Phagocytosis of the Malarial Pigment, Hemozoin, Impairs Expression of Major Histocompatibility Complex Class II Antigen, CD54, and CD11c in Human Monocytes

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Infect Immun, April 1998, p. 1601-1606, Vol. 66, No. 4
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Phagocytosis of the Malarial Pigment, Hemozoin, Impairs Expression of Major Histocompatibility Complex Class II Antigen, CD54, and CD11c in Human Monocytes

Evelin Schwarzer,¹^,² Massimo Alessio,³ Daniela Ulliers,¹ and Paolo Arese¹^,^*

Department of Genetics, Biology and Biochemistry, University of Turin Medical School, Turin,¹ and DIBIT, Istituto Scientifico San Raffaele, Milan,³ Italy, and Institute of Biochemistry, Humboldt University-Charité, Berlin, Germany²

Received 22 July 1997/Returned for modification 16 December 1997/Accepted 16 January 1998

	ABSTRACT

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In Plasmodium falciparum malaria, large proportions of resident macrophages and circulating monocytes and leukocytes containmassive amounts of the malarial pigment, hemozoin. Previous studieshave shown that important functions (e.g., the generation of theoxidative burst, the ability to repeat phagocytosis, and proteinkinase C activity) were severely impaired in hemozoin-loaded monocytes.Expression of membrane antigens directly involved in the immuneresponse and in the phagocytic process, and/or under protein kinaseC control, in hemozoin-loaded human monocytes was studied. Expressionof major histocompatibility complex (MHC) class II after gammainterferon stimulation was blocked in hemozoin-loaded monocytesat the protein expression and gene transcription levels but waspreserved in control monocytes loaded with opsonized latex beadsor anti-D(Rh_o)-immunoglobulin G (IgG)-opsonized human erythrocytes.Expression of CD54 (intracellular adhesion molecule 1) and CD11c(p150,95 integrin) was also decreased in hemozoin-loaded monocytes.Expression of MHC class I, CD16 (low-affinity Fc receptor foraggregated IgG), CD32 (low-affinity Fc receptor for aggregatedIgG), CD64 (high-affinity receptor for IgG), CD11b (receptor forcomplement component iC3b [CR3]), CD35 (receptor for complementcomponents C3b and C4b [CR1]), and CD36 (non-class-A scavengerreceptor) was not specifically affected by hemozoin loading. Theseresults suggest that hemozoin loading may contribute to the impairmentof the immune response and the derangement of antigen presentationreported in previous studies of P. falciparum malaria.

	INTRODUCTION

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During the 48-h intraerythrocytic life cycle of Plasmodium falciparum, a large portion of host hemoglobin is degraded (19).However, the parasite is unable to catabolyze heme, which aggregatesto form an insoluble polymer called malarial pigment or hemozoin(HE) (19, 20, 42). Crude, unpurified HE, as is present withinthe food vacuole (the parasite's digestive organelle), containslarge amounts of ferriprotoporphyrin IX, a globin related to hosthemoglobin, and a variety of lipids and proteins of host and parasiticorigin (6, 20, 48).

In vitro and in vivo studies have shown that monocytes and resident macrophages ingest HE or HE-containing parasitized erythrocytes(1, 16, 47). Large proportions of resident macrophagesand circulating monocytes and leukocytes are loaded with HE inmalaria (8, 16, 27). HE may persist, apparently unchanged,in macrophages for several months (16). In vitro studies haveshown that HE-fed monocytes are viable but functionally impaired.They are unable to digest HE or to repeat phagocytosis (40),to generate the oxidative burst upon appropriate stimulation (36)or to kill ingested bacteria, fungi, or tumor cells (15). Inaddition, membrane translocation and activity of protein kinaseC (PKC) were precociously and severely impaired (39). Moreover,HE-fed human and murine monocytes/macrophages were found to releaselarge amounts of tumor necrosis factor alpha (29, 31, 41),nitric oxide (30, 45), macrophage-inhibitory protein 1 $alpha$ andmacrophage-inhibitory protein 1 $beta$ (41), and reduced amounts ofinterleukin-6 (IL-6) (31).

Several studies have shown impaired immune responsiveness in P. falciparum malaria (see references 46 and 50 for reviews).Altered cellular responses to blood-stage Plasmodium antigens,reduced T-cell proliferation, and alterations of lymphocyte functionswere observed in acute malaria (see references 21 and 22 forreviews). Other studies also suggested depression of macrophagefunction (23, 25) and defects in antigen presentation (49,50).

Derangement of macrophage functions and the immune response in malaria, widespread HE presence in phagocytes, inhibition ofPKC in HE-loaded monocytes, and PKC involvement in the expressionof a number of surface molecules have prompted the present work,which was aimed at studying the expression of surface moleculesselected according to their roles in antigen presentation andthe T-cell-dependent immune response (major histocompatibilitycomplex [MHC] classes I and II), in cell adhesion (CD54, intracellularadhesion molecule 1 [ICAM-1], and CD11c [p150,95 integrin]), andin phagocytosis (CD16, a low-affinity Fc receptor for aggregatedimmunoglobulin G [IgG]; CD32, a low-affinity Fc receptor for aggregatedIgG; CD64, a high-affinity receptor for IgG; CD11b, a receptorfor complement component iC3b [CR3]; CD35, a receptor for complementcomponents C3b and C4b [CR1]; and CD36, a non-class-A scavengerreceptor) (24, 28).

	MATERIALS AND METHODS

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Preparation of human monocytes. Peripheral blood mononuclear cells (PBMC) were separated as previously indicated (7) from freshly collected platelet-poorbuffy coats discarded from blood samples from healthy adult donorsof both sexes. Separated cells were washed once with lukewarmphosphate-buffered saline (PBS) supplemented with 10 mM glucose(PBS-G) and resuspended at 5 × 10⁶ cells/ml in ice-cold RPMI 1640 medium supplemented with 23 mMNaHCO₃ and 25 mM HEPES, pH 7.4 (RMBH). Dynabeads M450 Pan B andPan T (Dynal) were added to the cells in a 4:1 ratio for 20 minat 4°C. B and T lymphocytes were removed as specified by the manufacturer.The remaining monocytes were washed twice in RMBH and resuspendedin AIM V cell culture medium (Gibco) at 10⁶ cell/ml. For fluorescence-activated cell sorter analysis, monocyteswere separated from washed PBMC by a second separation on hyperosmoticFicoll (Sigma). The original method of Recalde (33) was modifiedas follows. A total of 5 × 10⁸ PBMC were resuspended in 30 ml of PBS-G and kept for 10 min at37°C. Thereafter, 150 µl of a 9% NaCl solution was added and cellswere reincubated for 12 min at 37°C. An aliquot of 300 µl of a9% NaCl solution was added twice. Cells were incubated for 12min after each addition. Finally, cells were resuspended with60 ml of hyperosmotic PBS containing 2.5 mg of NaCl/ml and separatedon 30 ml of Ficoll containing 3 mg of NaCl/ml by centrifugationat 700 × g for 25 min. The monocyte layer was collected, washedwith PBS-G at 37°C, and resuspended in AIM V medium at 10⁶ cells/ml. Purified cells were >90% monocytes as assessed by CD14expression.

Preparation and opsonization of HE. HE was prepared from P. falciparum cultures (strain FCR-3) by osmotic shock and four washes with ice-cold distilled waterand opsonized without any further purification immediately beforephagocytosis with an equal volume of fresh human serum for 30min at 37°C as previously indicated (40). HE was quantifiedaccording its heme content by a luminescence method (38).

Phagocytosis of opsonized HE, opsonized human erythrocytes, and opsonized latex beads by adherent monocytes. Phagocytosis of fresh-serum-opsonized HE, of human erythrocytes opsonized with anti-D(Rh_o) IgG (40), and of fresh-serum-opsonizedlatex beads was initiated by mixing 10 erythrocytes per monocyte,an equivalent amount of HE in terms of heme content (for detailsof heme quantification, see reference 38), or 1 µl of opsonizedlatex bead (0.1-µm average diameter; Sigma) suspension (latexbeads, RMBH, and fresh human serum, 1:1:1 [vol/vol/vol]/10⁶ monocytes. Suspensions were briefly centrifuged (150 × g for5 s at room temperature) to improve contact between the erythrocytes,HE or latex beads, and monocytes. To avoid the attachment of monocytesafter centrifugation and during the whole incubation period, cellswere kept in suspension at 5 × 10⁶ cells/5 ml of AIM V medium in 6-cm-diameter Teflon-bottom dishes(Heraeus) in a humidified incubator (95% air, 5% CO₂) at 37°C.Stimulation with 200 U of human recombinant gamma interferon (IFN- $gamma$ )(a gift of G. Garotta, Roche, Basel, Switzerland)/ml was performed12 h after the start of phagocytosis, if not indicated otherwise.On average, $>=$ 90% of the monocytes phagocytosed HE or latex beads,and $>=$ 80% of monocytes phagocytosed opsonized erythrocytes, asassessed by microscopic inspection. Control cells were kept undersimilar conditions without phagocytosis and with and without additionof IFN- $gamma$ .

Flow cytometry analysis. Before phagocytosis and 48 h after the beginning of phagocytosis, monocytes were harvested by aspiration. Residual adherentmonocytes were scraped off without noticeable alterations. Afterthree washings with PBS, an indirect immunofluorescence test wasperformed by reacting 10⁶ cells in suspension with appropriate dilutions of purified monoclonalantibody (MAb) or hybridoma cell culture supernatants for 30 minat 4°C. MAbs used in this study were as follows: NL07 (2),anti-CD36; W6/32 (American Type Culture Collection), anti-MHCclass I; OKMI (Ortho Diagnostics), anti-CD11b; 2.9 (9), anti-MHCclass II-DR, -DP, and -DQ; MC105 (The Binding Site), anti-CD11c;3C10 (American Type Culture Collection), anti-CD14; 3G8 (Immunotech),anti-CD16; IV.3 (American Type Culture Collection), anti-CD32;CD54 (Serotec), anti-CD54; 32.2 (Medarex), anti-CD64; and CB04(26), anti-CD35. Controls were class-matched irrelevant MAbs.Bound antibody was revealed by fluoroscein isothiocyanate (FITC)-conjugatedF(ab')₂ goat anti-mouse Ig (Technogenetics). Cells were then analyzedon a FACScan flow cytometer (Becton Dickinson), by PC-LYSYS software.

Expression of specific mRNA for MHC class I and class II antigens. Forty-eight hours after the start of phagocytosis and 24 h after addition of 200 U of IFN- $gamma$ /ml, monocytes were harvested andsedimented by centrifugation. The supernatant was discarded andtotal RNA was isolated from 5 × 10⁶ monocytes by RNAzol B extraction as specified by the manufacturer(Biotech X Laboratories) and quantified by optical density (OD)measurement. The cDNA synthesis from 15 ng of total cellular RNAfrom each extract was performed with 25 ng of random primers (GibcoBRL), 200 U of Moloney murine leukemia virus reverse transcriptase(Gibco BRL), and 20 U of RNase inhibitor (Boehringer Mannheim).Reverse transcription was terminated after 60 min of incubationat 37°C by a 95°C treatment of samples for 5 min. Subsequently,PCR was carried out in the same tube used for reverse transcription,adding 20 pmol of each oligonucleotide primer and 5 U of AmpliTaq DNA polymerase (Perkin-Elmer) in a final volume of 100 µl.The volume was adjusted with PCR buffer. Oligonucleotide primerswere designed for conserved sequences coding for the human MHCclass I B (sense oligonucleotide, 5'-ACA GTG CCC AGG GCT CTG AT-3';antisense oligonucleotide, 5'-AGA GGC TCT TGA AGT CAC AA-3') andclass II B (sense oligonucleotide, 5'-GAT TGG ACC TTC CAG ACCCTG-3'; antisense oligonucleotide, 5'-ACT TGG GTG CTC CAC TTGGCA-3') chains from the DR1 haplotype and were synthesized byC. Bernd, Institute of Pathological and Clinical Biochemistry,Humboldt University, Berlin, Germany. Samples were subjected to25 cycles consisting of 45 s at 95°C, 45 s at 48°C, and 60 s at70°C and to an additional extension step of 5 min at 70°C in aBiometra Uni Thermoblock. Portions of 18 µl of the PCR productswere electrophoresed on a 3% agarose gel (NuSieve GTG; Biozym)in Tris-borate-EDTA buffer containing ethidium bromide. Bandswere detected by ethidium bromide-dependent fluorescence. ThePCR products of MHC class I and class II genes had 118 and 81bp, respectively. The quantity of PCR products for MHC class Iand class II obtained was dependent on the amount of MHC-specificmRNA in the cells when total mRNA extract was employed in therange of 7.5 to 60 ng for reverse transcription and PCR.

	RESULTS

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HE phagocytosis abrogates the IFN- $gamma$ effect on MHC class II expression. Flow cytometry analysis showed that the constitutive expression of MHC class II antigens on the surfaces of suspended humanmonocytes was very low in HE-fed and in unfed monocytes examined48 h after the start of phagocytosis. Expression of class II antigensin HE-fed monocytes was not increased after IFN- $gamma$ stimulation(200 U/ml was added for 36 h 12 h after the start of phagocytosis)(Fig. 1, left panel). By contrast, phagocytosis of serum-opsonizedlatex beads enhanced expression of MHC class II antigens 3.6-foldwithout IFN- $gamma$ stimulation and 33-fold with IFN- $gamma$ stimulation (200U/ml was added for 36 h 12 h after the start of phagocytosis)(Fig. 1, right panel). Similar results were obtained when IFN- $gamma$ stimulation was applied 5 h after the start of phagocytosis (notshown). Ingestion of serum-opsonized HE and latex beads did notmodify the physical characteristics of suspended monocytes, asindicated by the constancy of the forward-scatter and side-scatterdata (not shown).

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FIG. 1. Expression of MHC class II antigens in human monocytes after phagocytosis of serum-opsonized HE or latex beads with or without IFN- $gamma$ stimulation. Suspended human monocytes were allowed to phagocytose HE (left panel) or latex beads (right panel) in Teflon-bottom dishes kept in a humidified incubator at 37°C. Twelve hours after the start of phagocytosis, 200 U of IFN- $gamma$ /ml was added to a part of each dish. Forty-eight hours after the start of phagocytosis, monocytes were harvested by aspiration. After being washed, monocytes were immunostained with anti-MHC class II MAb and bound MAb was revealed by FITC-conjugated F(ab')₂ goat anti-mouse Ig. Flow cytometry analysis of surface antigens was performed on a FACScan flow cytometer (Becton Dickinson). The first peak at the left in both panels represents MHC class II antigen expression in unstimulated monocytes incubated for 48 h without phagocytosis. The y axis represents cell number and the x axis represents fluorescence intensity. This was one of four similar experiments.

MHC class I and class II mRNA contents of monocytes were compared by reverse transcriptase PCR (RT-PCR). The amount of PCRproducts for MHC classes I and II reflected the amount of specificcellular RNA when total cellular RNA was used in the range of7.5 to 60 ng in the RT-PCR. Increases in fluorescence intensityof PCR products for MHC class I (118 bp) and class II (84 bp)were observed in the above range with increasing amounts of totalRNA extract (Fig. 2). For each of the following RT-PCRs, 15 ngof total RNA extract was employed. This allowed us to comparethe amounts of PCR products for MHC class I and class II fromdifferently treated cells and to extrapolate them to differencesin cellular content of MHC class I and class II mRNA at the timeof RNA extraction.

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FIG. 2. Quantification of MHC class I and class II mRNA by RT-PCR. Increasing amounts (7.5 to 60 ng, quantified by OD, as indicated under the lanes) of total RNA extracted from human monocytes were employed in reverse transcription with Moloney murine leukemia virus reverse transcriptase for 1 h, followed by PCR in the same tube (100-µl final volume, 25 cycles). RT-PCR was performed in duplicate with each of the indicated total RNA amounts. Specific primers for conserved regions in MHC class I and class II genes were utilized to obtain PCR products of 118 and 81 bp, respectively. PCR products were separated on a 3% agarose gel and stained with ethidium bromide. DNA size standards are indicated on the right.

Similar to the expression of protein product in HE-fed monocytes examined 48 h after the start of phagocytosis, the steady-statelevel of MHC class II mRNA was very low and almost unresponsiveto IFN- $gamma$ stimulation. In unfed monocytes, the expression of MHCclass II mRNA did not change over 48 h but was remarkably enhancedafter IFN- $gamma$ stimulation (Fig. 3, upper panel). Based on the dependencyof output of class II-specific products on the amount of RNA usedin the RT-PCR (Fig. 2), we can estimate by OD quantification thatthe amount of class II mRNA was at least three times lower inIFN- $gamma$ -stimulated, HE-loaded monocytes than in IFN- $gamma$ -stimulatedcontrol cells. Compared to that in time-matched unfed monocytes,expression of MHC class II mRNA was slightly increased 48 h afterphagocytosis of opsonized latex beads or opsonized erythrocytesand was remarkably increased after IFN- $gamma$ stimulation (Fig. 3,lower panel). Thus, HE phagocytosis apparently hindered upregulationof MHC class II expression at the mRNA and protein levels. Theremarkable differences in the IFN- $gamma$ response observed in HE-fedand latex-bead-fed cells may exclude nonspecific effects due tolysosomal occupancy related to the phagocytic process and mayindicate a specific effect of HE. Expression of MHC class I mRNAwas not modified after phagocytosis of any of the phagocytic targetsused here and did not respond to IFN- $gamma$ stimulation (Fig. 3). Also,the amounts of extracted total RNA did not differ significantlyin differently treated cells. Contrary to expectations, the stimulationof unfed monocytes with 200 U of IFN- $gamma$ /ml for 2, 6, 12, or 24h did not modify the level of MHC class I-specific mRNA (datanot shown). Consequently, in the present experimental system,class I mRNA can be considered an internal standard for RT-PCR.The higher expression of class I mRNA in untreated control cellsand the relatively lower expression of class I mRNA in IFN- $gamma$ -treatedcontrol cells (shown in the upper panel of Fig. 3) was detectedoccasionally and was probably caused by usage of a larger amountof RNA in untreated control cells due to imprecise quantificationvia OD.

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FIG. 3. (Upper panel) steady-state levels of MHC class I and class II mRNA in human monocytes (C) and monocytes after phagocytosis of serum-opsonized HE (H) with (+) or without ( $-$ ) IFN- $gamma$ stimulation. After the start of HE phagocytosis, monocytes were incubated for 24 h before addition of IFN- $gamma$ (200 U/ml). After a further 24 h of incubation, total RNA was extracted, RT-PCR was performed in duplicate with 15 ng of total RNA, and amplified MHC class I and class II gene products of 118 and 81 bp, respectively, were analyzed as indicated in the legend to Fig. 2. DNA size standards are indicated on the right. This was one of five similar experiments. (Lower panel) steady-state levels of MHC class I and class II mRNA in human monocytes (C) and monocytes after phagocytosis of opsonized latex beads (L) or opsonized erythrocytes (R) with (+) or without ( $-$ ) IFN- $gamma$ stimulation. After the start of phagocytosis of the latex beads or erythrocytes, monocytes were incubated for 24 h before addition of IFN- $gamma$ (200 U/ml). After a further 24 h of incubation, total RNA was extracted, RT-PCR was performed with 15 ng of total RNA, and amplified MHC class I and class II gene products of 118 and 81 bp, respectively, were analyzed as indicated in the legend to Fig. 2. DNA size standards are indicated on the right. This was one of five similar experiments.

Effect of HE phagocytosis on expression of membrane antigens. Flow cytometry analysis was performed on the following cell surface antigens constitutively expressed on monocytes: MHC classI, CD32 (low-affinity Fc receptor for aggregated IgG), CD11c (p150,95integrin), and CD54 (ICAM-1). These cell surface antigens werestudied 48 h after phagocytosis of HE and latex beads. As shownin Fig. 4, after 48 h of culturing, expression of MHC class Iand CD11c did not change, while expression of CD32 and CD54 wasstimulated in unfed control monocytes. Phagocytosis of eitherHE or latex beads slightly reduced class I expression and abrogatedthe increase in CD32, while only HE phagocytosis downregulatedexpression of CD11c and reduced upregulation of CD54. Thus, HEphagocytosis seems to interfere specifically with expression ofCD11c and CD54.

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FIG. 4. Expression of surface antigens in unstimulated human monocytes after phagocytosis of serum-opsonized HE or latex beads. Suspended monocytes were allowed to phagocytose HE or latex beads in Teflon-bottom dishes kept in a humidified incubator at 37°C. Forty-eight hours after the start of phagocytosis, monocytes were harvested by aspiration. After being washed, monocytes were immunostained with purified MAb and bound MAb was revealed by FITC-conjugated goat anti-mouse Ig. Flow cytometry analysis of the surface antigens MHC class I, CD32 (low-affinity receptor for aggregated Ig), CD11c (p150,95 integrin), and CD54 (ICAM-1) was performed on a FACScan (Becton Dickinson) flow cytometer. (A) unfed monocytes at time zero ( $---$ $---$ ) and after 48 h in culture (); (B) HE-fed ( $---$ $---$ ) and unfed () monocytes after 48 h in culture; (C) latex-fed ( $---$ $---$ ) and unfed () monocytes after 48 h in culture. Black profiles on the left represent the fluorescence background of monocytes incubated with irrelevant mouse Ig. The y axis represents cell number and the x axis represents fluorescence intensity. This was one of four similar experiments.

The study also included expression of the following cell surface antigens: CD16 (low-affinity Fc receptor for aggregated IgG),CD64 (high-affinity receptor for IgG,, CD11b (receptor for complementcomponent iC3b [CR3]), CD35 (receptor for complement componentsC3b and C4b [CR1]), and CD36 (non-class-A scavenger receptor [28]).These results are not shown, either because changes (for example,drops in CD16 and CD64) elicited by phagocytosis of latex beadsand HE were similar or because HE-specific effects were small(for example, a minor drop in CD11b and CD35 in HE-fed versuslatex-fed cells) and not significant.

	DISCUSSION

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The reduction or lack of immune responsiveness toward a wide range of antigens has been noted in both human and experimentalmalaria. Altered immune reactivity involves both lower productionof specific antibodies and reduced lymphocyte proliferation inculture in the presence of a given antigen. In human malaria,immunosuppression appears late in the acute phase of the diseaseand can last a long time after the clearance of parasites fromthe circulation (see references 23 and 46 for reviews). Nigerianchildren with acute P. falciparum malaria showed diminished antibodyresponses to the O antigen of Salmonella typhi and to tetanustoxoid (21). Similar results were observed after the vaccinationof Nigerian children with meningococcal vaccine (51). Therewas a significant correlation between the degrees of immunosuppressionand parasitemia (5, 51). The mechanism of altered immunereactivity is not clear, although the functional defect of splenicmacrophages as antigen-presenting cells has been implicated (49).

The aim of the present work was to determine functional alterations in the monocyte/macrophage system that may be causallyconnected with altered T-cell-dependent immune reactivity andpossibly with defective antigen presentation in the organs ofP. falciparum-harboring patients.

Isolated circulating monocytes can be functionally similar to resident macrophages and professional dendritic leukocytes thatexpress MHC class II and adhesive protein, and they can act asantigen-presenting and T-cell-immunostimulating cells in the microenvironmentof blood-filtering organs, such as the spleen, the liver, andthe bone marrow (24). Macrophages residing in blood-filteringorgans and young monocytes under constitutive renewal in bonemarrow may take up locally released HE and HE-containing lateparasite forms. Dendritic leukocytes reside in the marginal zonebetween the blood-filtering (red pulp) and the lymphoid (whitepulp) compartments. These cells may also take up HE and can beimpaired in their T-cell-targeted immunostimulating functions(24).

HE loading in resident macrophages and in circulating leukocytes and monocytes is massive in malaria (8, 16, 27); ofnote, the percentages of heavily HE-laden leukocytes and macrophagesseem to roughly correlate with the severity of the disease (27).In vitro, monocytes also ingest large amounts of HE (38, 40).HE is persistently present in monocytes, where it can be observedto be apparently unmodified after several days in vitro (40)and after several months in vivo after clearance of parasites(8, 16). Under these conditions, HE-laden phagocytes arealive and metabolically active although impaired in importantfunctions (15, 36-40).

The main result of the present work was the defective induction of MHC class II in response to IFN- $gamma$ stimulation in HE-ladenmonocytes. Class II is upregulated in human macrophages by IFN- $gamma$ (the major physiological inducer), tumor necrosis factor, IL-4,and granulocyte-macrophage colony-stimulating factor and downregulatedby prostaglandin E2, IFN- $alpha$ / $beta$ , colony-stimulating factor 1, $alpha$ -macroglobulin, $alpha$ -fetoprotein, and corticosteroids (see reference 18 for a review).The abrogation of MHC class II expression observed here was presentat the protein expression level, where no upregulation of classII antigens could be elicited even after 36 h of stimulation withIFN- $gamma$ . The effect was also evident at the mRNA level. Low inductionof expression of specific MHC class II mRNA was seen under similarconditions of IFN- $gamma$ stimulation. Phagocytosis of serum-opsonizedlatex beads and IgG-opsonized, nonparasitized erythrocytes substantiallyincreased the expression of class II mRNA and class II antigensbut did not modify the IFN- $gamma$ -induced increase of MHC class II.Thus, the HE-elicited effect seems to be specific and not dueto the phagocytic process per se. The effect of HE was seen ratherquickly, since occupancy of monocytes by HE for 5 h did not modifythe basal level of class II expression but was sufficient to fullyabrogate its upregulation.

In bacterial or parasitic diseases such as malaria, upregulation of MHC class II for antigen presentation is important toensure adequate helper-T-cell development and to determine theoutcomes of disease and secondary infections. Consequently, thelack of expression at the cell surface of MHC class II followinga specific stimulus such as IFN- $gamma$ may also explain defects inT-cell activation observed in malaria and be consistent with manifestationsof altered T-cell-dependent immune reactivity mentioned above.

The HE-induced inability of monocytes to upregulate expression of MHC class II after IFN- $gamma$ stimulation described in the presentstudy adds to a series of analogous yet very heterogenous observationsin other bacterial and parasitic diseases for which impaired classII responses have been described (see reference 34 for a review).For example, it has been observed that after ingestion of Mycobacterium,macrophages showed reduced expression of class II antigens (17);that Leishmania donovani, an obligate intracellular protozoan,suppressed macrophage expression of class II (and class I) inresponse to IFN- $gamma$ stimulation (34, 35); and that supernatantsfrom monocytes inoculated with L. donovani contained a solublefactor which prevented class II upregulation by IFN- $gamma$ in naivemonocytes (12). An impaired class II response was accompaniedby defective antigen presentation and suppression of the T-cellresponse in mycobacterial (17) and Leishmania (32) infections.

The present data suggest a link between the HE loading of phagocytes, the suppression of IFN- $gamma$ responsiveness, the failureof MHC class II upregulation, and disturbances in antigen presentationand immunodepression in malaria. Mechanistically, the abrogationof the IFN- $gamma$ signal is unexplained. PKC-mediated phosphorylationshave been involved in IFN- $gamma$ -mediated enhancement of MHC classII (14, 43). Previous work by our group has shown that HEinhibited PKC translocation and PKC activity (39). Recent data(37) indicate that PKC inhibition may be the consequence ofmarkedly increased levels of 4-hydroxynonenal (HNE) in HE-loadedmonocytes. HNE, a highly potent toxic aldehyde originating fromlipoperoxidation of unsaturated fatty acids (see reference 13for a review), accumulates in membranes and may inactivate otherprotein kinase-dependent processes. Preliminary experiments (35a)showing that low micromolar concentrations of HNE inhibited IFN- $gamma$ -mediatedMHC class II expression and mimicked HE action seem to substantiatethe involvement of PKC.

Quite recently, it has been shown that HE-fed, but not erythrocyte-fed, human monocytes produce high levels of IL-10 (27a).IL-10 seems to be important for the downregulation of the immuneresponse, because it decreases expression of class II and leadsto reduced proliferation of human T cells (11). However, otherIL-10 effects (increased expression of CD14, CD64, and class Iand an increase in phagocytic activity [44]) were not observedafter HE phagocytosis. Thus, IL-10 may be only partially responsiblefor the HE effects reported here.

CD54 (ICAM-1), an adhesion molecule present on the surfaces of monocytes and other antigen-presenting cells, contributes considerablyto the capacity of these cells to adhere and stimulate T-cellproliferation by reinforcing the signal from the T-cell receptor(4, 10). CD54 is very weakly expressed in nonstimulated monocytesand is upregulated upon maturation, as confirmed by present data.Our observation that HE-laden but not latex-bead-laden monocyteshave reduced spontaneous upregulation of CD54 may help to explainthe defective T-cell response in malaria.

CD11c, which belongs to the $beta$ ₂ family of integrins, is expressed mostly on monocytes and granulocytes but also on activatedT and B cells (3). By using a CD8⁺ T-cell line which expressed a high level of CD11c, CD11c hasbeen recently identified as the ligand for ICAM-1 in the rabbit(3). If these data can be confirmed for humans, the lack ofspontaneous upregulation of CD11c in HE-laden monocytes may addto the defective response of ICAM-1 as a negative factor for theT-cell response in malaria.

In conclusion only expression of molecules that play essential roles in antigen presentation and the T-cell response, namely,MHC class II, CD54, and CD11c, appeared to be specifically hinderedor blocked after HE phagocytosis. Thus, despite their phenomenologicalcharacter, the present data may offer a way to identify a defectiveprocess (IFN- $gamma$ -responsive upregulation of critical molecules)and toxic mediators (HE and HNE) as possible causes of alterationsof the immune response in human malaria.

	ACKNOWLEDGMENTS

This work was supported by grants from WHO/UNDP/World Bank (TDR-Pathogenesis Programme, grant no. 940445), the Italian Ministryof University (MURST), and Compagnia di San Paolo, Torino, Italy.

	FOOTNOTES

^* Corresponding author. Mailing address: Dipartimento di Genetica, Biologia e Biochimica, Università di Torino, Via Santena5 bis, I-10126 Torino, Italy. Phone: 39-11-6706 686. Fax: 39-11-6635663. E-mail: arese{at}molinette.unito.it.

Editor: S. H. E. Kaufmann

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Top Abstract Introduction Materials & Methods Results Discussion References

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