key: cord-0695274-a4txd8qz authors: Maehara, Toko; Fujimori, Ko title: Inhibition of Prostaglandin F(2)(α) Receptors Exaggerates HCl-Induced Lung Inflammation in Mice date: 2021-11-27 journal: Int J Mol Sci DOI: 10.3390/ijms222312843 sha: d7a063fcac0c64cc9f392847c5f75525a84efa42 doc_id: 695274 cord_uid: a4txd8qz Acute lung injury (ALI) and acute respiratory distress syndrome (ARDS) are severe respiratory disorders that are caused by aspiration, sepsis, trauma, and pneumonia. A clinical feature of ALI/ARDS is the acute onset of severe hypoxemia, and the mortality rate, which is estimated at 38–50%, remains high. Although prostaglandins (PGs) are detected in the bronchoalveolar lavage fluid of patients with ALI/ARDS, the role of PGF(2α) in ALI remains unclear. We aimed to clarify the role of PGF(2α)/PGF(2α) receptor (FP) signaling in acid-induced ALI using an FP receptor antagonist, AL8810. Intratracheal injection of hydrochloric acid (HCl) increased neutrophil migration into the lungs, leading to respiratory dysfunction. Pre-administration of AL8810 further increased these features. Moreover, pre-treatment with AL8810 enhanced the HCl-induced expression of pro-inflammatory cytokines and neutrophil migratory factors in the lungs. Administration of HCl decreased the gene expression of lung surfactant proteins, which was further reduced by co-administration of AL8810. Administration of AL8810 also increased lung edema and reduced mRNA expression of epithelial sodium channel in the lungs, indicating that AL8810 reduced fluid clearance. Furthermore, AL8810 also increased lipopolysaccharide-induced expression of adhesion molecules such as intracellular adhesion molecule-1 and E-selectin in human umbilical vein endothelial cells. These results indicate that inhibition of FP receptors by AL8810 exacerbated HCl-induced ALI. Acute pulmonary disease, coronavirus disease 2019 (COVID- 19) , has rapidly evolved into a global pandemic [1] . The number of patients with COVID-19 is over 100 million, and 5 million people have died in just 3 years. Research on and development of therapeutic agents and vaccines against COVID-19 are progressing [2] . However, further research regarding the pathogenesis of COVID-19 and the development of treatments is indispensable. Acute lung injury (ALI) and acute respiratory distress syndrome (ARDS) are severe respiratory diseases caused by aspiration, sepsis, trauma, and pneumonia [3, 4] . The clinical characteristics of ALI/ARDS include severe hypoxemia. Morbidity and mortality rates remain high, with an estimated mortality rate of 38-50% [5] . Several clinical studies have shown that pharmacological trials have not been effective in the treatment of ALI/ARDS [6, 7] ; thus, the development of novel therapeutic strategies for ALI/ARDS is highly necessary. The pathological features of ALI/ARDS include increased neutrophil migration into the alveolar space, alveolar epithelial injury, vascular endothelial injury, and lung edema. Acute inflammation disrupts the endothelial and epithelial barriers [8] . Disruption of the endothelial barriers increases vascular permeability, which results in the efflux of protein-rich fluid into the bronchoalveolar lavage fluid (BALF) [9] . It also reduces alveolar fluid clearance and the production and function of surfactants. Endothelial cell injury upregulates the expression of intracellular adhesion molecule-1 (ICAM-1), which regulates neutrophil adhesion and migration [10] . Infiltrating neutrophils produce reactive oxygen species (ROS) and myeloperoxidase, leading to tissue damage [11] . We first investigated the effect of AL8810 on HCl-induced ALI. The levels of SpO 2 were measured as an index of pulmonary function. The SpO 2 levels in saline-treated mice were approximately 98% ( Figure 1A) . However, the SpO 2 levels were decreased with HCl treatment, as compared with those of the saline-treated mice, and were further decreased in AL8810-pretreated HCl-administered mice. Administration of HCl-induced lung hemorrhage (indicated by an arrow in Figure 1B , middle panel). Moreover, administration of HCl + AL8810 caused more severe lung hemorrhage than did the administration of HCl alone (indicated by arrows in Figure 1B , right panel). These morphological changes were not observed in the hematoxylin and eosin (HE)-stained sections of saline-treated mice ( Figure 1C , left panel). In addition, macrophages were detected in alveolar spaces, which were characterized by a large cytoplasm and round nucleus ( Figure 1C , left panel). However, HCl administration resulted in the accumulation of immune cells, mainly neutrophils that were identified by segmented nuclei ( Figure 1C , middle panel). Moreover, pretreatment with AL8810 increased HCl-induced neutrophil migration and disruption of alveolar structures ( Figure 1C , right panel). Then, we counted the cell population of macrophages and neutrophils in BALF. In the saline-treated mice, macrophages were a major cell population in BALF ( Figure 1D ). On the other hand, administration of HCl increased the ratio of neutrophils, which was further enhanced in BALF of AL8810-treated mice ( Figure 1D ). Administration of AL8810 alone did not affect the SpO 2 level ( Figure S1A ) or the ratios of macrophages and neutrophils in BALF ( Figure S1B ), compared with salinetreated mice. At one hour after HCl administration, the PGF 2α level in BALF was increased, compared with naïve mice (0 h; Figure 1E) . The PGE 2 level in BALF also tended to increase by HCl administration, compared with naïve mice ( Figure S2 ). Taken together, these results indicate that inhibition of FP receptors exacerbated HCl-induced ALI. Figure 1 . Pretreatment with AL8810 promoted HCl-induced lung inflammation. AL8810 (10 mg/kg, i.p.) was administered to mice 1 h before HCl (0.1 M, 2 µ L/g, i.t.) administration. (A) SpO2 level was used as a measure of pulmonary function (n = 3-4). * p < 0.05 vs. saline, # p < 0.05 vs. HCl. (B) Representative images of the lung tissues of saline-, HCl-, and HCl + AL8810-administered mice (n = 4-8). (C) Representative images of HE-stained sections of the lung tissues of saline-, HCl-, and HCl + AL8810-treated mice (scale bar 50 µ m) (n = 6-10). (D) The cell numbers in BALF were measured at 6 h after administration of saline or HCl (n = 5-6). * p < 0.05 vs. saline, # p < 0.05 vs. HCl. (E) The PGF2α levels in BALF were measured by ELISA (n = 6). * p < 0.05 vs. 0 h. Next, we assessed the gene expression levels of pro-inflammatory mediators associated with ALI. The expression of COX-2 was increased in the lungs of AL8810-pretreated mice, as compared with that in the HCl-administered mice ( Figure 2 ). The gene expression of pro-inflammatory mediators, such as tumor necrosis factor (TNF)-α, interleukin (IL)-1β, and IL-6, was also increased in the lungs of HCl+AL8810-administered mice, as compared with that in HCl-administered mice ( Figure 2 ). IL-12, IL-22, and IL-23 are key regulators of lung inflammation. IL-23 is also known to induce IL-22 production [20] . Bronchial epithelial cells express IL-22, which is associated with the repair of damaged tissues [21] . Pre-treatment with AL8810 elevated the gene expression of IL-12, IL-22, IL-23, and interferon (IFN)-γ in the lungs of mice, as compared with HCl treatment (Figure 2 ). Keratinocyte-derived chemokine (KC) and macrophage inflammatory protein (MIP)-2 are known as neutrophil chemoattractant chemokines. Pre-administration with AL8810 significantly enhanced these genes' expression, as compared with HCl treatment (Figure 2 ). Administration of AL8810 alone did not change the expression levels of TNF-α, IL-1β, and IL-6 ( Figure S3 ). These results suggest that inhibition of FP receptors elevated the expression levels of pro-inflammatory mediators in HCl-treated mice. Next, we assessed the gene expression levels of pro-inflammatory mediators associated with ALI. The expression of COX-2 was increased in the lungs of AL8810-pretreated mice, as compared with that in the HCl-administered mice ( Figure 2 ). The gene expression of proinflammatory mediators, such as tumor necrosis factor (TNF)-α, interleukin (IL)-1β, and IL-6, was also increased in the lungs of HCl+AL8810-administered mice, as compared with that in HCl-administered mice ( Figure 2 ). IL-12, IL-22, and IL-23 are key regulators of lung inflammation. IL-23 is also known to induce IL-22 production [20] . Bronchial epithelial cells express IL-22, which is associated with the repair of damaged tissues [21] . Pre-treatment with AL8810 elevated the gene expression of IL-12, IL-22, IL-23, and interferon (IFN)-γ in the lungs of mice, as compared with HCl treatment (Figure 2 ). Keratinocyte-derived chemokine (KC) and macrophage inflammatory protein (MIP)-2 are known as neutrophil chemoattractant chemokines. Pre-administration with AL8810 significantly enhanced these genes' expression, as compared with HCl treatment (Figure 2 ). Administration of AL8810 alone did not change the expression levels of TNF-α, IL-1β, and IL-6 ( Figure S3 ). Administration of AL8810 promoted the expression of pro-inflammatory mediators. AL8810 (10 mg/kg, i.p.) was administered to mice at 1 h prior to HCl (0.1 M, 2 µ L/g, i.t.) administration. The lung was extracted at 6 h after HCl administration. The gene expression levels of COX-2, TNF-α, IL-1β, IL-6, IL-12, IL-22, IL-23, IFN-γ, MIP-2, and KC in the lungs of HCl-and AL8810-treated mice were measured (n = 7). * p < 0.05 vs. HCl. We performed immunostaining analysis to identify the type of cells expressing FP receptors in the lungs of HCl-administered mice. In inflamed lungs, FP receptors were expressed in bronchial epithelial cells ( Figure 3A ) and alveolar macrophage-like cells, which were characterized by a large cytoplasm and round nucleus ( Figure 3B ). FP receptors were not detected when no primary antibody was used ( Figure 3C ). We performed immunostaining analysis to identify the type of cells expressing FP receptors in the lungs of HCl-administered mice. In inflamed lungs, FP receptors were expressed in bronchial epithelial cells ( Figure 3A ) and alveolar macrophage-like cells, which were characterized by a large cytoplasm and round nucleus ( Figure 3B ). FP receptors were not detected when no primary antibody was used ( Figure 3C ). Lung SFTPs are synthesized by epithelial cells to prevent alveolar collapse. SFTPs are key regulators of immune responses in the lungs and alveolar surface tension [22] . Thus, we investigated whether AL8810 affects the expression levels of SFTPs. The expression levels of SFTP-A, SFTP-B, and SFTP-C were significantly decreased in the lungs of HCladministered mice ( Figure 4 ). Administration of HCl tended to lower the expression level of SFTP-D. Moreover, pre-administration of AL8810 lowered the gene expression of SFTP-A, SFTP-B, and SFTP-C, as compared with that in HCl-administered mice ( Figure 4 ). On the other hand, the expression level of SFTP-D was increased in the lungs of AL8810treated mice. These results reveal that pharmacological inhibition of FP receptors reduced the gene expression levels of SFTPs in the lungs of HCl-administered mice. Lung SFTPs are synthesized by epithelial cells to prevent alveolar collapse. SFTPs are key regulators of immune responses in the lungs and alveolar surface tension [22] . Thus, we investigated whether AL8810 affects the expression levels of SFTPs. The expression levels of SFTP-A, SFTP-B, and SFTP-C were significantly decreased in the lungs of HCladministered mice (Figure 4 ). Administration of HCl tended to lower the expression level of SFTP-D. Moreover, pre-administration of AL8810 lowered the gene expression of SFTP-A, SFTP-B, and SFTP-C, as compared with that in HCl-administered mice ( Figure 4 ). On the other hand, the expression level of SFTP-D was increased in the lungs of AL8810-treated mice. These results reveal that pharmacological inhibition of FP receptors reduced the gene expression levels of SFTPs in the lungs of HCl-administered mice. Lung edema is often observed in patients with ALI and is associated with mortality. We thus examined whether an FP receptor antagonist affects lung edema. Administration of HCl increased the wet/dry weight ratio in the lungs, indicating that HCl administration enhanced lung edema ( Figure 5A ). In addition, pre-administration of AL8810 significantly enhanced HCl-induced lung edema ( Figure 5A ). The epithelium sodium channel (ENaC) has a pivotal role in lung edema in ARDS/ALI [21] . Activation of ENaC attenuated LPSinduced ALI in mice [23, 24] . We examined the effect of AL8810 on the gene expression of ENaC in the lungs. Administration with HCl decreased the gene expression of ENaC, as compared with saline-treated mice, which was further diminished in AL8810-preadministered mice ( Figure 5B ). In patients with ALI, the expression levels of adhesion molecules in the epithelium, such as ICAM-1 and E-selectin, are increased [25] . An increase in the expression of ICAM-1 and E-selectin causes infiltration of inflammatory cells to tissues from blood vessels [26] . We first examined whether FP receptors are expressed in HUVECs. FP receptors were not expressed in no-treated HUVECs ( Figure 6A ). LPS stimulation upregulated the mRNA expression of FP receptors, but there were no differences in their expression levels between LPS-and LPS+AL8810-stimulated cells ( Figure 6A ). We then assessed the effect of AL8810 on the expression of adhesion molecules in HUVECs. Administration of LPS increased the gene expression of ICAM-1 in HUVECs, compared with no-treated cells ( Figure 6B ). In contrast, E-selectin gene expression was not detected in no-treated cells. Pretreatment with 3 µM AL8810 elevated the expression levels of both ICAM-1 and E-selectin, as compared with those in LPS-stimulated cells. These results suggest that treatment with AL8810 increased the LPS-induced expression levels of ICAM-1 and E-selectin in endothelial cells. levels of SFTP-A, SFTP-B, and SFTP-C were significantly decreased in the lungs of HCladministered mice (Figure 4) . Administration of HCl tended to lower the expression level of SFTP-D. Moreover, pre-administration of AL8810 lowered the gene expression of SFTP-A, SFTP-B, and SFTP-C, as compared with that in HCl-administered mice (Figure 4) . On the other hand, the expression level of SFTP-D was increased in the lungs of AL8810treated mice. These results reveal that pharmacological inhibition of FP receptors reduced the gene expression levels of SFTPs in the lungs of HCl-administered mice. Lung edema is often observed in patients with ALI and is associated with mortality. We thus examined whether an FP receptor antagonist affects lung edema. Administration of HCl increased the wet/dry weight ratio in the lungs, indicating that HCl administration enhanced lung edema ( Figure 5A ). In addition, pre-administration of AL8810 significantly enhanced HCl-induced lung edema ( Figure 5A ). The epithelium sodium channel (ENaC) has a pivotal role in lung edema in ARDS/ALI [21] . Activation of ENaC attenuated LPSinduced ALI in mice [23, 24] . We examined the effect of AL8810 on the gene expression of ENaC in the lungs. Administration with HCl decreased the gene expression of ENaC, as compared with saline-treated mice, which was further diminished in AL8810-pre-administered mice ( Figure 5B ). In patients with ALI, the expression levels of adhesion molecules in the epithelium, such as ICAM-1 and E-selectin, are increased [25] . An increase in the expression of ICAM-1 and E-selectin causes infiltration of inflammatory cells to tissues from blood vessels [26] . We first examined whether FP receptors are expressed in HUVECs. FP receptors were not expressed in no-treated HUVECs ( Figure 6A ). LPS stimulation upregulated the mRNA ALI and ARDS are severe respiratory disorders, characterized by severe hypoxemia [4] . According to previous reports, the mortality rate of ALI/ARDS has remained high [5, 27] . To investigate the mechanism of ALI/ARDS progression, several animal models, such as mechanical ventilation-, LPS-, hypoxia-, bleomycin-, and acid aspiration-induced ALI, have been used [28] . In addition, it has been reported that there is a gender difference in pneumonia. However, these different animal models show distinct clinical and pathological features and mechanisms of progression of ALI/ARDS. Aspiration of gastric contents is an important risk factor for ALI [29] . Intratracheal injection of acid causes neutrophil migration and injures the airways, alveolar epithelium, and capillary endothelium [28] . Acid aspiration also changes alveolar clearance. In this study, we used an acid aspiration-induced ALI mouse model to elucidate the role of PGF2α/FP signaling. Inhibition of FP receptors by AL8810 enhanced HCl-induced pulmonary dysfunction, neutrophil migration, and lung edema, while it decreased SFTP expression. Thus, we showed that PGF2α/FP signaling is involved in regulating the progression of acid-induced ALI, which is summarized in Figure S4 . Neutrophils are major immune cells that are observed in BALF and the lungs of patients with ALI/ARDS. In response to pro-inflammatory mediators, neutrophils migrate to the alveolar space [30] . Infiltrating neutrophils cause tissue damage due to the production of histotoxic mediators, such as ROS and neutrophil extracellular traps. There are four steps involved in the recruitment of neutrophils to tissues from blood vessels: (ⅰ) integrinmediated rolling; (ⅱ) activation; (ⅲ) adhesion to vascular endothelium; and (ⅳ) transendothelial migration [31, 32] . Upregulation of adhesion molecules such as ICAM-1 and Eselectin in the vascular endothelium induces neutrophil migration [26] . In an in vitro assay, exogenous PGF2α administration upregulated CXCR1 expression and increased neutrophil migration [18] . However, we showed that the inhibition of FP receptors promoted neutrophil migration into the lungs and BALF ( Figure 1C,D) . We also demonstrated that AL8810 increased the LPS-induced gene expression of ICAM-1 and E-selectin in HUVECs ( Figure 6 ). Taken together, these results indicate that inhibition of FP receptors in the vascular endothelium increased the expression of molecular adhesion factors, which promoted neutrophil migration into the lungs. Adhesion molecules are also expressed in bronchial epithelium [33] . Upregulation of the expression of adhesion molecules promotes leucocyte infiltration into bronchi. It is possible that inhibition of FP receptors in bronchial epithelium also regulates the expression of adhesion molecules such as ICAM-1 and Eselectin, which increases neutrophil migration into the lungs. Further investigation is needed to clarify the regulatory mechanism of PGF2α/FP signaling on neutrophil migration. ALI and ARDS are severe respiratory disorders, characterized by severe hypoxemia [4] . According to previous reports, the mortality rate of ALI/ARDS has remained high [5, 27] . To investigate the mechanism of ALI/ARDS progression, several animal models, such as mechanical ventilation-, LPS-, hypoxia-, bleomycin-, and acid aspiration-induced ALI, have been used [28] . In addition, it has been reported that there is a gender difference in pneumonia. However, these different animal models show distinct clinical and pathological features and mechanisms of progression of ALI/ARDS. Aspiration of gastric contents is an important risk factor for ALI [29] . Intratracheal injection of acid causes neutrophil migration and injures the airways, alveolar epithelium, and capillary endothelium [28] . Acid aspiration also changes alveolar clearance. In this study, we used an acid aspirationinduced ALI mouse model to elucidate the role of PGF 2α /FP signaling. Inhibition of FP receptors by AL8810 enhanced HCl-induced pulmonary dysfunction, neutrophil migration, and lung edema, while it decreased SFTP expression. Thus, we showed that PGF 2α /FP signaling is involved in regulating the progression of acid-induced ALI, which is summarized in Figure S4 . Neutrophils are major immune cells that are observed in BALF and the lungs of patients with ALI/ARDS. In response to pro-inflammatory mediators, neutrophils migrate to the alveolar space [30] . Infiltrating neutrophils cause tissue damage due to the production of histotoxic mediators, such as ROS and neutrophil extracellular traps. There are four steps involved in the recruitment of neutrophils to tissues from blood vessels: (i) integrin-mediated rolling; (ii) activation; (iii) adhesion to vascular endothelium; and (iv) transendothelial migration [31, 32] . Upregulation of adhesion molecules such as ICAM-1 and E-selectin in the vascular endothelium induces neutrophil migration [26] . In an in vitro assay, exogenous PGF 2α administration upregulated CXCR1 expression and increased neutrophil migration [18] . However, we showed that the inhibition of FP receptors promoted neutrophil migration into the lungs and BALF ( Figure 1C,D) . We also demonstrated that AL8810 increased the LPS-induced gene expression of ICAM-1 and E-selectin in HUVECs ( Figure 6 ). Taken together, these results indicate that inhibition of FP receptors in the vascular endothelium increased the expression of molecular adhesion factors, which promoted neutrophil migration into the lungs. Adhesion molecules are also expressed in bronchial epithelium [33] . Upregulation of the expression of adhesion molecules promotes leucocyte infiltration into bronchi. It is possible that inhibition of FP receptors in bronchial epithelium also regulates the expression of adhesion molecules such as ICAM-1 and E-selectin, which increases neutrophil migration into the lungs. Further investigation is needed to clarify the regulatory mechanism of PGF 2α /FP signaling on neutrophil migration. Pulmonary surfactant is composed of lipids and proteins, and it is produced in type 2 alveolar epithelial cells [34] . Surfactant lipids are synthesized in the endoplasmic retic- 8 of 12 ulum. The components of alveolar surfactant proteins are SFTP-A, SFTP-B, SFTP-C, and SFTP-D. The lack of surfactant lipids leads to death in patients with ARDS [35] . Intratracheal injection of SFTP-B and SFTP-C significantly improves mortality and morbidity in patients with ARDS [36] . SFTP-A and SFTP-D regulate alveolar surface tension. Gene deficiency of SFTP-B is lethal due to atelectasis and respiratory failure [37] . Inhibition of FP receptors decreased the expression of SFTP-A, SFTP-B, SFTP-C, and SFTP-D (Figure 4) . We assessed the mRNA expression of SFTP but not the protein expressions. Previous studies have shown that mRNA expression patterns are not necessarily correlated with protein expression [38, 39] . Further studies are needed to clarify the details of the regulatory mechanism of PGF 2α /FP signaling on the production of pulmonary surfactant, including the control of these proteins' expression. FP receptors were expressed in the bronchial epithelium and macrophage-like cells (Figure 3 ). It has been reported that alveolar macrophage-derived pro-inflammatory mediators are initiators of inflammation in ALI [40] . We previously reported that the inhibition of FP receptors promoted the gene expression of pro-inflammatory mediators such as IL-1β, TNF-α, and inducible nitric oxide synthase in LPS + IFN-γ-stimulated macrophages [41] . In this model, inhibition of FP receptors in alveolar macrophages may produce pro-inflammatory mediators, which results in increased neutrophil migration. The airway epithelium plays a critical role in fluid transport. Patients with ALI/ARDS with protein-rich fluid in the alveolar space show higher mortality rates than those without protein-rich fluid [3] . ENaC and cystic fibrosis transmembrane regulator (CFTR) are major transporters that regulate alveolar fluid clearance [42] . ENaC and CFTR are expressed in the epithelium and endothelium. PGF 2α enhances ENaC activity in cortical collecting duct cells [43] . In this HCl-induced ALI model, administration with AL8810 enhanced HCl-induced lung edema ( Figure 5A ). Administration with AL8810 also decreased the gene expression of ENaC in the lungs ( Figure 5B ). Therefore, it is possible that the FP receptors expressed in the bronchial epithelium are involved in the regulation of ENaC activation, which maintains fluid clearance. In the present study, we showed that inhibition of FP receptors increased the gene expression of pro-inflammatory mediators, neutrophil migration into BALF, and lung edema in HCl-administered mice. This is the first report that PGF 2α /FP signaling is important in regulating the progression of HCl-induced ALI. Inhibition of FP receptors increased the gene expression of pro-inflammatory mediators and neutrophil migration into the lung, and it enhanced lung permeability and disruption of vascular endothelial cells in HCl-administered mice. Moreover, pharmacological inhibition of FP receptors elevated the expression of adhesion molecules in HUVECs. Furthermore, inhibition of FP receptors promoted the endothelial barrier dysfunction and the expression of adhesion molecules, which exacerbated HCl-induced ALI in mice. Therefore, PGF 2α /FP signaling is important in regulating the progression of HCl-induced ALI. In addition, FP receptor agonists may have future pharmaceutical potential to treat ALI in human patients. All experiments and animal care were conducted in accordance with the institutional guidelines of the Osaka Medical and Pharmaceutical University. C57BL/6J mice (8-weekold females; Japan SLC, Shizuoka, Japan) were used to induce lung inflammation. Mice were anesthetized with 3% (v/v) isoflurane (FUJIFILM Wako Pure Chemical, Osaka, Japan) and 50 mg/kg pentobarbital sodium (Nacalai Tesque, Kyoto, Japan). Acute lung injury was induced by intratracheal (i.t.) administration of HCl (0.1 M, 2 µL/g). AL8810 (10 mg/kg in 1% DMSO, Cayman Chemical, Ann Arbor, MI, USA) was administered intraperitoneally at 1 h before HCl administration. Mice were randomly divided into three groups: ad-ministration of saline (1% DMSO in 200 µL saline, i.p.), HCl (1% DMSO in 200 µL saline, 30 min before HCl administration, i.p.), and HCl+AL8810 (n = 3-5 per group/experiment, repeated 4 times). At six hours after saline or HCl administration, SpO 2 levels were measured using a mouseOx pulse oximeter (Starr Life Sciences, Oakmont, PA, USA). The pulse oximeter was placed around the neck of mice that were anesthetized using isoflurane (induction; 3% (v/v), maintenance; 1.5-2% (v/v)). The levels of SpO 2 were measured every second for 1 min while maintaining the breathing rate at 120-160 breaths per minute (bpm). The data are represented as the average of the SpO 2 levels measured for 1 min. At six hours after saline or HCl administration, total RNA was extracted using RNAiso Plus (Takara Bio, Kyoto, Japan), and the concentration of total RNA was adjusted to 0.5 µg/µL. RNA was reverse-transcribed to cDNA using a random 9-mer primer (Takara Bio) and ReverTra Ace (Toyobo, Osaka, Japan). Reverse transcription was carried out at 30 • C for 10 min, followed by incubation at 42 • C for 60 min. Subsequently, the reaction was stopped by heat inactivation at 95 • C for 5 min. The cDNAs were used for quantitative analysis of target gene expression levels using a Power SYBR Green PCR Master Mix (Thermo Fisher Scientific, Waltham, MA, USA) and a LightCycler 96 System (Roche Life Science, Penzberg, Germany). The mRNA expression levels were normalized to 18S rRNA levels and calculated using the ∆∆Ct method. Details of the primer sets used in the qPCR analysis are shown in Table 1 . At six hours after administration of saline or HCl, the lung was extracted and weighed (wet weight). Then, the lung was dried at 50 • C, and after 24 h, the dried weight was measured (dry weight). The lung wet/dry weight ratio was used as an index of lung water accumulation. Cells in BALF were attached to glass slides by cytospin centrifugation at 2000 rpm for 5 min (Thermo Fisher Scientific). The glass slides were stained with Diff Quick (Sys-mex Corporation, Hyogo, Japan) according to the manufacturer's instructions. The cell populations were counted for 4 randomly selected fields. PGF 2α and PGE 2 levels in BALF were measured using the respective ELISA kits (Cayman Chemical) according to the manufacturer's instructions. Briefly, BALF was centrifuged at 450× g for 3 min at 4 • C, and the resulting supernatant was used for the measurement of PGF 2α and PGE 2 levels. At six hours after saline or HCl administration, the lung was extracted. The lung was fixed in 4% (w/v) paraformaldehyde for 48 h and embedded in paraffin. The tissue block was cut into 4 µm sections. To perform the antigen retrieval, the glass slides were incubated with sodium citrate (10 mM, pH 6.0) for 10 min at 95 • C, followed by incubation for 30 min at 25 • C. To block endogenous peroxidase activity, the glass slides were incubated with 3% (v/v) hydrogen peroxidase for 10 min at 25 • C. After washing, to block the non-specific protein adherence to sections and permeabilize the lung, the sections were incubated with 10% (v/v) normal goat serum and 0.1% (v/v) Triton-X in PBS for 15 min at 25 • C. Then, the glass slides were washed with PBS and incubated with anti-FP receptor antibody (Cayman Chemical) [44] for 16 h at 4 • C. After washing with PBS, the glass slides were incubated with biotin-conjugated anti-rabbit IgG secondary antibody (Santa Cruz Biotechnology, Dallas, TX, USA) for 3 h at 25 • C. The glass slides were incubated with avidin-biotin complex reagent (Nacalai Tesque) for 30 min at 25 • C, followed by staining using a DAB substrate staining kit (Nacalai Tesque). Nuclear counterstaining was performed with hematoxylin as described previously [26] . Human umbilical vein endothelial cells (HUVECs) were obtained from the JCRB cell bank (National Institutes of Biomedical Innovation, Health and Nutrition, Osaka, Japan). HUVECs were cultured in Endothelial Cell Basal Medium (EBM)-2 medium with Endothelial Cell Growth Medium 2, containing 2% (v/v) fetal bovine serum (PromoCell GmbH, Heidelberg, Germany), 100 U/mL penicillin, and 100 µg/mL streptomycin (Nacalai Tesque) at 37 • C in an atmosphere of 5% CO 2 . The HUVECs were stimulated with 100 ng/mL LPS (Sigma, St. Louis, MO, USA) for 24 h. AL8810 (1 and 3 µM) was treated at 30 min before LPS stimulation. The data are presented as mean ± S.D. Statistical analysis between two groups was conducted using Student's t-test. For more than three groups, statistical analysis was conducted using a one-way ANOVA. Statistical significance was set at p < 0.05. A novel coronavirus from patients with pneumonia in China SARS-CoV-2 vaccines in development The acute respiratory distress syndrome Acute lung injury: Epidemiology, pathogenesis, and treatment Epidemiology, patterns of care, and mortality for patients with acute respiratory distress syndrome in intensive care units in 50 countries Effect of vitamin C infusion on organ failure and biomarkers of inflammation and vascular injury in patients with sepsis and severe acute respiratory failure: The CITRIS-ALI randomized clinical trial -agonist for treatment of acute lung injury The role of endothelial cells in the resolution of acute inflammation Acute respiratory distress in adults Adhesion receptors of the immune system Neutrophils in tissue injury and repair Enzymes of the cyclooxygenase pathways of prostanoid biosynthesis Physiology and pathophysiology of prostanoid receptors Cyclooxygenase 2 plays a pivotal role in the resolution of acute lung injury Anti-inflammatory role of PGD 2 in acute lung inflammation and therapeutic application of its signal enhancement Prostaglandin E 2 mediates IL-1β-related fibroblast mitogenic effects in acute lung injury through differential utilization of prostanoid receptors Recent reports about enzymes related to the synthesis of prostaglandin (PG) F 2 (PGF 2α and 9α, 11β-PGF 2 ) Prostaglandin F 2α -F-prostanoid receptor signaling promotes neutrophil chemotaxis via chemokine (C-X-C motif) ligand 1 in endometrial adenocarcinoma Prostaglandin F 2α receptor signaling facilitates bleomycin-induced pulmonary fibrosis independently of transforming growth factor-β IL-22 production is regulated by IL-23 during Listeria monocytogenes infection but is not required for bacterial clearance or tissue protection Interleukin-22: Immunobiology and pathology Immunomodulatory roles of surfactant proteins A and D: Implications in lung disease Netrin-1 promotes epithelial sodium channel-mediated alveolar fluid clearance via activation of the adenosine 2B receptor in lipopolysaccharide-induced acute lung injury Oxymatrine attenuates lipopolysaccharide-induced acute lung injury by activating the epithelial sodium channel and suppressing the JNK signaling pathway Increased plasma soluble adhesion molecules; ICAM-1, VCAM-1, and E-selectin levels in patients with slow coronary flow Neutrophil tethering on E-selectin activates β2 integrin binding to ICAM-1 through a mitogen-activated protein kinase signal transduction pathway Past and present ARDS mortality rates: A systematic review Animal models of acute lung injury Clinical risks for development of the acute respiratory distress syndrome Neutrophils in the initiation and resolution of acute pulmonary inflammation: Understanding biological function and therapeutic potential Neutrophil heterogeneity: Implications for homeostasis and pathogenesis ICAM-1 signaling in endothelial cells Cell adhesion molecules and the bronchial epithelium Role of pulmonary surfactant components in surface film formation and dynamics Surfactant alteration and replacement in acute respiratory distress syndrome Surfactant protein-B polymorphisms and mortality in the acute respiratory distress syndrome Prolonged survival in hereditary surfactant protein B (SP-B) deficiency associated with a novel splicing mutation On the dependency of cellular protein levels on mRNA abundance Correlation between protein and mRNA abundance in yeast The acute respiratory distress syndrome: From mechanism to translation Contribution of FP receptors in M1 macrophage polarization via IL-10-regulated nuclear translocation of NF-kB p65 Regulation of ENaC-mediated alveolar fluid clearance by insulin via PI3K/Akt pathway in LPS-induced acute lung injury Effects of lipids on ENaC activity in cultured mouse cortical collecting duct cells Failure of parturition in mice lacking the prostaglandin F receptor Informed Consent Statement: "Not applicable" for studies not involving humans. The data presented in this study are available on request from the corresponding author. The authors declare no conflict of interest.