Losartan, a Selective Inhibitor of Subtype AT1 Receptors for Angiotensin II, Inhibits the Binding of N-Formylmethionyl-leucyl-phenylalanine to Neutrophil Receptors

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LOSARTAN POTASSIUM

Vol. 281, Issue 2, 624-628, 1997

Losartan, a Selective Inhibitor of Subtype AT1 Receptors for Angiotensin II, Inhibits the Binding of N-Formylmethionyl-leucyl-phenylalanine to Neutrophil Receptors¹

Silvina Raiden , Mirta Giordano, Graciela Andonegui, Analía S. Trevani, Daniel H. López, Victor Nahmod and Jorge R. Geffner

Laboratorio de Inmunología, Instituto de Investigaciones Hematológicas, Academia Nacional de Medicina (S.R., M.G., G.A., A.S.T., D.H.L., J.R.G.), and Instituto de Investigaciones Médicas, Facultad de Medicina, Universidad de Buenos Aires (S.R., V.N.), Buenos Aires, Argentina

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

Losartan, a selective antagonist of AT1 receptors for angiotensin II, is widely used clinically to manage hypertension. Wereport here that losartan markedly inhibits neutrophil shape change,adherence and chemiluminescence responses triggered by N-formylmethionyl-leucyl-phenylalanine(fMLP), without affecting responses induced by immune complexes,zymosan or concanavalin A. Neither saralasin, another antagonistof angiotensin II receptors, nor captopril, an angiotensin-convertingenzyme inhibitor, reproduced the effects of losartan. It was alsoobserved that neutrophil responses triggered by fMLP were notaffected by exogenously added angiotensin II. The effect of losartanon the binding of fMLP was measured using [³H]fMLP. It was found that losartan inhibits the binding of [³H]fMLP to neutrophil receptors. As observed for neutrophils, studiesperformed with monocytes showed that losartan inhibits chemiluminescenceemission triggered by fMLP, without affecting chemiluminescenceresponses triggered by immune complexes, zymosan or concanavalinA.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

The renin-angiotensin system is a bioenzymatic cascade in which renin acts on angiotensinogen to form angiotensin I, whichis then converted by ACE to AII. AII is an important moleculecontrolling blood pressure and volume in the cardiovascular system.Its importance is manifested by the efficacy of ACE inhibitorsin the treatment of hypertension and congestive heart failure(Peach, 1977; Vidt et al., 1982; Smith et al., 1992). ACE inhibitorsare widely used in therapy, and many nonpeptide AII receptor antagonistsare in various stages of clinical development, with losartan beingthe first such drug available for clinical use since 1990 (Testaet al., 1993; Keilani et al., 1995; Johnston, 1995; Clauser etal., 1996). Losartan, moreover, has become the prototypical toolused to determine the role of AII in biological systems and isthe reference standard for AT1 receptors (Timmermans et al., 1993).

Previous work has shown that mononuclear phagocytes synthesize angiotensinogen, angiotensin I and AII and express receptorswith high affinity for AII (Thomas and Hoffman, 1984; Gomez etal., 1993; Kitazono et al., 1995; Suzuki et al., 1995). AII appearsto be able to modulate mononuclear phagocyte functions. In thisregard, Dezsö and Fóris (1981) and Fóris et al. (1983) showedthat AII regulates the activity of receptors for the Fc fragmentof IgG, whereas Hahn et al. (1994) found that AII stimulates tumornecrosis factor- $alpha$ production.

Leukocytes migrate from the blood to sites of inflammation in response to locally produced chemoattractants that activatespecific cell surface receptors. All of these receptors, includingthe receptors for bacterial N-formyl peptides, belong to the classof G-protein-coupled seven-transmembrane domain receptors (Murphy,1994). AT1 receptors for AII also belong to this family of receptors(Timmermans et al., 1993; Clauser et al., 1996). Moreover, a databasesearch revealed that the AT1 receptor for AII and the high affinityreceptor for fMLP share 25 to 30% sequence identity (Bernsteinand Alexander, 1992).

Considering the stimulatory activities of AII on mononuclear phagocyte responses and the relationship between the AT1 receptorfor AII and the high-affinity receptor for fMLP, we chose to initiateresearch to define whether AII may modulate neutrophil activationtriggered by the chemoattractant peptide fMLP. Unexpectedly, duringthe course of these experiments, we observed that losartan selectivelyinhibits neutrophil activation induced by fMLP, through a mechanismnot related to the ability of losartan to antagonize angiotensinreceptors.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Reagents. fMLP, AII, zymosan, Con A and saralasin were purchased from Sigma Chemical Co. (St. Louis, MO). Captopril was obtained fromSquibb Laboratory (Paris, France); losartan and [³H]fMLP were from DuPont (Boston, MA). Precipitating IC were preparedas previously described, using human IgG as antigen and rabbitIgG antibodies to human IgG (Schattner et al., 1993).

Preparation of neutrophils and monocytes. Blood samples were obtained from healthy donors who had taken no medication for at least 10 days before the day of sampling.Blood was obtained by venipuncture of the forearm vein, and itwas drawn directly into plastic tubes containing 3.8% sodium citrate(1:9, v/v). Human neutrophils were isolated by dextran sedimentationand Ficoll-Hypaque gradient centrifugation (Ficoll; Pharmacia,Uppsala, Sweden; Hypake; Winthrop Products Inc., Buenos Aires,Argentina), as described (Boyum, 1968). Contaminating erythrocyteswere removed by hypotonic lysis. After washing, the cells (>96%neutrophils in May Grunwald/giemsa-stained cytopreparations) wereresuspended at the desired concentration in RPMI 1640 medium (GIBCO,Detroit, MI). Peripheral blood mononuclear cells were harvestedfrom the interphase of the Ficoll-Hypaque gradient. After washing,the cells were resuspended in RPMI 1640 medium supplemented with10% heat-inactivated FCS (GIBCO), to a final concentration of5 × 10⁶ peripheral blood mononuclear cells/ml. Purified cells, containing95 to 98% mononuclear cells and 2 to 5% neutrophils, were placedin plastic Petri dishes that had been pretreated with autologousserum. After incubation for 2 hr at 37°C, nonadherent cells wereremoved by washing and adherent cells were detached with a rubberpoliceman and resuspended at the desired concentration in RPMI1640 medium. These cell suspensions contained 75 to 90% monocytes.

CL assays. Neutrophils and monocytes were suspended at 2.5 × 10⁶/ml in culture medium supplemented with 1% FCS. Luminescence responseswere measured with a Lumi-aggregometer (Chrono-Log Corp., Haverton,PA) at 1000 revolutions/min and 37°C, in the presence of luminol(0.1 µM), as previously described (Geffner et al., 1993). In allcases, light emission was continuously registered for 10 min.Data are expressed as the maximum response observed during thisperiod, in relative CL units. One CL unit was defined as 1-cmshifting of the light emission signal on the paper recorder.

Neutrophil adherence. Adherence was assessed as previously described (Geffner et al., 1991). Briefly, neutrophils were suspended in RPMI 1640 mediumsupplemented with 1% FCS and were labeled with Na₂CrO₄ (1 µCi/10⁶ cells) for 1 hr at 37°C. The cells were then washed four timeswith saline and resuspended in RPMI 1640 medium supplemented with10% FCS, to a density of 4 × 10⁶ cells/ml. One hundred microliters of this suspension were addedto each well in 96-well, flat-bottomed, polystyrene plates. Neutrophilswere incubated in the presence or absence of different compoundsfor 30 min at 37°C in 5% CO₂/95% humidified air and were washedthree times with culture medium to remove nonadherent neutrophils.Adherent neutrophils were then lysed with 1 N NH₄OH, and the radioactivitypresent in the lysates was measured. Cell adherence was expressedas the number of neutrophils that remained adherent to the plasticsurface after washing.

Shape change assay. This assay was performed as described previously (Craig Stocks et al., 1995). Briefly, neutrophils (1.5 × 10⁶) suspended in 100 µl of culture medium supplemented with 1% FCSwere incubated in the presence or absence of different compounds,in a shaking water bath, at 37°C for 15 min. After washing, cellswere suspended in phosphate-buffered saline and fixed by the additionof an equal volume of 0.5% glutaraldehyde in phosphate-bufferedsaline. Shape change was assayed in a fluorescence-activated cell-sortinganalyzer (Becton Dickinson Immunocytometry System, San Jose, CA).Results were expressed in mean forward light scatter units.

Neutrophil fMLP receptor binding assay. Binding of fMLP to neutrophil receptors was measured, as described previously (Weisbart et al., 1986), using [³H]fMLP (specific activity, 61.5 Ci/mmol). Increasing concentrationsof labeled peptide (2.5-80 nM final concentration) were addedto unstimulated neutrophils in the absence or presence of losartan(5 µg/ml). After 5 min at 22°C, radiolabeled fMLP and neutrophils(3 × 10⁶/tube, in a total volume of 250 µl) were incubated on a shakingplatform for 30 min in an ice bath. Nonspecific binding of [³H]fMLP to neutrophils was measured by mixing the radiolabeledligand with 10 µM unlabeled peptide and incubating the mixturefor 30 min in an ice bath. Nonspecific binding was similar inthe absence and presence of losartan (5 µg/ml) and accounted for $<=$ 11% of the binding. The values for nonspecific binding were subtractedfrom the corresponding values for total bound [³H]fMLP to yield the specifically bound radioligand. The numberof binding sites and the dissociation constant were determinedfrom a Scatchard plot analysis, using the computer program LIGAND(Munson and Rodbard, 1980).

Statistical analyses. Student's paired t test was used to determine the significance of differences between means, and P < .05 was taken as statisticallysignificant.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Effect of losartan on neutrophil responses triggered by different stimuli. The effect of losartan on neutrophil activation was examined by studying the following responses: CL emission, adherence andshape change. As shown in figure 1, responses induced by IC, zymosanand Con A were not affected by losartan, whereas responses inducedby fMLP were, in all cases, dramatically suppressed. A dose-responseexperiment is shown in figure 2. Doses of 5 µg/ml significantly(P < .01) inhibited CL and adherence responses triggered by 10nM fMLP. The ability of losartan to inhibit fMLP-triggered responseswas shown to be dependent on the concentrations of both losartanand fMLP. In fact, when CL responses induced by high concentrationsof fMLP (0.1 µM) were analyzed, it was observed that 10 µg/mllosartan was unable to exert any effect (data not shown). In contrast,with low concentrations of fMLP (1-3 nM), a significant inhibitionof CL (inhibition, 46 ± 9%; n = 6, P < .01) was observed at dosesof losartan as low as 0.5 µg/ml.

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Fig. 1. Effect of losartan on neutrophil responses triggered by different stimuli. CL emission (A), adherence (B) and shape change(C) were assessed as described in "Materials and Methods," inthe absence ( $square$ ) or presence (

) of losartan (10 µg/ml), whichwas added 5 min before the addition of stimuli. Results are expressedin relative CL units (RCLU), number of adherent cells and meanforward light scatter units (FSC), respectively. The followingstimuli were used: fMLP (10 nM), IC (50 µg/ml), zymosan (50 µg/ml)(Zy) and Con A (20 µg/ml). Data are expressed as the mean ± S.E.M.of 7 to 11 experiments performed in duplicate. *P < .005 vs. neutrophilsstimulated by fMLP in the absence of losartan.

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Fig. 2. Inhibition of fMLP-triggered neutrophil activation by different concentrations of losartan. CL emission ( $bullet$ ) and adherence( $open circle$ ) were triggered by fMLP (10 nM). Assays were performed as describedin "Materials and Methods." Percentages of inhibition were calculatedat each point by comparing the responses observed in the absenceand presence of losartan. Data are expressed as the mean ± S.E.M.of seven experiments performed in duplicate.

We then analyzed whether the effect of losartan on fMLP-triggered responses were related to its ability to antagonize AIIreceptors. To investigate this issue, the effects of saralasin,another inhibitor of AII receptors, and captopril, an ACE inhibitor,were assessed. Our results (fig. 3A) showed that these compoundsdid not affect fMLP-triggered responses, suggesting that the actionof losartan was not related to its ability to inhibit AII receptors.This presumption is also supported by results depicted in figure3B, showing that exogenously added AII exerted no effects on neutrophilactivation induced by fMLP.

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Fig. 3. Effect of saralasin, captopril and AII on neutrophil CL responses triggered by fMLP. A, CL responses measured in the absence( $square$ ) or presence of the renin-angiotensin system antagonists saralasin(

) and captopril (

) (5 µg/ml); B, responses measured in theabsence ( $square$ ) or presence of 1 µg/ml (

) and 0.01 µg/ml (

) AII.In all cases the drugs were added to neutrophils 5 min beforethe addition of fMLP. Data are expressed in relative CL unitsand represent the mean ± S.E.M. of five experiments performedin duplicate.

Effect of losartan on CL emission mediated by monocytes and triggered by different stimuli. In another set of experiments, we examined the effect of losartan on monocyte activation by studying CL emission triggeredby different stimuli. As observed for neutrophils, it was foundthat CL responses induced by IC, zymosan and Con A were not modifiedby losartan, whereas responses triggered by fMLP were markedlyinhibited (fig. 4).

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Fig. 4. Effect of losartan on CL emission mediated by monocytes triggered by different stimuli. CL assays were performed as describedin "Materials and Methods," in the absence ( $square$ ) or presence (

)of losartan (5 µg/ml), which was added 5 min before the additionof stimuli. Results are expressed in relative CL units (RCLU).The following stimuli were used: fMLP (10 nM), IC (100 µg/ml),zymosan (50 µg/ml) (Zy) and Con A (20 µg/ml). Data are expressedas the mean ± S.E.M. of six to eight experiments performed induplicate. *P < .01 vs. monocytes stimulated by fMLP in the absenceof losartan.

Effect of losartan on fMLP binding to neutrophil receptors. To examine the mechanisms by which losartan suppresses neutrophil activation by fMLP, its ability to inhibit [³H]fMLP binding to neutrophils was measured by adding increasingamounts of tritiated fMLP to fractions of 5 × 10⁶ neutrophils. Specific binding was determined by adding [³H]fMLP to neutrophils in the absence and presence of 10 µMunlabeledfMLP. Scatchard analysis of fMLP binding in the presence of losartan(5 µg/ml) showed that this compound did not modify the numberof binding sites but markedly decreased the binding affinity offMLP for neutrophil receptors, with a change in K_d from 36 nMto 88 nM (fig. 5).

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Fig. 5. Effect of losartan on the binding of fMLP to neutrophils. A representative Scatchard plot for [³H]fMLP binding to neutrophils in the absence ( $bullet$ ) and presence( $open circle$ ) of losartan (5 µg/ml) is shown. The assay was performed asdescribed in "Materials and Methods." Curve-fitting was done withthe LIGAND program. Each point represents the mean of duplicatedeterminations. The dissociation constant (K_d) of fMLP was significantlydifferent (P < .01) in the absence (36 nM) and presence (88 nM)of losartan.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

In this work we demonstrate that losartan, a selective antagonist of AT1 receptors for AII, markedly suppresses the activationof neutrophils by fMLP. This effect cannot be ascribed to theability of losartan to antagonize angiotensin receptors, because1) neither saralasin, an inhibitor of AT1 and AT2 receptors forAII, nor captopril, an inhibitor of ACE, reproduces the effectmediated by losartan and 2) neutrophil responses triggered byfMLP are not affected by exogenously added AII. Impairment offMLP-induced activation by losartan is due, at least in part,to its ability to inhibit neutrophil binding of fMLP. Scatchardanalysis showed that losartan markedly decreased the affinityof fMLP for neutrophil receptors without affecting the numberof binding sites. It is noteworthy that not only neutrophils butalso monocytes were affected by losartan. In fact, we observedthat losartan markedly inhibited CL emission by monocytes stimulatedwith fMLP.

Losartan and other AII AT1 receptor antagonists being developed for clinical use are phenyltetrazole-substituted imidazoles.Losartan potassium is a low molecular weight (molecular weight,461) nonpeptide (hence, orally active) that shows high selectivityfor the AT1 receptor subtype (Smith et al., 1992; Timmermans etal., 1993). At concentrations of 10 µM, it does not show affinityfor other hormonal receptors, such as Ca⁺⁺ channels and alpha and beta adrenergic, neurotensin, glycine,opioid (µ, $gamma$ and $kappa$ ), muscarinic, dopaminergic and serotonergicreceptors (Smith et al., 1992; Timmermans et al., 1993). Thesedata indicate that losartan is indeed a specific agent for AT1receptors. We show, for the first time, that losartan can effectivelyinhibit cellular specific binding of a peptide different fromAII.

After oral administration of clinically effective doses of losartan (50-100 mg), the blood concentration peak at 1 hr reachesvalues of 0.5 to 1.1 µg/ml (Smith et al., 1992; Timmermans etal., 1993). Our results showed that, in vitro, these concentrationsof losartan are able to inhibit neutrophil responses triggeredby low concentrations of fMLP. Considering the critical role thatN-formyl peptides play in the recruitment and activation of phagocyticcells in response to microbial injury (Marasco et al., 1984; Murphy,1994), it is tempting to speculate that, during therapy with losartan,there may be the risk of bacterial infectious diseases. However,observations from controlled clinical trials do not support thispresumption, because losartan is well tolerated and the incidenceof infectious diseases appears to be comparable to that in theplacebo group (Goodfriend et al., 1996). It should be emphasized,however, that so far no clinical trials have involved immunocompromisedpatients, for whom the impairment of phagocytic cell ability torespond to N-formyl peptides would be more harmful, compared withimmunocompetent patients. Additional studies will be requiredto determine whether losartan should be given to immunocompromisedpatients.

	Acknowledgments

The authors thank Dr. Juan C. Calvo for advice on Scatchard analysis.

	Footnotes

Accepted for publication January 29, 1997.

Received for publication November 13, 1996.

¹ This work was supported by grants from the "Consejo Nacional de Investigaciones Científicas y Técnicas," Buenos Aires UniversitySchool of Medicine, Fundación "Alberto J. Roemmers" and Fundación"Antorchas," Buenos Aires, Argentina.

Send reprint requests to: Dr. Silvina Raiden, Laboratorio de Inmunología, Instituto de Investigaciones Hematológicas, Academia Nacional de Medicina, Pacheco de Melo 3081, 1425 Buenos Aires, Argentina.

	Abbreviations

ACE, angiotensin-converting enzyme; AII, angiotensin II; CL, chemiluminescence; Con A, concanavalin A; FCS, fetal calf serum; fMLP, N-formylmethionyl-leucyl-phenylalanine; IC, immune complexes.

	References

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LOSARTAN POTASSIUM

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				S. Raiden, Y. Pereyra, V. Nahmod, C. Alvarez, L. Castello, M. Giordano, and J. Geffner Losartan, a selective inhibitor of subtype AT1 receptors for angiotensin II, inhibits neutrophil recruitment in the lung triggered by fMLP J. Leukoc. Biol., November 1, 2000; 68(5): 700 - 706. [Abstract] [Full Text]

				W. B Strawn, R. H Dean, and C. M Ferrario Novel mechanisms linking angiotensin II and early atherogenesis Journal of Renin-Angiotensin-Aldosterone System, March 1, 2000; 1(1): 11 - 17. [PDF]

Losartan, a Selective Inhibitor of Subtype AT1 Receptors for Angiotensin II, Inhibits the Binding of N-Formylmethionyl-leucyl-phenylalanine to Neutrophil Receptors1

Losartan, a Selective Inhibitor of Subtype AT1 Receptors for Angiotensin II, Inhibits the Binding of N-Formylmethionyl-leucyl-phenylalanine to Neutrophil Receptors¹