Molecular clock REV-ERBα regulates cigarette smoke–induced pulmonary inflammation and epithelial-mesenchymal transition

It has been shown that CS induces EMT in lung epithelial cells in culture and the lungs of smokers compared with health control. As shown in, we observed a significant increase in the abundance of type-1 collagen (COL1A1) in smokers compared with nonsmokers as well as a nonsignificant increasing trend of TGF-β and vimentin between smokers and nonsmokers. There was no change in the protein level of plasminogen activator inhibitor-1 (PAI-1) between smokers and nonsmokers. Overall, our results confirm the upregulation in mesenchymal transition markers in the lungs of smokers compared with nonsmokers. In our previous study, we have shown decreased protein levels of REV-ERBα in smokers compared with nonsmokers (). Here, we proposed to determine how REV-ERBα affects EMT activation. Figure 1 ¹⁴

To determine how subchronic CS exposure affects circadian clock gene targets in mouse lungs, we have employed a customized NanoString nCounter panel for gene transcription analysis. Subchronic CS exposure causes circadian clock dysregulation in the lungs (and; supplemental material available online with this article;). The core clock-controlled genes (CCGs), such as,,,, and, showed altered expression following subchronic CS exposure. Other circadian-related genes, such as D site of albumin promoter binding protein (), basic helix-loop-helix family, member e41 (), basic helix-loop-helix family, member e40 (), casein kinase 1 δ (), casein kinase 2 α 1 (), F-box and leucine-rich repeat protein 3 (), mitogen-activated protein kinase 14 (), methionine adenosyl transferase 2A (), nuclear receptor subfamily 2 group F member 6 (), and nuclear factor, IL-3 regulated (), were all dysregulated after subchronic CS exposure. In–KO mice, subchronic CS exposure further upregulated circadian gene transcription of selected genes, such as,,,, and hepatic leukemia factor () (and). Notably,,, andgenes showed a significant increase inKO mice exposed to CS compared with their respective air group control. However, we only observed a remarkable dysregulation in CCGs at the gene level. There was an increase in the protein abundance of BMAL1 after subchronic CS exposure (). Figure 2 Supplemental Figure 1 Figure 2 Supplemental Figure 1 Supplemental Figure 2 https://doi.org/10.1172/jci.insight.145200DS1↗ Arntl Per2 Per3 Cry2 Rora Dbp Bhlhe41 Bhlhe40 Csnk1d Csnk2a1 Fbxl3 Mapk14 Mat2a Nr2f6 Nfil3 REV-ERB α Per2 Per3 Dbp Bhlhe41 Hlf Dbp Bhlhe41 Per2 REV-ERB α –

To further investigate the correlation between REV-ERBα and CS-induced EMT, we examined EMT-associated gene expression and protein abundances/localizations in the lungs of subchronic CS-exposed WT and–KO mice (and). At the gene transcription level, only collagen type I α I () showed significant upregulation in CS-exposed REV-ERBα–KO mice compared with CS-exposed WT mice (). Most of the EMT markers, especially the mesenchymal markers, including vimentin (),, serpin family E member 1 (), collagen type III α I (), matrix metalloproteinase-2 (), and TIMP metallopeptidase inhibitor 1 (), were increased in CS-exposed mice compared with air group controls (,, and). Surprisingly, we showed a decreased gene expression of Snail (also known as) after CS exposure in both WT and KO mice (). In addition, the epithelial markerwas decreased in CS-exposed (WT or KO) mice (). REV-ERB α Col1a1 Vim Tgf β 1 Serpine1 Col3a1 Mmp2 Timp1 Snai1 Cdh1 Figures 3 4 Figure 3 Figure 3 Figure 4C Supplemental Figure 3 Supplemental Figure 3 Figure 4C

EMT-related protein abundances and localizations were measured to further determine the role of REV-ERBα in CS-induced EMT. All mesenchymal markers, including vimentin, COL1A1, TGF-β, PAI-1, and p53, were increased in CS-exposed mice (and). Additionally, vimentin, COL1A1, TGF-β, and snail-slug protein expressions were augmented in CS-exposed REV-ERBα–KO mice (). To further understand the altered expression and localization of mesenchymal markers, vimentin, αSMA, and snail-slug were stained immunohistochemically. In agreement with immunoblotting results, CS exposure significantly increased vimentin expression in the alveolar region (). InKO mice, further increase in the protein abundance of vimentin and snail-slug in the alveolar regions of the lungs was semiquantitatively analyzed (and). αSMA expression was also increased in alveolar epithelium of CS-exposed mice independent of REV-ERBα (and). Most of the EMT markers, such as αSMA, vimentin, and snail-slug, were expressed near the airway, whereas CS exposure augmented mesenchymal expression in alveoli (). PAI-1 and p53 protein levels were increased after subchronic CS exposure in both WT and–KO mice (). The epithelial markers E-cadherin and ZO-1 were decreased in CS-exposed WT andKO mice (). Figures 4 5 Figure 4A Figure 4B Figure 4B Supplemental Figure 4 Figure 4B Supplemental Figure 4 Supplemental Figure 4 Figure 5 Figure 5 REV-ERB α – REV-ERB α REV-ERB α –

MMPs are the essential components in ECM remodeling and deposition, and MMP2, MMP9, and MMP12 are upregulated after CS exposure. We evaluated the protein abundance of MMP2, MMP9, and MMP12 in mouse lung after 30 days of exposure (). We only found increased protein levels of MMP12 in CS-exposed REV-ERBα–KO mice, whereas MMP2 and MMP9 showed no alteration in protein abundance (). However, we observed an increase in MMP2 gene expression in both CS-exposed WT and–KO mice (). There was no difference in MMP9 gene expression among all the treatment groups (). Supplemental Figure 5 Supplemental Figure 5 Figure 3 Supplemental Figure 3 REV-ERB α

We showed that CS-induced mesenchymal transition is associated with circadian clock gene REV-ERBα in the lungs. We investigated this association by using histological analysis of lung sections for alveolar destruction/airspace enlargement and ECM remodeling (and). We measured lung mean linear intercept (Lm) analysis using H&E-stained images and Gomori’s Trichrome staining to quantify collagen deposition in the lungs from different experimental groups. Type I collagen and fibronectin were also immunohistochemically stained to determine the ECM remodeling. We found that the Lm of airspace was increased but not significantly in WT mice exposed to CS compared with air exposed controls. However,KO mice exposed to subchronic CS exhibited significantly increased Lm compared with their respective air group controls (and). As expected, various immune cells were found in the airspace of both CS-exposed WT and REV-ERBα–KO mice compared with respective air-exposed controls (and). Additionally, a significant increase in collagen deposition around the airway was found in CS-exposedKO mice, whereas CS-exposed WT mice showed similar collagen deposition compared with the air-exposed control (). We also found a higher type-1 collagen deposition in CS-exposedKO mice compared with air controls (), complementing the Gomori’s Trichrome staining results. However, we did not observe any significant difference in fibronectin localization and expression (). Figure 6 Supplemental Figure 6 Figure 6A Supplemental Figure 6 Figure 6A Supplemental Figure 6 Figure 6B Figure 6C Figure 6D REV-ERB α – REV-ERB α – REV-ERB α –

We exposed REV-ERBα Het and WT C57 mice to CS for 4 months and found similar alterations of lung morphometry and inflammation (). We found increased lung compliance and decreased lung resistance and elastance in CS-exposedHet mice compared with WT mice or those in the air group (). In concurrence with the increased compliance, we observed airspace enlargement in CS-exposedHet mice compared with that in WT mice (). We observed that the baseline Lm results varied between 1- and 4-month mouse groups, owing to mouse batch differences, such as their age and quantitation involved in scoring. Further, we found that chronic CS exposure increased inflammatory cell influx in bronchoalveolar lavage fluid (BALF) with increased macrophage, neutrophils, T lymphocytes, and total cells (). However,Het mice did not show significant difference in altered inflammatory cell counts compared with WT mice (). To support our finding for lung morphometry and inflammatory responses, we found a similar change histologically (and). Increased airspace enlargement was only observed inHet CS-exposed mice (original magnification, ×10 and ×20, denoted by green arrows); lung injury and infiltration of inflammatory cells in airspace were observed in both WT andHet CS-exposed mice (original magnification, ×10 and ×20, denoted by red arrows) (). Figure 7 Figure 7A Figure 7B Figure 7C Figure 7C Figure 7B Supplemental Figure 7 Supplemental Figure 7 REV-ERB α REV-ERB α REV-ERB α REV-ERB α REV-ERB α

We have shown that REV-ERBα deficiency promotes abnormal mesenchymal transition, and our previous study has shown that REV-ERBα is associated with increased lung inflammation induced by subchronic CS exposure (). Here, we demonstrate the therapeutic potential of REV-ERBα agonist (SR9009) in acute CS-induced inflammation. After 10 days of CS exposure, total cells from BAL fluid increased in both vehicle and Rev-erb agonist (SR9009) treatment groups (). The percentages of inflammatory cells were determined by flow cytometry, and the percentages of macrophages, CD4 T cells, and CD8 T cells were similar in acute CS-exposed mice treated with vehicle or SR9009 (). Intriguingly, acute CS-induced increase in neutrophils was inhibited by REV-ERBα agonist (SR9009) treatment (). ¹³ Figure 8A Figure 8A Figure 8A

We measured the BAL fluid cytokines by Luminex to identify the inflammatory responses induced by acute CS exposure with or without SR9009 treatment. We found that only CS-induced increases in IL-5 (= 0.06) and GM-CSF (= 0.07) were inhibited by SR9009 treatment without significant differences. Other BAL fluid cytokines, such as MCP-1 and KC, had significantly increased in the CS alone and CS+SR9009 treatment groups (and). P P Figure 8B Table 1

We have shown that subchronic CS exposure resulted in mesenchymal transition in a REV-ERBα–dependent manner. Here, we demonstrate the protective role of SR9009 against dysregulated EMT following acute CS exposure (and). As expected, vimentin, COL1A1, TGF-β, and snail-slug were upregulated by acute CS exposure, and SR9009 treatment significantly reduced COL1A1 and snail-slug protein abundance. Additionally, SR9009 treatment also inhibited the CS-induced increase in vimentin and TGF-β, which was not significantly different between the air- and CS-exposed SR9009 treatment groups (). We also measured the gene expression levels of,,,, and(). We observed increasedandafter CS exposure, and SR9009 administration was able to inhibit the upregulation ofbut not(). There was no difference inexpression among groups (). Interestingly, we found decreased gene expression ofandafter 10 days of CS exposure (). Other mesenchymal markers (PAI-1 and p53) were increased after acute CS exposure in both CS alone and CS+SR9009 treatment groups (). We also measured the protein abundance of epithelial markers and found that acute CS exposure decreased E-cadherin protein levels, whereas CS+SR9009 treatment further decreased E-cadherin levels. Interestingly, there was no change in the protein levels of ZO-1 between air- and CS-exposed mice, whereas SR9009 treatment augments ZO-1 in air+SR9009 treatment group compared with both air alone and CS+SR9009 treatment groups (). Figures 9 10 Figure 9A Figure 9B Figure 9B Figure 9B Figure 9B Figure 10 Figure 10 Tgfb1 Col1a1 Vim Snai1 Snai2 Tgfb1 Col1a1 Tgfb1 Col1a1 Vim Snai1 Snai2

We showed increased protein abundance of MMP12 in mouse lungs after 30 days of CS exposure and increased gene transcript level of MMP2. We measured the protein expression levels of MMP2, MMP9, and MMP12 and gene levels of, andin 10-day-exposed mouse lungs as well (). Surprisingly, we observed a decreased protein expression level of MMP12 after 10 days of CS exposure (), whereas increased MMP12 was found after 30 days of CS exposure (). Similarly, gene expression of MMP2 was upregulated after CS exposure, and SR9009 administration failed to attenuate MMP2 gene expression. There was no difference in the protein expression of MMP9 and MMP2 as well as the gene transcripts ofand(). Mmp2, Serpine1 Fn1 Fn1 Serpine1 Supplemental Figure 8 Supplemental Figure 8 Supplemental Figure 5 Supplemental Figure 8

Finally, we measured the protein abundance of a few key circadian clock molecules to understand the possible protective role of SR9009 treatment in acute CS-exposed mice. Immunoblot analysis of circadian clock targets confirmed an increase in the protein abundance of REV-ERBα in both acute air- and CS-exposed mice treated with SR9009 (). We found increased protein abundance of RORα in CS-exposed mice treated with SR9009 compared with vehicle/CS-exposed controls. BMAL1 protein levels remain unaffected among different exposure and treatment groups, and CLOCK protein expression was decreased in CS+SR9009 treatment group compared with the air+SR9009 group (). Overall, results revealed REV-ERBα agonist treatment mediates attenuation of lung inflammation and EMT phenotype via augmenting REV-ERBα expression in the lungs. Supplemental Figure 9 Supplemental Figure 9

To determine if REV-ERBα plays an essential role in CS-induced EMT, we investigated the role of REV-ERBα in fibroblast differentiation. Human fetal lung fibroblast 1 (HFL-1) cells were treated with TGF-β with or without GSK4112 (REV-ERBα agonist) for 3 days (). The TGF-β–induced increase in gene expression of(αSMA) was significantly inhibited by GSK4112 treatment in HFL-1 cells, whereas mRNA levels ofand(fibronectin) were reduced by GSK4112 but not significantly. We also treated HFL-1 cells with CS extract (CSE) with or without GSK4112 and measured the same fibroblast differentiation markers (). We found a high concentration of CSE (0.25%) showed reduced expression ofand, whereas low 0.1% CSE increased gene expression ofandwithout change in the expression of(). Similarly, we showed a significant reduction in,, andgene expression after treatment with 0.1% CSE+GSK4112 (). These findings indirectly support the role REV-ERBα during inflammation induced mesenchymal differentiation in the lungs (). Figure 11A Figure 11B Supplemental Figure 10 Figure 11B Figure 11 ACTA2 COL1A1 FN1 ACTA2 FN1 ACTA2 COL1A1, FN1 ACTA2 COL1A1 FN1

Lung tissue specimens from 14 subjects, including 7 nonsmokers and 7 smokers, were procured from the National Disease Research Interchange (NDRI) and provided by Vuokko L. Kinnula (Pulmonary Division, Department of Medicine, University of Helsinki and Helsinki University Hospital, Helsinki, Finland) (). Lungs were homogenized in RIPA buffer, and protein concentration was determined by the Pierce BCA Assay Kit (23227; Thermo Fisher Scientific). Supplemental Table 1

HFL-1 cells were purchased from ATCC, and cultured in DMEM: F12K medium (11320033; Thermo Fisher Scientific) with 10% FBS (10082147; Thermo Fisher Scientific), 1% Penicillin-Streptomycin-Glutamine (10378016; Thermo Fisher Scientific), and 1% Non-Essential Amino Acids (11140076, Thermo Fisher Scientific). Before treatment, cells were serum deprived for 12 hours and then treated with 5 ng/mL TGF-β with or without 10 μM GSK4112 (3663; TOCRIS) for 3 days; or 0.1% CSE with or without 10 μM GSK4112 or 0.25% CSE for 2 days. CSE stock was always prepared freshly right before the treatment as described previously (). In brief, CS (3R4F, University of Kentucky) was bubbling into 10 mL FBS-free DMEM: F12K medium (Phenol-red free) as 10% CSE stock. The 0.25% and 0.1% CSE working solutions were diluted from the stock CSE. Quality control of the CSE was based on the absorbance at 320 nm (1.00 ± 0.05 nm). ¹³

Adult C57BL/6 (WT) andglobal KO (KO) mice (male and female mice,4–5 months old) were housed in a 12-hour-light/12-hour-dark cycle in the inhalation core facility at the University of Rochester.–KO mice were provided by Ronald Evans from the Salk Institute (La Jolla, California, USA) (). WT mice were injected i.p. (veh/SR9009, 100 mg/kg body weight) with SR9009 dissolved in 15% cremophor (vehicle) 1 hour before CS exposure, SR9009 or vehicle were injected at ZT5 (11 am EST), every day for 10 days. Mice were exposed to CS for 10 days or 30 days; 2 hours/day with approximately 300 total particular matter (TPM, mg/m), and exposed to CS for 4 months (chronic exposure) with approximately TPM 2 hours every day using the Baumgartner Jaeger mainstream smoking machine. Air group mice were i.p. injected with SR9009 or vehicle at the same time for 10 days without CS exposure. Body weight was recorded daily during the SR9009 treatment period. Mice were sacrificed 24 hours after the last exposure. Lungs were either snap-frozen for gene/protein analysis or fixed (10% formalin) for histological observation. BALF was collected for inflammatory measurement. Lung mechanical properties were analyzed 24 hours after the last exposure via Flexivent FX1 system (Scireq) as per the manufacturer’s instructions. Each measurement was performed 3 times per animal. REV-ERB α REV-ERB α REV-ERB α ¹⁹ 3

Mice were euthanized with ketamine/xylazine, and lungs were lavaged with total 1.8 mL saline (0.6 mL/each time, for a total of 3 times). The BAL fluids were spun down to collect inflammatory cells, and supernatants were transferred for cytokine analysis. The cells were suspended and labeled with specific antibodies to identify the differentiated inflammatory cells. Specific cells were identified by Guava easyCyte flow cytometer (Millipore Sigma) and analyzed by Guava InCyte (). Inflammatory cytokines were measured by Bio-plex Pro mouse cytokine 23-plex immunoassay kit (M60009RDPD; Bio-Rad), and plates were read through the Luminex Flexmap 3D (Luminex Corp). ⁵⁰

Proteins were isolated from the snap-frozen lungs (approximately 30 mg) in RIPA buffer with protease inhibitor (78440; Thermo Fisher Scientific) with mechanical homogenization. An equal amount of protein (20 μg/lane) was used and then separated through 10% SDS-polyacrylamide electrophoresis (SDS-PAGE). The gels with protein samples were transferred onto a nitrocellulose membrane (1620112; Bio-Rad). The membranes were blocked with 5% non-fat milk at room temperature for 1 hour, followed by primary antibody incubation (overnight at 4°C). After primary antibody probing, membranes were washed with TBS-T, 10 minutes each for 4 times, and probed with goat anti-rabbit secondary antibody (1:5000, 1706515; Bio-Rad) for 1 hour at room temperature. Membranes were developed with Pierce ECL Western Blotting Substrate (32106; Thermo Scientific) and imaged by Bio-Rad ChemiDoc MP imaging system (Bio-Rad). The normalization was done based on β-actin (1:2500, ab20272; Abcam) or GAPDH (1:1000, ab9482; Abcam), and fold change was normalized to the WT air group or the air group treated with vehicle. See complete unedited blots in the supplemental material.

First, snap frozen lung lobes were homogenized in QIAzol reagent (79306; Qiagen) mechanically. Lung homogenates were mixed with chloroform and vortexed for 10 seconds, followed by centrifugation at 15,000for 15 minutes in 4°C. After centrifugation, aqueous phase was transferred to new RNase-free tubes and then mixed with isopropanol. The mixtures were kept at –20°C for 2 hours and then spun down at 20,637for 15 minutes in 4°C, and the supernatant discarded. The RNA pellets were washed with 75% EtOH and spun down again at 20,637for 15 minutes in 4°C. The EtOH was discarded and resuspended in RNA with RNase-free water. All of the RNA samples were cleaned up by RNeasy Plus Mini Kit (74136, Qiagen) based on the manufacturer’s protocol. RNA samples were stored at –80°C until analysis. g g g

RNA samples isolated from lung lobes were quantified through NanoDrop spectrophotometer (ND-1000, NanoDrop Technologies), and 100 ng RNA samples were prepared for NanoString analysis. The customized panels from NanoString, including circadian genes and EMT genes, were used in this study. All the gene expressions were presented as normalized counts and measured by nCounter SPRINT Profiler (NanoString Technologies) and analyzed by nSolver 4.0 software.

RNA samples isolated from lung lobes were quantified by Nano-drop spectrophotometer (ND-1000, NanoDrop Technologies). RT was done by RTFirst Strand Kit (330401; Qiagen), and qRT-PCR was based on SYBR green expression master-mix (330509; Qiagen). qPCR was done by the Bio-Rad CFX96 qPCR instrument, and mRNA expression was determined by 2methods with normalization using GAPDH as housekeeping control. 2 -ΔΔCt

The staining protocol has been described in our previous study (). Briefly, lung sections (5 μm) were deparaffinized with xylene and rehydrated with gradient percentage of ethanol (100%, 95%, and 70%). Then, sections were soaked in hematoxylin for 1 minute and 7% ammonia-water for 10 seconds. The sections were stained with eosin for 1 minute and rinsed in 95% ethanol for 1 minute. After staining, slides were dehydrated in 95% ethanol and 100% xylene. All slides were mounted for further analysis. ⁵¹

The staining protocol has been described in our previous study (). Lung sections were stained using the Gomori’s Trichrome staining kit that was commercially available (87020; Thermo Fisher Scientific) based on the manufacturer’s protocol. The slides were dehydrated and mounted for observation and Ashcroft scoring (). The Ashcroft scoring was done based on the previous study in a blinded manner (,). ^{51 52 5 51}

The staining protocol has been described in our previous study (). Lung sections (5 μm) were deparaffinized and rehydrated, and then the antigens unmasked with antigen retrieval solution (10x) (S1699; Dako). Sections were blocked with 10% normal goat serum and then incubated with primary antibodies at 4°C overnight. Then, slides were soaked in 0.3% hydrogen peroxide for 15 minutes, then washed with TBS. Secondary antibody (1:1000, ab7090; Abcam) was applied to the section at room temperature for 1 hour. Slides were developed with DAB Quanto Chromogen and Substrate (TA-125-QHDX; Thermo Fisher Scientific) and then counter stained with hematoxylin. Slides then dehydrated and were mounted for further analysis. ⁵¹

The Lm of airspace was measured through H&E-stained lung section (×20) by MetaMorph software (Molecular Devices). Pictures were taken randomly from 2–4 sections per slide in a blinded manner, more than 8 pictures were used for Lm calculation, and all of the pictures were used for analysis following manual threshold as described previously (). ⁵³

Lung tissues were obtained from the NDRI and/or NIH Lung Tissue Research Consortium and/or provided by Vuokko L. Kinnula.

The statistical differences among samples were analyzed through either 1-way ANOVA or 2-tailed Student’stest in GraphPad Prism software (version 8.0). Results were presented as the mean ± SEM. Avalue of less than 0.05 was considered significant. t P

This study was performed according to the standards from the United States Animal Welfare Act, NIH. All of the animal experiments followed the protocol approved by the Animal Research Committee of the University of Rochester.