Stabilized epoxygenated fatty acids regulate inflammation, pain, angiogenesis and cancer

1.1. Overview of the CYP/sEH pathway

CYP epoxygenases catalyze epoxidation of the double bonds of ARA to generate EETs. The epoxidation can occur at all of the four double bonds of ARA, leading to formation of four regioisomers (5,6-, 8,9-, 11,12- and 14,15-EET) [3]. Among these regioisomers, 5,6-EET is chemically unstable and undergoes rapid cyclization and hydrolysis, the other isomers are chemically stable except under acidic conditions. The CYPs referred to as epoxygenases are by no means specific, for example, they also oxidize reactive methylenes in PUFAs. The biochemistry of CYP epoxygenases in EETs biosynthesis have been discussed in several reviews [3, 36, 37]. A series of CYP enzymes such as CYP1A, CYP2B, CYP2C, CYP2D, CYP2G, CYP2J, CYP2N, and CYP4A are capable of converting ARA to EETs [3]. Generally each enzyme produces EETs with different profiles of optical- and regioisomers. In mammals CYP2C and CYP2J isoforms appear to be the predominate epoxygenases. For human and rat, CYP2C isoforms are the most abundant in liver and kidney, and CYP2J are the major ones in heart [3]. CYP2C and CYP2J are also the major epoxygenases in endothelium [36]. Similar to other CYP enzymes, the expression of CYP epoxygenases can be modulated by environmental factors and cellular stimuli [3, 36, 38]. Among these, the most physiologically relevant stimulator of CYP epoxygenase expression is hypoxia [39, 40], which is a critical regulator to stimulate neovasculization [41], suggesting a role of CYP epoxygeanses in angiogenesis.

Once formed, EETs are rapidly metabolized by sEH to generate the corresponding fatty acid diols called DHETs [6]. Compared with EETs, DHETs are widely believed to be inactive or less-active [5]; a recent study shows that opposite to the anti-inflammatory effects of EETs, DHETs are pro-inflammatory in stimulating monocyte migration [42]. Therefore the sEH-mediated metabolic step is generally regarded as a loss of beneficial biological activities. The biochemistry, expression and regulation of sEH have been discussed in several reviews [4–6]. The mammalian sEH is a homodimer composed of two ~62 KDa monomers. Each monomer has a ~35 KDa C-terminal domain which displays epoxide hydrolase activity and a ~25 KDa N-terminal domain which appears to have phosphatase activity [43]. sEH is highly expressed in many tissues including liver, kidney, lung, heart, brain, spleen, endothelium and mammary gland [6]. The highest sEH activity was observed in liver, followed with kidney. Even in organs with relatively low sEH activity, the enzymatic activity can be high in individual cell types. The expression of sEH is inducible by peroxisome proliferator-activated receptor α (PPARα) and PPARγ agonists [6]. PPARγ agonists have been shown to inhibit tumor growth and metastasis by blocking angiogenesis [44, 45], the anti-cancer effect of these compounds could be partially mediated by reduction of the amount of EETs via stimulation of sEH [32]. The expression of sEH is also up-regulated by angiotensin II [46] and homocysteine [47]. The sEH catalyzes hydrolysis of EpFAs by addition of water, in a two-step, base-catalyzed mechanism via the formation of a covalent intermediate [6]. Pharmacological inhibitors, many of which have a urea, amide, or carbamate group as the central pharmacophore to mimic the reaction transition states, were designed based on the catalytic mechanism of sEH enzyme [15]. A sEHI APAU has been evaluated in a Phase IIA trial targeting hypertension as the primary indication, recently more potent and metabolically stable sEHIs have been developed and are being considered for evaluation in human trials. FDA-approved anti-cancer drugs sorafenib (Nexavar®) and regorafenib (Stivarga®) are also potent sEH inhibitors with IC50 values in the low nM to pM range [48, 49].

Besides the hydrolysis catalyzed by sEH, EpFAs are also metabolized by other pathways including β-oxidation, chain shortening and chain elongation [3]. EpFAs can be reincorporated into the membrane phospholipids by acyl transferase causing a significant proportion of EpFAs to exist as esterified forms in the membrane phospholipids. In comparison, the fatty acid diols are less readily incorporated in the membrane phospholipids [3]. The biological significance of the membrane-incorporated EpFAs remains poorly studied. To address this question, more reliable analytical methods are needed to quantify the membrane-incorporated EpFAs and diols and particularly to evaluate the kinetics of this process. EpFAs could also be further metabolized by COX, LOX and CYP enzymes to generate novel series of LMs, though little is known about the chemical structures and biological activities of these lipid metabolites. Both 5,6- and 8,9-EET have been shown to be substrates of COX enzymes, which convert them to metabolites which may have potent effects of vasodilation or stimulation of cell proliferation [50–52]. A COX metabolite of 8,9-EET, 11-hydroxy-8,9-epoxyeicosatrienoic acid, has been shown to be >1000-fold more potent than 8,9-EET in stimulating cell proliferation and c-fos expression in rat glomerular mesangial cells [52]. Previous research from our laboratory has shown that sEHIs dramatically synergize with COX or LOX inhibitors to reduce inflammation [53, 54]. It would be interesting to investigate whether the observed synergistic interactions are in part mediated by the LOX and COX-derived metabolites of EETs. It was recently shown that EPA-derived 17,18-EEQ is further metabolized to generate 12-OH-17,18-EEQ, which inhibited LTB4-induced neutrophil chemotaxis and polarization in vitro with EC50 = 0.6 nM [55]. Other pathways such as β-oxidation and chain elongation also participate in the metabolism of EETs. When sEH is inhibited, other metabolic pathways of EETs are up-regulated [56]. Since the fates of EETs are regulated by multiple metabolic pathways, pharmacological inhibition or genetic deletion of sEH only increases level of EETs in a limited range.

2.1. Biological activities of EETs on inflammation in vitro

Node et al. first reported the anti-inflammatory effects of EETs [85]. Synthetic EETs inhibited LPS-, IL-1α- or TNF-α-induced vascular cell adhesion molecule-1 (VCAM-1) expression in human endothelial cells. The anti-inflammatory effects of EETs are regio-selective: 11,12-EET showing the most potent effect, followed with 8,9- and 5,6-EET, while 14,15-EET was inactive. 11,12-EET also suppressed other endothelial cell adhesion molecules such as E-selectin and intercellular adhesion molecule 1 (ICAM-1) in TNF-α-stimulated endothelial cells. Over-expression of CYP2J2 produced similar anti-inflammatory response, which was abolished by co-treatment with SKF525A, a broad pharmacological inhibitor of CYP enzymes including epoxygenases [85]. A recent study indicated that 14,15-EET inhibited TNF-α-stimulated inflammation in human bronchi, suggesting this EET regioisomer is also biologically active to suppress inflammation in some systems [86]. In a recent study, Deng et al. studied LPS-induced inflammatory responses in primary lung endothelial cells isolated from transgenic mice with endothelial expression of human CYP2C8 and CYP2J2 [87]. Transgenic expression of CYP2C8 or CYP2J2, which has higher capacity to generate EETs, significantly inhibited LPS-induced expression of E-selectin and monocyte chemoattractant protein-1 (MCP-1) in isolated endothelial cells, and such anti-inflammatory effects were attenuated by a putative EET receptor antagonist 14,15-EEZE and a selective inhibitor of CYP epoxygenase MS-PPOH [87].

EETs were also shown to inhibit inflammation in inflammatory cells in vitro. The mRNA expression of CYP2J2 and CYP2C8 were detected in human peripheral leukocytes, monocytes (Mc) and the human monocyte THP-1 cell line, but not polymorphonuclear cells (PMNs) [88]. 11,12- and 8,9-EET inhibited basal TNF-α production in THP-1 cells; 11,12-EET abolished IL-1β + PMA-induced COX-2 expression, while the CYP inhibitor SKF525A dose-dependently increased basal COX-2 expression in THP-1 cells [88]. In LPS-stimulated rat monocytes, CYP epoxygenase inhibitors SKF525A and 1-aminobenzotriazole (ABT) increased production of PGE2, while 11,12-EET dose-dependently suppressed LPS-induced PGE2formation via a mechanism of inhibiting the enzymatic activity but not the expression of COX-2 [89]. The sEHI c-TUCB reduced levels of LPS-induced MCP-1 and TNF-α, but not IL-6 and macrophage inflammatory protein-1α (MIP-1α), in human monocytes [90].

The sEH metabolites of EETs, DHETs, are generally believed to be inactive or less-active in many assays [5]. However a recent study showed that opposite to the anti-inflammatory effects of EETs, DHETs are pro-inflammatory in stimulating monocyte migration in vitro and in vivo [42]. Pharmacological inhibition of COX and LOX pathways had no effect on MCP-1-induced monocyte chemotaxis; while inhibition of CYP or sEH enzymes dose-dependently blocked this process, which was rescued by DHETs, suggesting the contribution of DHETs in MCP-1-induced chemotaxis [42]. This study indicates that pharmacological inhibition of sEH not only stabilizes and increases level of EETs which are anti-inflammatory, but also reduces the formation of DHETs which are pro-inflammatory.

2.2. Biological activities of EETs on inflammation in vivo

Animal studies have shown that EETs inhibited inflammation in various disease models. Continuous infusion of 11,12-EET, but not 14,15-EET, inhibited TNF-α-induced endothelial VCAM-1 expression and the resulting mononuclear cells adhesion and rolling in murine carotid artery [85]. Pharmacological inhibition of sEH, which increased level of EETs, reduced LPS-induced mortality, systemic hypotension and tissue injury, as well as elevation of inflammatory cytokines in a LPS-induced sepsis model in mice [91]. Inhibition of sEH reduced tobacco smoke-induced lung inflammation in spontaneously hypertensive rats [92]. Treatment with sEHIs decreased total bronchoalveolar lavage cell number with significant reductions noted in neutrophils, alveolar macrophages and lymphocytes in tobacco smoke-exposed rats. Co-administration of sEHIs with EETs further enhanced the anti-inflammatory effect of sEHIs [92]. In a streptozotocin-induced type 1 murine diabetic model, genetic deletion of sEH significantly reduced urinary MCP-1 excretion and NF-κB activation in diabetic mice [93]. Triclocarban (TCC) is a widely used antimicrobial component in personal care products, which has been shown to be a potent sEHI with IC50 = 13 nM for human sEH. In a LPS-induced acute inflammation model, treatment with TCC increased plasma levels of EETs and attenuated LPS-induced hypotension and elevation of pro-inflammatory cytokines in plasma [94]. Inhibition of sEH also reduced inflammation related to cardiovascular diseases. The mRNA expression of pro-inflammatory cytokines in liver (TNF-α and IL-6) and adipose tissues (TNF-α, IL-6, IL-1β and MCP-1) stimulated by high-fat diet were significantly reduced by treatment with the sEHI t-AUCB [95]. In a deoxycorticosterone acetate plus high salt (DOCA-salt)-induced hypertensive model in mice, genetic deletion of sEH or treatment with t-AUCB reduced DOCA-salt-induced hypertension, renal inflammation and renal injury [96]. Deletion of sEH reduced DOCA-salt-induced production of pro-inflammatory cytokines, macrophage infiltration, NF-κB signaling activation in renal tissues and elevation of urinary MCP-1 [96]. Inhibition or deletion of sEH reduces vascular remodeling and pro-inflammatory gene expression in an inflammatory model of neointima formation in mice [97]. IL-10 is an important anti-inflammatory cytokine, for example, genetic deletion of IL-10 induces inflammation in tissues and is used as a model for inflammatory bowel disease [98]. To study the role of sEH in inflammation caused by IL-10 deficiency, Zhang et al. created transgenic IL-10 (−/−) sEH (−/−) double knockout mice [99]. Deletion of sEH reduced the inflammatory cell infiltration, pro-inflammatory cytokine expression and NF-κB signaling activation caused by IL-10 deficiency [99, 100]. Beside manipulating sEH to modulate EETs, transgenic expression of CYP2C8 or CYP2J2 in mice significantly attenuated LPS-induced production of pro-inflammatory cytokines such as IL-6, MCP-1, E-selection, IL-1β and ENA-78, as well as NF-κB signaling activation and inflammatory cell infiltration in lung tissues [87].

Together, these studies provide strong evidence to support the anti-inflammatory effects of EETs in various inflammatory models, suggesting that inhibiting sEH to stabilize EETs is a promising therapeutic strategy to treat inflammatory disorders. However it should be noted that there are inconsistent results of sEH inhibition in inflammation [101, 102], more studies are thus needed to characterize the effects and mechanisms of EETs in inflammatory diseases and to determine what animal models are indicative of human conditions.

2.3. Mechanisms of EETs on inflammation

EETs have been shown to inhibit inflammation via blocking NF-κB pathway, which is an important signaling cascade to regulate inflammation. Without cellular stimulation, the NF-κB complex is sequestered in the cytoplasm through binding to the inhibitory protein IκBα. When activated, IκBα is phosphorylated and then degraded, resulting in release of the NF-κB complex from IκBα. The released NF-κB translocates to the nucleus and activates the expression of multiple pro-inflammatory genes [103]. Node et al. showed that 11,12-EET, but not 14,15-EET, inhibited TNF-α-induced IκBα degradation and nuclear translocation of NF-κB in endothelial cells, suggesting that EETs inhibit inflammation via blocking NF-κB signaling activation [85]. Co-administration of the sEHI AUDA with individual EET regioisomers inhibited TNF-α-induced IκBα degradation in endothelial cells, which was attenuated by a PPAR-γ antagonist GW9662. These data suggest that EETs blocked NF-κB signaling via a PPAR-γ-dependent mechanism [104]. In human bronchi, 14,15-EET inhibited TNF-α-stimulated inflammation via inhibition of IκBα degradation [86]. In primary mouse neonatal cardiomyocytes, the sEHI AEPU suppressed ascending aortic constriction-induced IκBα phosphorylation and degradation, and nuclear accumulation of NF-κB subunit p65 [105]. In primary endothelial cells isolated from Tie2-CYP2J2-Tr mice, LPS-induced IκBα phosphorylation was attenuated compared with WT cells [87]. Animal experiments also support that EETs and CYP/sEH pathway modulate NF-κB signaling. LPS-induced IκBα phosphorylation in lung tissues was significantly attenuated in Tie2-CYP2C8-Tr, Tie2-CYP2J2-Tr and sEH-null mice compared with WT mice [87]. Genetic deletion of sEH suppressed activation of NF-κB signaling in IL-10-knockout mice [99, 100]. Inhibition or deletion of sEH suppressed DOCA-salt- and streptozotocin-induced NF-κB activation in renal tissues [93, 96].

Besides NF-κB, other signaling pathways have also been investigated. For example, treatment with the sEHI c-TUCB had no effect on LPS-induced NF-κB nuclear translocation, while it abolished LPS-induced phosphorylation of JNK in adherent human monocytes, suggesting that JNK pathway is a potential target of sEHIs or EETs in monocytes [90]. PPARs have also been shown to contribute to the anti-inflammatory effects of EETs [104, 106–108].

3.1. Mechanisms of EETs on inflammatory pain

EpFA modulation of inflammatory pain has multiple effects including changes in COX-2 regulation and prostaglandin synthesis, interactions with TRP receptors and activity of CB2 receptors. However, it is widely hypothesized that a yet undiscovered G-protein coupled receptor is the primary mechanism for modulating inflammatory pain [117].

Administration of sEHI during an inflamed state resulted in reduced COX-2 mRNA in the spinal cord [109] and protein [53] expression in the liver relative to inflammed controls. This change in COX-2 regulation is likely modulated by suppression of NF-κB stemming from EpFAs binding to PPARγ [53]. The combination of COX-2 and sEH inhibitors results in a synergistic effect on both reducing the pro-inflammatory prostaglandins and the nociception, perception of pain, associated with systemic inflammation [53]. From this synergistic effect, the development of COX-2/sEH dual inhibitors have resulted in particularly potent inhibitors of LPS-induced inflammatory pain with favorable PK profiles [112]. However, blocking pain is not completely dependent on modulation of the COX-2 pathway, as evidenced by sEHI-mediated analgesia during PGE2 stimulated pain [121]. Interestingly, evidence indicates that EpFAs induce analgesia using a mechanism that requires prostaglandin activity, which explains why sEHI work only in an already inflamed state or a state of enhanced pain perception. The necessary component of this mechanism is cAMP, a downstream product of the prostanoid receptor, which can be mimicked by addition of phosphodiesterase inhibitors (PDEI) [121]. Thus co-administration of sEHI and PDEI results in reduction in pain-related response in the absence of an inflammatory state [121]. These data also suggest that a combination of sEHI and PDEI will enhance the potency, increase the therapeutic index, and broaden the activity of both drug classes. However, in the absence of inflammatory pain and upregulated cAMP, direct administration of ARA or EET increases sensitivity to pain briefly. A higher dose of EETs are required to enhance in a naive state than to control pain in a hyperalgesic state. The mechanism of this activity is not understood [119].

Paradoxically, when investigators have looked at sEH knockout mice, there does not seem to be the same regulation of COX-2 or modulation of pro-inflammatory prostaglandins seen with administration of sEHI [122]. This apparent discrepancy may be due to other genetic and physiological changes associated with strain of sEH knockout mice [123]. Alternatively each monomer of the sEH dimer has a catalytically active phosphatase domain active on lipophilic but not protein phosphatases [43]. The physiological role of this highly conserved domain is not known but is absent in the sEH knock out animals. In addition to in vivoadministration to sEH knockout mice, adding 5,6-EET directly to dorsal root ganglia resulted in increased TRPA1-mediated sensitization [122]. Similar to the above results, direct addition of 5,6-EET to TRPV4 transfected cells resulted in generation of Ca2+ currents [124]. While these combined findings suggest that 5,6-EET could actually increase sensitivity to pain, the rapid cyclization of this regioisomer indicate a secondary metabolite is the active sensitizing component.

In addition to direct effects on inflammation and pain, mounting evidence suggests a component relating epoxygenated endocannabinoids to pain and inflammation. The best understood endocannabinoids, anandamide (an ethanolamine derivative) and 2-arachidonylglycerol (a glycerol derivative), are derivatives of ARA that bind to the cannabinoid (CB1 and CB2) receptors. These receptors and ligands are named for their relation to the natural product Δ9-tetrahydrocannabinol – the active component of Cannabis sativa[125]. Changes in the endogenous cannabinoids are associated with a large spectrum of diseases including but not limited to obesity, inflammation, cardiovascular and metabolic disorders, cancer and pain [126]. Activation of CB2 receptors inhibits nociception in multiple forms of sensitization [127, 128], mediated by both inflammatory and non-inflammatory mechanisms [129]. An epoxide of anandamide, 5,6-epoxyeicosatrienoic acid ethanolamide (5,6-EET-EA) binds to CB2 receptor with high affinity (Ki = 8.9 nM) and increased stability relative to the parent anandamide. Compared to anandamide, which is hydrolyzed by fatty acid amide hydrolase (FAAH), 5,6-EET-EA can also be hydrolyzed by sEH to the respective diol, which can be inhibited by administration of sEHI [130]. Additionally, the 5,6-EET methyl ester is also a ligand for CB2 receptor, although with significantly decreased potency (IC50 = 19 μM) [116]. To test the possibility that an epoxide may be directly effecting inflammatory pain through the CB2receptor, Wagner et al [118] used CB2 antagonists to show the antinociceptive effects of sEHI were reduced when blocking CB2 in an LPS model of localized inflammation. However, further experiments are necessary to determine the exact contribution of cannabinoid signaling to antinociception in both inflammatory and neuropathic pain.

4.1. Biological activities of EETs on angiogenesis in vitro

The first data to suggest the pro-angiogenic effect of EETs was that endogenous EETs released from astrocytes stimulated cellular proliferation and tube formation of co-cultured endothelial cells [142]. Further studies showed that treatment with synthetic EETs stimulated angiogenesis in endothelial cells [36, 143, 144]. 11,12- and 14,15-EET are the most studied EET regioisomers and they have been shown to increase endothelial cell proliferation, migration and invasion, which are critical cellular steps involved in angiogenesis [145–149]. 11,12-EET also increased activity of matrix metalloproteases (MMPs), though the identity of the MMP enzymes involved remain to be confirmed [39]. Besides 11,12- and 14,15-EET, 5,6- and 8,9-EET have also been shown to stimulate cellular proliferation and tube formation in pulmonary murine microvascular endothelial cells, while the diols (5,6-, 8,9-, 11,12- and 14,15-DHET) lacked such effects [150]. Overexpression of CYP epoxygenases or pharmacological inhibition of sEH produced similar pro-angiogenic effects in endothelial cells [39, 40, 148, 150–152], while pharmacological inhibition of CYP epoxygenases suppressed angiogenesis [148]. Over-expression of CYP2C9 or treatment with 11,12-EET increased the expression of COX-2 in endothelial cells, consistent with the pro-angiogenic effect of EETs [153]. CYP2C in endothelial cells is inducible by hypoxia which is a key regulator to stimulate angiogenesis, suggesting that EETs are involved in the hypoxia-induced angiogenic responses [39]. Together, these results support the pro-angiogenic effects of EETs in vitro.

4.2. Biological activities of EETs on angiogenesis in vivo

Animal studies were followed up to support the pro-angiogenic effects of EETs in vivo. iTreatment with 11,12- or 14,15-EET stimulated neovascularization in a Matrigel plug assay and a chck chorioallantoic membrane (CAM) assay [148, 151, 154]. 5,6- and 8,9-EET stimulated angiogenesis in a subcutaneous sponge assay in mice [150]. Local treatment with 11,12-EET, 14,15-EET or the sEHI t-AUCB accelerated wound epithelialization and neovascularization in mice [155]. Recently Panigrahy et al. demonstrated that endothelium-derived EETs accelerated organ and tissue regeneration by stimulation of angiogenesis [156]. This study used three transgenic mouse models which have high level of EETs: endothelial expression of human CYP2C8 and human CYP2J2 (Tie2-CYP2C8-Tr and Tie2-CYP2J2-Tr) and genetic knockout of sEH (sEH-null). In these high-EETs transgenic mouse models, accelerated liver regeneration, kidney compensatory growth, lung compensatory growth, wound healing, corneal neovascularization and retinal vascularization were observed. Continuous infusion of 14,15-EET or administration of sEHI also stimulated tissue regeneration, while transgenic over-expression of sEH which reduced EETs levels delayed normal organ and tissue growth. This study suggests that sEHIs could be novel therapeutics for a number of human diseases which requires stimulation of angiogenesis [156].

5.2. Biological activities of EETs on tumorigenesis in vivo

Over-expression of CYP2J2 in cancer cells has been shown to stimulate tumor growth and metastasis in vivo [164–166]. The endothelium is a major site for biosynthesis of EETs. Recently Panigrahy et al. demonstrated that endothelium-derived EETs stimulated tumor growth and metastasis in multiple tumor models [32]. High levels of EETs in transgenic Tie2-CYP2C8-Tr, Tie2-CYP2J2-Tr and sEH-null mice slightly increased primary tumor growth but dramatically stimulated tumor metastasis. Continuous infusion with 14,15-EET via osmotic mini-pumps or treatment with a high-dose sEHI t-AUCB (10 mg/kg/day) also increased tumor progression, while the corresponding diols DHETs have no such effects. Lowering EETs by transgenic over-expression of sEH or using the EET antagonist 14,15-EEZE reduced tumor progression. The biological effects of EETs are at least partially mediated by VEGF. The plasma levels of EETs were significantly elevated in Tie2-CYP2C8-Tr and sEH-null mice compared with WT mice. Continuous infusion of 14,15-EET also increased VEGF expression in tumor endothelium and stromal fibroblasts of LLC tumors. Depletion of VEGF using Ad-sFIt dramatically suppressed B16F10 tumor growth in Tie2-CYP2J2-Tr and sEH-null but not in WT mice [32]. This study demonstrates that EETs play a central role in tumor growth and metastasis by stimulation of tumor angiogenesis.

This study raises questions on the biological implication from the sEH inhibition regarding cancer risks. Currently sEHIs are considered for human clinical trials for multiple disorders such as pain and inflammation [5], thus this study raised potential safety concerns of sEHIs in cancer patients. However it should be noted that in animal experiments the doses of sEHIs to treat hypertension, pain, and inflammation are in low mg/kg range (0.1–1 mg/kg), while the active dose used in the tumor experiment was as high as 10 mg/kg/day [32]. Our study showed that at 1 mg/kg/day, t-AUCB had no effect on primary tumor growth and metastasis in mice [33]; while at 10 mg/kg/day, t-AUCB significantly increased tumor growth and metastasis [32]. These results indicate that the biological effects of sEHIs (or EETs) on tumorigenesis have a high threshold. This still leaves the question if the therapeutic index of sEHI is sufficiently high to justify long term chronic use as pharmaceuticals.

6.2. Biological activities of ω-3 EpFAs on angiogenesis

Opposite to the effects of EETs in stimulation of angiogenesis, our recent study demonstrated that DHA-derived EDPs are strongly anti-angiogenic [33]. In a Matrigel plug assay in mice, treatment with synthetic EDP regioisomers (7,8-, 10,11-, 13,14-, 16,17- and 19,20-EDP) inhibited VEGF-induced neovascularization in a dose-dependent manner with EC50 = 0.3 μg per mouse. The 5,6-EDP regioisomer was chemically unstable, thus it was not tested. 19,20-EDP also inhibited fibroblast growth factor-2 (FGF-2)-induced angiogenesis using the Matrigel plug assay, supporting the potential broad-spectrum anti-angiogenic effects of EDPs [33]. In contrary, previous studies in Matrigel plug assays showed that EETs stimulated angiogenesis when treated alone [148, 154], and further up-regulated VEGF-induced angiogenesis in the presence of VEGF [156]. Together, these results support the opposite effects of ω-6 and ω-3 EpFAs on angiogenesis. To test whether EDPs inhibits angiogenesis via targeting endothelial cells, we tested the effects of EDPs on angiogenesis in the primary endothelial cell line HUVECs. 19,20-EDP inhibited endothelial tube formation after 6-h treatment in HUVECs, supporting its anti-angiogenic effect in vitro. The process of angiogenesis composes of multiple cellular steps including cell proliferation, migration and production of MMPs. We found that 19,20-EDP potently inhibited VEGF-stimulated endothelial cell migration, with no effect on cell proliferation and weak inhibitory effect on MMP-2 activity in HUVECs, suggesting that EDPs inhibited angiogenesis primarily via suppressing endothelial cell migration [33]. The detailed mechanism by which EDPs suppressed endothelial cell migration requires more study.

19,20-EDP at 1 μM almost abolished VEGF-induced VEGFR2 activation after a 10-min treatment in HUVECs, supporting that 19,20-EDP inhibits angiogenesis via a VEGFR2-dependent mechanism [33]. VEGFR2 is a critical mediator of angiogenesis, regulating all known biology of VEGF [157]. Most anti-angiogenic drugs on the market target VEGFR2/VEGF pathway to inhibit angiogenesis. However, VEGF is also critical for cardiovascular system [157]; therefore, all of currently available anti-angiogenic drugs cause cardiovascular side effects such as hypertension [175]. Human studies support that ω-3 PUFA supplementation reduced hypertension [176–178], and DHA-derived EDPs are among the most potent vessel dilators ever discovered [31]. In this aspect, pharmacological or nutritional manipulation of tissue level of EDPs may have unique advantages in anti-angiogenic therapy with reduced adverse effects on pain, blood pressure and other cardiovascular functions than current therapies.

Interestingly, our study also suggested potential roles of EDPs in lymphangiogenesis, an important process involved in tumor metastasis and other human diseases [179]. An angiogenesis assay (>80 genes correlated with angiogenesis) showed that the most down-regulated gene by 19,20-EDP is VEGF-C. RT-PCR analysis further confirmed that treatment of 19,20-EDP in HUVECs inhibited transcription of VEGF-C in a dose-dependent manner, while it has no effect on mRNA expression of VEGF-A [33]. VEGF-C is a critical mediator to regulate formation of new lymphatic vessels [179], suggesting a potential role of EDPs in inhibiting lymphangiogenesis. Currently no lymphangiogenesis inhibitors have been approved in therapy and a VEGF-C antibody is in Phase I human trials to treat cancers. More studies are needed to characterize the effects of EDPs on lymphangiogenesis and associated diseases.

The opposite effect of EETs and EDPs may explain away some inconsistent results in previous studies. Substantial studies have demonstrated that pharmacological inhibition or genetic deletion of sEH increases angiogenesis. For example, Panigrahy et al. showed that genetic deletion of sEH increased tissue regenerations in liver, lung and kidney via stimulation of angiogenesis [156]. However, recent studies showed that inhibition or deletion of sEH suppresses angiogenesis in zebrafish [76] and retina [180]. These “inconsistent” results could be partially explained by our findings of the opposite effects of EETs and EDPs on angiogenesis (Figure 3). The ω-6 ARA is the most abundant PUFA in membrane phospholipids in most tissues, pharmacological inhibition or genetic deletion of sEH would thus mainly accumulate ARA-derived EETs to stimulate angiogenesis. On the other hand, the ω-3 DHA is highly enriched in retina and brain tissues [17], inhibition or deletion of sEH is likely to mainly accumulate DHA-derived EDPs, leading to suppression of angiogenesis in these tissues. Currently there is no report of the tissue levels of EpFAs in retinal or brain tissues, while previous study has shown that EDPs are the most abundant EpFAs in zebrafish which is rich in ω-3 PUFAs, inhibition of sEH causes a 5-fold increase of the level of EDPs in zebrafish [76]. Since endogenous DHA is highly enriched in retinal tissues [17], pharmacological inhibition of sEH may be a potential strategy to suppress retinal angiogenesis and associated diseases such as macular degeneration. These studies emphasize that sEH inhibition is a ‘shot-gun” approach, modulating the levels of multiple EpFAs from several ω-3 and ω-6 PUFAs including ARA, EPA and DHA. The profiles of the EpFAs are tissue specific and can be modulated by nutrition. This modulation of lipid stores through nutrition offers more therapeutic opportunities by modulating sEH.

Fig. 3

Genetic deletion or pharmacological inhibition of sEH in ω-6-rich and ω-3-rich tissues leads to accumulation of EETs and EDPs respectively, leading to different effects on angiogenesis.

Besides our study, Cui et al. showed that 17,18-EEQ, but not other EEQ regioisomers derived from EPA, inhibited cell proliferation in the immortalized endothelial cell line bEND.3 at a dose of 10 μM, while EETs at the same dose showed opposite effects to increase cell proliferation in bEND.3 cells [181]. This study suggests that EPA epoxides may also suppress angiogenesis.

We acknowledge support from National Institute on Environmental Health Sciences R01 ES02710 and P42 ES04699, Research Investments in the Sciences and Engineering (RISE) Program of University of California Davis. B.D.H. is a George and Judy Marcus Senior Fellow of the American Asthma Society.