Inhibition of NADPH Oxidase Activation by 4-(2-Aminoethyl)-benzenesulfonyl Fluoride and Related Compounds*

(Received for publication, July 17, 1996, and in revised form, February 18, 1997)

Valery Diatchuk Dagger , Ofra Lotan Dagger , Vasilij Koshkin Dagger , Peter Wikstroem § and Edgar Pick Dagger

From the Dagger  Julius Friedrich Cohnheim-Minerva Center for Phagocyte Research, Department of Human Microbiology, Sackler School of Medicine, Tel Aviv University, Tel Aviv 69978, Israel and § Pentapharm Ltd., Engelgasse 109, CH-4002, Basel, Switzerland

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES


ABSTRACT

The elicitation of an oxidative burst in phagocytes rests on the assembly of a multicomponental complex (NADPH oxidase) consisting of a membrane-associated flavocytochrome (cytochrome b559), representing the redox element responsible for the NADPH-dependent reduction of oxygen to superoxide (Obardot 2), two cytosolic components (p47phox, p67phox), and the small GTPase Rac (1 or 2). We found that 4-(2-aminoethyl)-benzenesulfonyl fluoride (AEBSF), an irreversible serine protease inhibitor, prevented the elicitation of Obardot 2 production in intact macrophages and the amphiphile-dependent activation of NADPH oxidase in a cell-free system, consisting of solubilized membrane or purified cytochrome b559 combined with total cytosol or a mixture of recombinant p47phox, p67phox, and Rac1. AEBSF acted at the activation step and did not interfere with the ensuing electron flow. It did not scavenge oxygen radicals and did not affect assay reagents. Five other serine protease inhibitors (three irreversible and two reversible) were found to lack an inhibitory effect on cell-free activation of NADPH oxidase. A structure-function study of AEBSF analogues demonstrated that the presence of a sulfonyl fluoride group was essential for inhibitory activity and that compounds containing an aminoalkylbenzene moiety were more active than amidinobenzene derivatives. Exposure of the membrane fraction or of purified cytochrome b559, but not of cytosol or recombinant cytosolic components, to AEBSF, in the presence of a critical concentration of the activating amphiphile lithium dodecyl sulfate, resulted in a marked impairment of their ability to support cell-free NADPH oxidase activation upon complementation with untreated cytosol or cytosolic components. Kinetic analysis of the effect of varying the concentration of each of the three cytosolic components on the inhibitory potency of AEBSF indicated that this was inversely related to the concentrations of p47phox and, to a lesser degree, p67phox. AEBSF also prevented the amphiphile-elicited translocation of p47phox and p67phox to the membrane. These results are interpreted as indicating that AEBSF interferes with the binding of p47phox and/or p67phox to cytochrome b559, probably by a direct effect on cytochrome b559.


INTRODUCTION

The production of reactive oxygen radicals represents the major microbicidal mechanism of phagocytes (1). Oxygen radicals are also generated, in lesser amounts, by some nonphagocytic cells, sharing the enzymatic machinery characteristic of phagocytes (2), and, under certain conditions, by plant cells (3). Interest in reactive oxygen species has also been stimulated by accumulating evidence for their involvement in the pathogenesis of diseases, ranging from respiratory distress syndrome to ischemia-reperfusion injury in several organs (4).

The primordial oxygen radical produced by phagocytes is superoxide (Obardot 2).1 It is generated, in response to appropriate stimuli, by NADPH-derived one-electron reduction of molecular oxygen, a reaction catalyzed by a membrane-bound heterodimeric flavocytochrome (cytochrome b559) (reviewed in Refs. 5-7). Cytochrome b559 contains two redox centers, FAD and heme, and electron flow from NADPH to oxygen in initiated by the interaction of cytochrome with two cytosolic proteins, p47phox and p67phox, and the small GTPase, Rac1 or Rac2 (reviewed in Ref. 8). In the intact cell, this interaction is made possible by the stimulus-dependent translocation of the cytosolic components to the plasma membrane, leading to the assembly of what is known as the NADPH oxidase complex. Activation of NADPH oxidase, resulting in Obardot 2 generation, can be reproduced in vitro by a cell-free system consisting of either phagocyte membranes and cytosol (9, 10) or of a mixture of purified or recombinant components, exposed to a critical amount of an anionic amphiphile (arachidonate or SDS) (11, 12).

A number of inhibitors of the Obardot 2 generating NADPH oxidase have been described (reviewed in Ref. 13). The search for such inhibitors is propelled by two incentives: (a) to serve as tools for understanding the structure and mechanism of activation of the NADPH oxidase, and (b) their potential use as therapeutic agents in diseases associated with production of oxygen radicals at an inappropriate site or time. In most studies, inhibitors were tested for an effect on intact phagocytes. The main drawback of such an approach is that it does not permit a distinction between an effect on membrane receptors and signal transduction and a direct effect on the components of the NADPH oxidase complex. Alternative strategies rest on examining the effect of inhibitors on subcellular fractions originating from stimulated cells or on NADPH oxidase activation in the cell-free system. These latter approaches should allow the selection of inhibitors with a direct effect on the assembled complex or on individual components of the NADPH oxidase complex. So far, the only compound having gained wide acceptance as a relatively specific direct inhibitor of NADPH oxidase is diphenylene iodonium (14).

In the present paper we report that 4-(2-aminoethyl)-benzenesulfonyl fluoride (AEBSF; also known as Pefabloc SC), originally developed as an irreversible serine protease inhibitor, prevents the activation of the Obardot 2 generating NADPH oxidase in both intact stimulated macrophages and in cell-free systems. The effect is shared by some structurally related compounds, indicating that we are dealing with a new class of NADPH oxidase inhibitors. Evidence is presented in favor of the proposal that AEBSF interferes with the interaction of p47phox and/or p67phox with cytochrome b559, probably by chemical modification of cytochrome b559.


EXPERIMENTAL PROCEDURES

Chemicals and Reagents

AEBSF hydrochloride (>99% pure), lithium dodecyl sulfate (LiDS), and common laboratory chemicals (at the highest purity available) were from Merck. 4-(2-Aminoethyl)-benzenesulfonamide (AEBSNH2, 99% pure) was purchased from Aldrich. 4-(2-Aminoethyl)-benzenesulfonic acid hydrochloride (AEBSAc), 4-(2-N-methylaminoethyl)-benzenesulfonyl fluoride hydrochloride (MAEBSF), and 4-(amidino)-benzenesulfonyl fluoride hydrochloride (pABSF) were synthesized by Pentapharm Ltd., Basle, Switzerland. n-Octyl-beta -D-glucopyranoside (octyl glucoside) was a product of Pfanstiehl Laboratories. Aprotinin was obtained from Fluka. Guanosine 5'-3-O-(thio)triphosphate (GTPgamma S) was purchased from Boehringer. The following chemicals were obtained from Sigma: NADPH (tetrasodium salt, 95% pure), ferricytochrome c (from horse heart, 95% pure), superoxide dismutase (from bovine blood), xanthine, xanthine oxidase (from buttermilk), phorbol 12-myristate 13-acetate (PMA), N-formyl-Met-Leu-Phe (fMLP), calcium ionophore A23187, phenylmethanesulfonyl fluoride (PMSF), 4-(amidino)-phenylmethanesulfonyl fluoride hydrochloride (pAPMSF), benzamidine hydrochloride hydrate, leupeptin hemisulfate salt, n-tosyl-L-phenylalanine chloromethyl ketone (TPCK), and 3,4-dichloroisocoumarin (DCIC).

Protease inhibitors were dissolved in water at a concentration at least 50-fold higher than the highest concentration used in NADPH oxidase inhibition assays, witih the exception of PMSF, TPCK, and DCIC, which were dissolved in ethanol, methanol, and dimethyl sulfoxide, respectively.

Preparation of Macrophages and Subcellular Fractions

Macrophages were obtained from the peritoneal cavity of guinea pigs injected with mineral oil 5-6 days before cell harvest. The cells were washed and made erythrocyte-free, as described previously (10), and suspended in Earle's balanced salt solution (2 × 108 cells/ml), for assays involving intact cells. The membrane and cytosol fractions were obtained from cells disrupted by sonication, as described before (15), with some modifications (16).

Solubilization of Membranes and Purification of Cytochrome b559

Membranes were washed in 1 M KCl in cell homogenization buffer (15, 16) and solubilized in 40 mM octyl glucoside, as described (17). Before use in the cell-free assay, solubilized membrane was diluted in detergent-free solubilization buffer, to bring the concentration of octyl glucoside to 4-5 mM. Cytochrome b559 was purified from the original solubilized membrane and relipidated by a modification (18) of our original method (19). Spectral analysis of cytochrome b559 preparations was performed as described in Ref. 19.

Preparation of Recombinant Cytosolic NADPH Oxidase Components

Baculoviruses carrying cDNAs for human p47phox and p67phox were kind gifts of Dr. Thomas L. Leto (National Institutes of Health, Bethesda, MD). Suspension cultures of Sf9 cells (2 × 106 cells/ml), grown in serum-free medium (SF-900 II SFM, Life Technologies) were infected with the recombinant baculoviruses and harvested 72 h after infection. The recombinant proteins were prepared as described by Leto et al. (20). Briefly, the cells were disrupted by sonication using three 30-s pulses, in a 250 watt apparatus (Sonics and Materials), centrifuged at 12,000 × g for 10 min, and the supernatant fractions recentrifuged at 100,000 × g for 1 h. The recombinant proteins were purified by ion exchange chromatography of the high speed supernatants, referred to as "crude extracts." Thus, crude extract, containing p47phox, was applied to a SP Sepharose column (HiLoad 16/10, Pharmacia Biotech), equilibrated with 50 mM sodium phosphate buffer, pH 7.0, supplemented with 1 mM dithioerythritol, and was eluted with a 0-0.3 M NaCl gradient in the same buffer (210 ml, at a flow rate of 1.5 ml/min). Crude extract, containing p67phox, was applied to a Q-Sepharose column (HiLoad 16/10, Pharmacia Biotech Inc.) equilibrated with 20 mM Tris-HCl, pH 7.5, supplemented with 1 mM dithioerythritol, and eluted with a 0-0.5 M NaCl gradient in the same buffer (210 ml, at a flow rate of 1.5 ml/min). Purified recombinant proteins were analyzed by SDS-polyacrylamide gel electrophoresis; p47phox was 99% pure, whereas p67phox was 90% pure. Recombinant Rac1 was isolated from Escherichia coli transformed with Rac1 cDNA subcloned into the bacterial expression vector pGEX2T (a kind gift of Dr. Thomas L. Leto, National Institutes of Health, Bethesda, MD), as described by Kwong et al. (21). Briefly, the pellet of bacterial culture overexpressing the glutathione S-transferase-Rac1 fusion protein was disrupted by sonication, by three pulses of 30 s, and the homogenate was clarified by centrifugation at 12,000 × g for 5 min. The fusion protein was absorbed from the supernatant on glutathione-agarose (Sigma) and Rac1 was cleaved from the resin-bound fusion protein by thrombin. Thrombin was removed by absorption on benzamidine-Sepharose 6B (Pharmacia Biotech Inc.). Purified Rac1 was loaded with GTPgamma S, as described before (22).

Obardot 2 Production by Intact Macrophages

Macrophages (107 cells), in a volume of 50 µl, were added to 940 µl of Earle's balanced salt solution (containing 1.8 mM CaCl2), supplemented with 80 µM ferricytochrome c, in disposable spectrophotometer cuvettes. Inducers of an oxidative burst were added in a volume of 10 µl and the cuvettes placed in the thermostatted (37 °C) cuvette holder of a Uvikon 860 spectrophotometer (Kontron Instruments). Stimulus-dependent Obardot 2 production was assayed by the continuous recording of superoxide dismutase inhibitable ferricytochrome c reduction, measured at 550 nm, and the maximal rate was calculated from the linear sector of the change in absorbance curve (23).

Assays for Cell-free Activation of NADPH Oxidase

Obardot 2 Production

Anionic amphiphile (LiDS)-activated Obardot 2 production in vitro was assayed by ferricytochrome c reduction in mixtures consisting of solubilized membrane and either total cytosol or a combination of p47phox, p67phox, and Rac1-GTPgamma S, as described (10, 16). In some experiments, the membrane was replaced by purified relipidated cytochrome b559. Cell-free assays were performed either by the "one-step" method, in which activation by LiDS and NADPH-dependent Obardot 2 production occur simultaneously, or by the "two-step" method (24) permitting, at least partial, separation of the activation and catalytic stages of the reaction.

NADPH Oxidation

LiDS-dependent NADPH oxidation by cell-free mixtures, of a composition identical to those utilized in the Obardot 2 production assays, was measured as described in Ref. 25.

Oxygen Consumption

LiDS- and NADPH-dependent oxygen consumption by cell-free mixtures, consisting of membrane and recombinant cytosolic components, was assayed with the aid of a Clark oxygen electrode (Yellow Springs Instruments), as described (26).

Translocation of p47phox and p67phox to the Membrane

The translocation of p47phox and p67phox to the membrane fraction of macrophages was studied in the LiDS-activated cell free system. Macrophage membranes (equivalent to 1.6 × 107 cells) were mixed with total macrophage cytosol (equivalent to 1.5 × 107 cells) in a total volume of 1 ml of NADPH oxidase assay buffer (10), not containing ferricytochrome c, and incubated for 5 min at 24 °C, in the absence or presence of 185 µM LiDS (a concentration found to induce maximal Obardot 2 production under these conditions). The mixture was centrifuged at 15,800 × g for 30 min at 4 °C and, after careful removal of the supernatant, the membrane pellet was resuspended in 1 ml of NADPH oxidase assay buffer and recentrifuged at 15,800 × g for 15 min. After removal of the supernatant, the sedimented membranes were resuspended in 30 µl of electrophoresis sample buffer containing 2% SDS, heated at 95 °C for 5 min, and subjected to SDS-polyacrylamide gel electrophoresis and immunoblotting, as described (19). The blots were probed with a mixture of goat polyclonal anti-recombinant p47phox and anti-recombinant p67phox antibodies (20) (kind gifts of Dr. Thomas L. Leto, National Institutes of Health, Bethesda, MD), followed by peroxidase-conjugated rabbit anti-goat IgG (Jackson ImmunoResearch). The reactive bands were detected by enhanced chemiluminescence, using reagents manufactured by Amersham International, and exposure to Rx medical x-ray film (Fuji).


RESULTS

AEBSF Inhibits Obardot 2 Production by Intact Macrophages

Obardot 2 production can be elicited in guinea pig peritoneal macrophages by a variety of stimulants (27). We chose three stimulants (PMA, fMLP, and the calcium ionophore, A23187), known to activate NADPH oxidase in intact cells by distinct transductional mechanisms, and used these at concentrations found to elicit maximal Obardot 2 generation in cells in suspension at 37 °C. In the presence of AEBSF, a dose-dependent inhibition of Obardot 2 production elicited by 2 µM PMA was observed (Fig. 1A). When AEBSF was added just before the addition of PMA, the IC50 was close to 1 mM and inhibition was almost complete at 5 mM AEBSF. At the latter concentration, AEBSF also caused a total suppression of Obardot 2 production elicited by 1 µM fMLP or 10 µM A23187 (results not shown). This result was compatible with three interpretations: (a) AEBSF acts as a scavenger of Obardot 2; (b) it acts on a signal transduction path shared by all three stimulants; and (c) it has a direct effect on the NADPH oxidase complex.


Fig. 1. Inhibition of NADPH oxidase activation in intact macrophages, broken cell preparation, and semi-recombinant cell-free system. A, 107 macrophages were exposed to 2 µM PMA for 30 s, in the absence or presence of AEBSF and Obardot 2 production measured. Control preparations produced 16.7 nmol of Obardot 2/min/107 cells. B, solubilized macrophage membrane (2.25 pmol of cytochrome b559) was combined with total cytosol (equivalent to 4.5 × 106 cells) in 1 ml of assay buffer and activated by 130 µM LiDS for 90 s, in the absence or presence of AEBSF, and NADPH-dependent Obardot 2 production assessed. NADPH oxidase activity in the absence of AEBSF was 117.7 mol of Obardot 2/s/mol of cytochrome b559. C, purified and relipidated cytochrome b559 (3.9 nM) was combined with p47phox (3.5 nM), p67phox (49 nM), and Rac1-GTPgamma S (54 nM), activated by 130 µM LiDS for 3 min, in the absence or presence of AEBSF, and NADPH-dependent Obardot 2 production assessed. NADPH oxidase activity in the absence of AEBSF was 61.4 mol of Obardot 2/s/mol of cytochrome b559. The concentration of p47phox was chosen to be subsaturating for reasons described in the text. In this particular experiment, the IC50 of AEBSF was found to be 0.87 mM. All graphs illustrate representative experiments, in which each measurement was performed in duplicate.
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AEBSF Does Not Scavenge Obardot 2

We examined the effect of AEBSF on the ability to measure Obardot 2 generation by the xanthine-xanthine oxidase system, using the ferricytochrome c reduction assay. AEBSF (0.5-5 mM) did not interfere with the detection of Obardot 2 generated by xanthine (0.2 mM) and xanthine oxidase (0.018 units/ml); the difference between Obardot 2 detection in the absence or presence of AEBSF (up to 5 mM) was less than 10% of the control value.

AEBSF Inhibits Obardot 2 Production by a Cell-free System

NADPH oxidase can be activated in a cell-free system by certain anionic amphiphiles, a mechanism which circumvents the transductional pathways active in the intact phagocyte (9, 10). We, therefore, examined the effect of AEBSF on Obardot 2 production in several forms of cell-free activation systems. The simplest one consisted of solubilized macrophage membranes and unfractionated cytosol, both derived from unstimulated cells. AEBSF was found to exhibit a concentration-related, inhibitory influence on LiDS-induced Obardot 2 production, with an IC50 of 0.206 ± 0.014 mM (n = 8) (Fig. 1B). We next investigated the effect of AEBSF on a semi-recombinant cell-free system (11, 12), consisting of either solubilized macrophage membrane or purified cytochrome b559, incorporated in phospholipid liposomes, combined with recombinant p47phox, p67phox, and Rac1-GTPgamma S. AEBSF was found to act as an inhibitor of Obardot 2 production in this system, too, composed of four purified NADPH oxidase components in the virtual absence of any other protein (Fig. 1C). In the course of the latter experiments we became aware of an unexpected variability in the inhibitory potency of AEBSF which was not found in the cell-free system consisting of solubilized membrane and unfractionated cytosol. Analysis of this phenomenon revealed that, in the presence of a constant amount of membrane or purified cytochrome b559, the inhibitory effect of AEBSF was inversely related to the concentration of p47phox. A more detailed exploration of the mechanism of this correlation is provided in the penultimate section.

To further ascertain that inhibition by AEBSF of Obardot 2 production in the cell-free system is due to a direct effect on NADPH oxidase, we examined the influence of AEBSF on two additional indicators of NADPH oxidase activation. These were LiDS-elicited NADPH oxidation (25) and LiDS- and NADPH-dependent oxygen consumption (26), by mixtures of membrane and cytosol or membrane and recombinant cytosolic components. We found that AEBSF suppressed NADPH oxidation in a concentration-related manner; when cell-free mixtures were analyzed in parallel by ferricytochrome c reduction, the IC50 of AEBSF values were identical in the two assays. Also, at 5 mM, AEBSF inhibited oxygen consumption by 95%. We concluded that AEBSF acts by interacting with one or more of the components of the NADPH oxidase complex.

Inhibition by AEBSF Cannot Be Overcome by Excesses of Substrate, Cofactor, or Activator

The Obardot 2 generating NADPH oxidase has a Km for NADPH of 20-40 µM (6) and the enzyme activated by amphiphile under cell-free conditions exhibits the same kinetic characteristics (9, 10). The effect of AEBSF (2 mM) on NADPH oxidase activation in the cell-free system was examined at concentrations of NADPH varying from 10 to 400 µM and analyzed by Michaelis-Menten plotting. This demonstrated that inhibition of AEBSF was noncompetitive with NADPH. Membrane solubilization and purification of cytochrome b559 results in a partial loss of FAD from the cytochrome (11, 19, 28), which explains the dependence of NADPH oxidase activation, in the cell-free system, on exogenous FAD (9). We, therefore, investigated whether AEBSF interfered with the reflavination of cytochrome b559, by assessing the effect of varying the concentration of exogenous FAD on the inhibitory effect of AEBSF. We found that the degree of inhibition by AEBSF (IC50) was independent of the concentration of exogenous FAD (from 10 to 100 µM). Finally, we explored the possibility that AEBSF competes with the activating amphiphile for interaction with a component of the NADPH oxidase complex. We found that increasing the concentration of LiDS, from the optimal activating range of 120-140 µM to up to 180 µM, did not reverse or reduce the inhibitory effect of AEBSF (see also Fig. 4).


Fig. 4. The ability of AEBSF to prevent NADPH oxidase activation is not shared by other serine protease inhibitors. Solubilized macrophage membrane (2.52 pmol of cytochrome b559) was combined with total cytosol (equivalent to 4.5 × 106 cells) in 1 ml of assay buffer and activated with various concentrations of LiDS (40-180 µM) for 90 s, in the absence or presence of the indicated concentrations of serine protease inhibitors. Obardot 2 production was initiated by the addition of 0.2 mM NADPH. The figure was generated by the superposition of data from two characteristic experiments: one, comparing the effects of AEBSF, PMSF, and TPCK and the second, assessing the effect of DCIC. Each measurement was performed in triplicate and the values plotted on the y scale represent means ± S.E. of the amounts of Obardot 2 produced per assay mixture per min.
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AEBSF Interferes with Activation of NADPH Oxidase but Not with Electron Flow

Activation of NADPH oxidase, in intact cells and in broken cell preparations, is considered to be the result of the assembly of the individual components of the enzyme into a membrane-localized complex (reviewed in Ref. 8), this being followed by the induction of electron flow within the flavocytochrome b559 dimer. The "activation" and "electron flow" stages can be separated in a two-step cell-free activation assay (24). This consists of exposing a mixture of NADPH oxidase components to an optimal concentration of activating amphiphile in a small volume (100 µl) for a fixed time interval, in the absence of substrate NADPH, followed by 10-fold dilution and the initiation of electron flow by addition of NADPH. The 10-fold dilution results in a reduction in the concentration of amphiphile to a subactivating level and causes the virtual interruption of further assembly of the enzyme complex. We utilized this approach to identify the event affected by the inhibitor, by adding AEBSF either to the activation mixture at time 0 or after the completion of activation. As apparent in Fig. 2, AEBSF was a much more effective inhibitor when present during the assembly of the NADPH oxidase complex than when added at the completion of assembly. The finding that AEBSF was not totally inactive when added at the end of step one is probably due to the fact that some enzyme assembly continues taking place in the course of the second step. The ability of AEBSF to suppress Obardot 2 production when added to the components of the NADPH oxidase complex, in the absence of electron flow, also indicates that its mechanism of action is distinct from that of diphenylene iodonium, which acted as an inhibitor only under reducing conditions, such as those generated by NADPH oxidase turnover (29).


Fig. 2. AEBSF inhibits NADPH oxidase activation and has little effect on electron transport. Solubilized macrophage membrane (4.5 pmol of cytochrome b559) was incubated with total cytosol (equivalent to 4.5 × 106 cells) in 100 µl of assay buffer containing 300 µM LiDS, for 3 min, in the absence or presence of AEBSF. Following this, the reaction volume was brought to 1 ml with assay buffer and Obardot 2 production initiated by the addition of 0.2 mM NADPH. A parallel series of reaction mixtures were prepared, to which AEBSF was added at the completion of the 3-min activation interval. NADPH oxidase activity in the absence of AEBSF was 82.6 ± 4.6 mol of Obardot 2/s/mol of cytochrome b559. Results represent means ± S.E. of three experiments.
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Reversibility of Inhibition by AEBSF

Use was made of the two-step cell-free assay for determining whether inhibition of NADPH oxidase activation by AEBSF was reversible. For this purpose, activation mixtures were prepared in the absence and presence of a single concentration of AEBSF (2 mM) and incubated with an optimal concentration of LiDS for 5 min. Following this, the reaction mixtures were diluted in assay buffer to reduce the amphiphile concentration, and re-exposed or not to an activating concentration of LiDS for 3 min. The results illustrated in Fig. 3 demonstrate that re-exposure to LiDS of mixtures treated with 2 mM AEBSF partially reverses the inhibition. Thus, Obardot 2 production by activation mixtures treated with AEBSF was 22.67 ± 1.12% of that of control preparations, whereas re-exposure of the AEBSF-treated preparations to LiDS led to resurgence of Obardot 2 production, reaching 55.55 ± 1.99% of that measured in untreated preparations.


Fig. 3. Inhibition of NADPH oxidase activation by AEBSF is only partially reversible. Solubilized macrophage membrane (5.75 pmol of cytochrome b559) was mixed with total cytosol (equivalent to 4.5 × 106 cells) in 100 µl of assay buffer, containing 300 µM LiDS, and allowed to stand for 5 min, in the absence (1) or presence (2) of 2 mM AEBSF. This was followed by the addition of 0.9 ml of assay buffer, not containing LiDS, keeping the mixture for 3 min and initiating Obardot 2 production by the addition of 0.2 mM NADPH. In a parallel series of experiments, membrane/cytosol/LiDS mixtures were prepared as above, in the absence (3) or presence (4) of 2 mM AEBSF, but this was followed by the addition of 0.9 ml of assay buffer containing 120 µM LiDS and, after 3 min, by initiation of Obardot 2 production by the addition of 0.2 mM NADPH. To mixtures prepared in the absence of AEBSF (1 and 3), AEBSF was added at a concentration of 0.2 mM, together with the 0.9 ml of buffer, to reach a concentration of AEBSF equivalent to that present in samples 2 and 4, upon addition of 0.9 ml of buffer. The figure represents means ± S.E. of three experiments.
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Specificity of AEBSF-mediated Inhibition

AEBSF was developed originally as an irreversible serine protease inhibitor (30, 31). It was, therefore, essential to establish whether its inhibitory effect on NADPH oxidase activation was related to its anti-protease activity. Hence, we examined the ability of five additional serine protease inhibitors to affect NADPH oxidase activation in the cell-free system. These were the irreversible inhibitors PMSF (0.1-2 mM) and TPCK (10-200 µM), the "mechanism based" irreversible inhibitor, DCIC (0.25 mM), and the reversible inhibitors aprotinin (0.3 µM) and leupeptin (20 µM). None of these exhibited an inhibitory effect on NADPH oxidase activation. We next explored the possibility that inhibition might be related to the concentration of activating amphiphile. As apparent in Fig. 4, PMSF, TPCK, and DCIC did not possess an inhibitory effect at any LiDS concentration whereas AEBSF was a potent inhibitor over the whole range of amphiphile concentrations. On the contrary, PMSF, TPCK, and DCIC had an enhancing effect on NADPH oxidase activation, at concentrations of LiDS below those required for maximal activation.

Structural Requirements for Inhibitory Action

We investigated the capacity of several analogues of AEBSF to interfere with the activation of NADPH oxidase. One group consisted of aminoethylbenzene derivatives and included: MAEBSF, identical to AEBSF except for the presence of an amino-linked methyl group; AEBSAc, a product of alkaline hydrolysis of AEBSF, found to be inactive as a protease inhibitor (31); and AEBSNH2, in which an amide group replaces the fluoride found in AEBSF, also reported to lack protease inhibitory activity (32). As apparent in Fig. 5A, AEBSAc and AEBSNH2 were totally inactive, whereas MAEBSF exhibited an inhibitory potency identical to that of AEBSF (IC50 = 0.285 ± 0.005 mM; n = 3). The second group consisted of amidinobenzene derivatives. Among these, pAPMSF was reported to be a potent irreversible serine protease inhibitor (33), and benzamidine acts as a peptidase inhibitor (34). As seen in Fig. 5B, only pABSF was a moderate inhibitor of NADPH oxidase activation; its IC50 (1.49 ± 0.05; n = 3) was 7.5-fold higher than that of AEBSF. We also examined the influence of an excess of the two inactive analogues, AEBSAc and AEBSNH2, sharing the aminoethylbenzene structure with AEBSF, on inhibition of NADPH oxidase activation by AEBSF. Neither of the two analogues, at 5 mM, was capable of reducing the inhibitory effect of AEBSF, assayed at concentrations ranging from 0.1 to 5 mM. These results demonstrate that a sulfonyl fluoride group, adjacent to the benzene ring, is essential for inhibitory activity and that aminoalkylbenzene derivatives are more potent inhibitors than amidinobenzene compounds.


Fig. 5. Structure-function relationship in the NADPH oxidase inhibitory action of aminoethyl- and amidinobenzenesulfonyl fluorides. Mixtures of solubilized macrophage membranes (3.5-5.7 pmol of cytochrome b559) and total cytosol (equivalent to 4.5 × 106 cells), in 1 ml of assay buffer, were activated for 90 s by 130 µM LiDS, in the absence or presence of various concentrations of inhibitors, and Obardot 2 production, elicited by the addition of 0.2 mM NADPH, was assessed. For each compound, results represent the means ± S.E. of three experiments. A, AEBSF in comparison to aminoethylbenzene analogues. B, AEBSF in comparison to amidinobenzene analogues. NADPH oxidase activity of control mixtures was 60.8 ± 1.3 (A) and 80.9 ± 12.3 (B) mol of Obardot 2/s/mol of cytochrome b559 (means ± S.E.).
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Identification of the Molecular Target of AEBSF

We next investigated whether interaction between AEBSF and a specific NADPH oxidase component can be demonstrated. The basic design of these experiments was to expose subcellular fractions or individual NADPH oxidase components to AEBSF for a fixed time interval in a small volume, followed by 10-fold dilution into assay buffer containing the untreated complementary fraction or a mixture of the other, untreated NADPH oxidase components, activating LiDS and NADPH. Dilution resulted in a reduction in AEBSF concentration to subinhibitory levels, limiting its effect to the component initially exposed to the compound. We examined the effect of AEBSF on total membrane, total cytosol, relipidated cytochrome b559, and recombinant p47phox, p67phox, and Rac1-GTPgamma S. Each of these was exposed or not to AEBSF in the absence or presence of LiDS, the maximal concentration of amphiphile being chosen not to exceed that permitting the recovery of NADPH oxidase activity, upon complementation with untreated components.

As apparent in Table I, exposure of total solubilized membrane or purified and relipidated cytochrome b559 to AEBSF, in the presence but not in the absence of LiDS, resulted in marked inhibition of their capacity to support Obardot 2 production upon complementation with cytosol and activation by LiDS. Total cytosol as well as p47phox and Rac1 were insensitive to treatment by AEBSF; a minor effect of AEBSF on p67phox was evident but this result was difficult to interpret because of considerable interexperimental variability and because, among all NADPH oxidase components, p67phox was the most sensitive to denaturation by LiDS.

Table I. Effect of treating individual components of the NADPH oxidase complex with AEBSF on their ability to support Obardot 2 production in the cell-free system

Various components, at the concentrations shown in the footnotes, were incubated with 2 mM AEBSF for 5 min, at room temperature, in a volume of 100 µl, in the absence or presence of LiDS, at concentrations shown in the footnotes. This was followed by the addition of the missing untreated NADPH oxidase components at saturating concentration in 0.9 ml of assay buffer containing a concentration of LiDS, to result in a final concentration of 120 µM. Preparations, not exposed to AEBSF, were supplemented, at this stage, with 0.2 mM AEBSF, as a control for an eventual effect of AEBSF on electron flow. Obardot 2 production was elicited 90 s later by the addition of 0.2 mM NADPH. Results are expresses as % inhibition of NADPH oxidase activation by relating the activity of mixtures containing a component treated with 2 mM AEBSF to that of control mixtures containing untreated component and 0.2 mM AEBSF. Results represent means ± S.E. of four experiments, for each situation. Negative values were obtained when Obardot 2 production by a reaction mixture containing a component treated with AEBSF exceeded that of the control mixture containing the untreated component. Various components, at the concentrations shown in the footnotes, were incubated with 2 mM AEBSF for 5 min, at room temperature, in a volume of 100 µl, in the absence or presence of LiDS, at concentrations shown in the footnotes. This was followed by the addition of the missing untreated NADPH oxidase components at saturating concentration in 0.9 ml of assay buffer containing a concentration of LiDS, to result in a final concentration of 120 µM. Preparations, not exposed to AEBSF, were supplemented, at this stage, with 0.2 mM AEBSF, as a control for an eventual effect of AEBSF on electron flow. Obardot 2 production was elicited 90 s later by the addition of 0.2 mM NADPH. Results are expresses as % inhibition of NADPH oxidase activation by relating the activity of mixtures containing a component treated with 2 mM AEBSF to that of control mixtures containing untreated component and 0.2 mM AEBSF. Results represent means ± S.E. of four experiments, for each situation. Negative values were obtained when Obardot 2 production by a reaction mixture containing a component treated with AEBSF exceeded that of the control mixture containing the untreated component.

Material or component treated with AEBSF (2 mM) % Inhibition of NADPH oxidase activation in the reconstituted cell-free system
Treatment in the absence of LiDS Treatment in the presence of LiDS

Total solubilized membranea 1.42  ± 1.50 64.25  ± 4.78
Total cytosolb 0.15  ± 2.21 1.65  ± 0.22
Purified relipidated cytochrome b559c  -3.43  ± 1.16 43.98  ± 2.27
p47phox d 5.15  ± 4.51 2.24  ± 0.48
p67phox e  -0.33  ± 2.14 11.47  ± 10.27
Rac1-GTPgamma Sf 2.76  ± 1.56  -0.48  ± 1.72

a Solubilized membrane (2.4-4.5 pmol of cytochrome b559). In 100 µl, was exposed to AEBSF in the absence or presence of 300 µM LiDS. It was complemented with cytosol (equivalent to 4.5 × 106 cells) in 0.9 ml.
b Cytosol (equivalent to 4.5 × 106 cells), in 100 µl, was exposed to AEBSF in the absence or presence of 120 µM LiDS. It was complemented with solubilized membrane (4.5 pmol of cytochrome b599), in 0.9 ml.
c Purified cytochrome b559 (4.92 pmol), in 100 µl, was exposed to AEBSF in the absence or presence of 150 µM LiDS. It was complemented with cytosol (equivalent to 6 × 106 cells), in 0.9 ml.
d p47phox (12.2 pmol), in 100 µl, was exposed to AEBSF in the absence or presence of 140 µM LiDS. It was complemented with the missing components, in 0.9 ml, at the following final concentrations: solubilized membrane (2.4 nM cytochrome b599), p67phox (6 nM), and Rac1-GTPgamma S (100 nM).
e p67phox (6 pmol), in 100 µl, was exposed to AEBSF in the absence or presence of 140 µM LiDS. It was complemented with the missing components in 0.9 ml, at the following final concentrations: solubilized membrane (2.4 nM cytochrome b599), p47phox (12.2 nM), and Rac1-GTPgamma S (100 nM).
f Rac1-GTPgamma S (100 pmol), in 100 µl, was exposed to AEBSF in the absence or presence of 300 µM LiDS. It was complemented with the missing components in 0.9 ml, at the following final concentrations: solubilized membrane (2.4 nM cytochrome b559), p47phox (12.2 nM), and p67phox (6 nM).

The ability of AEBSF to inactivate cytochrome b559 was investigated in more detail by assessing the dose-dependence of the inactivation of solubilized membrane by AEBSF, in the presence and absence of LiDS. As seen in Fig. 6, AEBSF inhibited the capacity of the membrane to support Obardot 2 production only in the presence of LiDS, with an IC50 of 2.18 mM.


Fig. 6. Treatment of the membrane fraction with AEBSF results in impairment of its ability to cooperate with recombinant cytosolic components in NADPH oxidase assembly. Solubilized membrane (3.45 pmol of cytochrome b559) was exposed or not to various concentrations of AEBSF (0.5-10 mM), in the presence or absence of 300 µM LiDS, for 5 min at room temperature, in a total volume of 100 µl. This was followed by the addition of p47phox (24 nM), p67phox (19.8 nM), and Rac1-GTPgamma S (108 nM) in 0.9 ml of assay buffer containing 120 µM LiDS, bringing the total volume of the assay to 1 ml, and the mixture was kept for a further 90 s at room temperature, at which time Obardot 2 production was elicited by the addition of 0.2 mM NADPH. Reaction mixtures which contained solubilized membrane not pre-exposed to AEBSF were supplemented with AEBSF, at one-tenth of the concentration added to the membranes, at the stage of adding the cytosolic components, as a control for an effect of AEBSF on cytosolic components or electron flow. The figure illustrates the results of a typical experiment, with each measurement being performed in duplicate. For each measurement, the results are expressed as % inhibition of NADPH oxidase activation by relating NADPH oxidase activity of mixtures, containing membrane pretreated with AEBSF, to that of control preparations containing untreated membrane interacting with cytosolic components in the presence of AEBSF at 10-fold lower concentration. NADPH oxidase activity in control preparations was 99.3 mol of Obardot 2/s/mol of cytochrome b559, when the membrane was pretreated with LiDS, and 91.5 mol of Obardot 2/s/mol of cytochrome b559, when the membrane was not pretreated with LiDS.
[View Larger Version of this Image (21K GIF file)]

AEBSF Interferes with the Interaction between Cytochrome b559 and p47phox and/or p67phox

This series of experiments was initiated as an extension of the preliminary finding that, in the presence of a constant amount of cytochrome b559, the inhibitory effect of AEBSF could be overcome by increasing the concentration of cytosolic component p47phox. The consensus opinion is that an essential event in the assembly of the NADPH oxidase complex is the binding of p47phox to cytochrome b559 (reviewed in Ref. 8). In light of the results described in the preceding section, it seemed likely that AEBSF competes with p47phox for interaction with cytochrome b559. We, therefore, investigated the influence of varying the concentration of p47phox on the inhibition of NADPH oxidase activation by AEBSF, in the presence of a constant amount of membrane and saturating concentrations of p67phox and Rac1-GTPgamma S (Fig. 7A). In additional experiments, we varied the concentrations p67phox (Fig. 7B) and Rac1-GTPgamma S (Fig. 7C), in the presence of saturating concentrations of the other two cytosolic components. In all experiments, three concentrations of cytosolic component were chosen, two of which were on the ascending slope of previously established dose-response curves, whereas the third one represented a saturating concentration. The data were analyzed by plotting the "concentration of AEBSF" (on a logarithmic scale) against "inhibition of NADPH oxidase activation" and IC50 of AEBSF values, for each concentration of cytosolic component, were calculated. As seen in Fig. 7A, when p47phox was present in subsaturating concentrations, sigmoid curves were generated and IC50 values for AEBSF decreased with decreasing concentrations of p47phox. IC50 of AEBSF values were moderately reduced by lowering the concentration of p67phox (Fig. 7B) and not significantly affected by varying the concentration of Rac1-GTPgamma S (Fig. 7C). These results are compatible with the hypothesis that AEBSF interferes with the binding of p47phox to cytochrome b559 but we cannot rule out the possibility that AEBSF also inhibits a direct interaction between p67phox and cytochrome b559 (see "Discussion").


Fig. 7. Effect of concentration of cytosolic components on the inhibitory potency of AEBSF. Reaction mixtures contained solubilized membrane (40- 52.5 nM cytochrome b559), an excess of two out of three cytosolic components (240 nM p47phox, 300 nM p67phox, and 1.08 µM Rac1-GTPgamma S), various concentrations of the third cytosolic component (as indicated in each panel), 300 µM LiDS, and various concentrations of AEBSF (from 0 to 10 mM) in a volume of 100 µl. After incubation for 3 min at 24 °C, 0.9 ml of assay buffer were added and Obardot 2 production initiated by 0.2 mM NADPH. The panels present the effect of varying the concentration of p47phox (A), p67phox (B), and Rac1-GTPgamma S (C) on inhibition of NADPH oxidase activation by AEBSF. In all panels, % inhibition of NADPH oxidase activation values were plotted against a logarithmic scale presentation of the concentration of AEBSF. For each concentration of cytosolic components, the calculated IC50 of AEBSF is shown in brackets. In each panel, results represent means ± S.E. of four experiments.
[View Larger Version of this Image (26K GIF file)]

The hypothesis that AEBSF acts as a competitive inhibitor of p47phox was further tested by performing a Michaelis-Menten analysis of the effect of AEBSF on the activation of NADPH oxidase at four concentrations of p47phox (14, 21, 28, and 35 nM), all within the ascending slope of the concentration-response curve. As seen in the Lineweaver-Burk plot in Fig. 8, AEBSF, in the concentration range of 0.5 to 2 mM, behaves as a competitive inhibitor with respect to p47phox. At concentrations of AEBSF exceeding 2 mM, a noncompetitive or mixed type of inhibition pattern was obtained. Similar kinetic analysis of the effect of AEBSF on NADPH oxidase activation at varying concentrations of either p67phox or Rac1-GTPgamma S revealed noncompetitive or mixed type inhibition patterns.


Fig. 8. Kinetic analysis of the inhibition of NADPH oxidase activation by AEBSF. Reaction mixtures contained solubilized membrane (52.5 nM cytochrome b559), 198 nM p67phox, 540 nM Rac1-GTPgamma S, p47phox at four concentrations (14, 21, 28, and 35 nM) and 300 µM LiDS, in a total volume of 100 µl. Mixtures were supplemented or not with AEBSF (0.5, 1, or 2 mM). After 3 min, 0.9 ml of assay buffer were added and Obardot 2 production initiated by 0.2 mM NADPH. Data, presented as double reciprocal plots, represent means ± S.E. of four experiments.
[View Larger Version of this Image (19K GIF file)]

AEBSF Prevents Amphiphile-dependent Translocation of p47phox and p67phox to the Membrane

Activation of NADPH oxidase in intact cells is accompanied by translocation of fractions of p47phox and p67phox to the plasma membrane (35). The anchoring of both cytosolic components to the membrane is dependent on the presence of cytochrome b559 (36). Also, translocation of p67phox to the membrane occurs only in the presence of p47phox (36), suggesting that at least one of the functions of p47phox is to serve as an escort protein for p67phox. It was, therefore, of interest to investigate the effect of AEBSF on the translocation of cytosolic components to the membrane in the cell-free system (37). As seen in Fig. 9, the addition of AEBSF to mixtures of macrophage membranes and cytosol, activated by a concentration of LiDS to result in maximal NADPH-dependent Obardot 2 production, markedly inhibited the translocation of both p47phox and p67phox to the membrane. Parallel testing of the sedimented membranes, derived from cell-free mixtures activated in the absence and presence of 4.5 mM AEBSF, for Obardot 2 production, showed that lack of translocation was accompanied by an 82% inhibition of NADPH oxidase activation. As apparent in Fig. 9B, translocation of p47phox and p67phox (and its inhibition by AEBSF) was strictly dependent on the presence of membranes and was not the result of nonspecific precipitation of cytosolic components by LiDS (35).


Fig. 9. AEBSF interferes with the amphiphile-dependent translocation of p47phox and p67phox to the membrane in a cell-free system. A, macrophage membranes were incubated with total cytosol for 5 min at 24 °C, in the absence or presence of 185 µM LiDS, and in the absence or presence of 4.5 mM AEBSF. Translocation of p47phox and p67phox from cytosol to membranes was assessed as described under "Experimental Procedures." B, in this experiment, identical in design to that described in panel A, a mock control was included to demonstrate that LiDS-dependent translocation of p47phox and p67phox and its inhibition by AEBSF occur only in the presence of membranes. The band cathodal to p67phox is unrelated to p67phox and was detected independently of the presence of membrane or activation by LiDS.
[View Larger Version of this Image (28K GIF file)]


DISCUSSION

We found that AEBSF, originally developed as a water-soluble irreversible serine protease inhibitor of relatively low toxicity, interferes with the activation of the Obardot 2 generating NADPH oxidase both in intact macrophages and in cell-free systems in a concentration-dependent manner. A remarkable feature of this inhibition is that it affects all forms of cell-free activation, from broken cell systems, consisting of total membrane and unfractionated cytosol, to mixtures of purified cytochrome b559 and three recombinant cytosolic components. While this paper was in preparation, we became aware of the report by Remold-O'Donnell and Parent (38), describing the inhibitory effect of 2 mM AEBSF on Obardot 2 production by human neutrophils in response to PMA and opsonized zymosan. AEBSF (0.1-0.2 mM) was recently found to block priming of human monocytes for enhanced Obardot 2 production in response to PMA and fMLP but was reported not to affect the response of unprimed cells, in the above concentration range (32).

There is a large body of literature linking the elicitation of an oxidative burst to the activation of cellular proteases (summarized in Ref. 39). Some of the evidence for such a connection is based on the effect of synthetic or natural protease inhibitors, particularly serine protease inhibitors, on oxygen radical production by intact phagocytes. Results of such experiments have to be interpreted with caution since it became evident that the effects of protease inhibitors on Obardot 2 production were frequently unrelated to their antiproteolytic activity (39-42). Our results indicate, indeed, that AEBSF affects NADPH oxidase activation, at least in cell-free preparations, by a mechanism unrelated to its protease inhibitory activity. This claim is supported by the following arguments: (a) five other serine protease inhibitors (PMSF, TPCK, DCIC, leupeptin, and aprotinin) were found to be inactive when tested under identical conditions (it is of interest that DCIC which, like AEBSF, was found to block Obardot 2 production by intact neutrophils (38), did not inhibit NADPH oxidase activation in the cell-free system); (b) among protease inhibitors, structurally related to AEBSF (PMSF and pAPMSF), there was no relation between NADPH oxidase activation inhibitory and antiproteolytic activities, and (c) AEBSF was inhibitory in a cell-free system composed exclusively of purified native and recombinant proteins, and, therefore, free of contaminating proteases.

The inhibitory effect of AEBSF on NADPH oxidase activation exhibited a pronounced structural specificity. A number of derivatives of benzylamine and benzamidine, to which categories AEBSF is related, were shown to function as competitive serine protease inhibitors (43). The presence of a reactive sulfonyl fluoride group on the aromatic ring generates compounds capable of forming a covalent bond with their target enzymes (30, 44). We found that, among four compounds sharing an aminoethylbenzene moiety (AEBSF, AEBSAc, AEBSNH2, and MAEBSF), only AEBSF and MAEBSF, which possess a reactive sulfonyl fluoride group, were inhibitory. Among three amidinobenzene derivatives (benzamidine, pAPMSF, and pABSF) only pABSF, possessing a sulfonyl fluoride group adjacent to the benzene ring exhibited moderate NADPH oxidase inhibitory activity. PMSF and TPCK, two serine protease inhibitors bearing limited structural similarity to AEBSF, but lacking the basic amino group present in AEBSF, were found to be inactive in the cell-free system. We conclude that two structural elements are the minimal prerequisites for the possession of NADPH oxidase inhibitory property: a positively charged aminoalkyl moiety and a reactive sulfonyl fluoride group.

The search for the molecular target of AEBSF led to the conclusion that this is, most likely, cytochrome b559. This proposal is based principally on the finding that treatment of either total membrane fraction or purified and relipidated cytochrome b559 with AEBSF, in the presence of a critical concentration of LiDS, resulted in a dose-dependent reduction in their ability to cooperate with untreated components in the assembly of NADPH oxidase. Neither total cytosol nor any of the three cytosolic components were sensitive to AEBSF to a comparable degree. A remarkable feature of this effect is its absolute dependence on the simultaneous presence of an anionic amphiphile. The amphiphile may make the liposome-enclosed cytochrome b559 more accessible to AEBSF or may induce a conformational change in cytochrome b559 itself, normally associated with the process of activation, but also leading to exposure of an AEBSF-binding domain. Evidence for a direct effect of anionic amphiphiles, at NADPH oxidase activating concentrations, on cytochrome b559 was recently presented by the demonstration that arachidonate and SDS enhance interaction of cytochrome b559 with the NADPH oxidase inhibitory heme ligand, butyl isocyanide (45).

The results of systematic screening of the effect of varying the concentration of each of the three cytosolic components on the IC50 of AEBSF support the proposal that AEBSF prevents the binding of p47phox to cytochrome b559 and, consequently, interferes with the assembly of a functionally active NADPH oxidase complex. Such a mechanism is also in agreement with the Michaelis-Menten analysis of the inhibition of NADPH oxidase activation by AEBSF at various concentrations of p47phox. There is extensive evidence demonstrating interaction between p47phox and the small (46, 47) and large (48-50) subunits of cytochrome b559. Several groups also reported that, in p47phox, a region extending from residues 315 to 347, or part of it, represents a site of interaction with cytochrome b559 (51-53). This region is rich in basic residues, especially arginines, and it is possible that it forms electrostatic bonds with acidic residues on one of the two subunits of cytochrome b559.

However, the IC50 of AEBSF is also affected, albeit to a lesser degree, by the concentration of p67phox. This effect can be explained by assuming that p67phox binds to cytochrome b559 and that AEBSF interferes with this binding. There is, indeed, recent functional evidence for a direct interaction between p67phox and cytochrome b559 (54, 55). An alternative explanation could be provided by an indirect effect of varying the concentration of p67phox on the binding of p47phox to cytochrome b559. Thus, based on kinetic evidence, an enhancement of p47phox binding to cytochrome b559 by p67phox was demonstrated (56), and a marked reduction in the translocation of p47phox to the plasma membrane in neutrophils of p67phox-deficient patients, was recently reported (cited in Ref. 57). Our finding that AEBSF inhibits the activation-related translocation of both p47phox and p67phox to the membrane can be explained by either distinct effects on the binding of each of the two cytosolic components to cytochrome b559 or by an effect on the binding of one component affecting the binding of the other component.

When working as a protease inhibitor, AEBSF acts as a bifunctional reagent (30). The charged aminoethyl moiety acts as a substrate analogue, capable of forming ionic complexes with trypsin and related proteases because of its similarity to basic amino acids, whereas the chemically reactive sulfonyl fluoride group endows the inhibitor with the capacity of forming a stable covalent bond with the enzyme (30, 43, 44). We propose that AEBSF also acts as a bifunctional inhibitor of NADPH oxidase assembly, binding by the intermediary of its aminoethyl end, to an acidic domain on one of the subunits of cytochrome b559. This, essentially reversible step is followed by the formation of an irreversible bond, mediated by the sulfonyl fluoride group. The finding that, in the 0.5-2 mM range, AEBSF behaved as a competitive inhibitor, with respect to p47phox, but that this behavior was replaced by a noncompetitive pattern, at higher concentrations, suggests that the establishment of stable bonds becomes increasingly dominant with increasing concentrations of AEBSF. While this manuscript was under review, we became aware of a recent communication2 that AEBSF, under certain conditions (such as, at high concentrations), forms covalent adducts with proteins, other than serine proteases. These interactions appear to involve tyrosine and lysine residues and the free amino terminus.

Further exploration of the mechanism of inhibition of NADPH oxidase by AEBSF in particular and by aminoalkylbenzenesulfonyl fluorides in general is of both theoretical and practical relevance. Thus, it should lead to a better understanding of the molecular basis of the assembly of the NADPH oxidase complex and to the design of drugs to be used in circumstances associated with the undesired production of oxygen radicals. This latter aim, however, is dependent on the clarification of the relevance of effects found in the cell-free system to the situation in intact cells. Nevertheless, the fact that AEBSF is a stable, water-soluble and relatively nontoxic compound, possessing both NADPH oxidase suppressory and anti-proteolytic properties, makes it an interesting model compound for the design of antiinflammatory drugs.


FOOTNOTES

*   This work was supported by the Julius Friedrich Cohnheim-Minerva Center for Phagocyte Research, the Israel Science Foundation (Grant 10/94), the Israel Cancer Research Fund, and The David and Natalie Roberts Chair in Immunopharmacology.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
   To whom correspondence should be addressed: Dept. of Human Microbiology, Sackler School of Medicine, Tel Aviv University, Tel Aviv 69978, Israel. Tel.: 972-3-640-7872; Fax: 972-3-642-9119; E-mail: epick{at}ccsg.tau.ac.il.
1   The abbreviations used are: Obardot 2, superoxide; GTPgamma S, guanosine 5'-3-O-(thio)triphosphate; AEBSF, 4-(2-aminoethyl)-benzenesulfonyl fluoride; AEBSNH2, 4-(2-aminoethyl)-benzenesulfonamide; AEBSAc, 4-(2-aminoethyl)-benzenesulfonic acid; MAEBSF, 4-(2-N-methylaminoethyl)-benzenesulfonyl fluoride; pABSF, 4-(amidino)-benzenesulfonyl fluoride; octyl glucoside, n-octyl-beta -D-glucopyranoside; PMA, phorbol 12-myristate 13-acetate; fMLP, N-formyl-Met-Leu-Phe; PMSF, phenylmethanesulfonyl fluoride; pAPMSF, 4-(amidino)-phenylmethanesulfonyl fluoride; TPCK, n-tosyl-L-phenylalanine chloromethyl ketone; DCIC, 3,4-dichloroisocoumarin; LiDS, lithium dodecyl sulfate.
2   Data sheet on "Pefabloc SC PLUS" by Boehringer Mannheim.

ACKNOWLEDGEMENTS

We thank Dr. T. L. Leto (National Institutes of Health, Bethesda, MD) for providing baculoviruses carrying cDNAs for p47phox and p67phox and Rac1 plasmid in E. coli and S. Hanft for word processing.


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