ABSTRACT
Streptococcus suis is a common pathogen colonising the respiratory tract of pigs. It can cause meningitis, sepsis and pneumonia leading to economic losses in the pig industry worldwide. Cyclooxygenase-2 (COX-2) and its metabolites play an important regulatory role in different biological processes like modulation of inflammation and immune activation. In this report we analysed the induction of COX-2 and the production of its metabolite prostaglandin E2 (PGE2) in a porcine precision-cut lung slice (PCLS) model. Using Western blot analysis, we found a time-dependent induction of COX-2 in the infected tissue resulting in increased PGE2 levels. Immunohistological analysis revealed a strong COX-2 expression in the proximity of the bronchioles between the ciliated epithelial cells and the adjacent alveolar tissue. The morphology, location and vimentin staining suggested that these cells are subepithelial bronchial fibroblasts. Furthermore, we showed that COX-2 expression as well as PGE2 production was detected following infection with two prevalent S. suis serotypes and that the pore-forming toxin suilysin played an important role in this process. Therefore, this study provides new insights in the response of porcine lung cells to S. suis infections and serves as a basis for further studies to define the role of COX-2 and its metabolites in the inflammatory response in porcine lung tissue during infection with S. suis.
Introduction
Streptococcus suis is an important coloniser of the upper respiratory tract of pigs. It can cause a variety of disease manifestations ranging from pneumonia, septicaemia, meningitis to arthritis leading to great economic losses in the pig industry (reviewed in (1, 2)). S. suis is also considered as a zoonotic agent that can cause meningitis and septicaemia (3, 4). The bacterium shows a high diversity of more than 700 sequence types and can be classified into different serotypes based on its capsule polysaccharide (5). Although serotype 2 strains are considered the most common ones, causing infections in pigs and humans (1), infections with serotype 9 strains are increasing in importance in several countries particularly in Western Europe (1, 6). Pathogenesis of S. suis infections is not completely understood, but a strong inflammatory response is a hallmark of S. suis infections. Some virulence and virulence-associated factors have been identified and characterised including the capsule, muraminidase-released protein, the extracellular factor and the pore-forming toxin suilysin (SLY) (reviewed in (7)). SLY belongs to the group of cholesterol-dependent toxins that are produced by numerous Gram-positive bacteria. Oligomerisation of the toxin subunits in cholesterol rich membranes of host cells leads to the formation of large pores and consecutive cellular homeostatic changes culminating in immune activation and cell death (8).
Prostaglandin E2 (PGE2), a small-molecule derivative of arachidonic acid produced by a variety of cell types, participates in different biological processes like modulation of inflammation and immune activation (9). In the lung, PGE2 is considered to play an important regulatory role in the control of inflammatory responses and tissue repair processes (10). Generation of PGE2 starts with the liberation of arachidonic acid from cell membranes followed by conversion into prostaglandin H2 by the rate-limiting enzyme cyclooxygenase (COX), which can be further converted into PGE2 by PGE2 synthases (11, 12). Of the two isoforms, COX-1 is considered to be constitutively expressed and has homeostatic functions, whereas COX-2 is the inducible isoform involved in pathophysiological processes (12). Released PGE2 can signal via four different receptors and elicit different immunomodulatory effects (13).
Induction of COX-2 and production of PGE2 were demonstrated in tissue biopsies from S. pyogenes-infected patients as well as in the tissue of experimentally infected mice (14) and were also found in human lung tissue infected with S. pneumoniae (15). Furthermore, induction of COX-2/PGE2 was observed in swine infections with bacterial lung pathogens like Mycoplasma hyopneumoniae and Actinobacillus pleuropneumoniae (16, 17). Notably, to the best of our knowledge, COX-2 induction has not yet been reported for respiratory tract infections by S. suis. Thus, this study aimed at investigating whether COX-2, the rate-limiting en-zyme of PGE2 production, is induced by S. suis in porcine lung tissue and at identifying bacterial factors that might contribute to induction.
Materials and Methods
Reagents
PCLS culture media were obtained from Thermo Fisher Scientific (Waltham, MA, USA) and Sigma-Aldrich (St. Louis, MO, USA). If not stated otherwise, all other reagents were from Sigma-Aldrich or Roth (Karlsruhe, Germany). The experimental COX-2 inhibitor NS-398 and recombinant porcine IL-1β were purchased from Bio-Techne (Minneapolis, MN, USA). Fluorescently labelled phalloidin (Phalloidin-iFluor 647) was obtained from Abcam (Cambridge, UK). The following primary antibodies were used: monoclonal rabbit antibody against COX-2 (Clone SP21, Cat# SAB5500087-100UL, Sigma-Aldrich), mouse monoclonal anti-acetylated α-Tubulin antibody (Cat# sc-23950, RRID:AB_628409, St. Cruz (Dallas, TX, USA)), mouse monoclonal anti-vimentin antibody (Cat# GA630, RRID:AB_2827759, Agilent (St. Clara, CA, USA)) and rabbit monoclonal antibody against GAPDH (D16H11, RRID:AB_11129865, Cell Signaling Technology (Beverly, MA, USA)). Generation of the polyclonal antiserum against SLY was described previously (18). Secondary goat antimouse IgG (H+L) Alexa Fluor® 488 conjugated antibody (Cat# A-11029; RRID: AB_2534088), goat anti-rabbit IgG (H+L) Alexa Fluor® 488 conjugated antibody (Cat# A-11029; RRID: AB_2536097) and goat anti-rabbit IgG Alexa Fluor® 568 (Cat# A-27034; RRID: AB_143157) were obtained from Thermo Fisher Scientific. Secondary goat antirabbit IgG, HRP-linked (#7074, RRID:AB_2099233) was obtained from Cell Signaling Technology.
Bacterial strains and recombinant suilysin protein
The virulent, SLY-positive S. suis serotype 2 strain 10 (S10) was kindly provided by H. Smith (Lelystad, the Netherlands) (19). Its isogenic SLY-deficient mutant (S10Δsly) was constructed by the insertion of an erythromycin cassette in the sly gene (18). Complementation of S10Δsly (S10Δsly-C) was done by allelic exchange and was described in a previous publication (20). S. suis serotype 9 strain 8067 was isolated from a piglet and described earlier (21). All strains were grown on Columbia agar supplemented with 7% (v/v) sheep blood (Oxoid™, Thermo Fisher Scientific) overnight at 37°C under aerobic conditions. For infection experiments, cryoconserved bacterial stocks were prepared from liquid cultures in Todd-Hewitt Broth (THB; Bacto™, Becton Dickinson, Franklin Lakes, NJ, USA) at the late-exponential growth phase (OD600 = 1.1) as previously described (22). Recombinant suilysin (rSLY) was expressed, purified and characterised as described previously (18).
Generation of PCLS and infection with S. suis
Precision-cut lung slices were prepared as previously described (22) from lungs of freshly-slaughtered pigs (obtained from a local abattoir, Leine-Fleisch GmbH, Laatzen, Germany). In brief, the cranial, middle, and intermediated lobes were carefully removed and the bronchi were filled with 37°C low-melting agarose (GERBU, Heidelberg, Germany) in RPMI-1640 medium (Sigma-Aldrich). After solidifying on ice, cylindrical portions of lung tissue were punched out with a tissue coring tool so that the bronchus/bronchiole was in the middle. The approximately 300-μm thick slices were cut by a Krumdieck tissue slicer (model MD 4000-01; TSE Systems, Chesterfield, MO, USA). PCLS were collected in RPMI-1640 (Thermo Fisher Scientific) with antibiotics and antimycotics (1 μg/mL clotrimazole, 10 μg/mL enrofloxacin (Bayer, Leverkusen, Germany), 50 μg/mL kanamycin, 100 U/mL penicillin, 100 μg/mL streptomycin/ml, 50 μg/mL gentamicin, 2.5 μg/mL amphotericin B). For removal of the agarose, PCLS were bubbled with a normoxic gas mixture for two hours at 37°C as previously described (23). Then, the slices were transferred to 24-well plates (Greiner Bio-One, Frickenhausen, Germany) and incubated for one day in RPMI-1640 medium with antibiotics and antimycotics at 37°C and 5% CO2. On the following day, viability of the slices was analysed by observing the ciliary activity using a DMi1 light microscope (Leica, Wetzlar, Germany). PCLS with ciliary activity of at least 80-90% were selected and washed twice with phosphate-buffered saline (PBS; Sigma-Aldrich). Afterwards, the slices were incubated in RPMI-1640 medium containing no antibiotics and antimycotics for another day.
After washing the slices twice with PBS, they were inoculated with approximately 107 CFU/well of S. suis S10, S10Δsly, S10Δsly-C, and S8067 in 500 μL RPMI-1640, respectively. Slices were incubated for up to 24 hours (h) at 37°C and 5% CO2. In the experiments shown in Figure 1CD, slices were left uninfected or infected for 24 h at 37°C and 5% CO2 in the presence of 10 μM of the COX-2 inhibitor NS-398 or the vehicle DMSO. Supernatant and slices were collected at indicated time points for PGE2-ELISA, Western blot analysis and immunofluorescence staining. Slices were washed twice with PBS before collecting the samples. All experiments were performed in duplicates and repeated at least three times.
Isolatation of primary brochial fibroblasts and infection with S. suis
For isolating primary porcine bronchial fibroblasts, the bronchial tissue was carefully dissected, any parenchymal connective tissue was removed and the bronchus was cut into 5 mm thick rings. The pieces were placed in a 10 cm diameter cell culture dish in DMEM (Thermo Fisher Scientific) supplemented with 10% FCS, 1% glutamine and antibiotics (100 U/mL penicillin, 100 μg/mL streptomycin, 50 μg/mL gentamicin, 2.5 μg/mL amphotericin B) and incubated at 37°C and 5% CO2. After two weeks in culture, fibroblasts had grown out from the explanted tissue. The tissue pieces were removed and the cells were cultured for approx. 2-3 weeks until confluent cells islands were observed. Then, the cultures were passaged with a split ratio of 1:2 into 75-cm2 tissue culture flasks. Experiments were performed with cells between passages three and six showing typical fibroblast morphology and positive staining for vimentin by immunofluorescence microscopy. For infection with S. suis, fibroblasts were trypsinised, counted and 1.0 × 105 cells per well were seeded on glass coverslips placed in a 24-well plate in DMEM with 10% FCS and 1% glutamine. After incubation at 37°C and 5% CO2 over night, cells were infected for 8 h with S. suis using a multiplicity of infection (MOI) of one or five or left uninfected. As positive control, cells were stimulated with 40 ng/ml recombinant porcine IL-1β for 8 h.
SDS-PAGE and Western blotting
For protein analysis by Western blotting, whole tissue lysates were prepared in cell extraction buffer (Thermo Fisher Scientific) supplemented with protease inhibitor cocktail P8340, 1 mM AEBSF and Halt phosphatase inhibitor cocktail (Thermo Fisher Scientific) using an MP Biomedicals™ FastPrep-24™ 5G Instrument (St. Ana, CA, USA). Crude lysates were cleared by centrifugation and protein amounts were quantified by MicroBC Assay Protein Quantitation Kit (Interchim, Montluçon, France). Equal protein amounts (15 μg) were separated on 12% SDS-PAGE gels which were then blotted onto PVDF membranes. The latter were blocked in 5% (w/v) skimmed milk for 1 h at room temperature, washed and incubated overnight with the respective primary antibodies at 4°C. After washing, the blots were incubated for 1 h with secondary antibodies against rabbit IgG and washed. All washing steps were performed in TBS/0.05% (v/v) Tween® 20 (3 × 5 min). Blots were developed using SuperSignal West Pico Chemiluminescent Substrate (Thermo Fisher Scientific) and a ChemoCam Imager 3.2 (Intas, Göttingen, Germany). Densitometry was performed using LabImage 1D (Kapelan Bio-Imaging, Leipzig, Germany).
PGE2 ELISA
PGE2 levels in the supernatants were determined using the PGE2 ELISA kit (Enzo Life Science, Farmingdale, NY, USA) in accordance with the manufacturer’s recommendations.
Immunofluorescence staining of histological sections and primary fibroblasts
PCLS were fixed with 4% (v/v) formalin, embedded in paraffin blocks and sections of 3-4 μm were prepared. Sections were deparaffinised in Roti®Histol (Carl Roth), rehydrated in descending series of ethanol (100%, 95%, and 70%) and cooked in sodium-citrate buffer (10 mM, pH 6.0, 10 min) for antigen retrieval. To block unspecific binding sides, the samples were incubated in 1% (v/v) bovine serum albumin (BSA), 5% (v/v) goat serum, 0.3% (v/v) Triton-X-100 and 0.05% (v/v) Tween® 20 in PBS for one hour at room temperature. All antibodies were diluted in 1% (v/v) BSA and 0.05% (v/v) Tween® 20 in PBS and incubated for one hour at room temperature or overnight at 4°C. For visualisation of cilia, a monoclonal mouse antibody against acetylated α-tubulin (1:500), followed by an Alexa Fluor® 488 goat-anti-mouse IgG (H+L) antibody (1:500), was used. COX-2 was stained using an anti-COX-2 antibody (1:100) and a goat-anti-rabbit Alexa Fluor® 568 (1:500). Vimentin was visualised with a mouse monoclonal antibody diluted 1:100 in combination with an Alexa Fluor® 488 goat-anti-mouse IgG (H+L) antibody (1:500). Cell nuclei were visualized by 4’, 6 diamidino-2-phenylindole (DAPI, 0.5 μg/mL in PBS, Cell Signaling Technology). Stained sections were mounted with ProLong® Gold Antifade Reagent (Cell Signaling Technology) and stored at 4°C until examination. Fibroblasts were fixed with 3% (v/v) formaldehyde in PBS (methanol-free, Electron Microscopy Science, Hatfield, PA, USA) for 20 min at room temperature. Fixed cells were washed three times with PBS, permeabilised with 0.1% (v/v) Triton X-100 for 5 min and blocked in PBS containing 1% (w/v) BSA, 5% (v/v) goat serum and 0.05% (v/v) Tween® 20 for 30 min at room temperature. All antibodies were diluted in PBS containing 1% (v/v) BSA and 0.05% (v/v) Tween® 20 and cells were washed for 5 min with PBS between staining steps. COX-2 was stained using an anti-COX-2 antibody (1:100, 1 h) and a secondary goat-anti-rabbit Alexa Fluor® 488 antibody (1:500, 45 min) at ambient temperature. The actin cytoskeleton was stained with Phalloidin-iFluor 647 (1:500 in PBS) for 20 min at room temperature. Visualisation of nuclei and mounting was done as described above for PCLS.
Microscopy and image analysis
Confocal microscopy of PCLS was performed using a TCS SP5 confocal laser scanning microscope equipped with a 40× 1.25-NA oil HCX Plan Apochromat objective and a 63× 1.40-0.60-NA oil HCX Plan Apochromat objective (Leica). Overlapping image stacks with a z-distance of 1.0 μm per plane were acquired using a 1-Airy-unit pinhole diameter in sequential imaging mode to avoid bleed through. Maximum intensity projections were generated and the resulting images were stitched together using the pairwise stitching plugin (24) in Fiji-ImageJ (25). Widefield microscopy of fibroblasts was performed with a Nikon Eclipse Ti-S microscope equipped with a 20× 0.5-NA CFI Plan Fluor objective and a Nikon DS-QiMC-U2 camera controlled by NIS-Elements BR version 4.51.01 (Nikon, Tokyo, Japan). For display purposes, images were identically adjusted for brightness and contrast using Fiji-ImageJ.
COX-2 expression in fibroblasts was quantified using Cell-Profiler software version 4.0.7 (https://cellprofiler.org/) as previously described with modifications (26). First, individual cells were identified by segmenting nuclei based on the DAPI signal. Next, the identified primary objects were propagated to obtain a mask for the cytoplasm. Subsequently, the intensity in the COX-2 channel was measured using these cytoplasm masks with the built-in measurement modules in CellProfiler. Measurements were exported and final data analysis was done with Python 3.8 (Python Software Foundation, https://www.python.org/).
Statistical analysis
Values are expressed as means ± SD from at least three independent experiments. Statistical analysis was performed with Python 3.8 (Python Software Foundation, https://www.python.org/) and the Pingouin (0.3.8) package (27). Welch ANOVA followed by Games-Howell post-hoc test was used for comparison of three or more groups.
Results
S. suis induced expression of COX-2 in porcine lung tissue
Studies using different streptococcal pathogens indicated an up-regulation of COX-2 in streptococcal infections (14, 15). Since virtually no study has systematically analysed the biology of COX-2 in the porcine lung following S. suis infection, we used an ex vivo model of porcine precision-cut lung slices infected with S. suis to explore COX-2 induction and PGE2 synthesis.
To investigate whether COX-2 was expressed in S. suis-infected PCLS, slices were infected for the indicated time and COX-2 induction was analysed by Western blotting. In unin-fected control slices, no induction of COX-2 expression was detectable during the course of the experiment. In contrast, in slices infected with S. suis S10 increasing amounts of COX-2 were detected over time, which started to rise at 4 h and continuously increased until the end of the experiment (Figure 1A). Densitometric analysis revealed a robust and significant induction after 24 h (Figure 1B).
Next, we determined PGE2 levels in S. suis infected PCLS after 24 h to test whether the increased expression of COX-2 translated into increased COX-2 activity. The selective experimental inhibitor NS-389, that inhibits COX-2 activity, and thereby, production of prostaglandins by COX-2, was included to determine the amount PGE2 produced by COX-2. As shown in Figure 1C, PGE2 was significantly increased in the supernatants of infected tissue compared with uninfected PCLS. This increase of PGE2 was completely blocked by treatment of PCLS with 10 μM NS-398, indicating that the synthesis of PGE2 in response to S. suis infection was mainly mediated by COX-2 (Figure 1C). Western blot analysis revealed an increase of COX-2 protein induction in the presence of the inhibitor compared to PCLS infected in the presence of solely DMSO (Figure 1D).
Taken together, the data indicate that COX-2 is strongly up-regulated in porcine PCLS upon infection with S. suis which results in the production of PGE2.
Localisation of COX-2 induction in S. suis infected PCLS
In an ex vivo S. pneumoniae human lung infection model alveolar type II cells, the vascular endothelium, and alveolar macrophages were identified as primary COX-2 producing cells (15). To analyse which cells express COX-2 in our porcine PCLS model after infection with S. suis, we localised the COX-2 protein by immunohistochemistry.
COX-2 staining was more abundant and intense in infected lung tissue than in uninfected control tissue (Figure 2). Close examination of the histological sections demonstrated that COX-2 was mainly expressed in cells located in a region between the ciliated cells of the bronchioles and the corresponding proximal alveolar tissue, representing the connective tissue surrounding the bronchioles (Figure 2, S10, closed arrowheads). We only found a low expression of COX-2 in a few cells in the adjacent alveolar tissue (Figure 2, S10, open arrowheads) as well as in the more distant alveolar tissue (Figure 3A, S10, closed arrowheads). Furthermore, examination of COX-2 induction in blood vessels did not show any induction in endothelial cells lining the lumen of the vessels, but we observed induction in some cells located in the basement membrane (Figure 3B, closed arrowheads). Finally, staining for vimentin, a widely used marker for fibroblasts, showed a strong signal in elongated/spindle-shaped cells positive for COX-2 in the bronchiolar region (Figure 4, S10, closed arrowheads).
To test whether COX-2 can be directly induced in fibroblasts by S. suis, we isolated primary porcine bronchial fibroblasts and infected them with S. suis S10 using two different multiplicities of infection. Stimulation with recombinant IL1β was used as positive control. As shown in Supplementary Figure 1, we could not detect COX-2 induction by S. suis in isolated fibroblasts infected in vitro, while stimulation with IL1β resulted in a robust induction of COX-2 expression.
These results suggest that after infection of PCLS with S. suis, COX-2 is most likely primarily produced in fibroblasts in the bronchiolar area.
COX-2 is induced by two prevalent S. suis serotypes in porcine PCLS
To analyse whether COX-2 induction is specific for the serotype 2 strain S10, we next infected PCLS with the serotype 9 strain S. suis S8067 and compared COX-2 induction with that of S. suis S10. As shown in Figure 5A, Western blot analysis of infected PCLS after 24 h demonstrated a strong COX-2 induction in tissue infected with S8067 at a similar level as induced by S10, while no COX-2 induction was detectable in uninfected tissue. Densitometric analysis revealed a significant induction after infection with both strains when compared to control tissue, but no significant difference between the two strains (5B).
In line with increased COX-2 protein expression in PCLS infected with both strains, we also detected a significantly, 13.5-fold increased PGE2 level in tissue infected with S10 (Figure 5C). In tissue infected with S8076 we detected a 5.5-fold increased PGE2 level which is lower compared to infection with S10 but significantly increased compared to unstimulated PCLS (Figure 5C).
Immunohistochemical analysis of COX-2 induction in PCLS infected for 24 h revealed a similar localisation primarily in the bronchiolar region for both strains. Virtually no COX-2 induction was detectable in uninfected tissue (Figure 5D).
These results demonstrate that induction of COX-2 and PGE2 production in the PCLS model is not specific for S. suis S10, even though the level of produced PGE2 seems to vary between the two tested strains.
S. suis induced expression of COX-2 in porcine lung tissue is modulated by SLY
Finally, we analysed the role of the pore-forming toxin SLY in the induction of COX-2 as a role for pore-forming toxins in this process has been demonstrated for S. pyogenes (28).
For this, PCLS were infected for 24 h with S. suis S10, its isogenic suilysin deletion mutant S10Δsly or left uninfected. COX-2 induction was analysed by Western blotting of whole tissue lysates (WTL). As shown in Figure 6A, infection with the wild-type strain S10 induced COX-2 expression as demonstrated before. In contrast, tissue infected with S10Δsly showed a reduced COX-2 protein level compared to tissue infected with the wild-type strain (Figure 6A, WTL). Densitometric analysis revealed a significant induction after infection with the S10 wildtype strain when compared to control tissue. Although we also observed a significant induction in case of S10Δsly when compared to control tissue, there was significant difference in COX-2 induction between wildtype and mutant by densitometry (Figure 6B). Furthermore, we proved production of SLY by the wild-type strain S10 and absence of SLY production by S10Δsly by Western blotting of tissue culture supernatants (Figure 6A, SN). Reduced induction of COX-2 by S10Δsly was restored by infection with a complemented suilysin mutant strain (Supplementary Figure 2).
In accordance with reduced COX-2 protein expression, we observed a significantly reduced level of PGE2 in S10Δsly infected PCLS compared to tissue infected with the wild-type strain S10 (Figure 6C).
Furthermore, immunohistochemical analysis of COX-2 induction in PCLS revealed a reduced number of COX-2 positive cells with a strongly reduced COX-2 signal in the tissue infected with S10Δsly (Figure 6D).
Finally, we tested whether suilysin alone is sufficient to induce COX-2 expression by stimulation of PCLS with increasing amounts of recombinant suilysin (rSLY) for 24 h and sub-sequent analysis of COX-2 induction by Western blotting. As shown in Figure 7A, stimulation with rSLY resulted in a dose-dependent increase of COX-2 expression. Densitometric analysis revealed a significant COX-2 induction in tissues stimulated with 1000 ng/ml rSLY (Figure 7B). Taken together, these data indicate that the pore forming toxin of S. suis plays an important role in induction of COX-2 expression and PGE2 production in PCLS.
Discussion
COX-2 generates metabolites that are important regulators of inflammation (9). Studies using different streptococcal pathogens (14, 15) indicated a prominent immunomodulatory role of COX-2 in streptococcal infections of murine and human skin as well as human lung tissue. Since virtually no study has systematically analysed the biology of COX-2 in the porcine lung following S. suis infection, we used an ex vivo model of porcine precision-cut lung slices infected with S. suis to explore COX-2 induction and PGE2 synthesis.
PCLS represent a model system with the typical lung architecture containing all relevant cell types maintained in their differentiation state and preserving important functions like ciliary activity of the bronchiolar epithelial cells (22). This model also includes resident immune cells like dendritic cells and alveolar macrophages (29). Therefore, this model is suitable to investigate the inflammatory response of the resident cells induced by interactions of the bacteria within the bronchial and alveolar compartment. However, not all aspects of immunity like recruitment of immune cells and resolution of the inflammatory response can be studied because the tissue is disconnected from the blood stream. Nevertheless, we observed a reproducible induction of COX-2 expression and production of PGE2 after infection with S. suis in this model that is comparable to results obtained with S. pneumoniae in a human lung ex vivo infection model (15) and might contribute to chemo- and cytokine regulation in the lung (9). Interestingly and in contrast to the human lung ex vivo infection model, we observed an increase in COX-2 protein in the presence of the COX-2 inhibitor NS-389. This inhibitor mitigates the COX-2-mediated production of prostaglandins but does not inhibit the induction of COX-2. In one study using mouse lung fibroblast, PGE2 was shown to regulate COX-2 expression in a positive feedback loop (30), whereas other studies demonstrated a repressive effect of PGE2 in different cell/tissue systems (31, 32). The increase of COX-2 at the protein level in the presence of the inhibitor which almost completely reduces production of PGE2 at the used concentration in our model, also suggests a negative feedback loop.
We detected a strong COX-2 expression in the proximity of the bronchioles between the ciliated epithelial cells and the adjacent alveolar tissue. Morphology, location as well as the strong vimentin signal suggest that these cells are subepithelial bronchial fibroblasts. However, in future studies, staining with other fibroblast markers is required to further proof that these cells are indeed fibroblasts. We tested an antibody that is specific for human fibroblasts (TE-7 antibody) (33), but did not observe a specific staining in porcine lung tissue and isolated primary porcine fibroblasts, suggesting that the epitope recognised by the antibody is not present in porcine fibroblasts (data not shown). Lung fibroblasts play a key role in maintaining normal lung homeostasis and act as immune sentinels responding to inhaled toxic substances and cytokines like IL-1β (34). Furthermore, a recent study demonstrated that fibroblast activity integrates innate immune signals to regulate the adaptive immune environment of the lung after infection with influenza A virus (35). This study showed, that in virus-infected mouse lungs three different classes of fibroblasts can be distinguished: resting, ECM-synthesizing and inflammatory fibroblasts. Although COX-2 expression in the different classes of fibroblasts was not analysed in this study, it is tempting to speculate that the presence of functionally distinct fibroblasts may be the reason why we detect COX-2 expression only in a subset of the vimentin-positive cells. However, to proof that these fibroblast subgroups are also present in our model system and that COX-2 induction correlates with these subgroups, single cell transcriptomic analysis needs to be performed in future studies.
Induction of COX-2 in fibroblasts is in contrast to studies on COX-2 induction in lungs of pigs infected with M. hyopneu-moniae where induction was predominantly found in ciliated epithelial cells (17). This might be explained by the direct interaction of M. hyopneumoniae with the ciliated bronchial cells and a lack of cytolytic toxins that primarily results in the activation of signalling pathways, subsequently leading to COX-2 induction in these cells (36). Using a human lung ex vivo infection model, Szymanski et al. demonstrated that S. pneumoniae induces upregulation of COX-2 mainly in alveolar type II cells, but also in alveolar macrophages and endothelial cells (15). We also detected COX-2-positive cells in the alveolar compartment, but the observed level of the COX-2 signal, as well as the number of positive cells, was much lower compared to the bronchiolar region. The reason for this difference could be the lack of bronchial structures in this human lung model system leading to an induction of COX-2 primarily in the alveolar tissue (15).
At the protein level, both strains induced strong expression of COX-2 while the PGE2 levels were lower in case of infection with the serotype 9 strain 8067. The final step of PGE2 generation initiated by COX-2 depends on the membrane-bound enzyme PGE2 synthase (mPGES) which can be induced by pro-inflammatory factors (37). Although COX-2 and mPGES are thought to be functionally linked, the kinetics of COX-2 and mPGES induction are different in various cell types, suggesting different regulatory mechanisms controlling the expression of both enzymes (38–40). While COX-2 expression can be directly induced by poreforming toxins via, e.g. calcium signalling (28), induction of mPGES might be delayed due to lower induction of pro-inflammatory mediators required for its upregulation in case of infection with the serotype 9 strain 8067 and, therefore, leading to lower PGE2 levels. Interestingly, a recent study showed lower levels of pro-inflammatory cytokines in dendritic cells infected in vitro with a serotype 9 strain compared to infection with a serotype 2 strain (41). However, due to the fact, that only two different strains were tested in the present study, more strains need to be analysed in follow-up studies to definitely determine whether there are strain-specific differences in COX-2 induction or PGE2 production.
COX-2 induction has been demonstrated for several different bacterial toxins, e.g. LPS (42), C. difficile toxin A (43) as well as the S. pyogenes cytolysins SLS and SLO (28). SLY also belongs to the family of pore-forming toxins and exerts cytotoxic effects on various cell types such as epithelial cells, endothelial cells, phagocytes (18, 44, 45), but also on more complex tissue models like air-liquid interface cultures and PCLS (20, 22). In contrast to S. pyogenes expressing SLS and SLO, infection with a SLY-expressing S. suis strain does not induce COX-2 expression in isolated primary bronchial fibroblasts. However, in the study by Blaschke et al. macrophages were used that, as professional phagocytic cells, might have the capacity to directly upregulate COX-2 after infection. Interestingly, we observed COX-2 expression in isolated fibroblasts stimulated with recombinant IL-1β. S. suis has been shown to induce IL-1β in a SLY-dependent manner (46). Therefore, it is tempting to speculate, that COX-2 induction is facilitated indirectly in our model via inflammatory mediators like IL-1β and/or other cytokines produced by epithelial cells or resident immune cells in response to S. suis infection. Nevertheless, in this study, we provide evidence that SLY is involved in the induction of COX-2 and the synthesis of PGE2 in porcine lung tissue infected with S. suis, thus extending the list of functional activities of this toxin. In the future, the regulatory mechanisms underlying the induction of COX-2 by S. suis should be further investigated.
Conclusion
In summary, this study demonstrated that S. suis induces COX-2 expression and PGE2 production in porcine PCLS. COX-2 induction is most likely primarily induced in fibroblasts located in the bronchiolar region. Furthermore, COX-2 is induced by two different S. suis strains representing prevalent serotypes and the cytolysin SLY is a critical factor involved in the induction of COX-2 and the synthesis of PGE2 in the porcine PCLS model. Further studies are needed to verify the obtained results in animal models and to analyse the role of COX-2 and PGE2 in the inflammatory response in the porcine lung during infection with S. suis.
FUNDING
This project has received funding to P.V.-W. from the European Union’s Horizon 2020 research and innovation program under grant agreement no. 727966 and from the Deutsche Forschungsgemeinschaft, Bonn, Germany (Va 239/7-2). In part R2N Project funded by the Federal State of Lower Saxony, Germany (W.B.).
AUTHOR CONTRIBUTIONS
Conceptualization, A.N. and P.V.-W.; investigation, M.D., J.S., Y.B.W., D.V. and A.N.; formal analysis, M.D., J.S. and A.N.; resources, W.B.; writing—original draft preparation, M.D. and A.N.; writing—review and editing, all authors; funding acquisition, W.B. and P.V.-W. All authors have read and agreed to the published version of the manuscript.
COMPETING FINANCIAL INTERESTS
The authors declare no conflict of interest.
ACKNOWLEDGEMENTS
We thank Hilde E. Smith (Wageningen Bioveterinary Research, Lelystad, The Netherlands) for providing S. suis strains 10 and 8067 as well as Nina Janze for excellent technical assistance. Part of this work was contributed by M.D. in partial fulfilment of the requirements for a Ph.D. degree from the University of Veterinary Medicine Hannover.
Footnotes
Material and methods, results and discussion sections revised based on reviewer comments; new supplemental files added; author affilations updated; grammatical and spelling errors corrected.