Specialized pro-resolving mediators

Specialized pro-resolving mediators (SPM, also termed specialized proresolving mediators) are a large and growing class of cell signaling molecules formed in cells by the metabolism of polyunsaturated fatty acids (PUFA) by one or a combination of lipoxygenase, cyclooxygenase, and cytochrome P450 monooxygenase enzymes. Pre-clinical studies, primarily in animal models and human tissues, implicate SPM in orchestrating the resolution of inflammation. These studies suggest that synthetic SPM that are resistant to being metabolically inactivated hold promise of being clinically useful pharmacological tools for preventing and resolving a wide range of pathological inflammatory responses along with the tissue destruction and morbidity that these responses cause. Based on animal model studies, the inflammation-based diseases which may be treated by such metabolically resistant SPM analogs include not only pathological and tissue damaging responses to invading pathogens but also a wide array of pathological conditions in which inflammation is a contributing factor such as allergic inflammatory diseases (e.g. asthma, rhinitis), autoimmune diseases ( e.g. rheumatoid arthritis, systemic lupus erythematosis), psoriasis, atherosclerosis disease leading to heart attacks and strokes, type 1 and type 2 diabetes, the metabolic syndrome, and certain dementia syndromes (e.g. Alzheimer's disease, Huntingdon's disease).[1][2][3] SPM join the long list of other physiological agents which tend to limit inflammation (see Inflammation § Resolution of inflammation) including glucocorticoids, annexin A1, melanocortins, and the gaseous resolvins, carbon monoxide (see Carbon monoxide § Normal human physiology), nitric oxide (see Nitric oxide § Biological functions), and hydrogen sulfide (see Hydrogen sulfide § Function in the body and Hydrogen sulfide § Involvement in diseases).[4][5]

History

Through most of its early period of study, acute inflammatory responses were regarded as self-limiting innate immune system reactions to invading foreign organisms, tissue injuries, and other insults. These reactions were orchestrated by various soluble signaling agents such as a) foreign organism-derived N-formylated oligopeptide chemotactic factors like N-Formylmethionine-leucyl-phenylalanine; b) Complement component 5a and C3a (complement) chemotactic factors formed during the activation of the host's blood complement system by the invading organisms or injured tissues; and c) host cell-derived cytokines, chemokines, platelet-activating factor, and numerous PUFA metabolites including prostaglandins, leukotrienes such as leukotriene B4, Hydroxyeicosatetraenoic acids such as 5-HETE, and oxoeicosanoids such as 5-oxo-eicosatetraenoic acid. These agents act as cell signaling agents to increase the permeability of local blood vessels; activate nearby tissue-bound endothelial cells, mast cells, and macrophages; and attract to the nascent inflammatory site and further activated circulating neutrophils, monocytes, eosinophils, Gamma delta T cells, and Natural killer T cells. These reactions trended to neutralize invading organisms, limit tissue injury, and initiate tissue repair; they were viewed as resolving automatically consequential to the dissipation of signaling agents and thereby the recruitment and activation of pro-inflammatory cells.[6] In 1974, however, Charles N. Serhan and his renowned colleagues, Mats Hamberg and Bengt Samuelsson, discovered that human neutrophils metabolized arachidonic acid to two novel products that contained 3 hydroxyl residues and 4 double bonds viz., 5,6,15-trihydroxy-7,9,11,13-icosatetraenoic acid and 5,14,15-trihydroxy-6,8,10,12-icosatetraenoic acid.[7][8] These products are now termed lipoxin (Lx)A4 and LxB4, respectively. While initially found to have in vitro activity suggesting that they might act as pro-inflammatory agents, Serhan and colleagues as well as numerous other groups found that these lipoxins as well as many other newly discovered metabolites of various PUFA possess primarily if not exclusively anti-inflammatory activities in vivo as well as in vitro.[9] These many products were termed specialized pro-resolving mediators or SPM.[10]

SPM and inflammation

The production and activities of the SPM suggest a new view of inflammation wherein the initial response to foreign organisms, tissue injury, or other insults involves numerous soluble cell signaling molecules that not only recruit various cell types to promote inflammation but concurrently cause these cells to produce SPM which feed back on their parent and other cells to dampen their pro-inflammatory activity and to promote repair. Resolution of an inflammatory response is thus an active rather than self-limiting process which is set into motion at least in part by the initiating pro-inflammatory mediators (e.g. prostaglandin E2 and prostaglandin D2) which instruct relevant cells to produce SPM and to assume a more anti-inflammatory phenotype. Resolution of the normal inflammatory response, then, may involve switching production of pro-inflammatory to anti-inflammatory PUFA metabolites. Excessive inflammatory responses to insult as well as many pathological inflammatory responses that contribute to diverse diseases such as atherosclerosis, diabetes, Alzheimer's disease, Inflammatory bowel disease, etc. (see Inflammation#Inflammatory disorders) may reflect, in part, a failure in this class switching. Diseases caused or worsened by non-adaptive inflammatory responses may by amenable to treatment with SPM or synthetic SPM which, unlike natural SPM, resist in vivo metabolic inactivation.[2][11][12] The SPM possess overlapping activities which work to resolve inflammation. SPMs (typically more than one for each listed action) have the following anti-inflammatory activities on the indicated cell types as defined in animal and human model studies:[1][13][14][15]

SPMs also stimulate anti-inflammatory and tissue reparative types of responses in epithelium cells, endothelium cells, fibroblasts, smooth muscle cells, osteoclasts, osteoblasts, goblet cells, and kidney podocytes[1] as well as activate the heme oxygenase system of cells thereby increasing the production of the tissue-protective gaso-transmitter, carbon monoxide (see Carbon monoxide#Normal human physiology), in inflamed tissues.[16]

Biochemistry

SPM are metabolites of arachidonic acid (AA), eicosapentaenoic acid (EPA), docosahexaenoic acid (DHA), or n-3 DPA (i.e. 7,10Z,13Z,19Z-docosapentaenoic acid or clupanodonic acid); these metabolites are termed lipoxins (Lx), resolvins (Rv), protectins (PD) (also termed neuroprotectins [NP]), and maresins (MaR). EPA, DHA, and n-3 DPA are n-3 fatty acids; their conversions to SPM are proposed to be one mechanism by which n-3 fatty acids may ameliorate inflammatory diseases (see Omega-3 fatty acid#Inflammation).[17] SPM act, at least in part, by either activating or inhibiting cells through binding to and thereby activating or inhibiting the activation of specific cellular receptors.

Lipoxins

Human cells synthesize LxA4 and LxB4 by serially metabolizing arachidonic acid (5Z,8Z,11Z,14Z-eicosatrienoic acid) with a) ALOX15 (or possibly ALOX15B) followed by ALOX5; b) ALOX5 followed by ALOX15 (or possibly ALOX15B); or c) ALOX5 followed by ALOX12. Cells and, indeed, humans treated with aspirin form the 15R-hydroxy Epimer lipoxins of these two 15S-lipoxins viz., 15-epi-LXA4 and 15-epi-LXB4, through a pathway that involves ALOX5 followed by aspirin-treated cyclooxygenase 2 (COX2). Aspirin-treated COX-2, while inactive in metabolizing arachidonic acid to prostanoids, metabolizes this PUFA to 15R-hydroperoxy-eicosatetraenoic acid whereas the ALOX15 (or ALOX15B) pathway metabolizes arachidonic acid to 15S-hydroperoxy-eicosatetraenoic acid. The two aspirin-triggered lipoxins (AT-lipoxins) or epi-lipoxins differ structurally from LxA4 and LxB4 only in the S versus R chirality of their 15-hydroxyl residue. Numerous studies have found that these metabolites have potent anti-inflammatory activity in vitro and in animal models and in humans may stimulate cells by binding to certain Receptor (biochemistry)s in or on these cells.[11][18][19] The following table lists the structural formulae (ETE stands for eicosatetraenoic acid), major activities, cellular receptor targets (where known), and Wikipedia pages giving further information on the activity and synthesis of the lipoxins.

Trivial name Formula Activities Receptor(s) See Wikipedia page
LxA4 5S,6R,15S-trihydroxy-7E,9E,11Z,13E-ETE Anti-inflammatory, blocks pain perception[2][18] Stimulates FPR2, AHR[18][20] Lipoxin,15-Hydroxyicosatetraenoic acid#15S-HETE
LxB4 5S,14R,15S-trihydroxy-6E,8Z,10E,12E-ETE Anti-inflammatory, blocks pain perception[2][18] ? Lipoxin,15-Hydroxyicosatetraenoic acid#15S-HETE
15-epi-LxA4 (or AT-LxA4) 5S,6R,15R-trihydroxy-7E,9E,11Z,13E-eicosatetraenoic acid Anti-inflammatory, blocks pain perception[2][18] stimulates FPR2[18] Lipoxin, 15-Hydroxyicosatetraenoic acid#15R-HETE
15-epi-LxB4 (or AT-LxB4) 5S,14R,15R-trihydroxy-6E,8Z,10E,12E-eicosatrienoic acid Anti-inflammatory, blocks pain perception[2][18] ? Lipoxin, 15-Hydroxyicosatetraenoic acid#15R-HETE

Resolvins

Resolvins are metabolites of omega-3 fatty acids, EPA, DHA, and 7Z,10Z,13Z,16Z,19Z-docosapentaenoic acid (n-3 DPA). All three of these omega-3 fatty acids are abundant in salt water fish, fish oils, and other seafood.[17] n-3 DPA (also termed clupanodonic acid) is to be distinguished from its n-6 DPA isomer, i.e. 4Z,7Z,10Z,13Z,16Z-docosapentaenoic acid, also termed osbond acid.

EPA-derived resolvins

Cells metabolize EPA (5Z,8Z,11Z,14Z,17Z-eicosapentaenoic acid) by a cytochrome P450 monooxygenase(s) (in infected tissues a bacterial cytochrome P450 may supply this activity) or aspirin-treated cyclooxygenase-2 to 18R-hydroperoxy-EPA which is then reduced to 18R-hydroxy-EPA and further metabolized by ALOX5 to 5S-hydroperoxy-18R-hydroxy-EPA; the later product may be reduced to its 5,18-dihydroxy product, RvE2, or converted to its 5,6-epoxide and then acted on by an epoxide hydrolase to form a 5,12,18-trihydroxy derivative, RvE1. In vitro, ALOX5 can convert 18S-HETE to the 18S analog of RvE1 termed 18S-RvE1. 18R-HETE or 18S-HETE may also be metabolized by ALOX15 to its 17S-hydroperoxy and then reduced to its 17S-hydroxy product, Rv3. Rv3, as detected in in vitro studies, is a dihydroxy mixture of 18S-dihydroxy (i.e. 18S-RvE3) and 18R-dihydroxy (i.e. 18R-RvE3) isomers, both of which, similar to the other aforementioned metabolites possess potent SPM activity in in vitro and/or animal models.[22][23][24] In vitro studies find that ALOX5 can convert 18S-hydroperoxy-EPA to the 18S-hydroxy analog of RvE2 termed 18S-RvE2. 18S-RvE2, however has little or no SPM activity[24] and is therefore not considered to be a SPM here. The following table lists the structural formulae (EPA stands for eicosapentaenoic acid), major activities, cellular receptor targets (where known), and Wikipedia pages giving further information on the activity and syntheses.

Trivial name Formula Activities Receptor(s) See Wikipedia page
RvE1 5S,12R,18R-trihydroxy-6Z,8E,10E,14Z,16E-EPA Anti-inflammatory, blocks pain perception[1][25] stimulates CMKLR1, receptor antagonist of BLT, inhibits activation of TRPV1, TRPV3, NMDAR, and TNFR receptors[1][15][22] Resolvin#E series resolvins
18S-RvE1 5S,12R,18S-trihydroxy-6Z,8E,10E,14Z,16E-EPA Anti-inflammatory, blocks pain perception[1][25] stimulates CMKLR1, receptor antagonist of BLT[22][26] Resolvin#E series resolvins
RvE2 5S,18R-dihydroxy-6E,8Z,11Z,14Z,16E-EPA Anti-inflammatory[1] partial receptor agonist of CMKLR1, receptor antagonist of BLT[22][27] Resolvin#E series resolvins
RvE3 17R,18R/S-dihydroxy-5Z,8Z,11Z,13E,15E-EPA Anti-inflammatory[1] ? Resolvin#E series resolvins

DHA-derived resolvins

Cells metabolize DHA (4Z,7Z,10Z,13Z,16Z,19Z-docosahexaenoic acid) by either ALOX15 or a cytochrome P450 monooxygenase(s) (bacteria may supply the cytochrome P450 activity in infected tissues) or aspirin-treated cyclooxygenase-2 to 17S-hydroperoxy-DHA which is reduced to 17S-hydroxy-DHA. ALOX5 metabolizes this intermediate to a) 7S-hydroperoxy,17S-hydroxy-DHA which is then reduced to its 7S,17S-dihydroxy analog, RvD5; b) 4S-hydroperoxy,17S-hydroxy-DHA which is reduced to its 4S,17S-dihydroxy analog, RvD6; c) 7S,8S-epoxy-17S-DHA which is then hydrolyzed to 7,8,17-trihydroxy and 7,16,17-trihydorxy products, RvD1 and RvD2, respectively; and d) 4S,5S-epoxy-17S-DHA which is then hydrolyzed to 4,11,17-trihydroxy and 4,5,17-trihydroxy products, RvD3 and RvD4, respectively. These six RvDs possess a 17S-hydroxy residue; however, if aspirin-treated cyclooxygenase-2 is the initiating enzyme, they contain a 17R-hydroxy residue and are termed 17R-RvDs, aspirin-triggered-RvDs, or AT-RvDs 1 thru 6. In certain cases, the final structures of these AT-RvDs is assumed by analogy to the structures of their RvD counterparts. Studies have found that most (and presumably all) of these metabolites have potent anti-inflammatory activity in vitro and/or in animal models.[21][22][23][28] The following table lists the structural formulae, major activities with citations, cellular receptor targets, and Wikipedia pages giving further information on the activity and synthesis of these D series resolvins.

Trivial name Formula Activities Receptor(s) See Wikipedia pages
RvD1 7S,8R,17S-trihydroxy-4Z,9E,11E,13Z,15E,19Z-DHA Anti-inflammatory, blocks pain perception[1][29] stimulates GPR32, FPR2, inhibits activation of TRPV3, TRPV4, TRPA1[22] Resolvin#D series resolvins
RvD2 7S,16R,17S-trihydroxy-4Z,8E,10Z,12E,14E,19Z-DHA Anti-inflammatory, blocks pain perception[1][30] stimulates GPR32, GPR18, FPR2, inhibits activation of TRPV1 and TRPA1[15][16] Resolvin#D series resolvins
RvD3 4S,11R,17S-trihydroxy-5Z,7E,9E,13Z,15E,19Z-DHA Anti-inflammatory[1] stimulates GPR32[22] Resolvin#D series resolvins
RvD4 4S,5R,17S-trihydroxy-6E,8E,10Z,13Z,15E,19Z-DHA ? ? Resolvin#D series resolvins
RvD5 7S,17S-dihydroxy-4Z,8E,10Z,13Z,15E,19Z-DHA Anti-inflammatory[1] stimulates GPR32[22] Resolvin#D series resolvins
RvD6 4S,17S-dihydroxy-5E,7Z,10Z,13Z,15E,19Z-DHA ? ? Resolvin#D series resolvins
17R-RvD1 (AT-RvD1) 7S,8R,17R-trihydroxy-4Z,9E,11E,13Z,15E,19Z-DHA Anti-inflammatory,blocks pain perception[1][29] stimulates FPR2, GPR32, inhibits activation of TRPV3, TRPV4, and TNFR[15][22] Resolvin#Aspirin-triggered resolvin Ds
17R-RvD2 (AT-RvD2) 7S,16R,17R-trihydroxy-4Z,8E,10Z,12E,14E,19Z-DHA ? ? Resolvin#Aspirin-triggered resolvin Ds
17R-RvD3 (AT-RvD3) 4S,11R,17R-trihydroxy-5Z,7E,9E,13Z,15E,19Z-DHA Anti-inflammatory[1] stimulates GPR32[22] Resolvin#Aspirin-triggered resolvin Ds
17R-RvD4 (AT-RvD4) 4S,5R,17R-trihydroxy-6E,8E,10Z,13Z,15E,19ZDHA ? ? Resolvin#Aspirin-triggered resolvin Ds
17R-RvD5 (AT-RvD5) 7S,17R-dihydroxy-4Z,8E,10Z,13Z,15E,19Z-DHA ? ? Resolvin#Aspirin-triggered resolvin Ds
17R-RvD6 (AT-RvD6) 4S,17R-dihydroxy-5E,7Z,10Z,13Z,15E,19Z-DHA ? ? Resolvin#Aspirin-triggered resolvin Ds

n-3 DPA-derived resolvins

n-3 DPA (i.e. 7Z,10Z,13Z,16Z,19Z-docosahexaenoic acid)-derived resolvins are recently identified SPM. In the model system used to identify them, human platelets pretreated with aspirin to form acetylated COX2 or the statin, atorvastatin, to form S-ntrosylated and thereby modify this enzyme's activity metabolize n-3 DPA to form a 13R-hydroperoxy-n-3 DPA intermediate which is passed over to nearby human neutrophils; these cell then metabolize the intermediate to four poly-hydroxyl metabolites termed resolvin T1 (RvT1), RvT2, RvT3, and RvT4. (The chirality of their hydroxyl residues has not yet been determined.) These T series resolvins also form in mice undergoing experimental inflammatory responses and have potent in vitro and in vivo anti-inflammatory activity; they are particularly effective in reducing the systemic inflammation as well as increasing the survival of mice injected with lethal doses of E. coli bacteria.[23][35][36] Another set of newly described n-3 DPA resolvins, RvD1n-3, RvD2n-3, and RvD5n-3, have been named based on their presumed structural analogies to the DHS-derived resolvins RvD1, RvD2, and RvD5, respectively. These three n-3 DPA-derived resolvins have not been defined with respect to the chirality of their hydroxyl residues or the Cis–trans isomerism of their double bonds but do possess potent anti-inflammatory activity in animal models and human cells; they also have protective actions in increasing the survival of mice subjected to E. coli sepsis.[36] The following table lists the structural formulae (DPA stands for docosapentaenoic acid), major activities, cellular receptor targets (where known), and Wikipedia pages giving further information on the activity and syntheses.

Trivial name Formula Activities Receptor(s) See Wikipedia pages
RvT1 7,13R,20-trihydroxy-8E,10Z,14E,16Z,18E-DPA Anti-inflammatory[23][35] ? Resolvin#T series resolvins
RvT2 7,8,13R-trihydroxy-9E,11E,14E,16Z,19Z-DPA Anti-inflammatory[23][35] ? Resolvin#T series resolvins
RvT3 7,12,13R-trihydroxy-8Z,10E,14E,16Z,19Z-DPA Anti-inflammatory[23][35] ? Resolvin#T series resolvins
RvT4 7,13R-dihydroxy-8E,10Z,14E,16Z,19Z-DPA Anti-inflammatory[23][35] ? Resolvin#T series resolvins
RvD1n-3 7,8,17-trihydroxy-8,10,13,15,19-DPA Anti-inflammatory[36] ? Resolvin#Resolvin Dn-3DPA
RvD2n-3 7,16,17-trihydroxy-8,10,12,14,19-DPA Anti-inflammatory[36] ? Resolvin#Resolvin Dn-3DPA
RvD5n-3 7,17-dihydroxy-8,10,13,15,19-DPA Anti-inflammatory[36] ? Resolvin#Resolvin Dn-3DPA

Protectins/neuroprotectins

DHA-derived protectins/neuroprotectins

Cells metabolize DHA by either ALOX15, by a bacterial or mammalian cytochrome P450 monooxygenase (Cyp1a1, Cyp1a2, or Cyp1b1 in mice; see CYP450#CYP families in humans and CYP450#animals) or by aspirin-treated cyclooxygenase-2 to 17S-hydroperoxy or 17R-hydroperoxy intermediates (see previous subsection); this intermediate is then converted to a 16S,17S-epoxide which is then hydrolyzed (probably by a soluble epoxide hydrolase to protectin D1 (PD1, also termed neuroprotectin D1 [NPD1] when formed in neural tissue).[2] PDX is formed by the metabolism of DHA by two serial lipoxygenases, probably a 15-lipoxygenase and ALOX12. 22-Hydroxy-PD1 (also termed 22-hydroxy-NPD1) is formed by the Omega oxidation of PD1 probably by an unidentified cytochrome P450 enzyme. While omega-oxidation products of most bioactive PUFA metabolites are far weaker than their precursors, 22-hydroxy-PD1 is as potent as PD1 in inflammatory assays. Aspirin-triggered-PD1 (AT-PD1 or AP-NPD1) is the 17R-hydroxyl diastereomer of PD1 formed by the initial metabolism of DHA by aspirin-treated COX-2 or possibly a cytochrome P450 enzyme to 17R-hydroxy-DHA and its subsequent metabolism possibly in manner similar to that which forms PD1. 10-Epi-PD1 (ent-AT-NPD1), the 10S-hydroxy diastereomer of PD1, has been detected in small amounts in human neutrophils. While its in vivo synthetic pathway has not been defined, 10-epi-PD1 has anti-inflammatory activity.[23][37] The following table lists the structural formulae (DHA stands for docosahexaenoic acid), major activities, cellular receptor targets (where known), and Wikipedia pages giving further information on the activity and syntheses.

Trivial name Formula Activities Receptor(s) See Wikipedia pages
PD1 (NPD1) 10R,17S-dihydroxy-4Z,7Z,11E,13E,15Z,19Z-DHA anti-inflammatory, nerve protection/regeneration, blocks pain perception[38] inhibits the activation of TRPV1[15] Neuroprotectin D1
PDX 10S,17S-dihydroxy-4Z,7Z,11E,13Z,15E,19Z-DHA anti-inflammatory, inhibits platelet activation[39] ? Neuroprotectin D1#Protectin DX and Dihydroxy-E,Z,E-PUFA
22-hydroxy-PD1 10R,17S,22-trihydroxy-4Z,7Z,11E,13E,15Z,19Z-DHA anti-inflammatory[38] ? Neuroprotectin D1#Protectin DX and Dihydroxy-E,Z,E-PUFA
17-epi-PD1 (AT-PD1) 10R,17R-dihydroxy-4Z,7Z,11E,13E,15Z,19Z-DHA anti-inflammatory[12] ? Neuroprotectin D1#Aspirin-triggered PD1
10-epi-PD1 (ent-AT-NPD1) 10S,17S-Dihydroxy-4Z,7Z,11E,13E,15Z,19Z-DHA anti-inflammatory[38] ? Neuroprotectin D1#10-epi-PD1

n-3 DPA-derived protectins/neuroprotectins

n-3 DPA-derived protectins with structural similarities to PD1 and PD2 have been described, determined to be formed in vitro and in animal models, and termed PD1n-3 and PD2n-3, respectively. These products are presumed to be formed in mammals by the metabolism of n-3 DPA by an unidentified 15-lipoxygenase activity to 16,17-epoxide intermediate and the subsequent conversion of this intermediate to the di-hydroxyl products PD1n-3 and PD2n-3. PD1n-3 has anti-inflammatory activity in a mouse model of peritonitis; PD2n-3 has anti-inflammatory activity in an in vitro model.[36][41] The following table lists the structural formulae (DPA stands for docosapentaenoic acid), major activities, cellular receptor targets (where known), and Wikipedia pages giving further information on the activity and syntheses.

Trivial name Formula Activities Receptor(s) See Wikipedia pages
PD1n-3 10,17-dihydroxy-7,11,13,15,19-DPA ant-inflammatory[36] ? -
PD2n-3 16,17-dihydroxy-7,10,12,14,19-DPA anti-inflammatory[41] ? -

Maresins

DHA-derived Maresins

Cells metabolize DHA by ALOX12, other lipoxygenase, (12/15-lipoxygenase in mice), or an unidentified pathway to a 13S,14S-epoxide-4Z,7Z,9E,11E,16Z,19Z-DHA intermediate (13S,14S-epoxy-marisin MaR) and then hydrolyze this intermediate by an epoxide hydrolase activity (which ALOX 12 and mouse 12/15-lipoxygenase possess) to MaR1 and MaR2. During this metabolism, cells also form 7-epi-Mar1, i.e. the 7S-12E isomer of Mar1, as well as the 14S-hydroxy and 14R-hydroxy metabolites of DHA. The latter hydroxy metabolites can be converted by an unidentified cytochrome P450 enzyme to maresin like-1 (Mar-L1) and Mar-L2 by omega oxidation; alternatively, DHA may be first metabolized to 22-hydroxy-DHA by CYP1A2, CYP2C8, CYP2C9, CYP2D6, CYP2E1, or CYP3A4 and then metabolized through the cited epoxide-forming pathways to Mar-L1 and MaR-L2. Studies have found that these metabolites have potent anti-inflammatory activity in vitro and in animal models.[12][22][23] The following table lists the structural formulae (DHA stands for docosahexaenoic acid), major activities, cellular receptor targets (where known), and Wikipedia pages giving further information on the activity and syntheses.

Trivial name Formula Activities Receptor(s) See Wikipedia pages
MaR1 7R,14S-dihydroxy-4Z,8E,10E,12Z,16Z,19Z-DHA anti-inflammatory, tissue regeneration, blocks pain perception[12] Inhibits the activation of the vanilloid receptor TRPV1 and TRPA1[15][22] Maresin
MaR2 13R,14S-dihydroxy-4Z,7Z,9E,11E,16Z,19Z-DHA anti-inflammatory[12] ? Maresin
7-epi-MaR1 7S,14S-dihydroxy-4Z,8E,10Z,12E,16Z,19Z-DHA anti-inflammatory[38] ? Maresin
MaR-L1 14S,22-dihydroxy-4Z,7Z,10Z,12E,16Z,19Z-DHA anti-inflammatory[38][42] ? -
MaR-L2 14R,22-dihydroxy-4Z,7Z,10Z,12E,16Z,19Z-DHA anti-inflammatory[38][42] ? -

n-3 DPA-derived maresins

n-3 DPA-derived maresins are presumed to be formed in mammals by metabolism of n-3 DPA by an undefined 12-lipoxygenase activity to a 14-hydroperoxy-DPA intermediated and the subsequent conversion of this intermediate to di-hydroxyl products which have been termed MaR1n-3, MaR2n-3, and MaR3n-3 based on their structural analogies to MaR1, MaR2, and MaR3, respectively. MaR1n-3 and MaRn-3 have been found to possess anti-inflammatory activity in in vitro assays of human neutrophil function. These n-3 DPA-derived maresins have not been defined with respect to the chirality of their hydroxyl residues or the cis–trans isomerism of their double bonds.[36] The following table lists the structural formulae (DPA stands for docosapentaenoic acid), major activities, cellular receptor targets (where known), and Wikipedia pages giving further information on the activity and syntheses.

Trivial name Formula Activities Receptor(s) See Wikipedia pages
MaR1n-3 7S,14S-dihydroxy-8E,10E,12Z,16Z,19Z-DPA anti-inflammatory[36][38] ? -
MaR2n-3 13,14-dihydroxy-7,9,111,16,19-DPA anti-inflammatory[36] ? -
MaR3n-3 13,14-dihydroxy-7,9,111,16,19-DPA ? ? -

Other PUFA metabolites with SPM-like activity

The following PUFA metabolites, while not yet formally classified as SPM, have been recently described and determined to have anti-inflammatory activity.

n-3 DPA metabolites

10R,17S-dihydroxy-7Z,11E,13E,15Z,19Z-docosapentaenoic acid (10R,17S-diHDPAEEZ) has been found in inflamed exudates of animal models and possesses in vitro and in vivo anti-inflammatory activity almost as potently as PD1.[38]

n-6-DPA metabolites

n-6 DPA (i.e. 4Z,7Z,10Z,13Z,16Z-docosapentaenoic acid or osbond acid) is an isomer of n-3 DPA (clupanodonic acid) differing form the latter fatty acid only in the location of its 5 double bonds. Cells metabolize n-6 DPA to 7-hydroxy-DPAn-6, 10,17-dihydroxy-DPAn-6, and 7,17-dihydroxy-DPAn-3; the former two metabolites have been shown to possess anti-inflammatory activity in in vitro and in animal model studies.[36]

oxo-DHA and oxo-DPA metabolites

Cells metabolize DHA and n-3 DPA by COX2 to 13-hydroxy-DHA and 13-hydroxy-DPAn-3 products and by aspirin-treated COX2 to 17-hydroxy-DHA and 17-hydroxy-DPAn-3 products and may then oxidize these products to there corresponding oxo (i.e. ketone) derivatives, 13-oxo-DHA (also termed electrophilic fatty acid oxo derivative or EFOX-D6), 13-oxo-DPAn-3 (EFOX-D5), 17-oxo-DHA (17-EFOX-D6), and 17-oxo-DPAn-3 (17-EFOX-D3). These oxo metabolites directly activate the nuclear receptor Peroxisome proliferator-activated receptor gamma and possess anti-inflammatory activity as assesses in in vitro systems.[36]

Docosahexaenoyl ethanolamide metabolites

DHA ethanolamide ester (the DHA analog of arachindonyl ethanolamide [i.e. Anandamide]) is metabolized to 10,17-dihydroxydocosahexaenoyl ethanolamide (10,17-diHDHEA) and/or 15-hydroxy-16(17)-epoxy-docosapentaenoyl ethanolamide (15-HEDPEA) by mouse brain tissue and human neutrophils. Both compounds possess anti-inflammatory activity in vitro; 15-HEDPEA also has tissue-protective effects in mouse models of lung injury and tissue reperfusion. Like anandamide, both compounds activated the Cannabinoid receptor.[44][45]

Prostaglandins and Isoprostanes

PUFA derivatives containing a Cyclopentenone structure are chemically reactive and can form adducts with various tissue targets, particularly proteins. Certain of these PUFA-cyclopentenones bind to the sulfur residues in the KEAP1 component of the KEAP1-NFE2L2 protein complex in the cytosol of cells. This negates KEAP1's ability to bind NFE2L2; in consequence, NFE2L2 becomes free to translocate to the nuclease and stimulate the transcription of genes that encode proteins active in detoxifying reactive oxygen species; this effect tends to reduce inflammatory reactions. PUFA-cyclopentenones may likewise react with the IKK2 component of the cytosolic IKK2-NFκB protein complex thereby inhibiting NFκB from stimulating the transcription of genes that encode various pro-inflammatory proteins. One or both of these mechanisms appears to contribute to the ability of certain highly reactive PUFA-cyclopenetenones to exhibit SPM activity. The PUFA-cyclopentenones include two prostaglandins, (PG) Δ12-PGJ2 and 15-deoxy-Δ12,14-PGJ2, and two isoprostanes, 5,6-epoxyisoprostane E2 and 5,6-epoxyisoprostane A2. Both PGJ2's are arachidonic acid-derived metabolites made by cyclooxygenases, primarily COX-2, which is induced in many cell types during inflammation. Both isoprostanes form non-enzymatically as a result the attack on the arachidonic acid bond to cellular phospholipids by reactive oxygen species; they are then release from the phospholipids to become free in attacking their target proteins. All four products have been shown to form and possess SPM activity in various in vitro studies of human and animal tissue as well as in in vivo studies of animal models of inflammation; they have been termed pro-resolving mediators of inflammation[46]

Gene manipulation studies

Mice made deficient in their 12/15-lipoxygenase gene (Alox15) exhibit a prolonged inflammatory response along with various other aspects of a pathologically enhanced inflammatory response in experimental models of cornea injury, airway inflammation, and peritonitis. These mice also show an accelerated rate of progression of atherosclerosis whereas mice made to overexpress 12/15-lipoxygenase exhibit a delayed rate of atherosclerosis development. Alox15 overexpressing rabbits exhibited reduced tissue destruction and bone loss in a model of periodontitis.[2] Similarly, Alox5 deficient mice exhibit a worsened inflammatory component, failure to resolve, and/or decrease in survival in experimental models of respiratory syncytial virus disease, Lyme disease, Toxoplasma gondii disease, and corneal injury.[2] These studies indicate that the suppression of inflammation is a major function of 12/15-lipoxygenase and Alox5 along with the SPMs they make in at least certain rodent experimental inflammation models; although these rodent lipoxygenases differ from human ALOX15 and ALOX5 in the profile of the PUFA metabolites that they make as well as various other parameters (e.g. tissue distribution), these genetic studies allow that human ALOX15, ALOX5, and the SPMs they make may play a similar anti-inflammatory functions in humans.

Concurrent knockout of the three members of the CYP1 family of Cytochrome P450 enzymes in mice, i.e. Cyp1a1, Cyp1a2, and Cyp1b1, caused an increase in the recruitment of neutrophils to the peritoneum in mice undergoing experimental peritonitis; these triple knockout mice also exhibited an increase in the peritoneal fluid LTB4 level and decreases in the levels of peritoneal fluid NPD1 as well as the precursors to various SPMS including 5-hydroxyeicosatetraenoic acid, 15-Hydroxyeicosatetraenoic acid, 18-hydroxyeicosapentaenoic acid, 17-hydroxydocosahexaenoic acid, and 14-hydroxydocosahexaenoic. These results support the notion that Cyp1 enzymes contribute to the production of certain SPMs and inflammatory responses in mice; CYP1 enzymes may therefore play a similar role in humans.[47]

Clinical studies

In a randomized controlled trial, AT-LXA4 and a comparatively stable analog of LXB4, 15R/S-methyl-LXB4, reduced the severity of eczema in a study of 60 infants.[48][49] A synthetic analog of ReV1 is in clinical phase III testing (see Phases of clinical research) for the treatment of the inflammation-based dry eyesyndrome; along with this study, other clinical trials (NCT01639846, NCT01675570, NCT00799552 and NCT02329743) using an RvE1 analogue to treat various ocular conditions are underway.[14] RvE1, Mar1, and NPD1 are in clinical development studies for the treatment of neurodegenerative diseases and hearing loss.[2] And, in a single study, inhaled LXA4 decreased LTC4-initiated bronchoprovocation in patients with asthma.[14]

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