Activation of Leukotriene Synthesis in Human Neutrophils by Exogenous Arachidonic Acid: Inhibition by Adenosine A2a Receptor Agonists and Crucial Role of Autocrine Activation by Leukotriene B4

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Vol. 56, Issue 5, 1055-1062, November 1999

Activation of Leukotriene Synthesis in Human Neutrophils by Exogenous Arachidonic Acid: Inhibition by Adenosine A_2a Receptor Agonists and Crucial Role of Autocrine Activation by Leukotriene B₄

Marc E. Surette, Eric Krump, Serge Picard, and Pierre Borgeat

Centre de Recherche en Rhumatologie et Immunologie, Centre de Recherche du Centre Hospitalier Universitaire de Québec, Pavillon CHUL and Faculté de Médecine, Université Laval, Quebec, Canada

	Summary

Top Abstract Introduction Experimental Procedures Results Discussion References

We report here that the apparent inability of isolated human polymorphonuclear leukocytes (PMNs) to efficiently transformarachidonic acid (AA) is the consequence of A_2a receptor engagementby endogenous adenosine accumulating in incubation media. Indeed,when adenosine is eliminated from PMN suspensions by the additionof adenosine deaminase, or when cells are incubated with adenosineA_2a receptor antagonists, important quantities (40-80 pmol/10⁶ cells) of 5-lipoxygenase products are synthesized by PMN incubatedwith 1 to 5 µM exogenous AA. The selective A_2a receptor agonistCGS21680 was a very potent inhibitor of the AA-induced leukotriene(LT) synthesis, showing an IC₅₀ of ~1 nM. The mechanism of AA-inducedstimulation of LT synthesis observed in the absence of extracellularadenosine was investigated. In adenosine deaminase-treated PMN,exogenous AA induced Ca²⁺ mobilization and the translocation of 5-lipoxygenase to nuclearstructures. A time lag of 20 to 60 s (variable between PMN preparations)was observed consistently between the addition of AA and the elevationof intracellular Ca²⁺ concentration (and LT synthesis), indicating that AA itself didnot trigger the Ca²⁺ mobilization in PMN. This AA-induced Ca²⁺ mobilization, as well as the corresponding 5-lipoxygenase translocationand stimulation of LT synthesis, was blocked efficiently by theLT synthesis inhibitor MK0591, the LTB₄ receptor antagonists CP105696and LY223982, and the LTA₄ hydrolase inhibitor SC57461A. Thesedata demonstrate that AA is a highly potent and effective activatorof LT synthesis and acts through a mechanism that requires anautocrine stimulatory loop by LTB₄.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

The stimulation of human leukocytes by various agents such as calcium ionophores, soluble agonists, or phagocytic stimuliresults in the biosynthesis of the bioactive arachidonic acid(AA)-derived leukotrienes (LTs). In human polymorphonuclear leukocytes(PMN), the major AA-derived metabolites synthesized are LTs A₄and B₄ (LTA₄, LTB₄); LTB₄ is one of the most potent naturallyoccurring leukocyte chemoattractants (Borgeat and Naccache, 1990).Its synthesis after cell stimulation is the result of the calcium-dependentrelease of AA from cellular phospholipids after the activationof phospholipase(s) (PL) A₂ and the stereospecific transformationof AA to 5-hydroperoxyeicosatetraenoic acid (5-HpETE) by the 5-lipoxygenase(5-LO) (Borgeat and Naccache, 1990)_. 5-HpETE then can be reducedto 5-hydroxyeicosatetraenoic acid (5-HETE) or converted furtherby 5-LO to LTA₄, which then is rapidly converted to LTB₄ by LTA₄hydrolase. LTB₄ and 5-HETE are both biologically active compoundsthat stimulate leukocytes by interacting with distinct cell surfacereceptors (Yokomizo et al., 1997).

In addition to being transformed to oxygenated metabolites, free AA generated by PL A₂ activity also is released from activatedcells in vitro and also has been measured in inflammatory foci(Barr et al., 1984; Lundy et al., 1990). This extracellular AAcan be utilized for LT biosynthesis by agonist-stimulated neutrophils;such transcellular metabolism of AA is believed to play an importantrole in the overall production of the lipid mediators of inflammation(Maclouf et al., 1989; Serhan and Sheppard, 1990). AA also canact as a multifunctional agonist because the addition of AA toPMN stimulates the mobilization of calcium, degranulation, andsuperoxide anion production (Smith et al., 1987).

It is now well documented that adenosine acting via its A_2a receptor is a potent suppressor of PMN functions (Cronstein etal., 1983; Newby et al., 1983; Cronstein, 1994; Krump et al.,1997). Recently, it has been shown that PMN suspensions releaseadenosine in quantities that can severely inhibit functional responsesto various agonists (Cronstein et al., 1983; Newby et al., 1983;Krump et al., 1997). In particular, the accumulation of adenosinein the incubation medium after a 30-min preincubation period at37°C nearly completely inhibits LTB₄ production by formyl-methionyl-leucyl-phenylalanine(fMLP)- or platelet-activating factor (PAF)- stimulated PMN (Krumpet al., 1997).

In the present study, we have investigated the impact of adenosine A_2a receptor occupancy on the ability of exogenous AA tostimulate PMN for 5-LO product synthesis. These studies revealthat in the absence of the suppressive effect of adenosine, AAis a highly potent and efficient activator of LT synthesis involvingan autocrine stimulatory loop that includes LTB₄ itself. Thesestudies indicate further that adenosine exerts its potent inhibitoryeffect on AA-induced LTB₄ synthesis by inhibiting the abilityof exogenous AA to activate cellular 5-LO. Finally, these resultssuggest that the pharmacological manipulation of adenosine levelsat inflammatory sites may have an important impact on the transcellularbiosynthesis of LT.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials. Fura-2-acetoxymethly ester (fura-2/AM), prostaglandin B₂ (PGB₂), 19-hydroxy-PGB₂, leupeptin, aprotinin, phenylmethanesulfonylfluoride (PMSF), adenosine deaminase (ADA), and horseradish peroxidase-linkeddonkey anti-rabbit antibodies were obtained from Sigma ChemicalCo. (St. Louis, MO). Methyl arachidonyl fluorophosphonate, AA,and 5,8,11,14,17-eicosapentaenoic acid (EPA) were obtained fromCayman Chemical Co. (Ann Arbor, MI). CGS21680 HCl and CGS15943were obtained from Research Biochemicals International (Natick,MA). CP105696 was a gift from Dr. Henry Showell (Pfizer, Groton,CT), and MK0591 was a gift from Dr. Robert Young (Merck Frosst,Dorval, Canada). BN50730, LY223982, and L659989 were obtainedfrom the Institut Henri Beaufour (Paris, France), Eli Lilly Laboratories(Indianapolis, IN), and Merck Sharp and Dohme (Rahway, NJ), respectively.SC57461A was a gift from Dr. Walter G. Smith (Searle & Co., Skokie,IL). Drug stock solutions were in dimethyl sulfoxide (DMSO) andwere added directly to cell suspensions; the maximal final concentrationof DMSO in the cell suspensions was 0.2%.

Rabbit polyclonal anti-5-LO (5-LO 32) was kindly supplied by Dr. Jillian F. Evans of Merck Frosst. The enhanced chemiluminescencedetection kit was obtained from Amersham Canada (Oakville, Ontario,Canada). Immobilon-P polyvinylidene difluoride blotting membranewas obtained from Millipore (Mississauga, Ontario, Canada). Ficoll-Paquewas obtained from Pharmacia (Montréal,Canada).

Isolated Cell Preparations. Venous blood was obtained from healthy donors and collected into 10-ml glass tubes (100 × 16 mm; Vacutainer, Becton Dickinson,Franklin Lakes, NJ) containing 143 USP units of heparin. PMN wereisolated from peripheral blood after dextran sedimentation andcentrifugation on Ficoll-Paque cushions (Pharmacia, Dorval, Canada),as described previously (Boyum, 1968). Final preparations contained95% PMN, and viability was >95% as assessed by trypan blueexclusion.

Stimulation of Cells and Analysis of 5-LO. The cells were suspended in Hanks' balanced salt solution (HBSS) (1 × 10⁷ cells/ml) at 37°C and stimulated with the indicated concentrationsof fatty acid for the indicated time periods. For experimentsin which cells were pretreated with ADA, 0.4 U ADA/ml was addedto the cell suspension 2 min before stimulation. In some experiments,cells were preincubated at 37°C with the indicated concentrationsof receptor agonists or antagonists before stimulation. For thedetermination of 5-LO products, reactions were stopped at theindicated times by the addition of 1 volume of ice-cold methanol/acetonitrile(1:1, v/v) containing 12.5 ng each of PGB₂ and 19-hydroxy-PGB₂as internal standards, and the samples were processed and analyzedby reversed-phase (RP) HPLC with the use of an on-line extractionprocedure, as described previously (Borgeat et al., 1990).

Preparation of Nuclei. For the preparation of nuclei, neutrophils (2 × 10⁷ cells/2 ml) incubated under the conditions described were pelleted andresuspended in 600 µl of ice-cold Nonidet P-40 lysis buffer containing0.1% Nonidet P-40, 10 mM Tris-HCl, pH 7.4, 10 mM NaCl, 3 mM MgCl₂,1 mM EDTA, 10 µg/ml leupeptin, 10 µg/ml aprotinin, and 1 mM PMSF(Pouliot et al., 1996). The cells were vortexed for 15 s, kepton ice for 5 min, and centrifuged at 300g (10 min, 4°C). The resultingsupernatants (i.e., the non-nuclear fractions) and pellets (thenuclei-containing fractions) then were solubilized immediatelyin electrophoresis sample buffer containing 62.5 mM Tris-HCl,pH 6.8, 2% SDS, 100 mM dithiothreitol, 10% glycerol, 0.01% bromophenolblue, 10 µg/ml leupeptin, 10 µg/ml aprotinin, and 1 mM PMSF) andboiled for 5 min. Samples were analyzed by SDS-polyacrylamidegel electrophoresis, as described by Laemmli (1970) on 9% acrylamidegels. Proteins then were transferred at 0.5 A for 4 to 15 h at4°C onto an Immobilon-P polyvinylidene difluoride blotting membrane.Transfer efficiency was visualized by Ponceau Red staining. Forthe determination of 5-LO, the membranes were soaked for 30 minat 25°C in Tris-buffered saline (25 mM Tris-HCl, pH 7.6, 0.2 MNaCl, 0.15% Tween 20) containing 5% dried milk (w/v), blottedwith anti-5-LO, and revealed using a horseradish peroxidase-coupledmonoclonal antibody and the enhanced chemiluminescence detectionkit.

Measurement of Intracellular Calcium Concentration [Ca²⁺]_i. Fura-2 fluorescence was monitored, as described previously (Faucher and Naccache, 1987). Briefly, cells (1 × 10⁷/ml) were incubated for 30 min with 1 µM fura-2 AM at 37°C. Thecells then were washed, resuspended at 5 × 10⁶/ml, and transferred into the thermally controlled (37°C) andmagnetically stirred cuvette compartment of the spectrofluorometer(Aminco-Bowman series 2, SLM-Aminco, Urbana, IL). The excitationand emission wavelengths for Ca²⁺ measurements were 340 and 510,respectively.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

The Transformation of AA by 5-LO in Human PMN Is Inhibited by Endogenous Adenosine. A first series of experiments was designed to determine whether endogenous adenosine in isolated PMN preparations interfereswith the transformation of exogenous AA into 5-LO products. Itwas shown previously that isolated PMN release endogenous adenosineinto the incubation medium in a time- and cell concentration-dependentmanner and that this release affects cell functions (Cronsteinet al., 1983; Newby et al., 1983; Krump et al., 1997). As canbe seen on the HPLC chromatogram in Fig. 1A, the addition of 3µM AA to isolated PMN resulted in the synthesis of small amountsof LTB₄ and its $omega$ -oxidation products 20-hydroxy-LTB₄ (20-OH-LTB₄)and 20-carboxy-LTB₄ (20-COOH-LTB₄). This is in accord with resultsof many previous reports that AA is a weak stimulus for LT synthesisand that the threshold concentration of AA required to inducebasal LTB₄ synthesis is in the range of 3 to 10 µM (Clancy etal., 1983; McColl et al., 1989). However, when cells were pretreatedwith the adenosine A_2a receptor antagonist CGS15943 (Ghai et al.,1987), the capacity of the cells to synthesize LTB₄, its $omega$ -oxidationproducts, and the nonenzymatic hydrolysis products of LTA₄, 6-trans-LTB₄and 12-epi-6-trans-LTB₄, in response to 3 µM AA was greatly enhanced(greater than 10-fold), as shown in Fig. 1B. The cells' capacityto respond to exogenous AA was similarly enhanced when adenosinewas removed enzymatically from the incubation medium by the additionof ADA (Fig. 1C). However, when the adenosine A_2a receptor agonistCGS21680 was included in these incubations containing ADA, theenhanced response to AA was reversed (Fig. 1D). In fact, the adenosineA_2a receptor agonist CGS21680 was shown to be a very potent inhibitor(IC₅₀ of ~1 nM) of the AA-induced synthesis of 5-LO products inPMN (treated with ADA) (Fig. 2).

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Fig. 1. RP-HPLC chromatograms of eicosanoids from human PMN treated with exogenous AA. PMN (1 × 10⁷/ml) were preincubated for 5 min at 37°C in HBSS (A), in HBSS containing 1 µM CGS15943 (B), in HBSS containing 0.4 U/ml ADA (C), or in HBSS containing adenosine deaminase and 0.1 µM CGS21680 (D). The cells then were stimulated for 5 min with 3 µM AA and the reactions stopped by the addition of organic solvents containing the internal standards PGB₂ and 19-OH-PGB₂ (12.5 ng each), as described in Experimental Procedures. LTB₄, its $omega$ -oxidation products 20-OH-LTB₄ and 20-COOH-LTB₄, and the nonenzymatic hydrolysis products of LTA₄ (6-trans-LTB₄ and 12-epi-6-trans-LTB₄) were analyzed by RP-HPLC, as described in Experimental Procedures. Attenuation setting of the UV detector was 0.01 absorbance unit at full scale at 280 nm.

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Fig. 2. The effect of CGS21680 on the biosynthesis of 5-LO products by human PMN stimulated with exogenous AA. PMN (1 × 10⁷/ml) were preincubated at 37°C for 5 min in HBSS containing ADA (0.4 U/ml) and the indicated concentrations of CGS21680. The cells then were stimulated for 5 min with 3 µM AA and the reactions stopped by the addition of organic solvents containing the internal standards PGB₂ and 19-OH-PGB₂ (12.5 ng each), and 5-LO products were determined by RP-HPLC, as described in Experimental Procedures. The data show the relative amounts of LTB₄ and its metabolites generated. Values are the means ± S.E. of three separate experiments, each performed in duplicate.

In a parallel set of experiments, washing cells by centrifugation followed by immediate resuspension in prewarmed HBSS (37°C)and stimulation with 3 µM AA also resulted in an enhanced capacityto synthesize 5-LO products. When the washed cells (1 × 10⁷/ml) were allowed to incubate at 37°C for as little as 3 min beforestimulation, their response to AA was reduced to 60 to 70% ofthat of freshly washed cells and, within 15 min, the enhancedcapacity to respond had all but disappeared (data not shown).Therefore, the removal of endogenous adenosine by washing thecells, by the action of added ADA or the treatment of cells withthe A_2a receptor antagonist, resulted in a greatly enhanced abilityof the cells to synthesize 5-LO products in response to low micromolarconcentrations of exogenous AA.

Kinetics of the Synthesis of 5-LO Products. The synthesis of 5-LO products normally requires both AA release from phospholipids and activation of the 5-LO enzyme. However,because substrate availability should not be limiting when exogenousAA is added to the incubation media (as in the present experimentalconditions), the kinetics of the synthesis of 5-LO products undersuch conditions are likely only reliant on 5-LO activation. Thekinetics of 5-LO product synthesis in PMN exposed to AA in thepresence of ADA were evaluated; as can be seen in Fig. 3A, a lagperiod of approximately 40 s transpired before a measurable synthesisof 5-LO products could be detected, although the substrate AAshould be available immediately for transformation. This observedlag period varied between 20 and 60 s, depending on the PMN preparation.The addition of 3 µM AA to PMN induced a synthesis of 5-LO productsthat was maximal within 2 min. The decrease observed in the quantitiesof detectable 5-HETE when incubations are extended to >3 min isbecause 5-HETE is efficiently acylated into cellular glycerolipids(Stenson and Parker, 1979).

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Fig. 3. The kinetics and dose-response to exogenous AA for the biosynthesis of 5-LO products in human PMN. PMN (1 × 10⁷/ml) were preincubated at 37°C for 2 min in HBSS containing ADA (0.4 U/ml). A, cells were stimulated with 3 µM AA and, at the indicated times reactions, were stopped by the addition of organic solvents.

, LTB₄; $open circle$ , 5-HETE. B, cells were stimulated with the indicated concentrations of AA for 7 min and reactions stopped by the addition of organic solvents. LO products were determined by RP-HPLC, as described in Experimental Procedures.

, 5-LO products; $open circle$ , 15-HETE. Values for 5-LO products represent the sum of LTB₄, its $omega$ -oxidation products 20-OH-LTB₄ and 20-COOH-LTB₄, and the nonenzymatic hydrolysis products of LTA₄ (6-trans-LTB₄ and 12-epi-6-trans-LTB₄). Values are the means ± range of duplicate incubations from one experiment, which is representative of four separate experiments.

Figure 3B shows that when cells were stimulated with various concentrations of AA for 5 min, the optimal concentration for5-LO product synthesis was 3 µM. When the incubations containedthe higher AA concentrations of 10 to 30 µM, the cells eventuallysynthesized larger amounts of 5-LO products, but only after a15- to 20-min incubation period (data not shown). Another differencein the response to higher concentrations of AA is the synthesisof increasing quantities of the 15-LO product 15-HETE.15-HETEis known to exhibit inhibitory effects on PMN functions includingLT synthesis (Borgeat et al., 1983

). Therefore, its synthesismay be partially responsible for the slower accumulation of 5-LOproducts at high AAconcentrations.

LTB₄ Receptor Antagonists and an LTA₄ Hydrolase Inhibitor Block the AA-Induced Synthesis of 5-LO Products. Although no specific cell surface receptor capable of transmitting a signal has been described for fatty acids including AA,previous studies have shown that AA-induced signals can be blockedwith pertussis toxin, suggesting that AA may act either directlyor indirectly via G protein-coupled receptors (McColl et al.,1989). It also has been suggested that these may be LTB₄ receptors(Naccache et al., 1989). To determine whether the induction of5-LO product synthesis by AA may involve the LTB₄ receptor, PMNwere preincubated for 2 min with two different LTB₄ receptor antagonists,CP105696 and LY223982, before cell stimulation in the presenceof ADA. Figure 4 shows that both LTB₄ receptor antagonists blockedthe synthesis of 5-LO products induced by AA at concentrationsthat are consistent with their previously reported IC₅₀ for inhibitingPMN responses to LTB₄ (74 nM for LY223982 and 5 nM for CP105696)(Jackson et al., 1992; Showell et al., 1995). When AA was addedalong with the agonists fMLP and PAF, which stimulate PMN viatheir own receptors, LTB₄ receptor antagonists were without effecton 5-LO product synthesis, indicating that LTB₄ receptor antagonistswere acting in a receptor-specific manner (data not shown). Theseresults suggest that either AA itself can act as an agonist ofthe LTB₄ receptor or that small amounts of LTB₄ generated in responseto AA can then act in an autocrine manner on its receptor andstimulate the cell for a more important biosynthesis of 5-LO products.This hypothesis of an autocrine stimulation of the PMN by endogenousLTB₄ was verified further by using the LTA₄ hydrolase inhibitorSC57461A. As can be seen in Fig. 5A, pretreatment of PMN withSC57461A inhibited in a dose-dependent manner the ability of exogenousAA to induce the synthesis of all 5-LO products (including 5-HETEand 6-trans isomers of LTB₄, whose synthesis is not dependenton LTA₄-hydrolase activity), indicating that the transformationof LTA₄ to LTB₄ is absolutely required for the AA-induced synthesisof 5-LO products in the experimental conditions used. In contrast,when SC57461A-treated PMN were stimulated with the calcium ionophoreA23187, only LTB₄ synthesis was blocked, not that of LTA₄ (asevidenced by the detection of its nonenzymatic hydrolysis products6-trans-LTB₄ and 12-epi-6-trans-LTB₄) or 5-HETE (Fig. 5B). Thisis in agreement with our previous report that endogenous LTB₄does not exert a significant autocrine stimulatory effect on LTsynthesis in human PMN stimulated with 1 µM A23187 (McDonald etal., 1994).

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Fig. 4. Effect of LTB₄ receptor antagonists on the synthesis of 5-LO products in PMN stimulated with exogenous AA. PMN (1 × 10⁷/ml) were preincubated at 37°C for 5 min in HBSS containing ADA (0.4 U/ml) and the indicated concentrations of LTB₄ receptor antagonists. Cells then were stimulated with 3 µM AA for 7 min and the reactions stopped by the addition of organic solvents, and 5-LO products were determined by RP-HPLC, as described in Experimental Procedures. Values represent the sum of LTB₄, its $omega$ -oxidation products, and the nonenzymatic hydrolysis products of LTA₄. Values are the means ± S.D. of triplicate incubations from one experiment, which is representative of four separate experiments.

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Fig. 5. Effect of SC57461A on the biosynthesis of 5-LO products in PMN stimulated with exogenous AA or ionophore A23187. PMN (1 × 10⁷/ml) were preincubated for 5 min at 37°C in HBSS containing 0.4 U/ml ADA and SC57461A at the indicated concentrations. The cells then were stimulated for 5 min with 3 µM AA (A) or 1 µM A23187 (B), and the reactions were stopped by the addition of organic solvents containing the internal standards PGB₂ and 19-OH-PGB₂ (12.5 ng each), as described in Experimental Procedures. LTB₄ and its $omega$ -oxidation products 20-OH-LTB₄ and 20-COOH-LTB₄ ( $diamond$ , the nonenzymatic hydrolysis products of LTA₄ (6-trans-LTB₄ and 12-epi-6-trans-LTB₄) (

), and 5-HETE (

)were analyzed by RP-HPLC, as described in Experimental Procedures. Values are the means ± S.D. of triplicate incubations from one experiment, which is representative of three separate experiments.

AA Induces the Translocation of 5-LO to the Nucleus. One of the features of 5-LO activation after stimulation of human PMN is the translocation of the enzyme from the cytosolto the nuclear envelope where the 5-LO activating protein is present(Woods et al., 1993; Pouliot et al., 1996). Therefore, the translocationof 5-LO to the nucleus after activation of PMN by AA was assessedin cells treated with ADA alone and in combination with the adenosineA_2a receptor agonist CGS21680. Figure 6 shows that the stimulationof human PMN with 5 µM AA efficiently induces the translocationof 5-LO to the nucleus. Importantly, when cells were preincubatedwith the 5-LO activating protein antagonist MK0591, both 5-LOproduct biosynthesis and 5-LO translocation were inhibited. Stimulationof the adenosine A_2a receptor with the agonist CGS21680 also completelyblocked AA-induced translocation of 5-LO and 5-LO product synthesis.Similarly, the LTB₄ receptor antagonist CP105696 also blockedthe translocation of 5-LO, supporting the idea that a signal transmittedthrough this receptor is required for the AA-induced translocationof 5-LO. This is consistent with the effects of this antagoniston LTB₄ synthesis (Fig. 4). As with the biosynthesis of 5-LO products,the PAF receptor antagonist BN50730 did not block 5-LO translocationinduced by AA.

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Fig. 6. 5-LO product synthesis and immunoblot analysis of 5-LO translocation to nuclei in AA-stimulated human PMN. Human PMN were pretreated for 5 min with ADA (0.4 U/ml) and the indicated compounds (0.1 µM), except for BN50730, which was at 1.0 µM. Cells then were stimulated with 3 µM AA for 5 min and centrifuged, and the supernatants were evaluated for 5-LO products. Nuclei were isolated from the cell pellets and prepared for gel electrophoresis and immunoblot analysis, as described in Experimental Procedures. Each lane was loaded with nuclei obtained from 15 × 10⁶-cell equivalents of PMN. Results are from one experiment, which is representative of four separate experiments

AA Induces Calcium Mobilization: Effect of CGS21680, MK0591, CP105696, and SC57461A. The mechanism of the stimulation of 5-LO product biosynthesis by exogenous AA in human PMN and the inhibitory effects of adenosineon this process was investigated further in Ca²⁺ mobilization studies. As shown in Fig. 7, stimulation of PMNwith 3 µM AA induced a transient elevation of [Ca²⁺]i; furthermore, as observed in the kinetics of AA-induced 5-LOproduct biosynthesis, a 20- to 60-s lag was observed between thetime of addition of AA to the PMN suspensions and the elevationof intracellular Ca²⁺ concentrations, clearly indicating that AA does not directlytrigger the Ca²⁺ mobilization, and supporting a causal relationship between theseevents. The treatment of cells with CGS21680 resulted in a profoundinhibition of the biosynthesis of 5-LO products and 5-LO translocationinduced by AA; similarly, the adenosine A_2a receptor agonist CGS21680showed a concentration-dependent inhibitory effect on the Ca²⁺ transient induced by AA (Fig. 7A).

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Fig. 7. Effect of CGS21680, CP105696, MK0591, and SC57461A on AA-induced calcium mobilization in human PMN. Fura-2-loaded PMN (5 × 10⁶/ml) in HBSS were preincubated for 5 min at 37°C with ADA (0.4 U/ml) in the presence of CGS21680 at 0, 10, and 100 nM (A); CP105696 at 0, 1, and 10 nM (B); MK0591 at 0, 10, and 100 nM (C); and SC57461 at 0, 10, and 100 nM (D) before stimulation with 3 µM AA. Unstimulated cells (dotted lines) were incubated with diluent only (0.1% DMSO). $down-arrow$ indicate the time of AA additions; the fluorescence was monitored at the excitation and emission wavelengths of 340 nm and 510 nm, respectively, as described in Experimental Procedures. The results are representative of two to five separate experiments. Full traces indicate no drug added; dashed lines, low drug concentrations; interrupted lines, high drug concentrations.

The LTB₄ receptor antagonist CP105696, which effectively blocked both AA-induced 5-LO product biosynthesis and 5-LO translocation,was also investigated for its effect on Ca²⁺ mobilization. As shown in Fig. 7B, blocking the LTB₄ receptoralso completely prevented the AA-induced mobilization of Ca²⁺. When cells were treated with the 5-LO biosynthesis inhibitorMK0591 or with the LTA4 hydrolase inhibitor SC57461A, calciummobilization also was completely blocked (Fig. 7, C and D). Theseresults demonstrate that the synthesis of a 5-LO product is involvedin AA-induced calcium mobilization and that LTB₄ itself ultimatelystimulates PMN in an autocrine manner. Thus, the data also suggestthat engagement of the A_2a receptor blocks AA-induced LT biosynthesisby preventing the autocrine activation of the PMN by LTB₄.

EPA Is a Weak Stimulus of Ca²⁺ Mobilization and 5-LO Product Biosynthesis. Another polyunsaturated fatty acid, EPA, which is also a substrate for 5-LO, was evaluated for its ability to induce the biosynthesisof 5-LO products in human PMN. Despite the fact that EPA is asgood a substrate for 5-LO as is AA (Lee et al., 1984), the additionof 1 to 5 µM EPA to ADA-treated PMN resulted in little or no detectablesynthesis of its 5-LO products (data not shown). Accordingly,EPA also was a much weaker stimulus than AA for the inductionof Ca²⁺ mobilization in PMN (data not shown). Such data are entirelycompatible with the hypothesis proposed above, inasmuch as LTB₅,the product of EPA transformation by 5-LO, is a much weaker (25-fold)agonist of the LTB₄ receptor (as assessed by Ca²⁺ mobilization in human PMN) (Powell et al., 1996), which likelyexplains the inability of EPA to trigger the formation of 5-LOproducts. Interestingly, the addition of small concentrations(1 nM) of exogenous LTB₄ to ADA-treated PMN exposed to 5 µM EPAresulted in an enhanced biosynthesis of 5-LO products from EPA(26 ± 2 pmol/10⁶ cells, n =3).

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

The incubation of isolated human PMN in vitro results in the rapid accumulation of endogenous adenosine, which has profoundinhibitory effects on many cell functions, including LT synthesis.In the present study, we show that when endogenous adenosine iseliminated enzymatically from PMN suspensions, or its actionsblocked with receptor antagonists, human PMN respond very stronglyto low micromolar concentrations of AA for the synthesis of 5-LOproducts. This observation contrasts with the widely held perceptionthat resting human PMN respond poorly to exogenous AA for LTB₄synthesis and that the measurable synthesis of 5-LO products inthe presence of AA requires the simultaneous stimulation withanother agonist. Thus, our studies establish clearly that AA cantrigger, in the absence of other added PMN stimuli, an importantgeneration of 5-LO products and that the effect of exogenous AAis highly sensitive to the inhibitory effect of adenosine A_2areceptor engagement on PMN. Therefore, these findings are in linewith our previous observations that A_2a receptor agonists as wellas endogenous adenosine accumulating in PMN suspensions down-regulateagonist-induced LT biosynthesis in PMN (Krump et al., 1996, 1997)and add to the potential importance of adenosine as a naturalregulator of LTsynthesis.

The present observation that PMN do efficiently utilize exogenous AA (when released from the inhibitory constraint of adenosine)strongly supports the concept that the transcellular metabolismof exogenous AA by PMN could be an important source of biologicallyactive eicosanoids such as lipoxins and LTs at inflammatory sites.Indeed, PMN can be exposed to elevated concentrations of freeAA on close contact with activated cells releasing AA into theextracellular milieu. Such transcellular metabolism of AA hasbeen shown to be an important pathway for the synthesis of a numberof AA metabolites. In particular, AA released by stimulated plateletscan be utilized by stimulated PMN for LTA₄ and LTB₄ synthesis(Palmantier and Borgeat, 1991), whereas LTA₄ released by stimulatedPMN can be converted to lipoxins by the platelet 12-LO (Serhanand Sheppard, 1990). Thus, the present data indicate that PMNlikely utilize exogenous AA in a much more efficient manner thanwas thought previously. In fact, the quantities of LTB₄ producedby PMN in the presence of 3 µM AA (without the addition of otherstimulatory agents) exceed the quantities reported previouslyunder most conditions of PMN stimulation involving priming agentsand receptor-mediated agonists that activate PL A₂ and 5-LO forLT synthesis (Dahinden et al., 1988; Surette et al., 1998). Moreover,such efficient utilization of exogenous AA may take place in pathologicalsituations in which secreted PL(s) A₂ accumulation and associatedAA release occur, such as in adult respiratory distress syndrome,in the synovial fluid of arthritic patients, and in the asthmaticlung (Nevalainen, 1993). The two potent anti-inflammatory drugsmethotrexate and sulfalazine have been shown to promote adenosineaccumulation at inflammatory sites (Cronstein, 1995), an effectbelieved to be involved in their anti-inflammatory activity. Therefore,our data support the concept that the pharmacologically mediatedaccumulation of adenosine in inflammatory sites constitutes apromising approach for the treatment of inflammatory diseases,inasmuch as LTB₄ might play important roles in some diseasestates.

AA-induced 5-LO product biosynthesis showed intriguing features that suggested a role of de novo synthesized LTB₄ in the activationof PMN. Indeed, our data demonstrate that the observed biosynthesisof 5-LO products in response to exogenous AA involves an absoluterequirement for an autocrine/paracrine activation of the PMN byendogenous LTB₄, resulting in Ca²⁺ release from intracellular stores, the translocation and activationof 5-LO, and the important transformation of exogenous AA into5-LO products (Fig. 8). Several lines of evidence support thismechanism. First, the addition of AA to PMN did not result inan immediate mobilization of Ca²⁺ or synthesis of 5-LO products, because a lag of 20 to 60 s (variablebetween PMN preparations) was observed consistently. This indicatesthat AA itself is not acting directly in a receptor-dependentmanner as is observed when cells are stimulated with agonistssuch as fMLP, PAF, or LTB₄. Second, blocking the LTB₄ receptorwith specific receptor antagonists strikingly inhibited the AA-induceddelayed mobilization of Ca²⁺, 5-LO translocation, and the delayed biosynthesis of 5-LO products.This suggests that LTB₄ receptor occupation is required for AA-inducedPMN stimulation leading to 5-LO translocation and activation.Third, the specific LT synthesis inhibitor MK0591 also inhibitedthe mobilization of calcium, clearly indicating that 5-LO activityis required for this response to exogenous AA. That LTB₄ itselfis responsible for this autocrine effect is supported furtherby studies with the LTA₄ hydrolase inhibitor SC57461A, which preventsthe transformation of LTA₄ to LTB₄, but not the synthesis of other5-LO product such as 5-HETE. In the present studies, SC57461Ainhibited AA-induced synthesis of all 5-LO products and Ca²⁺ mobilization in PMN, indicating that LTB₄ formation is specificallyrequired for these responses to exogenous AA. Additional evidencethat an initial biosynthesis of LTB₄ is required for the furtherbiosynthesis of large amounts of 5-LO products on the additionof AA to ADA-treated cells was obtained by using EPA instead ofAA in similar experiments. Indeed EPA, which is as good a substratefor 5-LO as AA (Lee et al., 1984), did not induce an importantsynthesis of its 5-LO products (such as LTB₅) when added to PMN.This is likely because LTB₅, which is a much weaker agonist thanLTB₄ for the LTB₄ receptor, did not induce cell activation asmeasured herein by Ca²⁺ mobilization. Altogether, these observations point to a requirementfor an initial LTB₄ synthesis in response to exogenous AA, whichtriggers through an autocrine/paracrine mechanism the full activationof PMN for 5-LO product synthesis.

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Fig. 8. Hypothetical mechanism of 5-LO product biosynthesis involving autocrine activation by LTB₄ in PMN exposed to exogenous AA. Unstimulated PMN exposed to AA generate LTA₄ and LTB₄; this initial synthesis might involve a small quantity of 5-LO present on the nuclear envelope and is likely Ca²⁺-independent (Skorey and Gresser, 1998

). The LTB₄ generated initially then plays a pivotal role in activating further the PMN through engagement of the LTB₄ receptors, which results in Ca²⁺ release from intracellular stores, stimulation of the translocation of cytosolic 5-LO, and enhanced LTA₄ and LTB₄ biosynthesis from exogenous AA. In these experimental conditions, this autocrine/paracrine stimulatory loop by endogenous LTB₄ is required for the full activation of LT biosynthesis by exogenous AA, as demonstrated by the almost complete inhibition of 5-LO product formation by LTB₄ receptor antagonists and an LTA₄-hydrolase inhibitor. Engagement of the A_2a receptor appears to interfere with the autocrine/paracrine activation loop by inhibiting 5-LO translocation (through a yet-unidentified mechanism; see Discussion).

This scheme of events in AA-induced 5-LO product biosynthesis (Fig. 8) implies that the initial synthesis of LTB₄ responsiblefor the autocrine/paracrine activation of the PMN can occur inthe absence of a measurable Ca²⁺ mobilization. In support of such a mechanism, a recent reportindicated that in the presence of phosphatidylcholine-rich phospholipidvesicles, the 5-LO catalyzes the conversion of AA in the absenceof Ca²⁺ (Skorey and Gresser, 1998). Therefore, it seems reasonable tospeculate that the small amount of 5-LO detected in/on the nucleiof unstimulated PMN (Fig. 6) (Surette et al., 1998) could generatethe small amounts of LTA₄ required to initiate the activationof the PMN through engagement of LTB₄ receptors. The 20- to 60-seclag observed in these experiments between addition of AA and theoccurrence of 5-LO product biosynthesis may reflect the time requiredfor the hydroperoxide-mediated activation of the 5-LO, i.e., theoxidation of the nonheme iron of 5-LO (Chasteen et al., 1993).A similar time lag has been observed between PMN stimulation withagonists (GM-CSF/PAF or fMLP) or ionophore A23187 and the occurrenceof LT biosynthesis (Krump and Borgeat, 1994).

Finally, it is noteworthy that the present studies with this particular model (AA-induced LT biosynthesis) unraveled an additionalinhibitory mechanism of A_2a receptor engagement on LT synthesisin PMN. In previous studies, it was clearly established that theA_2a receptor agonist CGS21680 is a potent inhibitor of AA releasein agonist-activated human PMN (Krump et al., 1999), stronglysupporting that such a mechanism was involved in the inhibitoryeffects of the adenosine analog on LT synthesis. Because in theseand other previous studies, the inhibition of AA release alsowas observed with a variety of other agents known to cause anelevation of intracellular cAMP in PMN (E-type prostaglandins,the $beta$ -adrenergic agent isoproterenol, and the type IV phosphodiesteraseinhibitor Rolipram (Schering AG, Berlin, Germany) (Ham et al.,1983; Fonteh et al., 1993; Krump et al., 1999), it was proposedthat the effect of CGS21680 on AA release was cAMP-dependent.In the present studies, it is demonstrated that CGS21680 is apotent inhibitor of LT synthesis, even under conditions of PMNstimulation by exogenous substrate (AA), clearly indicating anothersite of action of A_2a receptor agonists in the inhibition of LTsynthesis. CGS21680 does not inhibit the release of Ca²⁺ from intracellular stores induced by LTB₄ in human PMN (datanot shown). However, as shown herein, CGS21680 interferes withthe activation/translocation process of the 5-LO. Hypothetically,A_2a receptor engagement might down-regulate phosphorylation eventsnecessary for 5-LO translocation; indeed, recent studies by Lepleyet al. (1996) described the inhibitory effects of various tyrosinekinase inhibitors on LT synthesis and 5-LO phosphorylation andtranslocation in human PMN. Studies are in progress to definefurther the molecular events involved in the inhibition of AArelease and 5-LO activation by A_2a agonists in humanneutrophils.

	Acknowledgments

We acknowledge the technical assistance of Nathalie Jean and TaniaLevesque.

	Footnotes

Received May 24, 1999; Accepted August 2, 1999

These studies were supported by grants from The Arthritis Society of Canada and The Medical Research Council of Canada. P.B.and M.E.S. are recipients of scholarships from Le Fonds de laRecherche en Santé du Québec. These studies were presented inpart at Experimental Biology '99, April 18, 1999, Washington,DC.

Send reprint requests to: Dr. Pierre Borgeat, Centre de Recherche en Rhumatologie et Immunologie, Centre Hospitalier Universitaire de Québec, Pavillon CHUL, 2705 Boul. Laurier, Room T 1-49, Ste-Foy, Québec, G1V 4G2, Canada. Email: pierre.borgeat{at}crchul.ulaval.ca

	Abbreviations

AA, arachidonic acid; PMN, polymorphonuclear leukocytes; ADA, adenosine deaminase; fura-2-acetoxymethly ester (fura-2/AM), 5-LO, 5-lipoxygenase; LT, leukotriene; 5-HpETE, 5-hydroperoxyeicosatetraenoic acid; 5-HETE, 5-hydroxyeicosatetraenoic acid; PG, prostaglandin; PMSF, phenylmethanesulphonyl fluoride; EPA, 5,8,11,14,17-eicosapentaenoic acid; 20-OH-LTB₄, 20-hydroxy-LTB₄; 20-COOH-LTB₄, 20-carboxy-LTB₄; DMSO, dimethyl sulfoxide; RP, reversed phase; HBSS, Hanks' balanced salt solution; PL, phospholipase; fMLP, formyl-methionyl-leucyl-phenylalanine; PAF, platelet-activating factor; PGB₂, prostaglandin B₂.

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