15-Hydroxyprostaglandin Dehydrogenase Generation of Electrophilic Lipid Signaling Mediators from Hydroxy Ω-3 Fatty Acids*

Background: 15-Hydroxyprostaglandin dehydrogenase (15PGDH) catalyzes the oxidation of hydroxylated polyunsaturated fatty acids to α,β-unsaturated carbonyl-containing electrophiles. Results: Hydroxylated docosahexaenoic acid (DHA) metabolites are substrates for 15PGDH, yielding electrophilic oxoDHA products that are anti-inflammatory. Conclusion: Hydroxylated Ω-3 fatty acid species are conferred with cell signaling capabilities after oxidation by 15PGDH. Significance: Formation of biologically active metabolites by 15PGDH contributes to the salutary signaling actions of Ω-3 fatty acids. 15-Hydroxyprostaglandin dehydrogenase (15PGDH) is the primary enzyme catalyzing the conversion of hydroxylated arachidonic acid species to their corresponding oxidized metabolites. The oxidation of hydroxylated fatty acids, such as the conversion of prostaglandin (PG) E2 to 15-ketoPGE2, by 15PGDH is viewed to inactivate signaling responses. In contrast, the typically electrophilic products can also induce anti-inflammatory and anti-proliferative responses. This study determined that hydroxylated docosahexaenoic acid metabolites (HDoHEs) are substrates for 15PGDH. Examination of 15PGDH substrate specificity was conducted in cell culture (A549 and primary human airway epithelia and alveolar macrophages) using chemical inhibition and shRNA knockdown of 15PGDH. Substrate specificity is broad and relies on the carbon position of the acyl chain hydroxyl group. 14-HDoHE was determined to be the optimal DHA substrate for 15PGDH, resulting in the formation of its electrophilic metabolite, 14-oxoDHA. Consistent with this, 14-HDoHE was detected in bronchoalveolar lavage cells of mild to moderate asthmatics, and the exogenous addition of 14-oxoDHA to primary alveolar macrophages inhibited LPS-induced proinflammatory cytokine mRNA expression. These data reveal that 15PGDH-derived DHA metabolites are biologically active and can contribute to the salutary signaling actions of Ω-3 fatty acids.

From a different perspective, oxo metabolites of hydroxyfatty acids are ␣,␤-unsaturated ketones that can mediate significant cell signaling and functional responses. For example, 15-ketoPGE 2 formation not only decreases the levels of the proproliferative PGE 2 but also inhibits growth of hepatocellular carcinoma and cholangiocarcinoma by peroxisome proliferator activator receptor ␥ (PPAR␥) activation (12,13). Studies in human umbilical vein endothelial cells affirm that 11-oxoETE and 15-oxoETE mediate anti-proliferative properties (5,6).
Electrophilic lipids such as fatty acid nitroalkene derivatives and ⍀-6 and ⍀-3-derived ␣,␤-unsaturated ketones are products of metabolic and oxidative inflammatory reactions that also act as signaling mediators. Mechanisms of action include induction of the expression of anti-inflammatory genes regulated by the transcription factor nuclear factor-erythroid 2-related factor 2 (Nrf2). Electrophilic fatty acids form Michael adducts with cysteines, for example primarily the Cys 273 and Cys 288 in KEAP1 (Kelch-like ECH-associated protein 1), which is responsible for sequestering Nrf2 in the cytosol and regulating its proteasomal degradation (14). This adduction promotes the release of Nrf2 and its translocation to the nucleus, where it promotes antioxidant response element gene expression (14,15). Electrophilic fatty acids also induce heat shock factor expression and suppress proinflammatory gene expression through Cys 38 alkylation and inhibition of DNA binding by the p65 subunit of NF-B (14, 16 -18). By these mechanisms, electrophilic fatty acids can act as pleiotropic signaling molecules that form reversible Michael addition adducts with nucleophilic species, including low molecular weight thiols and cysteine residues of proteins (16). In this context, 17-oxoDHA and 7Z,10Z,13Z,15E,19Z-17-keto-docosapentaenoic acid (17-ox-oDPA) and 15-oxoETE can induce Nrf2 expression, activate Nrf2-dependent gene expression (heme oxygenase-1 (HO-1), glutamate cysteine ligase modifier (GCLM), NAPDH oxidoreductase 1 (NQO1)), decrease the protein expression of inducible nitric-oxide synthase and COX-2 in Raw264.7 cells, and suppress NF-B-mediated mRNA cytokine expression in THP-1 cells (19,20).
This study evaluated the substrate specificity of 15PGDH for hydroxylated DHA (HDoHE) species and revealed the signaling actions of 15PGDH-derived electrophilic products in human primary alveolar macrophages. These results support two key precepts. First, a broad array of hydroxy-polyunsaturated fatty acids are substrates for 15PGDH. Second, the products of hydroxy-fatty acid dehydrogenation are electrophilic and can thus be conferred with pleiotropic anti-inflammatory signaling activities.
Bronchoscopy and Primary Cell Culture-Bronchoscopy of mild to moderate asthmatics with endobronchial epithelial brushing and primary airway epithelial cell (AEC) culture was performed as described previously and with University of Pittsburgh IRB approval (PRO11010186) (21,22). Briefly, a total of six brushings were obtained, and cells were placed into 10 ml of phosphate-buffered saline, centrifuged, and resuspended in 1 ml of serum-free hormonally supplemented bronchial epithelial growth medium (Clonetics, San Diego, CA) containing 50 g/ml gentamicin and 50 g/ml amphotericin. The cells were plated at ϳ3 ϫ 10 5 /plate in bronchial epithelial growth medium in 60-mm tissue culture dishes coated with rat tail type I collagen (BD Discovery Labware, Bedford, MA). Cells were cultured at 37°C in a 5% CO 2 environment. When cells were almost 100% confluent they were either plated at the air-liquid interface in 12-well transwell plates as described previously (21) or frozen for future use. When needed, frozen primary AECs were thawed, recounted, and plated at ϳ5 ϫ 10 5 cells per 60-mm collagen-coated dish and grown to confluency in Lifeline (Lifeline Cell Technology, Frederick, MD) serum-free media containing bronchial life factors. Upon 80% confluency, cells were trypsinized (0.25%) and plated on collagen-coated 6-well plates (Corning, Corning, NY) in serum-free Lifeline Bronchial Life Media with growth factors and 1% penicillin/streptomycin for metabolism studies (Lifeline Cell Technology, Frederick, MD). Primary alveolar macrophages were separated from bronchoalveolar lavage (BAL) fluid at the time of bronchoscopy, counted, and plated at 5 ϫ 10 5 cells/well in a 24-well plate in RPMI 1640 supplemented with 10% FBS and penicillin/streptomycin. After 90 min, media were changed to remove non-adherent cells (23)(24)(25).
Cell Treatment-Primary AECs were treated with 10 M DHA for 2 h or with 2 M HDoHEs, 2 M 5-HETE, or 2 M PGE 2 for 4 h in cell growth media. After determining optimal inhibitor concentrations, treatments were conducted with and without 50 M CAY10397. Media was extracted for LC-MS analysis as described below. A549 and A549 shRNA cell growth media were replaced with serum-free Hanks' balanced salt solution for cell treatments. Cells were treated for 4 h with either 10 M AA, 10 M DHA or 2 M PGE 2 , 5-HETE, or HDoHEs for 4 h with or without 50 M CAY10397 inhibitor. Primary alveolar macrophages were treated in RPMI with 1% FBS for 4 h and with 2 M 14-HDoHE with and without 50 M CAY10397 inhibitor. Media were collected for LC-MS analysis as described below. Results are an average of Ն3 individual treatments, and statistical significance was determined by either t test or one-way analysis of variance as appropriate.
BAL Cell Pellets-BAL obtained from bronchoscopies of 6 mild to moderate asthmatics was centrifuged to separate fluid from the cellular content. BAL cell pellets (1.5 ϫ 10 6 cells/sample) were lysed briefly in liquid nitrogen, and 10 ng of 5-oxo-ETE-d 7 was added as an internal standard. The cell pellet was incubated with 500 mM ␤-mercaptoethanol (BME) in 20 l of 50 mM phosphate buffer, pH 7.4, for 1 h at 37°C. The reaction was stopped with 80 l of cold acetonitrile with 1% formic acid. The samples were centrifuged at 10,000 ϫ g for 5 min, and the supernatant was used for LC-MS analysis of HDoHEs and electrophilic BME adducts (27).
RT-PCR-Primary alveolar macrophage media was replaced with 1% FBS in RPMI and treated for 6 h with vehicle, 100 ng/ml LPS, 10 M 14-oxoDHA, or the combination of LPS and 14-oxo-DHA. Results are representative of three individual treatments, and statistical significance was determined by one-way analysis of variance.
LC-Single Reaction Monitoring/MS-Free fatty acid metabolites in the media were extracted using diethyl ether. Briefly, media were collected, and 20 ng of 5-oxoETE-d 7 and 10 ng of PGE 2 -d 9 internal standards were added to each sample. The samples were allowed to equilibrate for 5 min before shaking for 10 min. Next, samples were centrifuged at 2800 ϫ g for 10 min. The top layer (organic) was transferred to a clean vial and dried under a stream of nitrogen. Samples were reconstituted in 100 l methanol before analysis. A Shimadzu HPLC (Columbia, MD) coupled to an AB Sciex (Framingham, MA) 5000 triple quadrupole mass spectrometer was used for the quantification of fatty acids. Sample (10 l) was separated on a Phenomenex (Torrence, CA) C18(2) ODS column, 2.1 ϫ 150 mm, 5-m bead size, 100 Å pore size. The solvent system employed aqueous 0.1% acetic acid (A) and 0.1% acetic acid in acetonitrile (B). The 60-min gradient with a flow rate of 0.25 ml/min started at 35% B and ramped to 90% B over 46 min. This was followed by a wash using 100% B for 6 min. The gradient then returned to starting conditions at 35% B for 8 min. MS analyses by electrospray ionization were run in negative mode with the collision gas set at 4 units, curtain gas at 40 units, ion source gas 1 and 2 at 40 units, ion spray voltage Ϫ4500 V, and temperature at 550°C. The declustering potential was set to Ϫ50, entrance potential Ϫ5, collision energy Ϫ17, and the collision exit potential Ϫ18.4. Single reaction monitoring was used for sample analysis and quantification. The following transitions were used: HDoHE and oxoDPA 343. 2  Structural characterization and retention time confirmation of 14-oxoDHA and 14-oxoDPA were confirmed using an Orbitrap Velos accurate mass, high resolution mass spectrometer (Thermo Scientific, Waltham, MA). The LC conditions were the same as described above for the quantification on the triple quadrupole mass spectrometer except the injection volume was 20 l. Both scans were performed in Fourier transform mass spectrometry negative ion mode at 30,000 resolution with an acquisition time of 30 ms, an ActQ of 0.25, and collision energy of 35. The ion spray voltage was maintained at 4 kV, and the heater and capillary temperatures were set to 300°C and 270°C, respectively. The sheath, auxiliary, and sweep gases were adjusted to 20, 18, and 12 arbitrary units. Mass accuracy was Ͻ5 ppm for all confirmed structures.
Identification of Lipid Electrophiles-Confirmation of electrophilicity was determined using the nucleophile BME (27). Media were incubated with 50 mM BME for 1 h at 37°C and then extracted with diethyl ether and dried under nitrogen before LC-MS analysis. Fatty acid BME adducts were analyzed on the AB Sciex 5000 triple quadrupole mass spectrometer described above. The oxoDPA species was monitored at 421.2 3 343.2 for the loss of 78 atomic mass units (BME), and the electrophilic 5-oxoETE-d 7 was used as a positive control for BME adduct formation (402.2 3 324.2).

Formation of Electrophilic Species from DHA-Primary
AECs were treated with 10 M DHA for 2 h and the formation of HDoHEs and the corresponding electrophilic oxoDHA species was determined. Analysis of control cell lysate and media did ⍀-3-Derived 15PGDH Products Are Bioactive not result in detectable levels of endogenous DHA-derived HDoHE metabolites monitored by the nonspecific transition (loss of CO 2 ) 343.2 3 299.2 (Fig. 1A). Additionally, the incubation of cell-free Hanks' balanced salt solution or media with DHA resulted in minimal generation of HDoHEs from DHA autoxidation (data not shown), whereas the addition of exogenous DHA to primary AEC resulted in the generation of HDo-HEs (Fig. 1B) via enzymatic and non-enzymatic reactions that could be quantitated in the media using 5-oxoETE-d 7 as the internal standard (Fig. 1C) (28 -33).
Regardless of the route of HDoHE formation, these DHAderived species are potential substrates of 15-PGDH. Simultaneous treatment of primary AEC with DHA and the 15PGDH inhibitor CAY10397 (50 M) resulted in a significant decrease in what was suspected to be 14-oxoDHA, the product of 15PGDH oxidation of 14-HDoHE ( Fig. 2A). The identity of 14-oxoDHA was confirmed using the 14-HDoHE standard that was oxidized to its corresponding electrophile using the Dess Martin periodinane reaction as no commercial standard was available. Characterization of the oxidized product confirmed the identity of the 14-oxoDHA species using retention time and MS 2 spectra from high resolution accurate mass LC-MS/MS (Fig. 2, B and C).
15PGDH Substrate Specificity-Metabolism was further investigated in primary AECs using HDoHE species (2 M) having the hydroxyl group at C4, C7, C8, C10, C11, C13, C14, C16, C17, and C20. HDoHEs were added to cells cultured in Hanks' balanced salt solution (HBSS) with and without 50 M CAY10397 for 4 h. Both HBSS and cell lysates were extracted; however, HDoHEs and downstream metabolites were predominantly detected in the media. The corresponding oxoDHA species could be detected for all HDoHE substrates except for 8-HDoHE (Fig. 3, A-I). HDoHE metabolism to their corresponding oxoDHA metabolite was only significantly inhibited by CAY10397 for the oxidation of 14-HDoHE to 14-oxoDHA, consistent with the inhibition of 15PGDH after exogenous DHA addition (Fig. 3F). PGE 2 and 5-HETE were used as positive and negative controls, respectively. CAY10397 significantly inhibited the formation of 15-ketoPGE 2 and its non-electro-philic metabolite 13,14-dihydro-15-ketoPGE 2 , whereas 5-oxo-ETE formation did not change as 5-HETE is a substrate for 5-hydroxyeicosanoid dehydrogenase, not 15PGDH (Fig. 3, J-L). The same analyses were repeated in A549 cells in which results varied significantly from the primary AEC (Fig. 4, A-L). 14-oxoDHA was abundantly formed in A549 cells, and its formation was significantly inhibited with CAY10397. However, CAY10397 also significantly inhibited oxoDHA formation for substrates with the hydroxyl group position ranging from 11-HDoHE to 20-HDoHE (Fig. 4, D-I). These data provide a clear indication that (a) dehydrogenase expression is cell linespecific, (b) CAY10397 is not specific for 15PGDH, and (c) transformed cell lines do not recapitulate what is observed in primary cells. To further confirm that 14-oxoDHA is a product of 15PGDH in a more specific manner, A549 cells were transduced with lentiviruses expressing either a scrambled or 15PGDH-specific shRNA. Loss of expression was validated by immunoblot (data not shown). Scrambled (Scr) control and 15PGDH knockdown (KD) cells were treated with 10 M DHA ⍀-3-Derived 15PGDH Products Are Bioactive for 4 h, and AA-derived 5-HETE was used as a control. The formation of 14-oxoDHA was significantly decreased in the 15PGDH KD cells compared with the Scr control, whereas there was no decrease in 5-oxoETE formation (Fig. 5). Scr A549 cells were treated with 2 M 14-HDoHE with and without 50 M CAY10397 and 15PGDH KD cells were treated with 2 M 14-HDoHE for 4 h (Fig. 6A). The PGE 2 metabolite 15-ketoPGE 2 was used as the positive control. 15-ketoPGE 2 was significantly decreased to the same extent in Scr A549 cells treated with 15PGDH inhibitor and 15PGDH KD cells (Fig. 6B). 14-oxo-DHA formation was also significantly decreased with inhibitor in Scr A549 cells and in 15PGDH KD cells (Fig. 6A). In both 15PGDH KD treatments 14-oxoDHA formation was not completely inhibited (Figs. 5A and 6A). In fact, Scr A549 cells treated with CAY10397 resulted in lower levels of 14-oxoDHA compared with the 15PGDH KD cells (Fig. 6A). These differences underscore the lower specificity of the CAY10397 inhibitor and highlight that other dehydrogenases may also contribute to 14-oxoDHA formation.
Electrophilic Metabolites-The formation of oxoDHA metabolites is also affected by 15PGDH. LC-MS analysis revealed a key metabolite of 14-oxoDHA is its reduced metabolite, 14-oxo- DPA. This product was detected in the transition 343.2 3 299.2, which is used to monitor the loss of CO 2 from any HDoHE species; however, reduced keto species can also be detected in this transition. The retention time of 14-oxoDPA is increased compared with 14-HDoHE due to the increase in hydrophobicity. The formation of 14-oxoDPA significantly decreased with either CAY10397 inhibition or 15PGDH KD (Fig. 7A).
Prostaglandin reductase (PTGR1) is the enzyme responsible for the conversion of the 15-ketoPGE 2 to its reduced metabolite 13,14-dihydro-15ketoPGE 2 (34). This reduction occurs at the double bond adjacent to the carbonyl group rendering 13,14-dihydro-15-ketoPGE 2 non-electrophilic. To test the electrophilicity of 14-oxoDPA, media were incubated with the nucleophile BME yielding a Michael adduct with the electrophilic ␣, ␤-unsaturated carbon (27). The top panel of Fig. 7B shows a transition for 421.2 3 343.2 that represents the loss of BME from an electrophilic metabolite with a parent mass of 343.2. In A549 cell-derived media without BME, there is no peak in the 421.  ⍀-3-Derived 15PGDH Products Are Bioactive min (Fig. 7B). However, upon incubation with BME (Fig. 7C), the peak at 32.1 min disappears concomitantly with the appearance of a more hydrophilic peak in the 421.2 3 343.2 transition for the 14-oxoDPA-BME Michael adduct, monitoring for a loss of BME (m/z 78). It is proposed that prostaglandin reductase is not the main reductase responsible for double-bond saturation because 14-oxoDPA maintains electrophilic characteristics. Characterization of the 14-oxoDPA species using high accuracy MS/MS resulted in similar fragment ions as seen for 14-oxo-DHA (Fig. 7, D and F), except that they were 2 mass units higher and the parent mass was 343.2279 (Ͻ0.5 ppm). The 14-oxo-DHA fragment ion with m/z 205.1235 (M-H ϩ -C 9 H 14 O, Ͻ1 ppm), representing cleavage between the carbonyl and ␣,␤-unsaturated carbon, was not a major fragment in the 14-oxoDPA MS 2 ; rather, m/z 207.1389 (M-H ϩ -C 9 H 12 O, Ͻ1ppm) was detected. This is indicative of saturation on the ⍀ side of the carbonyl (Fig. 7, F and G). The fragment with m/z 205.1597 (M-H ϩ -C 8 H 10 O 2 ) coming from the MS 2 of 14-oxoDPA provides evidence that the two saturated double bonds closest to the ⍀ end are present. Additionally, 14-oxoDHA has a characteristic fragmentation of 243.1751 (M-H ϩ -C 5 H 6 O 2 ), whereas the MS 2 of 14-oxoDPA contains a fragment ion with m/z 245.1911 (M-H ϩ -C 5 H 6 O 2 ) representing the same loss, indicating that the double bond closest to the carbonyl is not reduced. Therefore, it can be deduced from the MS 2 comparisons that the saturation occurs at the ␥,⌬-unsaturated double bond (Fig.  7, F and G).

Detection of HDoHEs and oxoDHA Metabolites in Bronchoalveolar Lavage Cells-
The clinical generation of electrophilic oxoDHA metabolites and HDoHE precursors occurred in cells from the BAL of six mild to moderate asthmatics. Electrophilic species were captured via reaction with added BME and then analyzed by LC-MS, where electrophilic species were monitored by the loss of BME. The chromatogram of a BAL cell pellet extracted after BME incubation reveals electrophilic species when monitored at 419.2 3 341.2 (Fig. 8A), with the 5-oxo-ETE-d 7 internal standard serving as the BME control monitored at 402.2 3 324.2 (not shown). Electrophilic BME adducts are more hydrophilic, and their retention shifts to the left by ϳ5.5 min. The non-electrophilic HDoHEs do not adduct to BME and could be detected at their specific single reaction monitoring transitions without a shift in retention time. 14-HDoHE was detected in the clinical samples using the transition 343.2 3 205.2 at 27.4 min (Fig. 8B). The levels of 14-HDoHE detected in BAL cell pellets ranged from not detectable to 0.95 ng/1.5 ϫ 10 6 cells (Fig. 8C). Primary alveolar macrophages were also separated from BAL fluid at the time of bronchoscopy from mild to moderate asthmatics and plated. Macrophages were treated with 2 M 14-HDoHE with and without CAY10397, and metabolites were monitored after 4 h. 14-oxoDHA and 14-oxoDPA were both detected, and their formation was significantly inhibited with the CAY10397 (Fig. 8, D  and E).  15PGDH Regulation of Inflammatory Signaling-Electrophilic lipids mediate a broad array of cell signaling responses (16). Primary alveolar macrophages were treated for 6 h with vehicle control, 10 M 14-oxoDHA, 100 ng/ml LPS, or concurrent treatment of 100 ng/ml LPS and 10 M 14-HDoHE or 100 ng/ml LPS and 10 M 14-oxoDHA (Fig. 9). LPS treatment significantly increased the mRNA expression of NF-B-driven cytokines, TNF␣, IL-6, and IL-1␤. Concurrent LPS treatment with 14-oxoDHA resulted in significant abrogation of cytokine mRNA expression. Interestingly, IL-6 mRNA expression was also significantly blunted by 14-HDoHE (Fig. 9).

DISCUSSION
15PGDH is noted for inactivating the pro-proliferative PGE 2 and the polyhydroxylated fatty acid derivatives termed lipoxin A 4 and resolvin E1. These oxidations catalyzed by 15PGDH are deemed inactivation reactions because of putative attenuation of G protein-coupled receptor ligand activity and downstream signaling responses. Notably, the oxidized products of 15PGDH become electrophilic species that can also mediate anti-inflammatory and anti-proliferative actions via pleiotropic G protein-coupled receptor-independent signaling mechanisms.
The inverse relationship between COX-2 and 15PGDH that leads to an excess of pro-proliferative signaling in many cancers highlights the importance of 15PGDH in the regulation of fatty acid metabolism and signaling (3,4,35). However, these studies only demonstrated that 15PGDH metabolites were products of the metabolism of pro-proliferative signaling molecules and not potentially conferred with alternative signaling potential. More recent studies of hepatocellular carcinoma and cholangiocarcinoma show that 15-ketoPGE 2 formation not only decreases the levels of the pro-proliferative PGE 2 but also inhibits cell growth via activation of PPAR␥ (12,13). The hepatocellular carcinoma model determined that cell proliferation was inhibited by an increase in p21 WAF1/Cip1 (cyclin-dependent kinase inhibitor 1) expression, leading to downstream association with cyclin-dependent kinase (CDK2), CDK4, and proliferating cell nuclear antigen (12). In the cholangiocarcinoma model, inhibition of proliferation is acquired through PPAR␥-, (SMAD2/3)-, and Tap63 (tumor protein)-mediated signaling actions (13). This study also linked 15-ketoPGE 2 generation with the induction of SMAD 2/3 dissociation from PPAR␥, thus promoting SMAD 2/3 complex formation with transforming growth factor B receptor 1 and SMAD anchor receptor for acti- ⍀-3-Derived 15PGDH Products Are Bioactive vation. In a related context, 15-oxoETE significantly up-regulated Nrf2-activated heme oxygenase-1 and NAPDH oxidoreductase 1 (NQO1) protein expression and inhibited TNF␣, IL-6, and IL-1␤ mRNA expression in THP-1 cells (20). Moreover, 11-oxoETE and 15-oxoETE demonstrated anti-proliferative properties in human umbilical vein endothelial cells using a bromodeoxyuridine-based cell proliferation assay. The IC 50 of 11-oxoETE for the inhibition of human umbilical vein endothelial cell proliferation was 2.1 M, similar to that of the electrophilic prostaglandin 15-deoxy prostaglandin J 2 (6). In aggregate, these observations indicate that 15PGDH and the oxo-fatty acid products it generates can profoundly influence cell function.
The present study reveals that hydroxylated ⍀-3 fatty acids are substrates for 15PGDH and potentially other dehydrogenases. These species, like 15-ketoPGE 2 and AA-derived oxoETEs, are electrophilic and possess anti-inflammatory signaling properties. Primary human AEC and A549 cell-based studies indicated that the most abundant 15-PGDH-derived oxoDHA metabolite is 14-oxoDHA, which was characterized by high resolution accurate mass LC-MS/MS (Fig. 2). When individual HDoHE metabolites were added to cell culture, the position of the hydroxyl group on the acyl chain dictated substrate specificity for 15PGDH in primary AEC (Fig. 3). Consistent with this, 15PGDH inhibition led to the most extensive decrease in 14-oxoDHA formation by A549 and primary AEC (Figs. 3D and 4D). 11,13,16,17, and 20-oxoDHA formation was also significantly inhibited in A549 cells, but not in primary AEC. This could be a result of differences in the expression of cell-specific dehydrogenase activities or the specificity of the CAY inhibitor for 15PGDH. Additionally, A549 cells are metabolically more active and in a more oxidative state, which may FIGURE 8. Detection of oxoDHA-BME adducts and 14-HDoHE in BAL cells. Bronchoalveolar lavage cell pellets were incubated with 500 mM BME and extracted for LC-MS analysis. The loss of BME (78 atomic mass units) was monitored for oxoDHA-BME adducts (419.2 3 341.2) (A). Endogenous levels of 14-HDoHE (343.3 3 205.2) were detected in BAL cell pellets (B). Endogenous 14-HDoHE levels ranged from not detectable to 0.95 ng/10 6 cells in the clinical samples (C). Primary alveolar macrophages taken from bronchoscopies were plated at a confluency of 5 ϫ 10 5 cells/well in a 24 well plate. Alveolar macrophages were incubated for 4 h with 2 M 14-HDoHE Ϯ 50 M CAY10397, and 14-oxoDHA (D) and 14-oxoDPA (E) metabolites were quantified. **, p Յ 0.01; ***, p Յ 0.001. ⍀-3-Derived 15PGDH Products Are Bioactive FEBRUARY 27, 2015 • VOLUME 290 • NUMBER 9 influence the extent of formation of various electrophilic oxoDHA species. This also highlights the concern of using transformed carcinogenic cell lines for metabolism studies as the results do not always correlate with primary cell lines.
The specificity of CAY10397 for 15PGDH inhibition of 14-oxoDHA formation was confirmed in A549 cells transduced with lentiviruses expressing either 15PGDH-specific shRNA or a scrambled shRNA control. 14-OxoDHA generation was significantly decreased in 15PGDH KD cells supplemented with either DHA or 14-HDoHE (Figs. 5 and 6). Interestingly, CAY10397 treatment of Scr A549 cells resulted in a greater inhibition of 14-oxoDHA formation compared with 15PGDH KD cells. This reiterates that CAY10397 is not specific for 15PGDH and that other cellular dehydrogenases are capable of forming oxoDHA species.
Electrophilic oxoDHA species are also substrates for further metabolism, particularly the reduction of a double bond. In the case of PGE 2 metabolism, 15-ketoPGE 2 is reduced by prostaglandin reductase at the ␣,␤-unsaturated bond, yielding the non-electrophilic metabolite 13,14-dihydro-15ketoPGE 2 . The 14-oxoDHA metabolite was also reduced to its corresponding oxoDPA species; however, this metabolite retained its electrophilic nature, as indicated by retention of BME reactivity (Fig. 7, B and C). Further characterization by MS 2 and comparison of fragmentation patterns point to saturation of the ␥,⌬-double bond (Fig. 7, D-G). These data support that although prostaglandin reductase is expressed in human lung epithelium (36), 14-oxoDHA is not a substrate for prostaglandin reductase reduction. The identity of an enzyme responsible for 14-oxo-DHA reduction remains to be investigated.
The observation that oxoDHA species abrogate proinflammatory cytokine expression (Fig. 9) reinforces the concept that electrophilic 15PGDH metabolites can acquire additional and unique biological activities (5,6,13,19). Herein and in other 15-oxoETE, 17-oxoDHA, and 15d-PGJ 2 signaling studies, higher than physiological concentrations of the electrophile have been added to culture systems. In each instance, the intracellular concentrations of electrophile are in the nM range, affirming that these model systems are biologically relevant (19,20,37). These and other electrophilic fatty acids signal in vitro and in vivo via Michael adduction to key nucleophilic cysteines in transcriptional regulatory proteins that regulate the inflammatory response including Nrf2 and NF-B (16, 19, 20, 38 -41). We have demonstrated that 15PGDH-derived 14-oxoDHA can inhibit NF-B-mediated cytokine expression after LPS treatment. Similar results are obtained using FAT-1 mice, where the inflammatory response to methacholine after ovalbumin challenge is suppressed. FAT-1 mice express a Caenorhabditis elegans desaturase that converts ⍀-6 to ⍀-3 fatty acids, providing endogenously elevated levels of DHA and eicosapentaenoic acid in lung tissue (42) and presumably elevated oxoDHA products described in the present study. Compared with wild type mice, FAT-1 mice that underwent ovalbumin challenge showed a decrease in allergic airway inflammation as measured by proinflammatory cytokine and chemokine levels and a reduced response to methacholine (42).
In summary, the ⍀-3 class of fatty acids instigates anti-inflammatory signaling actions by modulating multiple target molecules and signaling pathways. Most commonly, ⍀-3 fatty acids are viewed to compete with their ⍀-6 fatty acids as substrates for enzymes such as COX, lipoxygenase, and cytochrome P450 to limit the formation of proinflammatory ⍀-6 metabolites. The tri-hydroxylated lipid mediators termed resolvins, maresins, and protectins are also proposed to transduce signaling responses of ⍀-3 fatty acids through ligand activity toward the G-protein-coupled chemerin, ALX, and orphan GPR23 receptors (11,32,43). We show herein that additional signaling events are operative downstream of ⍀-3 and ⍀-6 fatty acid hydroxylation. These actions are mediated by the further oxidation of mono-, di-, and tri-hydroxylated species to electrophilic product. This represents a mechanism whereby metabolic and inflammatory fatty acid oxygenation yields a common class of oxo metabolites that mediate adaptive anti-inflammatory effects through less restrictive and more pleiotropic mechanisms. Specifically, this involves the kinetically facile oxo-fatty acid formation of Michael adducts with nucleophilic cysteines present in established redox-sensing transcriptional regulatory proteins that regulate metabolism FIGURE 9. 14-oxoDHA inhibits NF-B-derived cytokine mRNA expression. Primary alveolar macrophages were treated with 100 ng/ml LPS, 100 ng/ml LPS, and 10 M 14-HDoHE or 100 ng/ml LPS and 10 M 14-oxoDHA for 6 h. LPS induced cytokine mRNA expression, which was abrogated by 14-oxoDHA for TNF␣ (A), IL-6 (B), and IL-1␤ (C). ** p Յ 0.01. 14-HDoHE treatment resulted in a significant inhibition of IL-6.
⍀-3-Derived 15PGDH Products Are Bioactive and inflammation. Thus, 15PGDH and related dehydrogenases not only regulate fatty acid catabolism but also yield electrophilic metabolites with metabolic, anti-proliferative, and antiinflammatory signaling activities.