approved by the University of Pittsburgh Institutional Animal Care and Use Committee. All experiments were performed in accordance with IACUC guidelines and regulations.
In vitro differentiation of Th17 cells
CD4+ CD62L+ naïve T cells from the spleens of DO11.10 TCR-transgenic mice were enriched using a CD4+ CD62L+ T cell Isolation Kit II (Miltenyi Biotec) and were cultured for 6 days with antiCD3/antiCD28 mouse Dynabeads (Invitrogen) under Th17 cell polarizing conditions (10 ng/mL IL-23, 1 ng/mL TGFβ, 2 ng/mL IL-6, 10 μg/mL anti-IL-4, and 10 μg/mL anti-IFNγ purchased from R&D Systems) as previously described3.
Th17-induced, neutrophil-dominant allergic airway disease model
BALB/c SCID mice were challenged with 50 μg of ovalbumin (Sigma-Aldrich) via oropharyngeal aspiration (OA) on Day 0. On Day 1, 1 × 106 Th17 cells were adoptively transferred by retro-orbital injection. Mice were subsequently challenged with 50 μg ovalbumin OA daily for three consecutive days after cell transfer (Days 2–4). Twenty-four hours after the last challenge, mice were euthanized (Day 5) and allergic airway disease was assessed as detailed below. Control mice received all ovalbumin challenges, but received phosphate buffered saline retro-orbitally at time of cell transfer. To inhibit BET bromodomains, mice were treated with 2.5 mg/kg BET inhibitor CPI-203 (Constellation Pharmaceuticals) via intraperitoneal injection twice daily on Days 1–4.
Lung Mechanics Measurements
Pulmonary function was assessed by mechanical ventilation of anesthetized (90 mg/kg pentobarbital-NA, IP) and tracheotomized mice using a computer-controlled small-animal mechanical ventilator (FlexiVent; SCIREQ) as previously described3031. Respiratory mechanics measurements were made prior to and following inhalation of aerosolized methacholine (0, 0.75, 3.125, 12.5, and 25 mg/mL).
Bronchoalveolar lavage (BAL) and lung processing
After lung mechanics analyses, BAL fluid was collected via the intratracheal instillation and recovery of 1 mL of PBS. Total cells in the recovered BAL fluid were counted using a hemocytometer and the number of neutrophils, eosinophils, macrophages and lymphocytes were quantified from modified Wright-Giemsa-stained cytospin preparations of BAL cells (200 cells/slide). Lung lobes were separated and processed as follows: flash frozen in liquid nitrogen for cytokine and chemokine analyses by Lincoplex according to manufacturer’s instructions (Bio-Plex Pro™ Mouse Cytokine Group I Panel 23-Plex, BioRad) or gene expression analyses using quantitative RT-PCR, or inflation-fixed with 10% buffered formalin and paraffin embedded for histology3233. For Lincoplex analyses, the following cytokines and chemokines were measured (the limit of detection): IL-1α (2 pg/mL), IL-1β (7 pg/mL), IL-2 (3 pg/mL), IL-3 (2 pg/mL), IL-4 (3 pg/mL), IL-5 (2 pg/mL), IL-6 (2 pg/mL), IL-9 (15 pg/mL), IL-10 (2 pg/mL), IL-12p40 (2 pg/mL), IL-12p70 (4 pg/mL), IL-13 (9 pg/mL), IL-17A (1 pg/mL), EOTAXIN (148 pg/mL), G-CSF (1 pg/mL), GM-CSF (7 pg/mL), IFNγ 6 pg/mL), CXCL1 (3 pg/mL), MCP-1 (14 pg/mL), MIP-1α (24 pg/mL), MIP-1β (2 pg/mL), CCL5 (5 pg/mL), TNFα (6 pg/mL).
Gene expression analysis
RNA was isolated from lung tissue using an Absolutely RNA Miniprep Kit (Agilent Technologies, Santa Clara, CA). One μg of RNA was then converted to cDNA using iScript cDNA Synthesis Kit (Bio-Rad, Hercules, CA). Gene expression analysis was performed using Taqman Fast Mastermix and Assay On Demand TaqMan primer and probe sets for the following murine genes of interest: Muc5ac, Muc5b, Clca3, Spp1 (Life Technologies, Grand Island, NY).
Histological Scoring of Inflammation and Mucus Metaplasia
To characterize tissue inflammation in the lung, standard H&E-stained lung sections were scored by observers (JFA and MLM), who were blinded to the sample group identity. The entire lung section was observed with a light microscope (×40 magnification) and peribronchial, perivascular, and parenchymal inflammation were scored as previously described731. Briefly, cellular inflammation present in each area was scored according to the following scale: 0 = no inflammation, 1 = up to 25%, 2 = 25–50%, 3 = 50–75%, and 4 = 75–100%. The inflammation score was reported as the mean of the scores for each sample group. Mucus production was quantified through the observation of Periodic Acid-Schiff (PAS) stained lung sections by observers (JFA and MLM) blinded to the identity of the sample groups. The entire lung section was observed with a light microscope (100x magnification) and the amount of PAS staining in the entire lung section was scored using the following scale: 0 = no staining present, 1 = light staining in large airway only, 2 = staining present in all large airways and some small bronchioles, 3 = staining present in large and small airways, and 4= dense staining in all airways. The PAS score was reported as the mean of the scores for each sample group.
Statistical analyses
Data were analyzed using GraphPad Prism 5.0 (GraphPad Software Inc., La Jolla, CA). Experiments involving 2 variables were analyzed by two-way analysis of variance with a Bonferonni post-hoc test. Data with one variable were analyzed using one-way analysis of variance with Tukey’s post-hoc test. Data comparing two groups were analyzed using an unpaired t-test. Data was log transformed for statistical analyses where indicated. Data shown are mean ± SEM. A value of p < 0.05 was considered to be statistically significant.
Results
Inhibition of BET proteins decreases pulmonary inflammation and alters cytokine and chemokine production in the lungs during Th17-induced allergic airway disease
Previous work has shown that adoptive transfer of OVA-specific Th17 cells into OVA-treated BALB/c SCID mice is sufficient to promote neutrophilic inflammation, AHR, and mucus metaplasia, which are not affected by glucocorticoid treatment3. Utilizing this model, we investigated the therapeutic potential of CPI-203, a highly selective and potent inhibitor of BET proteins (Fig. 1A). Similar to previous work37, adoptive transfer of OVA-specific Th17 cells into OVA-treated BALB/c SCID mice increased cellular inflammation in the airspaces, resulting in higher levels of macrophages, neutrophils, and lymphocytes (Fig. 1B,C). CPI-203 treatment during Th17-driven allergic airway disease attenuated inflammation in the airspaces of the lungs and resulted in significantly lower levels of macrophages, lymphocytes, and neutrophils (Fig. 1B,C). Overall, these results suggest that the steroid-insensitive neutrophilia in the airspaces that was induced by Th17-mediated allergic airway disease, was reduced by CPI-203 treatment.
Figure 1
BET bromodomain inhibition reduces Th17-induced airspace inflammation in the lungs during allergic airway disease in mice.
(A) BALB/c SCID mice were treated with ovalbumin (OVA) and adoptively transferred with Th17 cells to induce allergic airway disease and the therapeutic potential of CPI-203 was investigated in this model. Cellular inflammation in the airspaces was measured by (B) total cells in the BAL fluid and (C) BAL fluid cell differential counts. Mice in control and CPI-203 groups received all OVA challenges, but phosphate buffered saline retro-orbitally at time of cell transfer. Graphs show data for control (n = 5), CPI-203 (n = 6), Th17 (n = 8), Th17+ CPI-203 (n = 8) combined from three independent experiments. *p < 0.05 when compared to all other groups, †p < 0.05 when compared to the CPI-203 group.
In addition to reducing cellular inflammation present in the airspaces, inhibition of BET proteins during Th17-induced allergic airway disease also decreased inflammation present in the lung tissue. Histological assessment of hematoxylin and eosin-stained lung sections showed that perivascular, peribronchial, and parenchymal inflammation were all lessened by CPI-203 treatment in this murine model of Th17-induced allergic airway disease (Fig. 2). Furthermore, treatment with CPI-203 altered cytokine and chemokine levels in the lungs of Th17 adoptive transfer, OVA challenged mice. Specifically, IL-1α, IL-1β, IL-2, IL-6, IL-10, IL-12p40, IL-12p70, IL-13, IL-17A, and eotaxin increased in response to CPI-203 treatment, while G-CSF, CXCL1, MIP-1β, and CCL5 decreased (Table 1). Several cytokines and chemokines were also unaffected by CPI-203 treatment, which included IL-3, IL-4, IL-5, IL-9, GM-CSF, IFNγ, MCP-1, MIP-1α and TNFα. These data demonstrate that inhibition of BET proteins alters Th17 cell-driven inflammation by modulating downstream pro-inflammatory mediators, which promote neutrophil recruitment into the lungs.
Figure 2
Inhibition of BET protein and chromatin interactions alters tissue-associated inflammation in the lungs of mice with Th17-induced allergic airway disease.
(A) Representative images of hematoxylin and eosin-stained lung sections (100x magnification) from OVA-treated BALB/c SCID mice that received Th17 cells (Th17 group) or PBS (control group) with and without CPI-203 treatment. (B) Perivascular, peribronchial, and parenchymal-associated inflammation in the entire lung section were quantified by an observer blinded to the identity of the samples. Graph shows data for control (n = 5), CPI-203 (n = 6), Th17 (n = 8), Th17+ CPI-203 (n = 8) combined from three independent experiments. *p < 0.05 when compared to all other groups, †p < 0.05 when compared to the CPI-203 group.
Table 1
Inflammatory cytokine and chemokine levels in the lungs following CPI-203 treatment in a murine model of Th17-induced allergic airway disease.
Control (n = 5)
CPI-203 (n = 6)
Th17 (n = 8)
Th17+CPI-203 (n = 8)
IL-1α
22.57 ± 1.97
22.81 ± 1.00
142.75 ± 4.33*
166.47 ± 8.83*
IL-1β
233.89 ± 14.18
240.68 ± 5.64
2067.55 ± 37.30*
2415.43 ± 85.61*
IL-2
55.99 ± 4.25
58.81 ± 2.25
189.90 ± 7.53*
248.55 ± 13.99*
IL-3
11.50 ± 0.80
11.32 ± 1.24
15.05 ± 1.31
19.24 ± 2.29†
IL-4
3.51 ± 0.14
3.57 ± 0.05
59.88 ± 7.47
98.92 ± 25.54†
IL-5
11.87 ± 0.99
13.05 ± 0.54
26.95 ± 2.55†
33.30 ± 4.16†
IL-6
0.00
0.00
89.40 ± 3.40
108.37 ± 4.69‡
IL-9
0.00
0.00
968.40 ± 33.54
1030.62 ± 30.50
IL-10
24.35 ± 0.90
27.18 ± 0.67
373.72 ± 7.87*
462.43 ± 17.65*
IL-12p40
78.45 ± 17.87
49.06 ± 15.88
261.17 ± 31.22*
467.50 ± 44.09*
IL-12p70
96.28 ± 9.40
105.46 ± 5.66
510.79 ± 25.30*
691.97 ± 34.71*
IL-13
281.83 ± 15.57
307.55 ± 15.96
1720.70 ± 74.47*
2329.93 ± 150.05*
IL-17A
8.41 ± 0.35
9.41 ± 0.53
90.03 ± 3.20*
110.35 ± 6.73*
EOTAXIN
467.54 ± 24.21
538.83 ± 28.85
2255.97 ± 99.10*
2753.50 ± 87.87*
G-CSF
0.00
0.00
227.80 ± 28.41
126.43 ± 13.84‡
GM-CSF
123.00 ± 3.81
134.20 ± 5.47
184.52 ± 4.30†
186.91 ± 4.35†
IFNγ
28.26 ± 2.96
34.22 ± 3.71
65.86 ± 5.07
206.78 ± 80.14
CXCL1
32.33 ± 1.61
26.85 ± 1.56
346.10 ± 29.10*
268.39 ± 17.61*
MCP-1
85.90 ± 8.74
90.21 ± 5.75
851.93 ± 64.59†
1031.35 ± 99.39†
MIP-1α
36.29 ± 1.95
30.04 ± 2.20
197.01 ± 12.89†
178.24 ± 7.44†
MIP-1β
51.48 ± 2.39
50.75 ± 1.69
126.71 ± 7.14*
102.83 ± 6.50*
CCL5
45.90 ± 1.37
28.06 ± 1.72
680.98 ± 34.69*
516.05 ± 27.07*
TNFα
176.06 ± 5.68
194.75 ± 4.66
497.21 ± 10.94†
567.25 ± 37.35†
Values shown are mean ± SEM. Comparisons were made using an unpaired t-test (IL-6, IL-9, G-CSF) or an one-way ANOVA and Tukey’s post-test (all other analytes). Mice in control and CPI-203 groups received all ovalbumin challenges, but received phosphate buffered saline (PBS) retro-orbitally at time of cell transfer. *p < 0.05 when compared to all other groups, †p < 0.05 when compared to control and CPI-203 groups, and ‡p < 0.05 when compared to the Th17 group.
BET bromodomain inhibition with CPI-203 alters respiratory mechanics in mice with Th17-induced allergic airway disease
To further characterize the role of BET proteins in Th17-dominant allergic airway disease, lung function was assessed by measuring Newtonian resistance (Rn), tissue damping (G), and tissue elastance (H), in response to increasing doses of methacholine as well as by measuring quasi-static lung compliance. Inhibition of BET proteins with CPI-203 treatment did not affect Rn, a parameter that is representative of central or conducting airway resistance, and G, a parameter that relates to tissue or parenchymal resistance, in this model of Th17-driven allergic airway disease (Fig. 3A,B). However, blocking BET bromodomains significantly lowered tissue elastance (H), a parameter related to parenchymal recoil, in Th17 cell adoptive transfer, OVA challenge mice (Fig. 3C). CPI-203 treatment also trended to improve quasi-static lung compliance in mice with Th17-induced allergic airway disease (Fig. 3D).
Figure 3
Blocking BET protein chromatin signaling via CPI-203 treatment alters tissue elastance in the lungs of mice with Th17-induced allergic airway disease.
Lung function was evaluated following CPI-203 treatment in a model of Th17-induced allergic airway disease. (A–C) Airway responsiveness to inhaled aerosolized methacholine (Newtonian resistance (Rn), tissue damping (G), and tissue elastance (H)), and (D) quasi-static lung compliance were measured using a FlexiVent system. Graphs show data for control (n = 5), CPI-203 (n = 6), Th17 (n = 8), Th17 + CPI-203 (n = 8) combined from three independent experiments. *p < 0.05 when compared to control and CPI-203 group, †p < 0.05 when compared to the control group, ‡p < 0.05 when compared to all other groups.
Inhibition of BET bromodomains limits Th17-mediated mucus production in the lungs of mice during allergic airway disease
As previously reported3, adoptive transfer of Th17 cells into OVA-treated BALB/c SCID mice increased pulmonary mRNA expression of mucus-associated genes, Muc5ac and Clca3, and increased mucus production as evident by PAS staining present in the airways (Fig. 4). In this study, inhibition of BET bromodomains during Th17-induced allergic airway disease significantly reduced PAS-positive airways, while not significantly altering Muc5ac and Clca3 mRNA expression (Fig. 4). These results suggest that BET proteins are important drivers of mucus production in the airways during allergic airway disease, independent of promoting mucin gene expression.
Figure 4
BET bromodomain inhibition via CPI-203 treatment alters goblet cell hyperplasia and mucus production in the lungs of mice with Th17-induced allergic airway disease.
(A) Pulmonary expression of Muc5ac and (B) Clca3 as well as (C) representative images of Periodic Acid Schiff (PAS)-stained lung sections (200x magnification) from OVA-treated BALB/c SCID mice that received Th17 cells (Th17 group) or PBS (control group) with and without CPI-203 treatment. (D) Mucus production in the PAS-stained lung sections was quantified by an observer blinded to the identity of the samples. Data shown for control (n = 5), CPI-203 (n = 6), Th17 (n = 8), Th17+ CPI-203 (n = 8) combined from three independent experiments. *p < 0.05 when compared to control and CPI-203 group, †p < 0.05 when compared to all other groups.
Discussion
In this study, we show that BET inhibition limits neutrophilia and Th17-driven cytokine and chemokine release in the lungs in a murine model of severe, steroid-insensitive asthma. Inhibition of BET proteins also improved lung function, specifically quasi-static lung compliance and tissue-related AHR, and reduced mucus production in the airways. To our knowledge, these results are novel and demonstrate that BET proteins are important regulators of asthma pathogenesis, and more significantly can affect severe, steroid-insensitive disease. Therefore, our work herein demonstrates that BET inhibitors may provide therapeutic benefit to patients with asthma, especially those with neutrophilia and/or severe refractory disease.Previous work has suggested that cellular infiltration into the airspaces during Th17-induced allergic airway disease correlated with quasi-static lung compliance, whereas AHR was associated with tissue-based inflammation7. The findings of this current study support these results, which demonstrate that when Th17-induced cellular inflammation is limited via BET protein inhibition, quasi-static lung compliance is also improved. Similarly, we also observe a marked reduction in Th17-induced tissue inflammation following BET protein inhibition and lower tissue-related AHR parameters. Although quasi-static lung compliance and tissue-related AHR may be associated with pulmonary inflammation, our results imply that central airway resistance is likely an inflammation-independent process. Alterations in airway resistance have been attributed to direct effects on airway remodeling and contractility. Specifically, IL-17 is known to induce airway smooth muscle cell contraction, thereby altering airway hyperresponsiveness343536. Overall, these results highlight the complexity of the underlying biology that contributes to asthma pathologies. Further work is needed to establish how histone modifications affect tissue responses in asthma.IL-17 is a cytokine mainly produced by Th17 cells and is thought to regulate neutrophilic inflammation and steroid resistance in severe asthmatics. BET chromatin modulators directly regulate Th17 responses and critically mediate Th17 biology via bromodomain-dependent association with acetylated histones at the IL17 locus in Th17 cells16. Further, BET inhibition was shown to limit Th17-mediated autoimmunity and pulmonary infection1620. Thus, we hypothesized that BET inhibition would alter Th17 cell-driven allergic airway disease. In this study, we did not observe a direct change in IL-17 protein following CPI-203 treatment, but did find lower levels of IL-17-driven cytokines and chemokines (G-CSF, CXCL1), neutrophils in the airspaces, and tissue inflammation in the lungs. The murine model of asthma utilized for this work is a neutrophil-dominant allergic airway disease model induced by antigen-specific Th17 cells, which presumably produce IL-17 as early as the first antigen challenge (Day 2, Fig. 1A). The lung tissue is collected for analyses several days after this initial challenge and thus may account for the unchanged pulmonary levels of IL-17 observed. The reduction of pulmonary neutrophilia and IL-17-driven cytokines implies however that the inhibition of BET proteins reduced the activity of IL-17 in the lungs in this murine model of severe, steroid-insensitive asthma.Our data provides evidence that the inhibition of BET proteins lessens neutrophilic inflammation likely by altering downstream pro-inflammatory mediators, which promote neutrophil recruitment into the lungs. Other studies using BET mimics have also established that BET proteins can modulate neutrophilia by regulating IL-6 and CXCL8 release from human bronchial epithelial cells and airway smooth muscle cells from healthy controls and asthmatics2122. BET protein function was also shown to be required for murine macrophage inflammatory processes18, which may influence their phenotype and role in asthma pathogenesis. Analyses of the cytokine and chemokine milieu following BET inhibition in mice with Th17 cell-driven allergic airway disease revealed a complex inflammatory environment even when cellular inflammation in the airspace and interstitium was significantly reduced. Overall, BET proteins clearly function as modulators of the inflammatory responses in this murine model of severe, steroid-insensitive asthma.JQ1 and CPI-203, an analog of JQ1, are well-characterized BET bromodomain inhibitors that are extremely selective, with no off-target effects at biologically relevant or suprapharmalogical concentrations373839. Clinical trials using BET bromodomain inhibitors for treatment of leukemias, lymphomas, myelomas, and other cancers are ongoing40. Recent studies have suggested the utility of BET mimics in Th17 cell-driven autoimmunity, pulmonary infection, and idiopathic pulmonary fibrosis162024. Our original work herein demonstrates a pivotal role of BET proteins in asthma and more importantly, provides evidence that BET inhibition may be beneficial in a steroid-insensitive disease setting. As some asthmatics with severe glucocorticoid resistance show abnormal histone acetylation patterns26, pharmacological intervention targeting BET adaptor proteins may be efficacious to lessen disease burden for patients with refractory disease.
Additional Information
How to cite this article: Manni, M. L. et al. Bromodomain and Extra-Terminal Protein Inhibition Attenuates Neutrophil-dominant Allergic Airway Disease. Sci. Rep.
7, 43139; doi: 10.1038/srep43139 (2017).Publisher's note: Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
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