Macrophage Nitric Oxide Synthase Associates with Cortical Actin but Is Not Recruited to Phagosomes

doi:10.1128/IAI.69.10.6391-6400.2001

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Webb, J. L.
	Articles by Evans, T. J.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Webb, J. L.
	Articles by Evans, T. J.

Previous Article | Next Article

Infection and Immunity, October 2001, p. 6391-6400, Vol. 69, No. 10
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.10.6391-6400.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Macrophage Nitric Oxide Synthase Associates with Cortical Actin but Is Not Recruited to Phagosomes

J. L. Webb, M. W. Harvey, David W. Holden, and T. J. Evans^*

Department of Infectious Diseases, Imperial College School of Medicine, Hammersmith Hospital, London W12 0NN, United Kingdom

Received 24 January 2001/Returned for modification 24 April 2001/Accepted 11 July 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Nitric oxide (NO) produced from inducible NO synthase (iNOS) is an important component of host defense against intracellularpathogens. To understand how phagocytes deliver NO to ingestedmicroorganisms while avoiding cytotoxicity, we set out to studythe subcellular localization of iNOS within macrophages followingphagocytosis. Confocal microscopy of immunostained cells showedthat iNOS was located not only diffusely within cytoplasm butalso in vesicles, as well as immediately adjacent to the peripheralcell membrane. This peripheral iNOS colocalized with the corticalactin cytoskeleton and was removed by the actin-depolymerizingdrug cytochalasin B. Biochemical fractionation of RAW 264 macrophagesshowed that 32.75% (±5.11%; n = 3) of iNOS was present in a particulatefraction, which cosedimented with low-density cellular vesicles.Following phagocytosis of latex beads, zymosan, immunoglobulinG-coated beads, or complement-coated zymosan, submembranous corticaliNOS was not recruited to phagosomes, nor was there any relocalizationof intracellular iNOS. Similarly, following phagocytosis of Salmonellaenterica serovar Typhimurium there was no recruitment of iNOSto the Salmonella vacuole at any stage after internalization.NO mediated significant killing of intracellular S. enterica serovarTyphimurium in RAW macrophages treated with lipopolysaccharideand gamma interferon; this was evident 4 h after infection. Althoughnot recruited to phagosomes, iNOS association with the submembranouscortical actin cytoskeleton is ideally suited to deliver NO tomicrobes in contact with the cell surface and may contribute toearly killing of ingested Salmonella.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Nitric oxide (NO) plays important roles in many different aspects of mammalian biology (25). In phagocytes, NO is producedin large quantities by the action of the enzyme inducible NO synthase(iNOS), also known as type II NOS (20, 33). This isoform isproduced following stimulation of cells with agents such as inflammatorycytokines and lipopolysaccharide (LPS). Studies using NOS inhibitorsand mice with targeted disruption of the iNOS gene have demonstratedan important role of NO release from this enzyme in host defenseagainst a number of intracellular pathogens, including Mycobacteriumtuberculosis, Leishmania major, Listeria monocytogenes, and Salmonellaenterica serovar Typhimurium (26, 32).

NO is a highly reactive free radical with antimicrobial activity on its own, but it also can form a number of oxidation productssuch as NO₂, NO₂, N₂O₃, and S-nitrosothiols. In addition, it reacts with superoxideto yield the extremely reactive and microbicidal peroxynitriteanion, ONOO (2, 41). Collectively, these reactive nitrogen intermediateshave a spectrum of antimicrobial activity mediated by their abilityto react with key protein and lipid molecules in microbes (18,29). These cytotoxic effects are not restricted to microbes,as reactive nitrogen intermediates can act on host cells to producecell necrosis or apoptosis, thus potentially exacerbating tissueinjury where produced (5, 19).

This balance between microbicidal activity and potential cytotoxicity applies to many of the antimicrobial products producedby phagocytes, such as lysosomal enzyme products and superoxide.How do these cells avoid the damaging effects of these chemicals,while still efficiently killing invading pathogens? One mechanismis by compartmentalizing these toxic compounds within the cellso that they are released in close proximity to the pathogen,for example, by fusion of lysosomes with phagosomes or targetingof the superoxide-generating cytochrome b to neutrophil-specificgranules (4, 8, 23). Pathogens also have strategies toavoid these compartmentalized killing compounds. For example,S. enterica serovar Typhimurium disrupts intracellular traffickingand avoids fusion with lysosomal contents (7). It also preventsmovement of active NADPH oxidase to the Salmonella vacuole (38).This effect on the movement of NADPH oxidase is mediated by atype III secretion system encoded within Salmonella pathogenicityisland 2 (SPI-2) (38). However, NO still has an important antimicrobialeffect against serovar Typhimurium, mainly by exerting a relativelydelayed bacteriostatic effect within macrophages (37).

In neutrophils, we have shown that iNOS is localized to primary granules, where it is able to mediate nitration of ingestedbacteria, most likely through the generation of peroxynitrite(13). In macrophages, although the enzyme is frequently describedas cytoplasmic, some reports have shown that a proportion of theenzyme is localized to a particulate fraction within the cell(17, 30). One study has addressed the subcellular localizationof iNOS within primary macrophages, using immunoelectron microscopy(39). This found that a proportion of iNOS was present in apopulation of vesicles, most notably in the trans-Golgi network.The authors reported that iNOS was not associated with phagosomescontaining Mycobacterium avium or Leishmania mexicana, althougha preliminary association of iNOS vesicles with phagosomes containingimmunoglobulin G (IgG)-coated beads was mentioned. However, noimages of the distribution of iNOS following phagocytosis werepresented.

Once iNOS has been induced within the macrophage, there appear to be few further controls over its activity (27), althoughthe availability of tetrahydrobiopterin and L-arginine may beimportant (31, 34). Given the high reactivity of NO, we postulatedthat one way in which the cell could control the delivery of NOto its targets would be by subcellular compartmentalization, specificallyto phagosomes. Using high-resolution laser confocal immunofluorescencemicroscopy and biochemical techniques, we found in both primarymurine macrophages and the macrophage cell line RAW264 stimulatedwith LPS and gamma interferon (IFN- $gamma$ ) that a proportion of iNOSwas associated with the cortical submembranous actin cytoskeleton,as well as in intracytoplasmic vesicles and in free cytoplasm.Following phagocytosis of a variety of particles or the pathogenS. enterica serovar Typhimurium, membrane-associated iNOS didnot relocalize around phagosomes, nor was there recruitment ofcytoplasmic iNOS to phagosomes. However, NO mediated a significantkilling effect against serovar Typhimurium within 4 h of infectionin LPS- and IFN- $gamma$ -treated cells that may be mediated by membrane-associatediNOS.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Reagents and antibodies. Rabbit polyclonal (N32030) and murine monoclonal (N39120) antibodies to iNOS were from Transduction Laboratories, Lexington,Ky., as was mouse monoclonal antibody to GM130. Goat polyclonalanti-LAMP1 was from Santa Cruz Biotechnology. Secondary antibodiesconjugated to Alexafluors were from Molecular Probes (Eugene,Oreg.). Biotinylated secondary antibodies to mouse, rabbit, orgoat immunoglobulin were from Jackson ImmunoResearch Laboratories,West Grove, Pa., or Vector Laboratories, Peterborough, UnitedKingdom. Fluorescein isothiocyanate or Texas red avidin was boughtfrom Vector Laboratories. Latex beads and zymosan particles werefrom Sigma-Aldrich, Poole, United Kingdom. Wild-type Salmonellaenterica serovar Typhimurium 12023, its corresponding SPI-2 mutant,and the green fluorescence protein-labeled wild-type strain wereas previously described (3).

Cell culture. To obtain peritoneal macrophages, CD1 mice were primed with thioglycolate broth or BioGel P100 beads (Bio-Rad, Hercules, Calif.).Three days later, peritoneal fluid was collected and cells werewashed in Hanks balanced salt solution (Life Technologies Ltd.,Paisley, United Kingdom) and plated out for 2 h at 37°C. Adherentmacrophages were then washed free of other cells. Cells were seededonto glass coverslips (Merck Ltd., Poole, United Kingdom) in 24-welldishes (Corning Costar, High Wycombe, United Kingdom) at 10⁶ cells ml¹. Both RAW 264 cells and primary macrophages were cultured inDulbecco's modified Eagle's medium (Life Technologies Ltd.) with10% heat-inactivated fetal calf serum (Labtech International,Ringmer, United Kingdom) and 1 mM glutamine (Life TechnologiesLtd.). Where indicated, cells were stimulated for 18 h with 10ng of IFN- $gamma$ (Peprotech EC Ltd., London, United Kingdom) ml¹ and 2 µg of LPS from Escherichia coli serotype 0111:B4 (Sigma-Aldrich)ml¹. If used, cytochalasin B (Sigma-Aldrich) was added to cells at10 µM for 30 min. Particles were centrifuged onto the macrophagesat 450 × g for 2 min, normally at a ratio of 10 to 1. Zymosanwas prepared by being boiled in phosphate-buffered saline (PBS;0.01 M sodium phosphate buffer [pH 7.3], 0.15 M NaCl) for 30 min.Bacteria were used at stationary phase or logarithmic phase, opsonizedin 10% mouse serum (Serotec Ltd., Oxford, United Kingdom) for15 min at 37°C, and then washed three times with PBS before beingadded tomacrophages.

Immunostaining. iNOS was detected by immunocytochemistry using either a murine monoclonal iNOS antibody or a rabbit polyclonal anti-iNOS (bothfrom Transduction Laboratories). The monoclonal antibody recognizesa single 135-kDa protein, the expected weight of iNOS, in cytokine-treatedhuman and murine cells (28, 40). After incubation, cells werewashed gently three times with PBS and left to dry. Cells werefixed in 1% paraformaldehyde for 30 min, washed in PBS, and thenblocked in 0.2 M glycine in PBS for 15 min. Cells were washedthree times in PBS and then permeabilized in 0.1% Triton X-100in PBS for 15 min. After further washes in PBS, cells were blockedin 10% serum (Serotec Ltd.), using animal serum correspondingto the host in which the secondary antibody was derived. Afterat least 30 min of incubation, the block was removed and primaryantibody to iNOS was added. Cells were incubated for 18 h at 4°C.After three 5-min washes in PBS, secondary antibody to mouse orrabbit was added either using Alexafluor conjugates (MolecularProbes Europe BV, Leiden, The Netherlands) or adding the appropriatebiotinylated secondary antibody (Vector Laboratories or JacksonImmunoResearch Laboratories) and then adding fluorescein isothiocyanateor Texas red-conjugated avidin (Vector Laboratories). Tetramethylrhodamine isocyanate-phalloidin (Sigma-Aldrich) was used to detectfilamentous actin. After washing, DAPI (4',6'-diamidino-2-phenylindole)(Sigma-Aldrich) was added to stain nuclei. Cells were mountedin Vectashield (Vector Laboratories). Immunofluorescent imageswere acquired by confocal microscopy, using a Zeiss Axiovert microscopeand the Bio-Rad MRC 1024 Confocal system, running with LaserSharpsoftware.

Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and immunoblotting. To extract sufficient protein for Western analysis, 12 175-cm² flasks of RAW cells were used for each fractionation, using apublished method (35). Briefly, cells were stimulated with 10ng (200 U) of IFN- $gamma$ per ml and 2 µg of LPS ml¹ for 18 h and then scraped into 1 ml of lysis buffer (0.25 M sucrose,3 mM imidazole, 0.5 mM EDTA [pH 7.3]) containing 1 µg each ofleupeptin, aprotonin, chymotrypsin inhibitor, and antipain ml¹. Cells were centrifuged at 750 × g for 7 min, and the cell pelletwas resuspended in 100 µl of lysis buffer. This suspension waspassed through a 21-gauge needle until cell breakage occurred,and then it was centrifuged at 750 × g for 7 min to remove nuclei.The supernatant was then centrifuged at 100,000 × g for 2 h toseparate soluble and particulate fractions. The pellet, containingparticulate material, was resuspended in 1 ml of lysis buffer,vortexed gently, and left on ice for 30 min. It was then layeredonto 9 ml of 17% Percoll, which was above a cushion of 2 ml of64% sucrose, both made up in lysis buffer. Tubes were centrifugedat 56,000 × g for 1 h (without the brake) and 1-ml fractions wererecovered by puncturing the tube. Fractions were run on an 8%acrylamide sodium dodecyl sulfate-polyacrylamide gel electrophoresisgel and blotted onto a polyvinylidene difluoride membrane (AmershamPharmacia Biotech UK, Little Chalfont, United Kingdom). iNOS wasdetected with a monoclonal iNOS antibody (Transduction Laboratories)and biotinylated secondary anti-mouse antibody (Vector Laboratoriesand Jackson ImmunoResearch Laboratories), horseradish peroxidase-streptavidinreagent (Serotec Ltd.), and ECL plus detection (Amersham PharmaciaBiotech UK). To identify cell surface proteins, cells were treatedwith biotinylation reagent EZ-Link Sulfo-NHS-LC-Biotin (PierceChemical Company, Rockford, Ill.) before being scraped into lysisbuffer. To identify fractions containing transferrin (early endosomes),20 nM biotin-transferrin (Molecular Probes) was added to unstimulatedRAW cells and incubated for 20 min at 37°C before being washedwith PBS, and cells were scraped from the flask in 1 ml of lysisbuffer.

Quantification of iNOS protein within particulate and soluble fractions was determined by densitometric analysis of Westernblots in a linear range of exposure. Results are expressed asa percentage of the total iNOS present within the celllysate.

iNOS activity assay. Fractions and totals were assayed for iNOS activity by following the conversion of [³H]arginine to citrulline (NOSdetect Assay Kit; Stratagene, Amsterdam,The Netherlands). To duplicate reaction mixtures, we added 2 mML-NIL hydrochloride (Calbiochem-Novabiochem [UK] Ltd., Nottingham,United Kingdom) to identify iNOS-dependent conversion to L-citrulline.Reactions were carried out according to the kit instructions,and L-citrulline was recovered by adding the reaction mixtureto columns containing DOWEX 50WX8-400 ion-exchange resin (Sigma-Aldrich)and washing it three times with water to elute citrulline. Thequantity of isotope was measured by liquid scintillationcounting.

$beta$ -Glucuronidase assay. To identify fractions containing lysosomes, we assayed the presence of $beta$ -glucuronidase activity by using a diagnostic kit(Sigma-Aldrich). Briefly, 20 µl of each fraction was mixed with20 µl of phenolphthalein glucuronic acid solution and 60 µl ofacetate buffer solution and incubated at 56°C for 1 h. Five hundredmicroliters of 2-amino-2-methyl-1-propanol buffer was added, andabsorbance was read at 550nm.

Assay of intracellular Salmonella viability. Monolayers of RAW macrophages in 24-well plates (10⁶ cells per well) treated as described above were infected with opsonizedSalmonella enterica serovar Typhimurium 12023 in the stationaryphase of growth at a multiplicity of infection of 10. To ensurea synchronous infection, after the addition of bacteria plateswere centrifuged at 200 × g for 4 min and then incubated at 37°Cfor 30 min. Gentamicin (12 µg ml¹) was then added to kill extracellular bacteria, and incubationwas continued as required. Viable intracellular bacteria wereassayed by washing the well twice with PBS, lysing the cells in100 µl of 1% Triton X-100 for 10 min at room temperature, andplating serial dilutions onto prewarmed LB agar plates. Afterovernight culture at 37°C, CFU were enumerated. Each experimentalpoint was determined intriplicate.

Statistical analysis. Results are given as the means plus or minus standard deviations. To calculate the percentage of cells expressing iNOS inthe plasma membrane, a total of >50 iNOS-positive cells were scoredin three to four separateexperiments.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Immunofluorescent microscopic localization of iNOS within mouse macrophages. We used a mouse monoclonal anti-iNOS and a polyclonal rabbit anti-iNOS. The pattern of staining was identical with both antibodiesused; isotype-matched control sera gave no immunostaining usingboth anti-mouse and anti-rabbit secondary reagents. Unstimulatedcells showed only 0 to 1% iNOS-positivecells.

We first analyzed the pattern of iNOS staining in primary mouse peritoneal macrophages stimulated with IFN- $gamma$ or IFN- $gamma$ andLPS (Fig. 1A to C). Three main sites of staining could be visualized.First, virtually all cells showed a degree of diffuse intracytoplasmicstaining, although this differed in intensity from cell to cell.Secondly, we found staining in discrete intracellular punctatestructures, consistent with a vacuolar localization of iNOS. Thesewere either distributed fairly evenly within the cytoplasm (Fig.1A) or in 5 to 10% of cells aggregated in the perinuclear area(Fig. 1B). The third site of staining was at the periphery ofthe cell, apparently in the region of the plasma membrane (Fig.1B and C). Fifty-seven percent (±8.92%; n = 4) of cells showedsome iNOS staining localized to this site. As the limit of resolutionof confocal microscopy is about 0.5 µm, this immunostaining maybe either in association with the membrane or immediately belowit in the submembranous area. To avoid confusion, we term thisperipheral staining cortical iNOS localization. The relative amountof iNOS in this cortical location, compared to an intracytoplasmicsite, varied among different macrophage preparations. However,the cortical iNOS shown in Fig. 1B and C is representative ofall the preparations. Quantification of the proportion of iNOSat this location is considered further below and in Discussion.We noted that the majority of cells with cortical iNOS had a roundedshape, while those that had extended one or more pseudopodia tendednot to show peripheral iNOS staining (Fig. 1A and B).

View larger version (82K):
[in this window]
[in a new window]

FIG. 1. Localization of iNOS within macrophages. Primary mouse peritoneal macrophages (A to C) or RAW 264 cells (D) were stimulated with IFN- $gamma$ alone (A) or with IFN- $gamma$ and LPS (B to D) and immunostained for iNOS, using the mouse monoclonal antibody. All images were obtained using laser confocal microscopy. Magnification, ×2,000 (A), ×600 (B to C), or ×6,000 (D). Arrows indicate peripheral plasma membrane staining of iNOS. The solid arrowhead in panel B indicates iNOS staining in the perinuclear area.

We also examined the distribution of iNOS within IFN- $gamma$ - and LPS-treated RAW 264 cells, a mouse macrophage cell line. A similarpattern of distribution of staining was seen, with 43.3% (±8.79%;n = 3) of cells showing some cortical iNOS staining (Fig. 1D).In addition, in about 5 to 10% of cells we also observed the perinuclearstaining seen in the primary macrophages. To determine whetheriNOS in the perinuclear area was localized within the Golgi apparatus,we stained IFN- $gamma$ - and LPS-treated RAW cells for both iNOS andthe intrinsic Golgi membrane protein GM130. In cells showing perinucleariNOS (Fig. 2A), the pattern of GM130 staining (Fig. 2B) overlappedconsiderably with perinuclear iNOS staining (Fig. 2C). Not allthe iNOS-positive vesicles in this area, however, colocalizedwith GM130, as the merged image of Fig. 2C shows some vesiclesin the Golgi region that stain only with iNOS and thus are greenin the merged image. However, in all instances where there wasperinuclear iNOS staining we saw overlapping of most of the iNOSstaining with that for GM130. These data suggest that some ofthe perinuclear iNOS staining observed is in the Golgi apparatus,although at least a proportion is in a vesicle population thatdoes not contain GM130.

View larger version (10K):
[in this window]
[in a new window]

FIG. 2. iNOS can be found in the Golgi apparatus. RAW 264 cells were stimulated with LPS and IFN- $gamma$ and dually stained for iNOS using a rabbit polyclonal antibody, with red staining (A), and the intrinsic Golgi protein GM130, with green staining (B). (C) Merged images of panels A and B, with areas of colocalization in yellow. Magnification, ×1,000 for all panels.

iNOS associates with actin at the cell periphery. We examined whether there was an association between iNOS and the cortical actin cytoskeleton that might account for its localizationat the cell periphery. Using fluorescent phalloidin to visualizepolymerized actin, we found that iNOS and polymerized actin colocalizeat the cell periphery (Fig. 3A to C). When the cortical cytoskeletonwas disrupted with cytochalasin B, cortical iNOS was completelydisrupted, with iNOS distributed entirely within the cytoplasm(Fig. 3D to F). It is important to stress that following cytochalasintreatment, we were unable to detect any cell that showed corticaliNOS staining. These data suggest strongly that the peripheraliNOS is associated with the cortical actin cytoskeleton. To determineif any iNOS was exposed on the surface of cells, we immunostainedmacrophages for iNOS with no prior permeabilization step. Underthese conditions, we observed no iNOS staining (data not shown).Taken together, these data suggest that iNOS associates with thecortical actin cytoskeleton at the cytoplasmic face of the plasmamembrane.

View larger version (25K):
[in this window]
[in a new window]

FIG. 3. iNOS associates with the cortical actin cytoskeleton. Primary peritoneal macrophages were stimulated with LPS and IFN- $gamma$ and immunostained for iNOS with the mouse monoclonal antibody in green (B and E) or polymerized actin in red (A and D). Cells were either untreated before staining (A to C) or treated with cytochalasin B (D to F). Panels C and F show the merged actin and iNOS images from panels A and B and panels D and E, respectively; areas of colocalization are shown in yellow. Magnification, ×600 for all panels.

Biochemical fractionation of iNOS within RAW 264 cells. In order to explore the subcellular distribution of iNOS further, we fractionated RAW 264 cells using biochemical techniques.We chose these cells for further study, as it was difficult toobtain enough material from primary peritoneal macrophages withoutsacrificing large numbers of animals. Particulate and solublefractions were analyzed for the presence of iNOS by Western blotting.We found that 32.75% (±5.11%; n = 3) of total cellular iNOS wasrecovered in the particulate fraction as assayed by densitometryof immunoblots, in good agreement with other studies (30, 39).The activity of this particulate material was also measured andfound to be 16.47% (±0.15%; n = 3) of total cellular iNOS activity.The smaller amount of iNOS activity in the particulate material,compared to the amount of iNOS protein, may reflect poor accessof substrates and cofactors to the particulate enzyme or somedenaturation on centrifugation, or it may truly reflect a differencein specific activity of iNOS in cytosolic and particulatelocations.

We resuspended the particulate material and fractionated it by Percoll density centrifugation, using a protocol that separatedplasma membrane and early endosomes from late endosomal and lysosomalvesicles (35). Western blotting of fractions from this gradientshowed that most of the iNOS protein was found in the lightestfractions (Fig. 4A, lanes 1 to 3), although a small amount couldbe detected in the remaining denser fractions (Fig. 4A, lanes4 to 11). To detect iNOS in these denser fractions required afilm exposure that overexposes the iNOS signal in lanes 1 to 4,thus underestimating the percentage of iNOS in these fractions.Using shorter exposures, densitometry showed that 95% of particulateiNOS sedimented in fractions 1 to 3. Enzymatic assay of iNOS fromthese gradient fractions showed a similar distribution, confirmingthat this particulate iNOS was enzymatically active (Fig. 4B).Surface biotinylated proteins were identified exclusively in thelight region of the gradient (Fig. 4C, lanes 1 and 2), with adistribution similar but not completely identical to that of iNOS.Assay of the lysosomal enzyme $beta$ -glucuronidase showed two peaksof activity (Fig. 4D). There was a peak in the denser region ofthe gradient, consistent with previous reports showing that lysosomesare denser than early components of the endocytic pathway (8,35). There was, however, another peak in the lighter portionof the gradient, in the same fractions as the surface proteinand iNOS. This was a consistent feature of Percoll fractionationof LPS- and IFN- $gamma$ -stimulated RAW cells. This lighter density fractionmay result from intracellular acidification following macrophageactivation, a process that has been reported to lower the densityof lysosomes (21). Attempts were made to improve the resolutionof the Percoll density gradient separation, but these were notsuccessful. Although the separation is not complete, the datashow that particulate iNOS from lysed cells is contained in alight vesicle population that is enzymatically active and distinctfrom dense lysosomes but is of a density similar to that of vesiclesderived from plasma membrane.

View larger version (24K):
[in this window]
[in a new window]

FIG. 4. Density gradient centrifugation analysis of the particulate fraction of IFN- $gamma$ - and LPS-treated RAW 264 cells. Each panel shows an assay performed on each of 12 fractions from the density gradient, with the lighter fractions to the left (top) and the denser ones to the right (bottom). The experiment was repeated with similar results. (A) iNOS protein, detected by Western blotting. The band shown is the major band detected, at 135 kDa. So that the bands in lanes 6 to 11 could be seen, the blot was overexposed for lanes 1 to 3. (B) iNOS activity, as assayed by arginine-to-citrulline conversion. (C) Surface proteins of the cell, labeled by surface biotinylation, identified by probing the Western blot with horseradish peroxidase-streptavidin. The gel shows proteins ranging in size from 200 kDa at the top of the panel to 29 kDa at the bottom. (D) $beta$ -glucuronidase activity.

Patterns of iNOS localization following phagocytosis. Next, we examined the pattern of iNOS staining within macrophages following phagocytosis of a variety of particles. Theseincluded latex beads, zymosan, IgG-coated magnetic beads, andcomplement-coated zymosan particles. Representative results fromexperiments with primary macrophages are shown in Fig. 5. PanelsA and B show iNOS staining (green) following phagocytosis of latexbeads for a 30-min period. iNOS staining remained at the peripheryof the cells and did not localize to phagosomes. Similar resultswere seen at much earlier time points (2 and 5 min of particleinternalization; data not shown), with no localization of iNOSto phagosomes at any stage of bead uptake. Following internalizationof latex beads, phagosomes were allowed to mature for a further2 h and the pattern of iNOS distribution was analyzed (Fig. 5Dto F). This showed that the majority of latex bead-containingphagosomes had no accumulation of iNOS at their periphery (Fig.5D). There were occasional phagosomes that showed iNOS accumulationat their periphery (Fig. 5D). However, this was seen in only fewerthan 1% of the cells. In contrast, after this period of maturation,most phagosomes showed accumulation of the lysosomal marker LAMP-1(Fig. 5E and F) confirming the fusion of lysosomes with phagocytosedlatex beads at this time after ingestion.

View larger version (63K):
[in this window]
[in a new window]

FIG. 5. iNOS distribution following phagocytosis in mouse primary peritoneal macrophages. Cells treated with IFN- $gamma$ and LPS were used in all panels. (A and B) Uptake of latex beads at 30 min after addition. iNOS staining (mouse monoclonal) in green is shown alone (A) and also merged with the differential interference contrast (DIC) image of the same cell (B). (C) A cell, 2 min after addition of zymosan particles, stained for iNOS (mouse monoclonal) in green. Accumulation of iNOS at the tips of pseudopodia closing around zymosan just entering the cell is shown by arrows. (D to F) Cells, 2 h after being fed latex beads for 10 min, which were then removed by washing. The panels show the pattern of iNOS staining (mouse monoclonal) in green (D), LAMP-1 staining in red (E), and the merged images of panels D and E (F), where areas of colocalization are shown in yellow. Two areas showing apparent accumulation of iNOS around the outside of phagocytosed beads are indicated by arrows in panel D. (G and H) Uptake of IgG-coated magnetic beads at 5 min after addition. iNOS staining (rabbit polyclonal antibody) in green is shown alone (G) and merged with the DIC image of the same cell (H). (I) A cell, 10 min after the addition of complement-coated zymosan particles stained for iNOS (mouse monoclonal) in green. Magnification, ×2,000 for all panels.

Similarly, there was a lack of association of iNOS with phagosomes containing IgG and complement-coated particles at variousstages of maturation (Fig. 5G to I and data not shown). When macrophageswere allowed to phagocytose zymosan particles, at 2 min afteraddition cells in which pseudopodial arms were closing aroundthe ingested particle could be observed (Fig. 5C). iNOS appearedto be selectively localized to the point of fusion of the pseudopodialarms under these conditions (Fig. 5C). Fixation of cells exactlyat this point of pseudopodial fusion was a relatively rare event,so that the significance of the iNOS staining observed in thesecells is difficult to gauge. However, this was observed only withzymosanparticles.

iNOS localization following ingestion of S. enterica serovar Typhimurium. Using a virulent strain of S. enterica serovar Typhimurium labeled with green fluorescent protein, we analyzed the distributionof iNOS following phagocytosis of this microorganism (Fig. 6).In both primary cells (Fig. 6A) and RAW 264 macrophages (Fig.6B), there was no localization of iNOS around the Salmonella vacuoleat any stage of maturation (Fig. 6A and B and data not shown).Similar results were obtained using bacteria in either the stationaryor logarithmic phase of growth. Serovar Typhimurium prevents thetransport of NADPH oxidase to the Salmonella vacuole by a processthat is dependent on a type III secretory system encoded by apathogenicity island termed SPI-2 (32). We therefore examinedthe distribution of iNOS around phagosomes containing an SPI-2mutant strain (Fig. 6C). At a time when NADPH oxidase had accumulatedaround phagocytosed bacteria of this strain (38), we did notobserve any relocalization of iNOS (Fig. 6C). Furthermore, whenwe stained macrophages for nitrotyrosine, a marker of the formationof peroxynitrite anions, although this could be seen within cells,it did not localize around phagocytosed bacteria (Fig. 6D).

View larger version (29K):
[in this window]
[in a new window]

FIG. 6. iNOS and nitrotyrosine in macrophages following phagocytosis of serovar Typhimurium. In all cases, the bacteria are labeled green. (A) iNOS (red; mouse monoclonal) in a primary macrophage 2 h after phagocytosis of wild-type stationary phase serovar Typhimurium. (B) iNOS (red; rabbit polyclonal) in a RAW 264 cell 90 min after phagocytosis of wild-type stationary phase serovar Typhimurium. (C) iNOS (red; rabbit polyclonal) in a RAW 264 cell 4 h after phagocytosis of a SPI-2 mutant stationary-phase serovar Typhimurium. (D) Nitrotyrosine staining (red) in a RAW 264 cell 4 h after phagocytosis of wild-type stationary-phase serovar Typhimurium. Magnification, ×1,000 (B and D) or ×2,000 (A and C).

NO effects on bacterial uptake by macrophages. The presence of iNOS at the plasma membrane is ideal for delivery of NO to potentially pathogenic microorganisms as they undergophagocytosis. In a previous study of serovar Typhimurium survivalwithin macrophages using IFN- $gamma$ -primed macrophages, a delayed bacteriostaticeffect of NO production on bacterial proliferation was observed(37). Therefore, a possible explanation of the lack of recruitmentof iNOS to the Salmonella vacuole observed above is that we hadnot examined the cells at a point when NO was exerting its antibacterialeffect. Therefore, we measured the time course of survival ofSalmonella within RAW macrophages treated with (i) no additions,(ii) LPS and IFN- $gamma$ , (iii) LPS and IFN- $gamma$ and the NOS inhibitorL-NIL. Figure 7 shows that at 45 min after infection there wasno significant difference in survival of intracellular Salmonellaamong the three groups of cells. However, at 4 h after infectionthere was a significant reduction in the numbers of intracellularSalmonella in the LPS- and IFN- $gamma$ -treated cells compared to untreatedcells, a difference that was abolished by the NOS inhibitor L-NIL(Fig. 7). Numbers of intracellular bacteria increased by 20 hafter infection in all groups, although the difference betweenthe LPS- and IFN- $gamma$ -treated group and the others remained. Underthese conditions, the NOS inhibitor L-NIL inhibited macrophageNO output by >95%, as detected by a Griess assay (data not shown).Thus, NO does exert an antibacterial effect in these cells, whichis evident at 4 h after infection $---$ a time when we observed no recruitmentof iNOS to the Salmonella vacuole (Fig. 6C and data not shown).

View larger version (15K):
[in this window]
[in a new window]

FIG. 7. Survival of serovar Typhimurium within RAW macrophages. Cells were infected at a multiplicity of infection of 10 with 10⁷ bacteria at time zero. The graph shows the mean intracellular bacterial numbers found in RAW 264 cells either unstimulated (US), treated with LPS and IFN- $gamma$ (S), or treated with LPS and IFN- $gamma$ plus L-NIL (S+LNIL). Error bars, ± 1 standard deviation. A significant difference was found in intracellular Salmonella survival between cells treated with LPS and IFN- $gamma$ and cells treated with LPS, IFN- $gamma$ , and L-NIL at 4 and 20 h after infection. *, P < 0.05; ** P < 0.01 (two-tailed t test).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The work presented here reports the novel observation that a proportion of iNOS is associated with the cortical actin cytoskeletonin primary mouse macrophages and the murine macrophage cell lineRAW 264. iNOS was also found in an intracellular vesicle population,within the Golgi apparatus, and diffusely within the cytoplasm.Following phagocytosis of a variety of particles, there was littleevidence of recruitment of iNOS to phagosomes; neither was thererelocation of iNOS around phagocytosed serovar Typhimurium. Althoughnot recruited to the phagosome, cortical iNOS is ideally placedto deliver microbicidal NO to microorganisms in contact with thecellsurface.

We also found iNOS diffusely within the cytoplasm, within cytoplasmic vesicles, and in a Golgi compartment (Fig. 1 and 2).The relative distribution of iNOS between these different subcellularsites is difficult to gauge from confocal microscopy, as pixeldensities for each component would have to be calculated for multipleconfocal sections through each cell to calculate the total distributionof iNOS. From the combined imaging, biochemical fractionation,and activity assays, we estimate that about 20% of iNOS is localizedto the cortical region in macrophages following LPS and IFN- $gamma$ stimulation under the conditions usedhere.

What can we deduce about the functional role of the differentially distributed iNOS we have described? We originally hypothesizedthat iNOS would be targeted to phagosomes, in order to delivera high concentration of NO to ingested microbes and limit possibledamaging effects to the rest of the cell. Cortical iNOS is obviouslywell placed to deliver NO to incoming microorganisms that arebeing ingested. However, following phagocytosis of a variety ofparticles, cortical iNOS is not retained in or recruited to thephagosome (Fig. 5). Similarly, there was no association of iNOSwith phagocytosed serovar Typhimurium (Fig. 6). These experimentsutilized all the major molecular mechanisms for triggering phagocytosis $---$ theFc receptor, complement receptors, and the mannose receptor. Itseems unlikely, therefore, that failure to observe recruitmentof iNOS to the phagosome resulted from lack of signaling fromcell surface receptors engaged during phagocytosis. Phagocytosisinvolves the internalization of a large proportion of the macrophagecell membrane, but only a very small proportion of plasma membraneproteins are removed as a result of this process, the majoritybeing returned to their original locations (22). Integral membraneproteins such as Toll-like receptor 2 and natural resistance-associatedmacrophage protein 1 (N-RAMP1) are recruited to the phagosomalmembrane (16, 36), although in the case of Toll-like receptor2, this association can be transient. We analyzed iNOS localizationaround phagosomes at a range of times after formation, includingvery early stages at 2 min after particle internalization. Wedo not feel, therefore, that we missed a transient early recruitmentof iNOS to the phagosome. The association of iNOS with the corticalactin cytoskeleton, on the cytoplasmic side of the cell membrane(Fig. 3), suggested that it might move with actin to the phagosomalmembrane. However, not all actin-associated proteins show sucha redistribution. For example, in phagocytosis of unopsonizedzymosan, the actin-associated proteins vinculin and paxillin donot associate with phagosomes (1).

Despite the lack of recruitment of iNOS to phagosomes, NO clearly has important antimicrobial actions within macrophages,notably for serovar Typhimurium (37) (Fig. 7). In IFN- $gamma$ -treatedmacrophages (37), this effect, although noticeable at 2 h afterbacterial entry, was more marked 10 h after infection. We foundthat in LPS- and IFN- $gamma$ -stimulated cells, the effect was somewhatearlier, with clear NO-dependent killing at 4 h after bacterialentry (Fig. 7). This difference may reflect the time taken forinduction of iNOS in IFN- $gamma$ -treated macrophages following bacterialingestion. In LPS- and IFN- $gamma$ -stimulated cells, high levels ofiNOS are already present, so that the time course of Salmonellakilling more accurately reflects the time of antimicrobial actionof NO against the ingested microbe. However, in vivo, it may bemore likely that macrophages are first activated with IFN- $gamma$ andthen receive an LPS stimulus on phagocytosing Salmonella. Thus,the time course of Salmonella killing by macrophages in naturalinfection may be better reflected by cells activated with IFN- $gamma$ alone rather than LPS and IFN- $gamma$ .

iNOS association with the cortical actin cytoskeleton may be important in targeting NO to bacteria as they enter the cell,although the effects on phagocytosed serovar Typhimurium are notevident until 4 h after uptake of the bacteria into the cell.Alternatively, it may be that NO is capable of antimicrobial actionwithout producing cytotoxicity, even if it is not delivered directlyto the Salmonella vacuole. Unlike superoxide, NO can readily diffuseacross membranes (10) and thus could enter the phagosome fromthe cytosol. This might account for the localization of the NADPHoxidase but not iNOS to the phagosomal membrane. In addition,the exact identity of the reactive nitrogen species responsiblefor anti-Salmonella activity is unknown. For example, NO may alsoproduce potent antimicrobial compounds by reacting with cytosolicthiols to yield S-nitrosothiols. These reactions may be facilitatedby cytosolic localization of NO production by iNOS. To determinethe contribution of cortical actin-associated iNOS to Salmonellakilling will require the construction of iNOS mutants that arespecifically targeted to either plasma membrane or cytoplasm.Cells expressing these differently localized enzymes can thenbe assayed for their ability to affect intracellular Salmonellareplication.

Serovar Typhimurium has evolved mechanisms which enable it to avoid contact with the NADPH oxidase within macrophages, asrevealed by SPI-2 mutants (38). These mutants, however, alsofailed to show accumulation of iNOS around phagocytosed bacteria(Fig. 6C). Although Salmonella may have other genes which encodea factor able to prevent iNOS localization around phagosomes,we feel that this is very unlikely, since a variety of experimentalparticles also failed to show iNOS recruitment to the phagosome(Fig. 5). In addition, we did not observe any iNOS accumulationaround phagocytosed E. coli, which enters but does not proliferatewithin macrophages (data not shown). It has been assumed thatperoxynitrite, the product of NO and superoxide, is a major antimicrobialfactor within macrophages (41). However, Vazquez Torres et al.(37) showed no localization of nitrotyrosine around intracellularSalmonella and found that the peroxynitrite scavenger uric acidpotentiates rather than inhibits Salmonella killing. In addition,there was a clear temporal separation of the roles of NADPH oxidaseand iNOS in Salmonella killing. Thus, it seems unlikely that peroxynitriteis responsible for macrophage killing of intracellular Salmonella.Although there was evidence of nitrotyrosine generation withinmacrophages in our experiments, we too found no localization aroundphagocytosed bacteria (Fig. 6D), unlike the extensive nitrationaround phagocytosed Staphylococcus aureus within neutrophils (13).It may be that bacterial peroxiredoxins in Salmonella are ableto detoxify peroxynitrite within the vicinity of the bacterium,avoiding nitration (6). However, deletion of the gene for thesmall subunit of the peroxiredoxin alkylhydroperoxide reductasein serovar Typhimurium does not affect virulence, suggesting thatsuch a mechanism is not critical for pathogenesis. An alternativeexplanation for the absence of nitration of intracellular Salmonellamight be the abundance of periplasmic superoxide dismutase inthe bacteria, limiting in situ formation of peroxynitrite fromNO and superoxide (9, 14, 15).

One previous report analyzed the subcellular distribution of iNOS in primary macrophages using immunoelectron microscopy (39).These authors found that iNOS was both cytoplasmic and in a vesiclepopulation, particularly at the trans face of the Golgi apparatus,and with some staining at the cell periphery. A notable featureof the cells showing the most marked membrane iNOS staining inthe present study is that they had a rounded, nonactivated shape,even after LPS and IFN- $gamma$ stimulation. Thioglycolate-induced macrophagescan show a more activated macrophage phenotype, with extensionof multiple pseudopodia (12). Cells with this morphology tendednot to show plasma membrane iNOS, suggesting that the signal involvedin the generation of this phenotype leads to loss of iNOS fromthis site. Differences in macrophage activation state may thusaccount for differences in iNOSdistribution.

Cortical iNOS might be involved not in microbial killing but in some other function. Recently, an essential role for NO derivedfrom iNOS has been demonstrated in the signaling pathway of interleukin12 (IL-12) and IFN- $alpha$ / $beta$ within NK cells (11). Plasma membrane-associatediNOS would be well placed to deliver NO locally to the IL-12 receptorsignaling complex, maximizing its signaling effects while limitingtoxicity within the cell. Macrophages have recently been shownto respond to combined IL-12 and IL-18 stimulation with an increasedoutput of IFN- $gamma$ (24). Whether NO participates in the IL-12 signalingpathway in macrophages remains to bedetermined.

What mechanism underlies the association of iNOS with the cortical actin cytoskeleton? It has been found that in epithelialcells, iNOS is localized to the apical membrane of polarized cells(P. Glynne and T. J. Evans, submitted for publication). The interactionof iNOS with membranes from these epithelial cells shows thatiNOS is a tightly bound peripheral protein, associating with thecortical actin cytoskeleton and requiring mixtures of salt anddetergent for efficient solubilization. This suggests that similarmolecular mechanisms are involved in tethering iNOS to the corticalregion in all these cells. iNOS does not have an intrinsic membrane-spanningdomain, nor does it have known lipid modifications, suggestingthat the most likely mechanism is by a direct protein-proteininteraction with a component of the cortical actin cytoskeleton.The Golgi association may thus reflect the trafficking of iNOSin association with this protein through the cell on its way tothe cellcortex.

iNOS is an important part of the phagocyte's defensive capabilities, and the work described here sheds more light on the wayin which it is controlled by the cell. Further work with additionalpathogens will better define the precise role that membrane-associatediNOS has in microbial killing and may reveal additional functionsofiNOS.

	ACKNOWLEDGMENTS

We thank Julia Polak for providing facilities for confocalmicroscopy.

This work was supported by the Wellcome Trust and the Lister Institute by the award of a Jenner Fellowship to T.J.E.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Infectious Diseases, Imperial College School of Medicine, HammersmithHospital, Du Cane Rd., London W12 0NN, United Kingdom. Phone:44 20 8383 8576. Fax: 44 20 8383 3394. E-mail: tom.evans{at}ic.ac.uk.

Editor: V. J. DiRita

	REFERENCES

Top Abstract Introduction Materials and Methods Results Discussion References

1.	Allen, L. A., and A. Aderem. 1996. Molecular definition of distinct cytoskeletal structures involved in complement- and Fc receptor-mediated phagocytosis in macrophages. J. Exp. Med. 184:627-637[Abstract/Free Full Text].
2.	Beckman, J. S., and J. N. Siedow. 1985. Bactericidal agents generated by the peroxidase-catalyzed oxidation of para-hydroquinones. J. Biol. Chem. 260:14604-14609[Abstract/Free Full Text].
3.	Beuzon, C. R., S. Meresse, K. E. Unsworth, J. Ruiz-Albert, S. Garvis, S. R. Waterman, T. A. Ryder, E. Boucrot, and D. W. Holden. 2000. Salmonella maintains the integrity of its intracellular vacuole through the action of SifA. EMBO J. 19:3235-3249[CrossRef][Medline].
4.	Borregaard, N., J. M. Heiple, E. R. Simons, and R. A. Clark. 1983. Subcellular localization of the b-cytochrome component of the human neutrophil microbicidal oxidase: translocation during activation. J. Cell Biol. 97:52-61[Abstract/Free Full Text].
5.	Brune, B., A. von Knethen, and K. B. Sandau. 1998. Nitric oxide and its role in apoptosis. Eur. J. Pharmacol. 351:261-272[CrossRef][Medline].
6.	Bryk, R., P. Griffin, and C. Nathan. 2000. Peroxynitrite reductase activity of bacterial peroxiredoxins. Nature 407:211-215[CrossRef][Medline].
7.	Buchmeier, N. A., and F. Heffron. 1991. Inhibition of macrophage phagosome-lysosome fusion by Salmonella typhimurium. Infect. Immun. 59:2232-2238[Abstract/Free Full Text].
8.	Claus, V., A. Jahraus, T. Tjelle, T. Berg, H. Kirschke, H. Faulstich, and G. Griffiths. 1998. Lysosomal enzyme trafficking between phagosomes, endosomes, and lysosomes in J774 macrophages. Enrichment of cathepsin H in early endosomes. J. Biol. Chem. 273:9842-9851[Abstract/Free Full Text].
9.	De Groote, M. A., U. A. Ochsner, M. U. Shiloh, C. Nathan, J. M. McCord, M. C. Dinauer, S. J. Libby, A. Vazquez-Torres, Y. Xu, and F. C. Fang. 1997. Periplasmic superoxide dismutase protects Salmonella from products of phagocyte NADPH-oxidase and nitric oxide synthase. Proc. Natl. Acad. Sci. USA 94:13997-14001[Abstract/Free Full Text].
10.	Denicola, A., J. M. Souza, R. Radi, and E. Lissi. 1996. Nitric oxide diffusion in membranes determined by fluorescence quenching. Arch. Biochem. Biophys. 328:208-212[CrossRef][Medline].
11.	Diefenbach, A., H. Schindler, M. Rollinghoff, W. M. Yokoyama, and C. Bogdan. 1999. Requirement for type 2 NO synthase for IL-12 signaling in innate immunity. Science 284:951-955[Abstract/Free Full Text].
12.	Doyle, A. G., and I. P. Fraser. 1998. Murine macrophages: isolation, cultivation, and characterization, p. 154.1-154.8. In D. M. Weir (ed.), Experimental immunology, 5th ed. Blackwell Scientific, Oxford, United Kingdom.
13.	Evans, T. J., L. D. K. Buttery, A. Carpenter, D. R. Springall, J. M. Polak, and J. Cohen. 1996. Cytokine-treated human neutrophils contain inducible nitric oxide synthase that produces nitration of ingested bacteria. Proc. Natl. Acad. Sci. USA 93:9553-9558[Abstract/Free Full Text].
14.	Fang, F. C., M. A. DeGroote, J. W. Foster, A. J. Baumler, U. Ochsner, T. Testerman, S. Bearson, J. C. Giard, Y. Xu, G. Campbell, and T. Laessig. 1999. Virulent Salmonella typhimurium has two periplasmic Cu, Zn-superoxide dismutases. Proc. Natl. Acad. Sci. USA 96:7502-7507[Abstract/Free Full Text].
15.	Figueroa-Bossi, N., and L. Bossi. 1999. Inducible prophages contribute to Salmonella virulence in mice. Mol. Microbiol. 33:167-176[CrossRef][Medline].
16.	Gruenheid, S., E. Pinner, M. Desjardins, and P. Gros. 1997. Natural resistance to infection with intracellular pathogens: the Nramp1 protein is recruited to the membrane of the phagosome. J. Exp. Med. 185:717-730[Abstract/Free Full Text].
17.	Hiki, K., Y. Yui, R. Hattori, H. Eizawa, K. Kosuga, and C. Kawai. 1991. Cytosolic and membrane-bound nitric oxide synthase. Jpn. J. Pharmacol. 56:217-220[Medline].
18.	Ischiropoulos, H., L. Zhu, J. Chen, M. Tsai, J. C. Martin, C. D. Smith, and J. S. Beckman. 1992. Peroxynitrite-mediated tyrosine nitration catalysed by superoxide dismutase. Arch. Biochem. Biophys. 298:431-437[CrossRef][Medline].
19.	Kroncke, K. D., K. Fehsel, and V. Kolb-Bachofen. 1997. Nitric oxide: cytotoxicity versus cytoprotection $---$ how, why, when, and where? Nitric Oxide 1:107-120[CrossRef][Medline].
20.	MacMicking, J., Q. W. Xie, and C. Nathan. 1997. Nitric oxide and macrophage function. Annu. Rev. Immunol. 15:323-350[CrossRef][Medline].
21.	Mayorga, L. S., M. G. De Veca, M. I. Colombo, and F. Bertini. 1993. Effect of pH and ATP on the equilibrium density of lysosomes. J. Cell. Physiol. 156:303-310[CrossRef][Medline].
22.	Mellman, I. 2000. Quo vadis: polarized membrane recycling in motility and phagocytosis. J. Cell Biol. 149:529-530[Abstract/Free Full Text].
23.	Mullock, B. M., N. A. Bright, C. W. Fearon, S. R. Gray, and J. P. Luzio. 1998. Fusion of lysosomes with late endosomes produces a hybrid organelle of intermediate density and is NSF dependent. J. Cell Biol. 140:591-601[Abstract/Free Full Text].
24.	Munder, M., M. Mallo, K. Eichmann, and M. Modolell. 1998. Murine macrophages secrete interferon gamma upon combined stimulation with interleukin (IL)-12 and IL-18: a novel pathway of autocrine macrophage activation. J. Exp. Med. 187:2103-2108[Abstract/Free Full Text].
25.	Murad, F. 1998. Nitric oxide signaling: would you believe that a simple free radical could be a second messenger, autacoid, paracrine substance, neurotransmitter, and hormone? Recent Prog. Horm. Res. 53:43-60.
26.	Nathan, C. 1997. Inducible nitric oxide synthase: what difference does it make? J. Clin. Investig. 100:2417-2423[Medline].
27.	Nathan, C., and Q.-W. Xie. 1994. Regulation of biosynthesis of nitric oxide. J. Biol. Chem. 269:13725-13728[Free Full Text].
28.	Palacios, M., J. Padron, L. Glaria, A. Rojas, R. Delgado, R. Knowles, and S. Moncada. 1993. Chlorpromazine inhibits both the constitutive nitric oxide synthase and the induction of nitric oxide synthase after LPS challenge. Biochem. Biophys. Res. Commun. 196:280-286[CrossRef][Medline].
29.	Radi, R., J. S. Beckman, K. M. Bush, and B. A. Freeman. 1991. Peroxynitrite-induced membrane lipid peroxidation: the cytotoxic potential of superoxide and nitric oxide. Arch. Biochem. Biophys. 288:481-487[CrossRef][Medline].
30.	Schmidt, H. H., T. D. Warner, M. Nakane, U. Forstermann, and F. Murad. 1992. Regulation and subcellular location of nitrogen oxide synthases in RAW264.7 macrophages. Mol. Pharmacol. 41:615-624[Abstract].
31.	Schoedon, G., M. Schneemann, S. Hofer, L. Guerrero, N. Blau, and A. Schaffner. 1993. Regulation of the L-arginine-dependent and tetrahydrobiopterin-dependent biosynthesis of nitric oxide in murine macrophages. Eur. J. Biochem. 213:833-839[Medline].
32.	Shiloh, M. U., and C. F. Nathan. 2000. Reactive nitrogen intermediates and the pathogenesis of Salmonella and mycobacteria. Curr. Opin. Microbiol. 3:35-42[CrossRef][Medline].
33.	Stuehr, D. J. 1999. Mammalian nitric oxide synthases. Biochim. Biophys. Acta 1411:217-230[Medline].
34.	Tian, Y., Y. Xing, R. Magliozzo, K. Yu, B. R. Bloom, and J. Chan. 2000. A commercial preparation of catalase inhibits nitric oxide production by activated murine macrophages: role of arginase. Infect. Immun. 68:3015-3018[Abstract/Free Full Text].
35.	Tjelle, T. E., A. Brech, L. K. Juvet, G. Griffiths, and T. Berg. 1996. Isolation and characterization of early endosomes, late endosomes and terminal lysosomes: their role in protein degradation. J. Cell Sci. 109:2905-2914[Abstract].
36.	Underhill, D. M., A. Ozinsky, A. M. Hajjar, A. Stevens, C. B. Wilson, M. Bassetti, and A. Aderem. 1999. The Toll-like receptor 2 is recruited to macrophage phagosomes and discriminates between pathogens. Nature 401:811-815[CrossRef][Medline].
37.	Vazquez Torres, A., J. Jones Carson, P. Mastroeni, H. Ischiropoulos, and F. C. Fang. 2000. Antimicrobial actions of the NADPH phagocyte oxidase and inducible nitric oxide synthase in experimental salmonellosis. I. Effects on microbial killing by activated peritoneal macrophages in vitro. J. Exp. Med. 192:227-236[Abstract/Free Full Text].
38.	Vazquez Torres, A., Y. Xu, J. Jones Carson, D. W. Holden, S. M. Lucia, M. C. Dinauer, P. Mastroeni, and F. C. Fang. 2000. Salmonella pathogenicity island 2-dependent evasion of the phagocyte NADPH oxidase. Science 287:1655-1658[Abstract/Free Full Text].
39.	Vodovotz, Y., C. Bogdan, J. Paik, Q.-W. Xie, and C. Nathan. 1993. Mechanisms of suppression of macrophage nitric oxide release by transforming growth factor b. J. Exp. Med. 178:605-613[Abstract/Free Full Text].
40.	Xie, Q.-W., H. J. Cho, J. Calaycay, R. A. Mumford, K. M. Swiderek, T. D. Lee, A. Ding, T. Troso, and C. Nathan. 1992. Cloning and characterization of inducible nitric oxide synthase from mouse macrophages. Science 256:225-228[Abstract/Free Full Text].
41.	Zhu, L., C. Gunn, and J. Beckman. 1992. Bactericidal activity of peroxynitrite. Arch. Biochem. Biophys. 298:452-457[CrossRef][Medline].

This article has been cited by other articles:

Bourret, T. J., Song, M., Vazquez-Torres, A. (2009). Codependent and Independent Effects of Nitric Oxide-Mediated Suppression of PhoPQ and Salmonella Pathogenicity Island 2 on Intracellular Salmonella enterica Serovar Typhimurium Survival. Infect. Immun. 77: 5107-5115 [Abstract] [Full Text]
Eswarappa, S. M., Pareek, V., Chakravortty, D. (2008). Role of actin cytoskeleton in LPS-induced NF-{kappa}B activation and nitric oxide production in murine macrophages. Innate Immunity 14: 309-318 [Abstract]
Navarro-Lerida, I., Martinez-Moreno, M., Ventoso, I., Alvarez-Barrientos, A., Rodriguez-Crespo, I. (2007). Binding of CAP70 to Inducible Nitric Oxide Synthase and Implications for the Vectorial Release of Nitric Oxide in Polarized Cells. Mol. Biol. Cell 18: 2768-2777 [Abstract] [Full Text]
Sebbane, F., Lemaitre, N., Sturdevant, D. E., Rebeil, R., Virtaneva, K., Porcella, S. F., Hinnebusch, B. J. (2006). Adaptive response of Yersinia pestis to extracellular effectors of innate immunity during bubonic plague. Proc. Natl. Acad. Sci. USA 103: 11766-11771 [Abstract] [Full Text]
Roshick, C., Wood, H., Caldwell, H. D., McClarty, G. (2006). Comparison of Gamma Interferon-Mediated Antichlamydial Defense Mechanisms in Human and Mouse Cells. Infect. Immun. 74: 225-238 [Abstract] [Full Text]
McCollister, B. D., Bourret, T. J., Gill, R., Jones-Carson, J., Vazquez-Torres, A. (2005). Repression of SPI2 transcription by nitric oxide-producing, IFN{gamma}-activated macrophages promotes maturation of Salmonella phagosomes. JEM 202: 625-635 [Abstract] [Full Text]
Kolodziejska, K. E., Burns, A. R., Moore, R. H., Stenoien, D. L., Eissa, N. T. (2005). Regulation of inducible nitric oxide synthase by aggresome formation. Proc. Natl. Acad. Sci. USA 102: 4854-4859 [Abstract] [Full Text]
Suvarnapunya, A. E., Stein, M. A. (2005). DNA base excision repair potentiates the protective effect of Salmonella Pathogenicity Island 2 within macrophages. Microbiology 151: 557-567 [Abstract] [Full Text]
Daniliuc, S., Bitterman, H., Rahat, M. A., Kinarty, A., Rosenzweig, D., Nitza, L. (2003). Hypoxia Inactivates Inducible Nitric Oxide Synthase in Mouse Macrophages by Disrupting Its Interaction with {alpha}-Actinin 4. J. Immunol. 171: 3225-3232 [Abstract] [Full Text]
Kim, C. C., Monack, D., Falkow, S. (2003). Modulation of Virulence by Two Acidified Nitrite-Responsive Loci of Salmonella enterica Serovar Typhimurium. Infect. Immun. 71: 3196-3205 [Abstract] [Full Text]
Vallance, B. A., Deng, W., De Grado, M., Chan, C., Jacobson, K., Finlay, B. B. (2002). Modulation of Inducible Nitric Oxide Synthase Expression by the Attaching and Effacing Bacterial Pathogen Citrobacter rodentium in Infected Mice. Infect. Immun. 70: 6424-6435 [Abstract] [Full Text]
Koebernick, H., Grode, L., David, J. R., Rohde, W., Rolph, M. S., Mittrucker, H.-W., Kaufmann, S. H. E. (2002). Macrophage migration inhibitory factor (MIF) plays a pivotal role in immunity against Salmonella typhimurium. Proc. Natl. Acad. Sci. USA 99: 13681-13686 [Abstract] [Full Text]
Glynne, P. A., Darling, K. E. A., Picot, J., Evans, T. J. (2002). Epithelial Inducible Nitric-oxide Synthase Is an Apical EBP50-binding Protein That Directs Vectorial Nitric Oxide Output. J. Biol. Chem. 277: 33132-33138 [Abstract] [Full Text]
Stevanin, T. M., Poole, R. K., Demoncheaux, E. A. G., Read, R. C. (2002). Flavohemoglobin Hmp Protects Salmonella enterica Serovar Typhimurium from Nitric Oxide-Related Killing by Human Macrophages. Infect. Immun. 70: 4399-4405 [Abstract] [Full Text]
Anjum, M. F., Stevanin, T. M., Read, R. C., Moir, J. W. B. (2002). Nitric Oxide Metabolism in Neisseria meningitidis. J. Bacteriol. 184: 2987-2993 [Abstract] [Full Text]
Chakravortty, D., Hansen-Wester, I., Hensel, M. (2002). Salmonella Pathogenicity Island 2 Mediates Protection of Intracellular Salmonella from Reactive Nitrogen Intermediates. JEM 195: 1155-1166 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Webb, J. L.
	Articles by Evans, T. J.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Webb, J. L.
	Articles by Evans, T. J.