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Arachidonate 5-lipoxygenase

January 01, 1970

Arachidonate 5-lipoxygenase, also known as ALOX5, 5-lipoxygenase, 5-LOX, or 5-LO, is a non-heme iron-containing enzyme (EC 1.13.11.34) that in humans is encoded by the ALOX5 gene.[1] Arachidonate 5-lipoxygenase is a member of the lipoxygenase family of enzymes. It transforms essential fatty acids (EFA) substrates into leukotrienes as well as a wide range of other biologically active products. ALOX5 is a current target for pharmaceutical intervention in a number of diseases.

arachidonate 5-lipoxygenase
Identifiers
Aliases5-lipoxygenase
External IDsGeneCards: [1]
Orthologs
SpeciesHumanMouse
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arachidonate 5-lipoxygenase
Identifiers
EC no.1.13.11.34
CAS no.80619-02-9[permanent dead link]
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IntEnzIntEnz view
BRENDABRENDA entry
ExPASyNiceZyme view
KEGGKEGG entry
MetaCycmetabolic pathway
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PDB structuresRCSB PDB PDBe PDBsum
Gene OntologyAmiGO / QuickGO
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Gene edit

The ALOX5 gene, which occupies 71.9 kilobase pairs (kb) on chromosome 10 (all other human lipoxygenases are clustered together on chromosome 17), is composed of 14 exons divided by 13 introns encoding the mature 78 kilodalton (kDa) ALOX5 protein consisting of 673 amino acids. The gene promoter region of ALOX5 contains 8 GC boxes but lacks TATA boxes or CAT boxes and thus resembles the gene promoters of typical housekeeping genes. Five of the 8 GC boxes are arranged in tandem and are recognized by the transcription factors Sp1 and Egr-1. A novel Sp1-binding site occurs close to the major transcription start site (position – 65); a GC-rich core region including the Sp1/Egr-1 sites may be critical for basal 5-LO promoter activity.[2]

Expression edit

Cells primarily involved in regulating inflammation, allergy, and other immune responses, e.g. neutrophils, eosinophils, basophils, monocytes, macrophages, mast cells, dendritic cells, and B-lymphocytes express ALOX5. Platelets, T cells, and erythrocytes are ALOX5-negative. In skin, Langerhans cells strongly express ALOX5. Fibroblasts, smooth muscle cells and endothelial cells express low levels of ALOX5.[2][3] Up-regulation of ALOX5 may occur during the maturation of leukocytes and in human neutrophils treated with granulocyte macrophage colony-stimulating factor and then stimulated with physiological agents.

Aberrant expression of LOX5 is seen in various types of human cancer tumors in vivo as well as in various types of human cancer cell lines in vitro; these tumors and cell lines include those of the pancreas, prostate and colon. ALOX5 products, particularly 5-hydroxyeicosatetraenoic acid and 5-oxo-eicosatetraenoic acid, promote the proliferation of these ALOX5 aberrantly expressing tumor cell lines suggesting that ALOX5 acts as a pro-malignancy factor for them and by extension their parent tumors.[2]

Studies with cultured human cells have found that there are a large number of ALOX5 mRNA splice variants due to alternative splicing. The physiological and/or pathological consequences of this slicing has yet to be defined. In one study, however, human brain tumors were shown to express three mRNA splice variants (2.7, 3.1, and 6.4 kb) in addition to the full 8.6 lb species; the abundance of the variants correlated with the malignancy of these tumors suggesting that they may play a role in the development of these tumors.[2]

Biochemistry edit

Human ALOX5 is a soluble, monomeric protein consisting of 673 amino acids with a molecular weight of ~78 kDa. Structurally, ALOX5 possesses:[3][4]

  • A C-terminal catalytic domain (residues 126–673)
  • An N-terminal C2-like domain which promotes its binding to ligand substrates, Ca2+, cellular phospholipid membranes, Coactin-like protein (COL1), and Dicer protein
  • A PLAT domain within its C2-like domain; this domain, by analogy to other PLAT domain-bearing proteins, may serve as a mobile lid over ALOX5's substrate-binding site
  • An adenosine triphosphate (ATP) binding site; ATP is crucial for ALOX5's metabolic activity
  • A proline-rich region (residues 566–577), sometimes termed a SH3-binding domain, which promotes its binding to proteins with SH3 domains such as Grb2 and may thereby link the enzyme's regulation to tyrosine kinase receptors.

The enzyme possesses two catalytic activities as illustrated by its metabolism of arachidonic acid. ALOX5's dioxygenase activity adds a hydroperoxyl (i.e. HO2) residue to arachidonic acid (i.e. 5Z,8Z,11Z,14Z-eicosatetraenoic acid) at carbon 5 of its 1,4 diene group (i.e. its 5Z,8Z double bonds) to form 5(S)-hydroperoxy-6E,8Z,11Z,14Z-eicosatetraenoic acid (i.e. 5S-HpETE).[5] The 5S-HpETE intermediate may then be released by the enzyme and rapidly reduced by cellular glutathione peroxidases to its corresponding alcohol, 5(S)-hydroxy-6E,8Z,11Z,14Z-eicosatetraenoic acid (i.e. 5-HETE), or, alternatively, further metabolized by ALOX5's epoxidase (also termed LTA4 synthase) activity which converts 5S-HpETE to its epoxide, 5S,6S-hydroxy-6E,8Z,11Z,14Z-eicosatetraenoic acid (i.e. LTA4).[6] LTA4 is then acted on by a separate, soluble enzyme, leukotriene-A4 hydrolase, to form the dihydroxyl product, leukotriene B4 (LTB4, i.e. 5S,12R-dihydroxy-5S,6Z,8E,10E,12R,14Z-eicosatetraenoic acid) or by either LTC4 synthase or microsomal glutathione S-transferase 2 (MGST2), which bind the sulfur of cysteine's thio (i.e. SH) residue in the tripeptide glutamate-cysteine-glycine to carbon 6 of LTA4 thereby forming LTC4 (i.e. 5S-hydroxy,6R-(S-glutathionyl)-7E,9E,11Z,14Z-eicosatetraenoic acid). The Glu and Gly residues of LTC4 may be removed step-wise by gamma-glutamyltransferase and a dipeptidase to form sequentially LTD4 and LTE4.[4][7] To varying extents, the other PUFA substrates of ALOX5 follow similar metabolic pathways to form analogous products.

Sub-human mammalian Alox5 enzymes like those in rodents appear to have, at least in general, similar structures, distributions, activities, and functions as human ALOX5. Hence, model Alox5 studies in rodents appear to be valuable for defining the function of ALOX5 in humans (see Lipoxygenase § Mouse lipoxygenases).

Regulation edit

ALOX5 exists primarily in the cytoplasm and nucleoplasm of cells. Upon cell stimulation, ALOX5: a) may be phosphorylated on serine 663, 523, and/or 271 by mitogen-activated protein kinases, S6 kinase, protein kinase A (PKA), protein kinase C, Cdc2, and/or a Ca2+/calmodulin-dependent protein kinase; b) moves to bind with phospholipids in the nuclear membrane and, probably, endoplasmic reticulum membrane; c) is able to accept substrate fatty acids presented to it by the 5-lipoxygenase-activating protein (FLAP) which is embedded in these membranes; and d) thereby becomes suited for high metabolic activity. These events, along with rises in cytosolic Ca2+ levels, which promote the translocation of ALOX5 form the cytoplasm and nucleoplasm to the cited membranes, are induced by cell stimulation such as that caused by chemotactic factors on leukocytes. Rises in cytosolic Ca2+, ALOX5's movement to membranes, and ALOX5's interaction with FLAP are critical to the physiological activation of the enzyme.[3] Serine 271 and 663 phosphorylations do not appear to alter ALOX5's activity. Serine 523 phosphorylation (which is conducted by PKA) totally inactivates the enzyme and prevents its nuclear localization; stimuli which cause cells to activate PKA can thereby block production of ALOX5 metabolites.[4][8]

In addition to its activation, ALOX5 must gain access to its polyunsaturated fatty acid (PUFA) substrates, which commonly are bound in an ester linkage to the sn2 position of membrane phospholipids, in order to form biologically active products. This is accomplished by a large family of phospholipase A2 (PLA2) enzymes. The cytosolic PLA2 set (i.e. cPLA2s) of PLA2 enzymes (see Phospholipase A2 § Cytosolic phospholipases A2 (cPLA2)) in particular mediates many instances of stimulus-induced release of PUFA in inflammatory cells. For example, chemotactic factors stimulate human neutrophils to raise cytosolic Ca2+ which triggers cPLA2s, particularly the α isoform (cPLA2α), to move from its normal residence in the cytosol to cellular membranes. This chemotactic factor stimulation concurrently causes the activation of mitogen-activated protein kinases (MAPK) which in turn stimulates the activity of cPLA2α by phosphorylating it on ser-505 (other cell types may activate this or other cPLA2 isoforms using other kinases which phosphorylate them on different serine residues). These two events allow cPLA2s to release PUFA esterified to membrane phospholipids to FLAP which then presents them to ALOX5 for their metabolism.[9][10]

Other factors are known to regulate ALOX5 activity in vitro but have not been fully integrated into its physiological activation during cell stimulation. ALOX5 binds with the F actin-binding protein, coactin-like protein. Based on in vitro studies, this protein binding serves to stabilize ALOX5 by acting as a chaperone (protein) or scaffold, thereby averting the enzyme's inactivation to promote its metabolic activity; depending on circumstance such as the presence of phospholipids and levels of ambient Ca2+, this binding also alters the relative levels of hydroperoxy versus epoxide (see arachidonic acid section below) products made by ALOX5.[3][4] The binding of ALOX5 to membranes as well as its interaction with FLAP likewise cause the enzyme to alter its relative levels of hydroperoxy versus epoxide production, in these cases favoring the production of the epoxide products.[4] The presence of certain diacylglycerols such as 1-oleoyl-2-acetyl-sn-glycerol, 1-hexadecyl-2-acetyl-sn-glycerol, and 1-O-hexadecyl-2-acetyl-sn-glycerol, and 1,2-dioctanoyl-sn-glycerol but not 1-stearoyl-2-arachidonyl-sn-glycerol increase the catalytic activity of ALOX5 in vitro.[4]

Substrates, metabolites, and metabolite activities edit

ALOX5 metabolizes various omega-3 and omega-6 PUFA to a wide range of products with varying and sometimes opposing biological activities. A list of these substrates along with their principal metabolites and metabolite activities follows.  

Arachidonic acid edit

ALOX5 metabolizes the omega-6 fatty acid, arachidonic acid (AA, i.e. 5Z,8Z,11Z,14Z-eicosatetraenoic acid), to 5-hydroperoxyeicosatetraenoic acid (5-HpETE) which is then rapidly converted to physiologically and pathologically important products. Ubiquitous cellular glutathione peroxidases (GPXs) reduce 5-HpETE to 5-hydroxyeicosatetraenoic acid (5-HETE); 5-HETE may be further metabolized by 5-hydroxyeicosanoid dehydrogenase (5-HEDH) to 5-oxo-eicosatetraenoic acid (5-oxo-ETE). Alternatively, the intrinsic activity of ALOX5 may convert 5-HpETE to its 5,6 epoxide, leukotriene A4 LTA4, which is then either rapidly converted to leukotriene B4 (LTB4) by leukotriene-A4 hydrolase (LTA4H) or to leukotriene C4 (LTC4) by LTC4 synthase (LTC4S); LTC4 exits its cells of origin through the MRP1 transporter (ABCC1) and is rapidly converted to LTD4 and then to LTE4) by cell surface-attached gamma-glutamyltransferase and dipeptidase peptidase enzymes. In another pathway, ALOX5 may act in series with a second lipoxygenase enzyme, ALOX15, to metabolize AA to lipoxin A4 (LxA4) and LxB4 (see Specialized pro-resolving mediators § Lipoxins).[3][11][12][13] GPXs, 5-HEDH, LTA4H, LTC4S, ABCC1, and cell surface peptidases may act similarly on the ALOX5-derived metabolites of other PUFA.

LTB4, 5-HETE, and 5-oxo-ETE may contribute to the innate immune response as leukocyte chemotactic factors, i.e. they recruit and further activate circulating blood neutrophils and monocytes to sites of microbial invasion, tissue injury, and foreign bodies. When produced in excess, however, they may contribute to a wide range of pathological inflammatory responses (5-HETE and LTB4). 5-Oxo-ETE is a particularly potent chemotactic factor for and activator of eosinophils and may thereby contribute to eosinophil-based allergic reactions and diseases.[4][14] These metabolites may also contribute to the progression of certain cancers such as those of the prostate, breast, lung, ovary, and pancreas. ALOX5 may be overexpressed in some of these cancers; 5-Oxo-ETE and to a lesser extent 5-HETE stimulate human cell lines derived from these cancers to proliferate; and the pharmacological inhibition of ALOX5 in these human cell lines causes them to die by entering apoptosis.[14][15][16][17][18] ALOX5 and its LTB4 metabolite as well as this metabolite's BLT1 and BLT2 receptors have also been shown to promote the growth of various types of human cancer cell lines in culture.[19][20]

LTC4, LTD4, and LTE4 contribute to allergic airways reactions such as asthma, certain non-allergic hypersensitivity airways reactions, and other lung diseases involving bronchoconstriction by contracting these airways and promoting in these airways inflammation, micro-vascular permeability, and mucus secretion; they likewise contribute to various allergic and non-allergic reactions involving rhinitis, conjunctivitis, and urticaria.[3] Certain of these peptide-leukotrienes have been shown to promote the growth of cultured human breast cancer and chronic lymphocytic leukemia cell lines thereby suggesting that ALOX5 may contribute to the progression of these diseases.[19]

LxA4 and LxB4 are members of the specialized pro-resolving mediators class of polyunsaturated fatty acid metabolites. They form later than the ALOX5-derived chemotactic factors in the inflammatory response and are thought to limit or resolve these responses by, for example, inhibiting the entry of circulating leukocytes into inflamed tissues, inhibiting the pro-inflammatory action of the leukocytes, promoting leukocytes to exit from inflammatory sites, and stimulating leukocyte apoptosis (see Specialized pro-resolving mediators and Lipoxin).[11]

Mead acid edit

Mead acid (i.e. 5Z,8Z,11Z-eicosatrienoic acid) is identical to AA except that has a single rather than double bond between its 14 and 15 carbon. ALOX5 metabolizes mead acid to 3-series (i.e. containing 3 double bonds) analogs of its 4-series AA metabolites viz., 5(S)-hydroxy-6E,8Z,11Z-eicosatrienoic acid (5-HETrE), 5-oxo-6,8,11-eicosatrienoic acid (5-oxo-ETrE), LTA3, and LTC3; since LTA3 inhibits LTA hydrolase, mead acid metabolizing cells produce relatively little LTB3 and are blocked from metabolizing arachidonic acid to LTB4. On the other hand, 5-oxo-ETrE is almost as potent as 5-oxo-ETE as an eosinophil chemotactic factor and may thereby contribute to the development of physiological and pathological allergic responses.[12] Presumably, the same metabolic pathways that follow ALOX5 in metabolizing arachidonic acid to the 4-series metabolites likewise act on mead acid to form these products.

Eicosapentaenoic acid edit

ALOX5 metabolizes the omega-3 fatty acid, eicosapentaenoic acid (EPA, i.e. 4Z,8Z,11Z,14Z,17Z-eiosapentaenoic acid), to 5-hydroperoxy-eicosapentaenoic acid which is then converted to 5-series products that are structurally analogous to their arachidonic acid counterparts viz., 5-hydroxy-eicosapentaenoic acid (5-HEPE), 5-oxo-eiocosapentaenoic acid (5-oxo-HEPE), LTB5, LTC5, LTD5, and LTE5.[4][21] Presumably, the same metabolic pathways that follow ALOX5 in metabolizing arachidonic acid to the 4-series metabolites likewise act on EPA to form these 5-series products. ALOX5 also cooperates with other lipoxygenase, cyclooxygenase, or cytochrome P450 enzymes in serial metabolic pathways to metabolize EPA to resolvins of the E series (see Specialized pro-resolving mediators § EPA-derived resolvins for further details on this metabolism) viz., resolvin E1 (RvE1) and RvE2.[22][23]

5-HEPE, 5-oxo-HEPE, LTB5, LTC5, LTD5, and LTE5 are generally less potent in stimulating cells and tissues than their arachidonic acid-derived counterparts; since their production is associated with reduced production of their arachidonic acid-derived counterparts, they may indirectly serve to reduce the pro-inflammatory and pro-allergic activities of their arachidonic acid-derived counterparts.[4][21] RvE1 and ReV2 are specialized pro-resolving mediators that contribute to the resolution of inflammation and other reactions.[23]

Docosahexaenoic acid edit

ALOX5 acts in series with ALOX15 to metabolize the omega 3 fatty acid, docosahexaenoic acid (DHA, i.e. 4Z,7Z,10Z,13Z,16Z,19Z-docosahexaenoic acid), to D series resolvins (see Specialized pro-resolving mediators § DHA-derived resolvins for further details on this metabolism).[23][24]

The D series resolvins (i.e. RvD1, RvD2, RvD3, RvD4, RvD5, RvD6, AT-RVD1, AT-RVD2, AT-RVD3, AT-RVD4, AT-RVD5, and AT-RVD6) are specialized pro-resolving mediators that contribute to the resolution of inflammation, promote tissue healing, and reduce the perception of inflammation-based pain.[23][24]

Transgenic studies edit

Studies in model animal systems that delete or overexpress the Alox5 gene have given seemingly paradoxical results. In mice, for example, Alox5 overexpression may decrease the damage caused by some types yet increase the damage caused by other types of invasive pathogens. This may be a reflection of the array of metabolites made by the Alox5 enzyme some of which possess opposing activities like the pro-inflammatory chemotactic factors and the anti-inflammatory specialized pro-resolving mediators. Alox5 and presumably human ALOX5 functions may vary widely depending on: the agents stimulating their activity; the types of metabolites that they form; the specific tissues responding to these metabolites; the times (e.g. early versus delayed) at which observations are made; and very likely various other factors.

Alox5 gene knockout mice are more susceptible to the development and pathological complications of experimental infection with Klebsiella pneumoniae, Borrelia burgdorferi, and Paracoccidioides brasiliensis.[8][25] In a model of cecum perforation-induced sepsis, ALOX5 gene knockout mice exhibited a decrease in the number of neutrophils and an increase in the number of bacteria that accumulated in their peritoneum.[26] On the other hand, ALOX5 gene knockout mice demonstrate an enhanced resistance and lessened pathology to Brucella abortus infection[27] and, at least in its acute phase, Trypanosoma cruzi infection.[28] Furthermore, Alox5-null mice exhibit a worsened inflammatory component, failure to resolve inflammation-related responses, and decreased survival in experimental models of respiratory syncytial virus disease, Lyme disease, Toxoplasma gondii disease, and corneal injury. These studies indicate that Alox5 can serve a protective function presumably by generating metabolites such as chemotactic factors that mobilize the innate immunity system. However, the suppression of inflammation appears also to be a function of Alox5, presumably by contributing to the production of anti-inflammatory specialized pro-resolving mediators (SPMs), at least in certain rodent inflammation-based model systems. These genetic studies allow that ALOX5 along with the chemotactic factors and SPMs that they contribute to making may play similar opposing pro-inflammatory and anti-inflammatory functions in humans.[22][29]

Alox5 gene knockout mice exhibit an increase in the lung tumor volume and liver metastasis of Lewis lung carcinoma cells that were directly implanted into their lungs; this result differs from many in vitro studies which implicated human ALOX5 along with certain of its metabolites with promoting cancer cell growth in that it finds that mouse Alox5 and, perhaps, certain of its metabolites inhibit cancer cell growth. Studies in this model suggest that Alox5, acting through one or more of its metabolites, reduces growth and progression of the Lewis carcinoma by recruiting cancer-inhibiting CD4+ T helper cells and CD8+ T cytotoxic T cells to the sites of implantation.[30] This striking difference between human in vitro and mouse in vivo studies may reflect species differences, in vitro versus in vivo differences, or cancer cell type differences in the function of ALOX5/Alox5.

Clinical significance edit

Inflammation edit

Studies implicate ALOX5 in contributing to innate immunity by contributing to the mounting inflammatory responses to a wide range of diseases:

however, ALOX5 also contributes to the development and progression of excessive and chronic inflammatory responses such as:

(see Inflammation § Disorders).

These dual functions probably reflect ALOX5's ability to form the: a) potent chemotactic factor, LTB4, and possibly also weaker chemotactic factor, 5S-HETE, which serve to attract and otherwise activate inflammation-inducing cells such as circulating leukocytes and tissue macrophages and dendritic cells and b) lipoxin and resolvin subfamily of SPMs which tend to inhibit these cells as well as the overall inflammatory responses.[8][31][32]

Allergy edit

ALOX5 contributes to the development and progression of allergy and allergic inflammation reactions and diseases such as:

This activity reflects its formation of a) LTC4, LTD4, and LTE4 which promote vascular permeability, contract airways smooth muscle, and otherwise perturb these tissues and b) LTB4 and possibly 5-oxo-ETE which are chemotactic factors for, and activators of, the cell type promoting such reactions, the eosinophil.[8][14] 5-Oxo-ETE and, to a lesser extent, 5S-HETE, also act synergistically with another pro-allergic mediator, platelet-activating factor, to stimulate and otherwise activate eosinophils.[14][33][34][35]

Hypersensitivity reactions edit

ALOX5 contributes to non-allergic NSAID hypersensitivity reactions of the respiratory system and skin such as:

It may also contribute to hypersensitivity responses of the respiratory system to cold air and possibly even alcohol beverages. These pathological responses likely involve the same ALOX5-formed metabolites as those promoting allergic reactions.[13][8][36]

ALOX5-inhibiting drugs edit

Main article: Arachidonate 5-lipoxygenase inhibitor

The tissue, animal model, and animal and human genetic studies cited above implicate ALOX5 in a wide range of diseases:

(see Inflammation § Disorders)

However, clinical use of drugs that inhibit ALOX5 to treat any of these diseases has been successful with only Zileuton along with its controlled released preparation, Zileuton CR.

Zileuton is approved in the US for the prophylaxis and chronic treatment of allergic asthma; it is also used to treat chronic non-allergic reactions such as NSAID-induced non-allergic lung, nose, and conjunctiva reactions as well as exercise-induced asthma. Zileuton has shown some beneficial effects in clinical trials for the treatment of rheumatoid arthritis, inflammatory bowel disease, and psoriasis.[8][37] Zileuton is currently undergoing a phase II study for the treatment of acne vulgaris (mild-to-moderate inflammatory facial acne) and a phase I study (see Clinical trial § Phases) combining it with imatinib for treating chronic myeloid leukemia.[38][39] Zyleuton and zileuton CR cause elevations in liver enzymes in 2% of patients; the two drugs are therefore contraindicated in patients with active liver disease or persistent hepatic enzyme elevations greater than three times the upper limit of normal. Hepatic function should be assessed prior to initiating either of these drugs, monthly for the first 3 months, every 2–3 months for the remainder of the first year, and periodically thereafter; zileuton also has a rather unfavorable pharmacological profile (see Zileuton § Contraindications and warnings).[38] Given these deficiencies, other drugs targeting ALOX5 are under study.

Flavocoxid is a proprietary blend of purified plant derived bioflavonoids including Baicalin and Catechins. It inhibits COX-1, COX-2, and ALOX5 in vitro and in animal models. Flavocoxid has been approved for use as a medical food in the United States since 2004 and is available by prescription for use in chronic osteoarthritis in tablets of 500 mg under the commercial name Limbrel. However, in clinical trials serum liver enzyme elevations occurred in up to 10% of patients on flavocoxid therapy although elevations above 3 times the upper limit of normal occurred in only 1-2% of recipients. Since its release, however, there have been several reports of clinically apparent acute liver injury attributed to flavocoxid.[40]

Setileuton (MK-0633) has completed a Phase II clinical trial for the treatment of asthma, chronic obstructive lung disease, and atherosclerosis (NCT00404313, NCT00418613, and NCT00421278, respectively).[38][41] PF-4191834[42] has completed phase II studies for the treatment of asthma (NCT00723021).[38]

Hyperforin, an active constituent of the herb St John's wort, is active at micromolar concentrations in inhibiting ALOX5.[43] Indirubin-3'-monoxime, a derivative of the naturally occurring alkaloid, indirubin, is also described as selective ALOX5 inhibitor effective in a range of cell-free and cell-based model systems.[44] In addition, curcumin, a constituent of turmeric, is a 5-LO inhibitor as defined by in vitro studies of the enzyme.[45]

Acetyl-keto-beta-boswellic acid (AKBA), one of the bioactive boswellic acids found in Boswellia serrata (Indian Frankincense) has been found to inhibit 5-lipoxygenase. Boswellia reduces brain edema in patients irradiated for brain tumor and it's believed to be due to 5-lipoxygenase inhibition.[46][47]

While only one ALOX5-inhibiting drug has proven useful for treating human diseases, other drugs that act down-stream in the ALOX5-initiated pathway are in clinical use. Montelukast, Zafirlukast, and Pranlukast are receptor antagonists for the cysteinyl leukotriene receptor 1 which contributes to mediating the actions of LTC4, LTD4, and LTE4. These drugs are in common use as prophylaxis and chronic treatment of allergic and non-allergic asthma and rhinitis diseases[3] and also may be useful for treating acquired childhood sleep apnea due to adenotonsillar hypertrophy (see Acquired non-inflammatory myopathy § Diet and Trauma Induced Myopathy).[48]

To date, however, neither LTB4 synthesis inhibitors (i.e. blockers of ALOX5 or LTA4 hydrolase) nor inhibitors of LTB4 receptors (BLT1 and BLT2) have turned out to be effective anti-inflammatory drugs. Furthermore, blockers of LTC4, LTD4, and LTE4 synthesis (i.e. ALOX5 inhibitors) as well as of LTC4 and LTD4 receptor antagonists have proven inferior to corticosteroids as single drug therapy for persistent asthma, particularly in patients with airway obstruction. As a second drug added to corticosteroids, leukotriene inhibitors appear inferior to beta2-adrenergic agonist drugs in the treatment of asthma.[49]

Human genetics edit

ALOX5 contributes to the formation of PUFA metabolites that may promote (e.g. the leukotrienes, 5-oxo-ETE) but also to metabolites that inhibit (i.e. lipoxins, resolvins) diseases. Consequently, a given abnormality in the expression or activity of ALOX5 due to variations in its gene may promote or suppress inflammation depending on the relative roles these opposing metabolites have in regulating the particular type of reaction examined. Furthermore, the ALOX5-related tissue reactions studied to date are influenced by multiple genetic, environmental, and developmental variables that may influence the consequences of abnormalities in the expression or function of ALOX5. Consequently, abnormalities in the ALOX5 gene may vary with the population and individuals studied.

Allergic asthma edit

The upstream promoter in the human ALOX5 gene commonly possess five GGGCCGG repeats which bind the Sp1 transcription factor and thereby increase the gene's transcription of ALOX5. Homozygous variants for this five repeat promoter region in a study of 624 asthmatic children in Ankara, Turkey were much more likely to have severe asthma. These variants are associated with reduced levels of ALOX5 as well as reduced production of LTC4 in their eosinophils.[50] These data suggest that ALOX5 may contribute to dampening the severity of asthma, possibly by metabolizing PUFA to specialized pro-resolving mediators.[51] Single nucleotide polymorphism differences in the genes that promote ALOX5 activity (i.e. 5-lipoxygenase-activating protein), metabolize the initial product of ALOX5, 5S-HpETE, to LTB4 (i.e. leukotriene-A4 hydrolase), or are the cellular receptors responsible for mediating the cellular responses to the down-stream ALOX products LTC4 and LTD4 (i.e. CYSLTR1 and CYSLTR2) have been associated with the presence of asthma in single population studies. These studies suggest genetic variants may play a role, albeit a relatively minor one, in the overall susceptibility to allergic asthma.[50]

NSAID-induced non-allergic reactions edit

Aspirin and other non-steroidal anti-inflammatory drugs (NSAID) can cause NSAID-exacerbated diseases (N-ERD). These have been recently classified into 5 groups 3 of which are not caused by a classical immune mechanism and are relevant to the function of ALOX5: 1) NSAIDs-exacerbated respiratory disease (NERD), i.e. symptoms of bronchial airways obstruction, shortness of breath, and/or nasal congestion/rhinorrhea occurring shortly after NSAID ingestion in patients with a history of asthma and/or rhinosinusitis; 2) NSAIDs-exacerbated cutaneous disease (NECD), i.e. wheal responses and/or angioedema responses occurring shortly after NSAID ingestion in patients with a history of chronic urticaria; and 3) NSAIDs-induced urticaria/angioedema (NIUA) (i.e. wheals and/or angioedema symptoms occurring shortly after NSAID ingestion in patients with no history of chronic urticaria).[52] The genetic single-nucleotide polymorphism (SNP) variant in the ALOX5 gene, ALOX5-1708 G>A is associated with NSAID-induced asthma in Korean patients and three SNP ALOX5 variants, rs4948672,[53] rs1565096,[54] and rs7894352,[55] are associated with NSAID-induced cutaneous reactions in Spanish patients.[33]

Atherosclerosis edit

Bearers of two variations in the predominant five tandem repeat Sp1 binding motif (GGGCCGG) of the ALOX5 gene promoter in 470 subjects (non-Hispanic whites, 55.1%; Hispanics, 29.6%; Asian or Pacific Islander, 7.7&; African Americans, 5.3%, and others, 2.3%) were positively associated with the severity of atherosclerosis, as judged by carotid intima–media thickness measurements. Variant alleles involved deletions (one or two) or additions (one, two, or three) of Sp1 motifs to the five tandem motifs allele.[56]

See also edit

Arachidonate 5-lipoxygenase inhibitor

References edit

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  3. ^ a b c d e f g Anwar Y, Sabir JS, Qureshi MI, Saini KS (2014). "5-lipoxygenase: a promising drug target against inflammatory diseases-biochemical and pharmacological regulation". Current Drug Targets. 15 (4): 410–422. doi:10.2174/1389450114666131209110745. PMID 24313690.
  4. ^ a b c d e f g h i Rådmark O, Werz O, Steinhilber D, Samuelsson B (2015). "5-Lipoxygenase, a key enzyme for leukotriene biosynthesis in health and disease". Biochimica et Biophysica Acta (BBA) - Molecular and Cell Biology of Lipids. 1851 (4): 331–339. doi:10.1016/j.bbalip.2014.08.012. PMID 25152163.
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Further reading edit

  • Rådmark OP (2000). "The molecular biology and regulation of 5-lipoxygenase". Am. J. Respir. Crit. Care Med. 161 (2 Pt 2): S11–5. doi:10.1164/ajrccm.161.supplement_1.ltta-3. PMID 10673219.
  • Hammarberg T, Reddy KV, Persson B, Rådmark O (2002). "Calcium Binding to 5-Lipoxygenase". In Honn KV, Marnett LJ, Nigam S, Dennis E, Serhan C (eds.). Eicosanoids and Other Bioactive Lipids in Cancer, Inflammation, and Radiation Injury, 5. Advances in Experimental Medicine and Biology. Vol. 507. Springer. pp. 117–121. doi:10.1007/978-1-4615-0193-0_19. ISBN 978-0-306-47283-1. PMID 12664574.
  • Ishii S, Noguchi M, Miyano M, Matsumoto T, Noma M (1992). "Mutagenesis studies on the amino acid residues involved in the iron-binding and the activity of human 5-lipoxygenase". Biochem. Biophys. Res. Commun. 182 (3): 1482–1490. doi:10.1016/0006-291X(92)91901-2. PMID 1540191.
  • Nguyen T, Falgueyret JP, Abramovitz M, Riendeau D (1991). "Evaluation of the role of conserved His and Met residues among lipoxygenases by site-directed mutagenesis of recombinant human 5-lipoxygenase". J. Biol. Chem. 266 (32): 22057–22062. doi:10.1016/S0021-9258(18)54744-X. PMID 1939225.
  • Hoshiko S, Rådmark O, Samuelsson B (1990). "Characterization of the human 5-lipoxygenase gene promoter". Proc. Natl. Acad. Sci. U.S.A. 87 (23): 9073–9077. Bibcode:1990PNAS...87.9073H. doi:10.1073/pnas.87.23.9073. PMC 55106. PMID 2251250.
  • Matsumoto T, Funk CD, Rådmark O, Höög JO, Jörnvall H, Samuelsson B (1988). "Molecular cloning and amino acid sequence of human 5-lipoxygenase". Proc. Natl. Acad. Sci. U.S.A. 85 (1): 26–30. Bibcode:1988PNAS...85...26M. doi:10.1073/pnas.85.1.26. PMC 279474. PMID 2829172.
  • Rouzer CA, Kargman S (1988). "Translocation of 5-lipoxygenase to the membrane in human leukocytes challenged with ionophore A23187". J. Biol. Chem. 263 (22): 10980–10988. doi:10.1016/S0021-9258(18)38066-9. PMID 3134355.
  • Dixon RA, Jones RE, Diehl RE, Bennett CD, Kargman S, Rouzer CA (1988). "Cloning of the cDNA for human 5-lipoxygenase". Proc. Natl. Acad. Sci. U.S.A. 85 (2): 416–420. Bibcode:1988PNAS...85..416D. doi:10.1073/pnas.85.2.416. PMC 279559. PMID 3422434.
  • Jakobsson PJ, Shaskin P, Larsson P, Feltenmark S, Odlander B, Aguilar-Santelises M, Jondal M, Biberfeld P, Claesson HE (1995). "Studies on the regulation and localization of 5-lipoxygenase in human B-lymphocytes". Eur. J. Biochem. 232 (1): 37–46. doi:10.1111/j.1432-1033.1995.tb20778.x. PMID 7556168.
  • Janssen-Timmen U, Vickers PJ, Wittig U, Lehmann WD, Stark HJ, Fusenig NE, Rosenbach T, Rådmark O, Samuelsson B, Habenicht AJ (1995). "Expression of 5-lipoxygenase in differentiating human skin keratinocytes". Proc. Natl. Acad. Sci. U.S.A. 92 (15): 6966–6970. Bibcode:1995PNAS...92.6966J. doi:10.1073/pnas.92.15.6966. PMC 41452. PMID 7624354.
  • Lepley RA, Fitzpatrick FA (1994). "5-Lipoxygenase contains a functional Src homology 3-binding motif that interacts with the Src homology 3 domain of Grb2 and cytoskeletal proteins". J. Biol. Chem. 269 (39): 24163–24168. doi:10.1016/S0021-9258(19)51063-8. PMID 7929073.
  • Shaw KJ, Ng C, Kovacs BW (1994). "Cyclooxygenase gene expression in human endometrium and decidua". Prostaglandins Leukot. Essent. Fatty Acids. 50 (5): 239–243. doi:10.1016/0952-3278(94)90160-0. PMID 8066098.
  • Maruyama K, Sugano S (1994). "Oligo-capping: a simple method to replace the cap structure of eukaryotic mRNAs with oligoribonucleotides". Gene. 138 (1–2): 171–174. doi:10.1016/0378-1119(94)90802-8. PMID 8125298.
  • Woods JW, Evans JF, Ethier D, Scott S, Vickers PJ, Hearn L, Heibein JA, Charleson S, Singer II (1993). "5-lipoxygenase and 5-lipoxygenase-activating protein are localized in the nuclear envelope of activated human leukocytes". J. Exp. Med. 178 (6): 1935–1946. doi:10.1084/jem.178.6.1935. PMC 2191287. PMID 8245774.
  • Mancini JA, Li C, Vickers PJ (1993). "5-Lipoxygenase activity in the human pancreas". J Lipid Mediat. 8 (3): 145–150. PMID 8268460.
  • VanderNoot VA, Fitzpatrick FA (1995). "Competitive binding assay of src homology domain 3 interactions between 5-lipoxygenase and growth factor receptor binding protein 2". Anal. Biochem. 230 (1): 108–114. doi:10.1006/abio.1995.1444. PMID 8585605.
  • Brock TG, McNish RW, Bailie MB, Peters-Golden M (1997). "Rapid import of cytosolic 5-lipoxygenase into the nucleus of neutrophils after in vivo recruitment and in vitro adherence". J. Biol. Chem. 272 (13): 8276–8280. doi:10.1074/jbc.272.13.8276. PMID 9079648.
  • Nassar GM, Montero A, Fukunaga M, Badr KF (1997). "Contrasting effects of proinflammatory and T-helper lymphocyte subset-2 cytokines on the 5-lipoxygenase pathway in monocytes". Kidney Int. 51 (5): 1520–1528. doi:10.1038/ki.1997.209. PMID 9150468.
  • Suzuki Y, Yoshitomo-Nakagawa K, Maruyama K, Suyama A, Sugano S (1997). "Construction and characterization of a full length-enriched and a 5'-end-enriched cDNA library". Gene. 200 (1–2): 149–156. doi:10.1016/S0378-1119(97)00411-3. PMID 9373149.

External links edit

January 01, 1970
arachidonate, lipoxygenase, also, known, alox5, lipoxygenase, heme, iron, containing, enzyme, that, humans, encoded, alox5, gene, member, lipoxygenase, family, enzymes, transforms, essential, fatty, acids, substrates, into, leukotrienes, well, wide, range, oth. Arachidonate 5 lipoxygenase also known as ALOX5 5 lipoxygenase 5 LOX or 5 LO is a non heme iron containing enzyme EC 1 13 11 34 that in humans is encoded by the ALOX5 gene 1 Arachidonate 5 lipoxygenase is a member of the lipoxygenase family of enzymes It transforms essential fatty acids EFA substrates into leukotrienes as well as a wide range of other biologically active products ALOX5 is a current target for pharmaceutical intervention in a number of diseases arachidonate 5 lipoxygenaseIdentifiersAliases5 lipoxygenaseExternal IDsGeneCards 1 OrthologsSpeciesHumanMouseEntrezn an aEnsembln an aUniProtnan aRefSeq mRNA n an aRefSeq protein n an aLocation UCSC n an aPubMed searchn an aWikidataView Edit Human arachidonate 5 lipoxygenaseIdentifiersEC no 1 13 11 34CAS no 80619 02 9 permanent dead link DatabasesIntEnzIntEnz viewBRENDABRENDA entryExPASyNiceZyme viewKEGGKEGG entryMetaCycmetabolic pathwayPRIAMprofilePDB structuresRCSB PDB PDBe PDBsumGene OntologyAmiGO QuickGOSearchPMCarticlesPubMedarticlesNCBIproteins Contents 1 Gene 2 Expression 3 Biochemistry 4 Regulation 5 Substrates metabolites and metabolite activities 5 1 Arachidonic acid 5 2 Mead acid 5 3 Eicosapentaenoic acid 5 4 Docosahexaenoic acid 6 Transgenic studies 7 Clinical significance 7 1 Inflammation 7 2 Allergy 7 3 Hypersensitivity reactions 7 4 ALOX5 inhibiting drugs 8 Human genetics 8 1 Allergic asthma 8 2 NSAID induced non allergic reactions 8 3 Atherosclerosis 9 See also 10 References 11 Further reading 12 External linksGene editThe ALOX5 gene which occupies 71 9 kilobase pairs kb on chromosome 10 all other human lipoxygenases are clustered together on chromosome 17 is composed of 14 exons divided by 13 introns encoding the mature 78 kilodalton kDa ALOX5 protein consisting of 673 amino acids The gene promoter region of ALOX5 contains 8 GC boxes but lacks TATA boxes or CAT boxes and thus resembles the gene promoters of typical housekeeping genes Five of the 8 GC boxes are arranged in tandem and are recognized by the transcription factors Sp1 and Egr 1 A novel Sp1 binding site occurs close to the major transcription start site position 65 a GC rich core region including the Sp1 Egr 1 sites may be critical for basal 5 LO promoter activity 2 Expression editCells primarily involved in regulating inflammation allergy and other immune responses e g neutrophils eosinophils basophils monocytes macrophages mast cells dendritic cells and B lymphocytes express ALOX5 Platelets T cells and erythrocytes are ALOX5 negative In skin Langerhans cells strongly express ALOX5 Fibroblasts smooth muscle cells and endothelial cells express low levels of ALOX5 2 3 Up regulation of ALOX5 may occur during the maturation of leukocytes and in human neutrophils treated with granulocyte macrophage colony stimulating factor and then stimulated with physiological agents Aberrant expression of LOX5 is seen in various types of human cancer tumors in vivo as well as in various types of human cancer cell lines in vitro these tumors and cell lines include those of the pancreas prostate and colon ALOX5 products particularly 5 hydroxyeicosatetraenoic acid and 5 oxo eicosatetraenoic acid promote the proliferation of these ALOX5 aberrantly expressing tumor cell lines suggesting that ALOX5 acts as a pro malignancy factor for them and by extension their parent tumors 2 Studies with cultured human cells have found that there are a large number of ALOX5 mRNA splice variants due to alternative splicing The physiological and or pathological consequences of this slicing has yet to be defined In one study however human brain tumors were shown to express three mRNA splice variants 2 7 3 1 and 6 4 kb in addition to the full 8 6 lb species the abundance of the variants correlated with the malignancy of these tumors suggesting that they may play a role in the development of these tumors 2 Biochemistry editHuman ALOX5 is a soluble monomeric protein consisting of 673 amino acids with a molecular weight of 78 kDa Structurally ALOX5 possesses 3 4 A C terminal catalytic domain residues 126 673 An N terminal C2 like domain which promotes its binding to ligand substrates Ca2 cellular phospholipid membranes Coactin like protein COL1 and Dicer protein A PLAT domain within its C2 like domain this domain by analogy to other PLAT domain bearing proteins may serve as a mobile lid over ALOX5 s substrate binding site An adenosine triphosphate ATP binding site ATP is crucial for ALOX5 s metabolic activity A proline rich region residues 566 577 sometimes termed a SH3 binding domain which promotes its binding to proteins with SH3 domains such as Grb2 and may thereby link the enzyme s regulation to tyrosine kinase receptors The enzyme possesses two catalytic activities as illustrated by its metabolism of arachidonic acid ALOX5 s dioxygenase activity adds a hydroperoxyl i e HO2 residue to arachidonic acid i e 5Z 8Z 11Z 14Z eicosatetraenoic acid at carbon 5 of its 1 4 diene group i e its 5Z 8Z double bonds to form 5 S hydroperoxy 6E 8Z 11Z 14Z eicosatetraenoic acid i e 5S HpETE 5 The 5S HpETE intermediate may then be released by the enzyme and rapidly reduced by cellular glutathione peroxidases to its corresponding alcohol 5 S hydroxy 6E 8Z 11Z 14Z eicosatetraenoic acid i e 5 HETE or alternatively further metabolized by ALOX5 s epoxidase also termed LTA4 synthase activity which converts 5S HpETE to its epoxide 5S 6S hydroxy 6E 8Z 11Z 14Z eicosatetraenoic acid i e LTA4 6 LTA4 is then acted on by a separate soluble enzyme leukotriene A4 hydrolase to form the dihydroxyl product leukotriene B4 LTB4 i e 5S 12R dihydroxy 5S 6Z 8E 10E 12R 14Z eicosatetraenoic acid or by either LTC4 synthase or microsomal glutathione S transferase 2 MGST2 which bind the sulfur of cysteine s thio i e SH residue in the tripeptide glutamate cysteine glycine to carbon 6 of LTA4 thereby forming LTC4 i e 5S hydroxy 6R S glutathionyl 7E 9E 11Z 14Z eicosatetraenoic acid The Glu and Gly residues of LTC4 may be removed step wise by gamma glutamyltransferase and a dipeptidase to form sequentially LTD4 and LTE4 4 7 To varying extents the other PUFA substrates of ALOX5 follow similar metabolic pathways to form analogous products Sub human mammalian Alox5 enzymes like those in rodents appear to have at least in general similar structures distributions activities and functions as human ALOX5 Hence model Alox5 studies in rodents appear to be valuable for defining the function of ALOX5 in humans see Lipoxygenase Mouse lipoxygenases Regulation editALOX5 exists primarily in the cytoplasm and nucleoplasm of cells Upon cell stimulation ALOX5 a may be phosphorylated on serine 663 523 and or 271 by mitogen activated protein kinases S6 kinase protein kinase A PKA protein kinase C Cdc2 and or a Ca2 calmodulin dependent protein kinase b moves to bind with phospholipids in the nuclear membrane and probably endoplasmic reticulum membrane c is able to accept substrate fatty acids presented to it by the 5 lipoxygenase activating protein FLAP which is embedded in these membranes and d thereby becomes suited for high metabolic activity These events along with rises in cytosolic Ca2 levels which promote the translocation of ALOX5 form the cytoplasm and nucleoplasm to the cited membranes are induced by cell stimulation such as that caused by chemotactic factors on leukocytes Rises in cytosolic Ca2 ALOX5 s movement to membranes and ALOX5 s interaction with FLAP are critical to the physiological activation of the enzyme 3 Serine 271 and 663 phosphorylations do not appear to alter ALOX5 s activity Serine 523 phosphorylation which is conducted by PKA totally inactivates the enzyme and prevents its nuclear localization stimuli which cause cells to activate PKA can thereby block production of ALOX5 metabolites 4 8 In addition to its activation ALOX5 must gain access to its polyunsaturated fatty acid PUFA substrates which commonly are bound in an ester linkage to the sn2 position of membrane phospholipids in order to form biologically active products This is accomplished by a large family of phospholipase A2 PLA2 enzymes The cytosolic PLA2 set i e cPLA2s of PLA2 enzymes see Phospholipase A2 Cytosolic phospholipases A2 cPLA2 in particular mediates many instances of stimulus induced release of PUFA in inflammatory cells For example chemotactic factors stimulate human neutrophils to raise cytosolic Ca2 which triggers cPLA2s particularly the a isoform cPLA2a to move from its normal residence in the cytosol to cellular membranes This chemotactic factor stimulation concurrently causes the activation of mitogen activated protein kinases MAPK which in turn stimulates the activity of cPLA2a by phosphorylating it on ser 505 other cell types may activate this or other cPLA2 isoforms using other kinases which phosphorylate them on different serine residues These two events allow cPLA2s to release PUFA esterified to membrane phospholipids to FLAP which then presents them to ALOX5 for their metabolism 9 10 Other factors are known to regulate ALOX5 activity in vitro but have not been fully integrated into its physiological activation during cell stimulation ALOX5 binds with the F actin binding protein coactin like protein Based on in vitro studies this protein binding serves to stabilize ALOX5 by acting as a chaperone protein or scaffold thereby averting the enzyme s inactivation to promote its metabolic activity depending on circumstance such as the presence of phospholipids and levels of ambient Ca2 this binding also alters the relative levels of hydroperoxy versus epoxide see arachidonic acid section below products made by ALOX5 3 4 The binding of ALOX5 to membranes as well as its interaction with FLAP likewise cause the enzyme to alter its relative levels of hydroperoxy versus epoxide production in these cases favoring the production of the epoxide products 4 The presence of certain diacylglycerols such as 1 oleoyl 2 acetyl sn glycerol 1 hexadecyl 2 acetyl sn glycerol and 1 O hexadecyl 2 acetyl sn glycerol and 1 2 dioctanoyl sn glycerol but not 1 stearoyl 2 arachidonyl sn glycerol increase the catalytic activity of ALOX5 in vitro 4 Substrates metabolites and metabolite activities editALOX5 metabolizes various omega 3 and omega 6 PUFA to a wide range of products with varying and sometimes opposing biological activities A list of these substrates along with their principal metabolites and metabolite activities follows nbsp Arachidonic acid edit ALOX5 metabolizes the omega 6 fatty acid arachidonic acid AA i e 5Z 8Z 11Z 14Z eicosatetraenoic acid to 5 hydroperoxyeicosatetraenoic acid 5 HpETE which is then rapidly converted to physiologically and pathologically important products Ubiquitous cellular glutathione peroxidases GPXs reduce 5 HpETE to 5 hydroxyeicosatetraenoic acid 5 HETE 5 HETE may be further metabolized by 5 hydroxyeicosanoid dehydrogenase 5 HEDH to 5 oxo eicosatetraenoic acid 5 oxo ETE Alternatively the intrinsic activity of ALOX5 may convert 5 HpETE to its 5 6 epoxide leukotriene A4 LTA4 which is then either rapidly converted to leukotriene B4 LTB4 by leukotriene A4 hydrolase LTA4H or to leukotriene C4 LTC4 by LTC4 synthase LTC4S LTC4 exits its cells of origin through the MRP1 transporter ABCC1 and is rapidly converted to LTD4 and then to LTE4 by cell surface attached gamma glutamyltransferase and dipeptidase peptidase enzymes In another pathway ALOX5 may act in series with a second lipoxygenase enzyme ALOX15 to metabolize AA to lipoxin A4 LxA4 and LxB4 see Specialized pro resolving mediators Lipoxins 3 11 12 13 GPXs 5 HEDH LTA4H LTC4S ABCC1 and cell surface peptidases may act similarly on the ALOX5 derived metabolites of other PUFA LTB4 5 HETE and 5 oxo ETE may contribute to the innate immune response as leukocyte chemotactic factors i e they recruit and further activate circulating blood neutrophils and monocytes to sites of microbial invasion tissue injury and foreign bodies When produced in excess however they may contribute to a wide range of pathological inflammatory responses 5 HETE and LTB4 5 Oxo ETE is a particularly potent chemotactic factor for and activator of eosinophils and may thereby contribute to eosinophil based allergic reactions and diseases 4 14 These metabolites may also contribute to the progression of certain cancers such as those of the prostate breast lung ovary and pancreas ALOX5 may be overexpressed in some of these cancers 5 Oxo ETE and to a lesser extent 5 HETE stimulate human cell lines derived from these cancers to proliferate and the pharmacological inhibition of ALOX5 in these human cell lines causes them to die by entering apoptosis 14 15 16 17 18 ALOX5 and its LTB4 metabolite as well as this metabolite s BLT1 and BLT2 receptors have also been shown to promote the growth of various types of human cancer cell lines in culture 19 20 LTC4 LTD4 and LTE4 contribute to allergic airways reactions such as asthma certain non allergic hypersensitivity airways reactions and other lung diseases involving bronchoconstriction by contracting these airways and promoting in these airways inflammation micro vascular permeability and mucus secretion they likewise contribute to various allergic and non allergic reactions involving rhinitis conjunctivitis and urticaria 3 Certain of these peptide leukotrienes have been shown to promote the growth of cultured human breast cancer and chronic lymphocytic leukemia cell lines thereby suggesting that ALOX5 may contribute to the progression of these diseases 19 LxA4 and LxB4 are members of the specialized pro resolving mediators class of polyunsaturated fatty acid metabolites They form later than the ALOX5 derived chemotactic factors in the inflammatory response and are thought to limit or resolve these responses by for example inhibiting the entry of circulating leukocytes into inflamed tissues inhibiting the pro inflammatory action of the leukocytes promoting leukocytes to exit from inflammatory sites and stimulating leukocyte apoptosis see Specialized pro resolving mediators and Lipoxin 11 Mead acid edit Mead acid i e 5Z 8Z 11Z eicosatrienoic acid is identical to AA except that has a single rather than double bond between its 14 and 15 carbon ALOX5 metabolizes mead acid to 3 series i e containing 3 double bonds analogs of its 4 series AA metabolites viz 5 S hydroxy 6E 8Z 11Z eicosatrienoic acid 5 HETrE 5 oxo 6 8 11 eicosatrienoic acid 5 oxo ETrE LTA3 and LTC3 since LTA3 inhibits LTA hydrolase mead acid metabolizing cells produce relatively little LTB3 and are blocked from metabolizing arachidonic acid to LTB4 On the other hand 5 oxo ETrE is almost as potent as 5 oxo ETE as an eosinophil chemotactic factor and may thereby contribute to the development of physiological and pathological allergic responses 12 Presumably the same metabolic pathways that follow ALOX5 in metabolizing arachidonic acid to the 4 series metabolites likewise act on mead acid to form these products Eicosapentaenoic acid edit ALOX5 metabolizes the omega 3 fatty acid eicosapentaenoic acid EPA i e 4Z 8Z 11Z 14Z 17Z eiosapentaenoic acid to 5 hydroperoxy eicosapentaenoic acid which is then converted to 5 series products that are structurally analogous to their arachidonic acid counterparts viz 5 hydroxy eicosapentaenoic acid 5 HEPE 5 oxo eiocosapentaenoic acid 5 oxo HEPE LTB5 LTC5 LTD5 and LTE5 4 21 Presumably the same metabolic pathways that follow ALOX5 in metabolizing arachidonic acid to the 4 series metabolites likewise act on EPA to form these 5 series products ALOX5 also cooperates with other lipoxygenase cyclooxygenase or cytochrome P450 enzymes in serial metabolic pathways to metabolize EPA to resolvins of the E series see Specialized pro resolving mediators EPA derived resolvins for further details on this metabolism viz resolvin E1 RvE1 and RvE2 22 23 5 HEPE 5 oxo HEPE LTB5 LTC5 LTD5 and LTE5 are generally less potent in stimulating cells and tissues than their arachidonic acid derived counterparts since their production is associated with reduced production of their arachidonic acid derived counterparts they may indirectly serve to reduce the pro inflammatory and pro allergic activities of their arachidonic acid derived counterparts 4 21 RvE1 and ReV2 are specialized pro resolving mediators that contribute to the resolution of inflammation and other reactions 23 Docosahexaenoic acid edit ALOX5 acts in series with ALOX15 to metabolize the omega 3 fatty acid docosahexaenoic acid DHA i e 4Z 7Z 10Z 13Z 16Z 19Z docosahexaenoic acid to D series resolvins see Specialized pro resolving mediators DHA derived resolvins for further details on this metabolism 23 24 The D series resolvins i e RvD1 RvD2 RvD3 RvD4 RvD5 RvD6 AT RVD1 AT RVD2 AT RVD3 AT RVD4 AT RVD5 and AT RVD6 are specialized pro resolving mediators that contribute to the resolution of inflammation promote tissue healing and reduce the perception of inflammation based pain 23 24 Transgenic studies editStudies in model animal systems that delete or overexpress the Alox5 gene have given seemingly paradoxical results In mice for example Alox5 overexpression may decrease the damage caused by some types yet increase the damage caused by other types of invasive pathogens This may be a reflection of the array of metabolites made by the Alox5 enzyme some of which possess opposing activities like the pro inflammatory chemotactic factors and the anti inflammatory specialized pro resolving mediators Alox5 and presumably human ALOX5 functions may vary widely depending on the agents stimulating their activity the types of metabolites that they form the specific tissues responding to these metabolites the times e g early versus delayed at which observations are made and very likely various other factors Alox5 gene knockout mice are more susceptible to the development and pathological complications of experimental infection with Klebsiella pneumoniae Borrelia burgdorferi and Paracoccidioides brasiliensis 8 25 In a model of cecum perforation induced sepsis ALOX5 gene knockout mice exhibited a decrease in the number of neutrophils and an increase in the number of bacteria that accumulated in their peritoneum 26 On the other hand ALOX5 gene knockout mice demonstrate an enhanced resistance and lessened pathology to Brucella abortus infection 27 and at least in its acute phase Trypanosoma cruzi infection 28 Furthermore Alox5 null mice exhibit a worsened inflammatory component failure to resolve inflammation related responses and decreased survival in experimental models of respiratory syncytial virus disease Lyme disease Toxoplasma gondii disease and corneal injury These studies indicate that Alox5 can serve a protective function presumably by generating metabolites such as chemotactic factors that mobilize the innate immunity system However the suppression of inflammation appears also to be a function of Alox5 presumably by contributing to the production of anti inflammatory specialized pro resolving mediators SPMs at least in certain rodent inflammation based model systems These genetic studies allow that ALOX5 along with the chemotactic factors and SPMs that they contribute to making may play similar opposing pro inflammatory and anti inflammatory functions in humans 22 29 Alox5 gene knockout mice exhibit an increase in the lung tumor volume and liver metastasis of Lewis lung carcinoma cells that were directly implanted into their lungs this result differs from many in vitro studies which implicated human ALOX5 along with certain of its metabolites with promoting cancer cell growth in that it finds that mouse Alox5 and perhaps certain of its metabolites inhibit cancer cell growth Studies in this model suggest that Alox5 acting through one or more of its metabolites reduces growth and progression of the Lewis carcinoma by recruiting cancer inhibiting CD4 T helper cells and CD8 T cytotoxic T cells to the sites of implantation 30 This striking difference between human in vitro and mouse in vivo studies may reflect species differences in vitro versus in vivo differences or cancer cell type differences in the function of ALOX5 Alox5 Clinical significance editInflammation edit Studies implicate ALOX5 in contributing to innate immunity by contributing to the mounting inflammatory responses to a wide range of diseases acute pathogen invasion trauma and burns see Inflammation Causes however ALOX5 also contributes to the development and progression of excessive and chronic inflammatory responses such as rheumatoid arthritis atherosclerosis inflammatory bowel disease autoimmune diseases see Inflammation Disorders These dual functions probably reflect ALOX5 s ability to form the a potent chemotactic factor LTB4 and possibly also weaker chemotactic factor 5S HETE which serve to attract and otherwise activate inflammation inducing cells such as circulating leukocytes and tissue macrophages and dendritic cells and b lipoxin and resolvin subfamily of SPMs which tend to inhibit these cells as well as the overall inflammatory responses 8 31 32 Allergy edit ALOX5 contributes to the development and progression of allergy and allergic inflammation reactions and diseases such as allergic rhinitis conjunctivitis asthma rashes eczema see Allergy Signs and symptoms This activity reflects its formation of a LTC4 LTD4 and LTE4 which promote vascular permeability contract airways smooth muscle and otherwise perturb these tissues and b LTB4 and possibly 5 oxo ETE which are chemotactic factors for and activators of the cell type promoting such reactions the eosinophil 8 14 5 Oxo ETE and to a lesser extent 5S HETE also act synergistically with another pro allergic mediator platelet activating factor to stimulate and otherwise activate eosinophils 14 33 34 35 Hypersensitivity reactions edit ALOX5 contributes to non allergic NSAID hypersensitivity reactions of the respiratory system and skin such as aspirin exacerbated respiratory disease nonallergic rhinitis non allergic conjunctivitis angioedema urticarial It may also contribute to hypersensitivity responses of the respiratory system to cold air and possibly even alcohol beverages These pathological responses likely involve the same ALOX5 formed metabolites as those promoting allergic reactions 13 8 36 ALOX5 inhibiting drugs edit Main article Arachidonate 5 lipoxygenase inhibitor The tissue animal model and animal and human genetic studies cited above implicate ALOX5 in a wide range of diseases excessive inflammatory responses to pathogens trauma burns and other forms of tissue injury see Inflammation Causes chronic inflammatory conditions such as rheumatoid arthritis atherosclerosis inflammatory bowel disease autoimmune diseases Alzheimer s disease see Inflammation Disorders allergy and allergic inflammation reactions such as allergic rhinitis conjunctivitis asthma rashes eczema NSAID induced acute non allergic reactions such as asthma rhinitis conjunctivitis angioedema urticaria the progression of certain cancers such as those of the prostate and pancreas However clinical use of drugs that inhibit ALOX5 to treat any of these diseases has been successful with only Zileuton along with its controlled released preparation Zileuton CR Zileuton is approved in the US for the prophylaxis and chronic treatment of allergic asthma it is also used to treat chronic non allergic reactions such as NSAID induced non allergic lung nose and conjunctiva reactions as well as exercise induced asthma Zileuton has shown some beneficial effects in clinical trials for the treatment of rheumatoid arthritis inflammatory bowel disease and psoriasis 8 37 Zileuton is currently undergoing a phase II study for the treatment of acne vulgaris mild to moderate inflammatory facial acne and a phase I study see Clinical trial Phases combining it with imatinib for treating chronic myeloid leukemia 38 39 Zyleuton and zileuton CR cause elevations in liver enzymes in 2 of patients the two drugs are therefore contraindicated in patients with active liver disease or persistent hepatic enzyme elevations greater than three times the upper limit of normal Hepatic function should be assessed prior to initiating either of these drugs monthly for the first 3 months every 2 3 months for the remainder of the first year and periodically thereafter zileuton also has a rather unfavorable pharmacological profile see Zileuton Contraindications and warnings 38 Given these deficiencies other drugs targeting ALOX5 are under study Flavocoxid is a proprietary blend of purified plant derived bioflavonoids including Baicalin and Catechins It inhibits COX 1 COX 2 and ALOX5 in vitro and in animal models Flavocoxid has been approved for use as a medical food in the United States since 2004 and is available by prescription for use in chronic osteoarthritis in tablets of 500 mg under the commercial name Limbrel However in clinical trials serum liver enzyme elevations occurred in up to 10 of patients on flavocoxid therapy although elevations above 3 times the upper limit of normal occurred in only 1 2 of recipients Since its release however there have been several reports of clinically apparent acute liver injury attributed to flavocoxid 40 Setileuton MK 0633 has completed a Phase II clinical trial for the treatment of asthma chronic obstructive lung disease and atherosclerosis NCT00404313 NCT00418613 and NCT00421278 respectively 38 41 PF 4191834 42 has completed phase II studies for the treatment of asthma NCT00723021 38 Hyperforin an active constituent of the herb St John s wort is active at micromolar concentrations in inhibiting ALOX5 43 Indirubin 3 monoxime a derivative of the naturally occurring alkaloid indirubin is also described as selective ALOX5 inhibitor effective in a range of cell free and cell based model systems 44 In addition curcumin a constituent of turmeric is a 5 LO inhibitor as defined by in vitro studies of the enzyme 45 Acetyl keto beta boswellic acid AKBA one of the bioactive boswellic acids found in Boswellia serrata Indian Frankincense has been found to inhibit 5 lipoxygenase Boswellia reduces brain edema in patients irradiated for brain tumor and it s believed to be due to 5 lipoxygenase inhibition 46 47 While only one ALOX5 inhibiting drug has proven useful for treating human diseases other drugs that act down stream in the ALOX5 initiated pathway are in clinical use Montelukast Zafirlukast and Pranlukast are receptor antagonists for the cysteinyl leukotriene receptor 1 which contributes to mediating the actions of LTC4 LTD4 and LTE4 These drugs are in common use as prophylaxis and chronic treatment of allergic and non allergic asthma and rhinitis diseases 3 and also may be useful for treating acquired childhood sleep apnea due to adenotonsillar hypertrophy see Acquired non inflammatory myopathy Diet and Trauma Induced Myopathy 48 To date however neither LTB4 synthesis inhibitors i e blockers of ALOX5 or LTA4 hydrolase nor inhibitors of LTB4 receptors BLT1 and BLT2 have turned out to be effective anti inflammatory drugs Furthermore blockers of LTC4 LTD4 and LTE4 synthesis i e ALOX5 inhibitors as well as of LTC4 and LTD4 receptor antagonists have proven inferior to corticosteroids as single drug therapy for persistent asthma particularly in patients with airway obstruction As a second drug added to corticosteroids leukotriene inhibitors appear inferior to beta2 adrenergic agonist drugs in the treatment of asthma 49 Human genetics editALOX5 contributes to the formation of PUFA metabolites that may promote e g the leukotrienes 5 oxo ETE but also to metabolites that inhibit i e lipoxins resolvins diseases Consequently a given abnormality in the expression or activity of ALOX5 due to variations in its gene may promote or suppress inflammation depending on the relative roles these opposing metabolites have in regulating the particular type of reaction examined Furthermore the ALOX5 related tissue reactions studied to date are influenced by multiple genetic environmental and developmental variables that may influence the consequences of abnormalities in the expression or function of ALOX5 Consequently abnormalities in the ALOX5 gene may vary with the population and individuals studied Allergic asthma edit The upstream promoter in the human ALOX5 gene commonly possess five GGGCCGG repeats which bind the Sp1 transcription factor and thereby increase the gene s transcription of ALOX5 Homozygous variants for this five repeat promoter region in a study of 624 asthmatic children in Ankara Turkey were much more likely to have severe asthma These variants are associated with reduced levels of ALOX5 as well as reduced production of LTC4 in their eosinophils 50 These data suggest that ALOX5 may contribute to dampening the severity of asthma possibly by metabolizing PUFA to specialized pro resolving mediators 51 Single nucleotide polymorphism differences in the genes that promote ALOX5 activity i e 5 lipoxygenase activating protein metabolize the initial product of ALOX5 5S HpETE to LTB4 i e leukotriene A4 hydrolase or are the cellular receptors responsible for mediating the cellular responses to the down stream ALOX products LTC4 and LTD4 i e CYSLTR1 and CYSLTR2 have been associated with the presence of asthma in single population studies These studies suggest genetic variants may play a role albeit a relatively minor one in the overall susceptibility to allergic asthma 50 NSAID induced non allergic reactions edit Aspirin and other non steroidal anti inflammatory drugs NSAID can cause NSAID exacerbated diseases N ERD These have been recently classified into 5 groups 3 of which are not caused by a classical immune mechanism and are relevant to the function of ALOX5 1 NSAIDs exacerbated respiratory disease NERD i e symptoms of bronchial airways obstruction shortness of breath and or nasal congestion rhinorrhea occurring shortly after NSAID ingestion in patients with a history of asthma and or rhinosinusitis 2 NSAIDs exacerbated cutaneous disease NECD i e wheal responses and or angioedema responses occurring shortly after NSAID ingestion in patients with a history of chronic urticaria and 3 NSAIDs induced urticaria angioedema NIUA i e wheals and or angioedema symptoms occurring shortly after NSAID ingestion in patients with no history of chronic urticaria 52 The genetic single nucleotide polymorphism SNP variant in the ALOX5 gene ALOX5 1708 G gt A is associated with NSAID induced asthma in Korean patients and three SNP ALOX5 variants rs4948672 53 rs1565096 54 and rs7894352 55 are associated with NSAID induced cutaneous reactions in Spanish patients 33 Atherosclerosis edit Bearers of two variations in the predominant five tandem repeat Sp1 binding motif GGGCCGG of the ALOX5 gene promoter in 470 subjects non Hispanic whites 55 1 Hispanics 29 6 Asian or Pacific Islander 7 7 amp African Americans 5 3 and others 2 3 were positively associated with the severity of atherosclerosis 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Deletion of 5 Lipoxygenase in the Tumor Microenvironment Promotes Lung Cancer Progression and Metastasis through Regulating T Cell Recruitment Journal of Immunology 196 2 891 901 doi 10 4049 jimmunol 1501648 PMC 4705594 PMID 26663781 Rossi AG O Flaherty JT 1991 Bioactions of 5 hydroxyicosatetraenoate and its interaction with platelet activating factor Lipids 26 12 1184 1188 doi 10 1007 bf02536528 PMID 1668115 S2CID 3964822 Basil MC Levy BD 2016 Specialized pro resolving mediators endogenous regulators of infection and inflammation Nature Reviews Immunology 16 1 51 67 doi 10 1038 nri 2015 4 PMC 5242505 PMID 26688348 a b Oussalah A Mayorga C Blanca M Barbaud A Nakonechna A Cernadas J Gotua M Brockow K Caubet JC Bircher A Atanaskovic M Demoly P K Tanno L Terreehorst I Laguna JJ Romano A Gueant JL 2016 Genetic variants associated with drugs induced immediate hypersensitivity reactions a PRISMA compliant systematic review Allergy 71 4 443 462 doi 10 1111 all 12821 PMID 26678823 O Flaherty JT Kuroki M Nixon AB Wijkander J Yee E Lee SL Smitherman PK Wykle RL Daniel LW 1996 5 Oxo eicosatetraenoate is a broadly active eosinophil selective stimulus for human granulocytes Journal of Immunology 157 1 336 342 doi 10 4049 jimmunol 157 1 336 PMID 8683135 S2CID 35264541 Schauberger E Peinhaupt M Cazares T Lindsley AW 2016 Lipid Mediators of Allergic Disease Pathways Treatments and Emerging Therapeutic Targets Current Allergy and Asthma Reports 16 7 48 doi 10 1007 s11882 016 0628 3 PMC 5515624 PMID 27333777 Barros R Moreira A Padrao P Teixeira VH Carvalho P Delgado L Lopes C Severo M Moreira P 2015 Dietary patterns and asthma prevalence incidence and control Clinical amp Experimental Allergy 45 11 1673 1680 doi 10 1111 cea 12544 PMID 25818037 S2CID 32499209 Fanning LB Boyce JA 2013 Lipid mediators and allergic diseases Annals of Allergy Asthma amp Immunology 111 3 155 162 doi 10 1016 j anai 2013 06 031 PMC 4088989 PMID 23987187 a b c d Steinhilber D Hofmann B 2014 Recent advances in the search for novel 5 lipoxygenase inhibitors Basic amp Clinical Pharmacology amp Toxicology 114 1 70 77 doi 10 1111 bcpt 12114 PMID 23953428 Cingi C Muluk NB Ipci K Sahin E 2015 Antileukotrienes in upper airway inflammatory diseases Current Allergy and Asthma Reports 15 11 64 doi 10 1007 s11882 015 0564 7 PMID 26385352 S2CID 38854822 Flavocoxid Drug Record LiverTox United States National Library of Medicine Archived from the original on 2019 08 19 Retrieved 2016 08 22 Clinical trial number NCT00404313 for The Effect of MK0633 in Patients With Chronic Asthma at ClinicalTrials gov PF 4191834 MedKoo Biosciences Inc Albert D Zundorf I Dingermann T Muller WE Steinhilber D Werz O Dec 2002 Hyperforin is a dual inhibitor of cyclooxygenase 1 and 5 lipoxygenase Biochemical Pharmacology 64 12 1767 1775 doi 10 1016 s0006 2952 02 01387 4 PMID 12445866 Blazevic T Schaible AM Weinhaupl K Schachner D Nikels F Weinigel C Barz D Atanasov AG Pergola C Werz O Dirsch VM Heiss EH Mar 2014 Indirubin 3 monoxime exerts a dual mode of inhibition towards leukotriene mediated vascular smooth muscle cell migration Cardiovascular Research 101 3 522 532 doi 10 1093 cvr cvt339 PMC 3928003 PMID 24368834 Bishayee K Khuda Bukhsh AR Sep 2013 5 lipoxygenase antagonist therapy a new approach towards targeted cancer chemotherapy Acta Biochimica et Biophysica Sinica 45 9 709 719 doi 10 1093 abbs gmt064 PMID 23752617 Kirste S 2009 Antiodematose Wirkung von Boswellia serrata auf das Strahlentherapie assoziierte Hirnodem Anti edematous effect of Boswellia serrata on radiation therapy associated brain edema Ph D thesis in German Breisgau Germany University Freiburg Kirste S Treier M Wehrle SJ Becker G Abdel Tawab M Gerbeth K et al August 2011 Boswellia serrata acts on cerebral edema in patients irradiated for brain tumors a prospective randomized placebo controlled double blind pilot trial Cancer 117 16 3788 3795 doi 10 1002 cncr 25945 PMID 21287538 S2CID 11283379 Kar M Altintoprak N Muluk NB Ulusoy S Bafaqeeh SA Cingi C 2016 Antileukotrienes in adenotonsillar hypertrophy a review of the literature European Archives of Oto Rhino Laryngology 273 12 4111 4117 doi 10 1007 s00405 016 3983 8 PMID 26980339 S2CID 31311115 Kuhn H Banthiya S van Leyen K 2015 Mammalian lipoxygenases and their biological relevance Biochimica et Biophysica Acta BBA Molecular and Cell Biology of Lipids 1851 4 308 330 doi 10 1016 j bbalip 2014 10 002 PMC 4370320 PMID 25316652 a b Tantisira KG Drazen JM 2009 Genetics and pharmacogenetics of the leukotriene pathway The Journal of Allergy and Clinical Immunology 124 3 422 427 doi 10 1016 j jaci 2009 06 035 PMC 2794036 PMID 19665766 Duvall MG Levy BD 2016 DHA and EPA derived resolvins protectins and maresins in airway inflammation European Journal of Pharmacology 785 144 155 doi 10 1016 j ejphar 2015 11 001 PMC 4854800 PMID 26546247 Kowalski ML Asero R Bavbek S Blanca M Blanca Lopez N Bochenek G Brockow K Campo P Celik G Cernadas J Cortellini G Gomes E Nizankowska Mogilnicka E Romano A Szczeklik A Testi S Torres MJ Wohrl S Makowska J 2013 Classification and practical approach to the diagnosis and management of hypersensitivity to nonsteroidal anti inflammatory drugs Allergy 68 10 1219 1232 doi 10 1111 all 12260 PMID 24117484 S2CID 32169451 Reference SNP refSNP Cluster Report rs4948672 NCBI dbSNP Reference SNP refSNP Cluster Report rs1565096 NCBI dbSNP Reference SNP refSNP Cluster Report rs7894352 NCBI dbSNP Dwyer JH Allayee H Dwyer KM Fan J Wu H Mar R Lusis AJ Mehrabian M 2004 Arachidonate 5 lipoxygenase promoter genotype dietary arachidonic acid and atherosclerosis The New England Journal of Medicine 350 1 29 37 doi 10 1056 NEJMoa025079 PMID 14702425 Further reading editRadmark OP 2000 The molecular biology and regulation of 5 lipoxygenase Am J Respir Crit Care Med 161 2 Pt 2 S11 5 doi 10 1164 ajrccm 161 supplement 1 ltta 3 PMID 10673219 Hammarberg T Reddy KV Persson B Radmark O 2002 Calcium Binding to 5 Lipoxygenase In Honn KV Marnett LJ Nigam S Dennis E Serhan C eds Eicosanoids and Other Bioactive Lipids in Cancer Inflammation and Radiation Injury 5 Advances in Experimental Medicine and Biology Vol 507 Springer pp 117 121 doi 10 1007 978 1 4615 0193 0 19 ISBN 978 0 306 47283 1 PMID 12664574 Ishii S Noguchi M Miyano M Matsumoto T Noma M 1992 Mutagenesis studies on the amino acid residues involved in the iron binding and the activity of human 5 lipoxygenase Biochem Biophys Res Commun 182 3 1482 1490 doi 10 1016 0006 291X 92 91901 2 PMID 1540191 Nguyen T Falgueyret JP Abramovitz M Riendeau D 1991 Evaluation of the role of conserved His and Met residues among lipoxygenases by site directed mutagenesis of recombinant human 5 lipoxygenase J Biol Chem 266 32 22057 22062 doi 10 1016 S0021 9258 18 54744 X PMID 1939225 Hoshiko S Radmark O Samuelsson B 1990 Characterization of the human 5 lipoxygenase gene promoter Proc Natl Acad Sci U S A 87 23 9073 9077 Bibcode 1990PNAS 87 9073H doi 10 1073 pnas 87 23 9073 PMC 55106 PMID 2251250 Matsumoto T Funk CD Radmark O Hoog JO Jornvall H Samuelsson B 1988 Molecular cloning and amino acid sequence of human 5 lipoxygenase Proc Natl Acad Sci U S A 85 1 26 30 Bibcode 1988PNAS 85 26M doi 10 1073 pnas 85 1 26 PMC 279474 PMID 2829172 Rouzer CA Kargman S 1988 Translocation of 5 lipoxygenase to the membrane in human leukocytes challenged with ionophore A23187 J Biol Chem 263 22 10980 10988 doi 10 1016 S0021 9258 18 38066 9 PMID 3134355 Dixon RA Jones RE Diehl RE Bennett CD Kargman S Rouzer CA 1988 Cloning of the cDNA for human 5 lipoxygenase Proc Natl Acad Sci U S A 85 2 416 420 Bibcode 1988PNAS 85 416D doi 10 1073 pnas 85 2 416 PMC 279559 PMID 3422434 Jakobsson PJ Shaskin P Larsson P Feltenmark S Odlander B Aguilar Santelises M Jondal M Biberfeld P Claesson HE 1995 Studies on the regulation and localization of 5 lipoxygenase in human B lymphocytes Eur J Biochem 232 1 37 46 doi 10 1111 j 1432 1033 1995 tb20778 x PMID 7556168 Janssen Timmen U Vickers PJ Wittig U Lehmann WD Stark HJ Fusenig NE Rosenbach T Radmark O Samuelsson B Habenicht AJ 1995 Expression of 5 lipoxygenase in differentiating human skin keratinocytes Proc Natl Acad Sci U S A 92 15 6966 6970 Bibcode 1995PNAS 92 6966J doi 10 1073 pnas 92 15 6966 PMC 41452 PMID 7624354 Lepley RA Fitzpatrick FA 1994 5 Lipoxygenase contains a functional Src homology 3 binding motif that interacts with the Src homology 3 domain of Grb2 and cytoskeletal proteins J Biol Chem 269 39 24163 24168 doi 10 1016 S0021 9258 19 51063 8 PMID 7929073 Shaw KJ Ng C Kovacs BW 1994 Cyclooxygenase gene expression in human endometrium and decidua Prostaglandins Leukot Essent Fatty Acids 50 5 239 243 doi 10 1016 0952 3278 94 90160 0 PMID 8066098 Maruyama K Sugano S 1994 Oligo capping a simple method to replace the cap structure of eukaryotic mRNAs with oligoribonucleotides Gene 138 1 2 171 174 doi 10 1016 0378 1119 94 90802 8 PMID 8125298 Woods JW Evans JF Ethier D Scott S Vickers PJ Hearn L Heibein JA Charleson S Singer II 1993 5 lipoxygenase and 5 lipoxygenase activating protein are localized in the nuclear envelope of activated human leukocytes J Exp Med 178 6 1935 1946 doi 10 1084 jem 178 6 1935 PMC 2191287 PMID 8245774 Mancini JA Li C Vickers PJ 1993 5 Lipoxygenase activity in the human pancreas J Lipid Mediat 8 3 145 150 PMID 8268460 VanderNoot VA Fitzpatrick FA 1995 Competitive binding assay of src homology domain 3 interactions between 5 lipoxygenase and growth factor receptor binding protein 2 Anal Biochem 230 1 108 114 doi 10 1006 abio 1995 1444 PMID 8585605 Brock TG McNish RW Bailie MB Peters Golden M 1997 Rapid import of cytosolic 5 lipoxygenase into the nucleus of neutrophils after in vivo recruitment and in vitro adherence J Biol Chem 272 13 8276 8280 doi 10 1074 jbc 272 13 8276 PMID 9079648 Nassar GM Montero A Fukunaga M Badr KF 1997 Contrasting effects of proinflammatory and T helper lymphocyte subset 2 cytokines on the 5 lipoxygenase pathway in monocytes Kidney Int 51 5 1520 1528 doi 10 1038 ki 1997 209 PMID 9150468 Suzuki Y Yoshitomo Nakagawa K Maruyama K Suyama A Sugano S 1997 Construction and characterization of a full length enriched and a 5 end enriched cDNA library Gene 200 1 2 149 156 doi 10 1016 S0378 1119 97 00411 3 PMID 9373149 External links editArachidonate 5 Lipoxygenase at the U S National Library of Medicine Medical Subject Headings MeSH Human ALOX5 genome location and ALOX5 gene details page in the UCSC Genome Browser Portal nbsp Biology Retrieved from https en wikipedia org w index php title Arachidonate 5 lipoxygenase amp oldid 1220330869, wikipedia, wiki, book, books, library,

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