Binding and transfer of verocytotoxin by polymorphonuclear leukocytes in hemolytic uremic syndrome

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Blood, Vol. 95 No. 11 (June 1), 2000: pp. 3396-3402
HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY

Binding and transfer of verocytotoxin by polymorphonuclear leukocytes in hemolytic uremic syndrome

D. Maroeska W. M. te Loo, Leo A. H. Monnens, Thea J. A. M. van der Velden, Mario A. Vermeer, Frank Preyers, Pierre N. M. Demacker, Lambertus P. W. J. van den Heuvel, and Victor W. M. van Hinsbergh
From the Department of Pediatrics, University Hospital Nijmegen, The Netherlands; Gaubius Laboratory TNO-PG, Leiden, The Netherlands; Institute for Cardiovascular Research, Vrije Universiteit, Amsterdam, The Netherlands; Department of Hematology, University Hospital Nijmegen, Nijmegen, The Netherlands; and the Department of General Internal Medicine, University Hospital Nijmegen, Nijmegen, The Netherlands.

  Abstract

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

The hemolytic uremic syndrome (HUS) is the most common cause of acute renal failure in children. The role of a verocytotoxin(VT)-producing Escherichia coli has been strongly implicated inthe epidemic form of HUS. Although direct toxicity of VT on glomerularendothelial cells has been demonstrated, it remained still unclearhow the VT is transported from the intestine to the target organs.In this study we demonstrate that VT, when incubated in wholeblood, binds rapidly and completely to human polymorphonuclearleukocytes (PMNs) and not to other components of blood. Bindingstudies with ¹²⁵I-VT-1 showed a single class of binding sites on freshly isolated,nonstimulated human PMNs. The K_d of VT-binding to PMNs was 10^-8 mol/L, 100-fold less than that of the VT-receptor globotriaosylceramide.On incubation of VT-preloaded PMNs with human glomerular microvascularendothelial cells (GMVECs), transfer of VT-1 to the endothelialcells occurred. Incubation of nonstimulated GMVECs with VT-preloadedPMNs, but not with PMNs or VT-1 alone, caused inhibition of proteinsynthesis and cell death. Our data are in concert with a roleof PMNs in the transfer of VT from the intestine to the kidneyendothelium. This transfer occurs by selective binding to a specificreceptor on PMNs and subsequent passing of the ligand VT to theVT-receptor on GMVECs, which causes cell damage. This new mechanismfurther underpins the important role of PMNs inHUS. (Blood. 2000;95:3396-3402)

© 2000 by The American Society of Hematology.

  Introduction

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

The hemolytic uremic syndrome (HUS) is the most frequent cause of acute renal failure in children. The traditional diagnosticcriteria for this syndrome include hemolytic anemia with fragmentederythrocytes, thrombocytopenia, and renal failure.¹ The endotheliumof kidney arterioles and glomeruli plays a central role in thepathogenesis of HUS. Histopathological studies of the kidney ofHUS patients show characteristic lesions, consisting of swellingand detachment of the endothelial cells of glomeruli and depositsof fibrin in glomeruli and arterioles.²^,³ In severe cases,the cell damage is not limited to the kidney but other organs,such as brain and pancreas, are alsoinvolved.

The epidemic form of HUS, or (D+) HUS, occurs mostly following a prodromal phase of bloody diarrhea. In 90% of the cases with(D+) HUS, an infection with a verocytotoxin (VT)-producing Escherichiacoli is strongly implicated.^2-6 Strains of the VT-producing Ecoli associated with HUS can produce VT-1 or VT-2, or both. Thestructure of the VT is formed by a biologically active A subunitand 5 B subunits by which the toxin binds to specific glycolipidreceptors. The VT-producing E coli is transmitted by contaminatedfood or water or from person to person. After ingestion, the Ecoli binds to specific receptors to the intestinal wall, and VTenters the circulation via a still unknown mechanism.³^,⁷^,⁸VT is transported to the target organs and can bind specificallyto its receptor globotriaosylceramide, also called Gb3. This receptorhas been demonstrated in human renal tissue and in human endothelialcells.⁹^,¹⁰ After binding to Gb3, the active subunit of theVT enters the cell and causes inhibition of protein synthesis.^11-16

The route of transport of the VT from intestine to the kidney or other target organs is not solved yet. Although epidemiologicalstudies have pointed to a role of VT in (D+) HUS, no VT has beenencountered thus far in the plasma of patients with HUS. In vitroexperiments showed that VT could bind to erythrocytes, dependingon the P-blood group glycolipids, that are structurally relatedto the known VT receptor Gb3. It has been reported that VT canbind to the P1 phenotype (Pk, P1, P2 antigens) and, to a lesserextent, to the P2 phenotype (Pk and P antigens) but not to theP phenotype (lacking antigens).^17-20 In vitro experiments alsoshowed binding to activated human monocytes.²¹ Other possiblecandidates for transporting the VT are platelets²² and lipoproteins.²³^,²⁴In this study we evaluate which fractions of the blood contributeto VT binding and transfer. Our data suggest that polymorphonuclearleukocytes (PMNs) are responsible for transporting the VT in bloodand that the receptor responsible for binding VT to PMNs is differentfrom that found on endothelial cells. Furthermore, we demonstratethat VT is transferred from PMNs to human glomerular endothelialcells.

  Materials and methods

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Materials
Purified VT-1 was kindly provided by Dr M. A. Karmali (Toronto, ON, Canada). Ficoll was purchased from Pharmacia (Uppsula,Sweden). Plastic-coated silica gel F1500 thin-layer chromatography(TLC) plates were obtained from Schleicher and Schuell (Dassel,Germany). A standard mixture of pure neutral glycolipids was obtainedfrom Biocarb AB (Lund, Sweden). VT-1 labeled with fluoresceinisothiocyanate (VT-FITC) was kindly donated by Dr Lingwood (Hospitalfor Sick Children, Toronto, ON, Canada). Flow-activated cell sorter(FACS) lysing solution was purchased from Becton Dickinson ImmunocytometrySystems (San Jose, CA). CD13-PE, CD14-PE, and CD45-TRITC werepurchased from DAKO (Glostrup, Denmark). All other reagents wereof analytical grade or as described previously.²¹^,²⁵^,²⁶

FACS analysis and immunohistological study of whole blood
VT-FITC was used to determine binding of VT in whole blood. Blood was obtained from 10 different healthy donors, 8 adultsand 2 children (aged 10 and 6 years), and blood group of the adultswas determined according to established procedures. Two donorshad blood group O, 4 blood group A, and 2 had blood group B. Therewere 2 donors with the P1 blood group. Blood was immediately puton ice; 100 µL of blood was incubated for 20 minutes on ice withVT-FITC, followed by addition of FACS lysing solution to removeerythrocytes. The solution was centrifuged at 200g for 5 minutesat 4°C. The cells were washed twice with phosphate-buffered saline(PBS) containing 1% albumin. Cells were resuspended in 500 µLof a 0.5% paraformaldehyde solution for fixation. Flow cytometrywas used to determine binding of VT-FITC. Fluorescence was measuredin a histogram, using a log scale. The different cell types werecharacterized with the use of monoclonal antibodies; CD13-PE andCD16-PE for PMNs, CD14-PE for monocytes, and CD45-TRITC for lymphocytes.To exclude nonspecific binding, whole blood was previously incubatedwith unlabeled VT for 20 minutes, followed by incubation withVT-FITC. The same procedure as above was used for direct immunofluorescencestudies. Briefly, cells were incubated for 20 minutes with VT-FITCand a monoclonal antibody to indicate the cell type. Cells werewashed twice with PBS and were then resuspended in 500 µL of 0.5%paraformaldehyde. Cells were centrifuged at 200g. Subsequently,cells were analyzed by a Zeiss fluorescence microscope (Aksioscope)with standard FITC filter (09) and PE-filter (014) (excludingthe possibility of interference of FITC and PE-staining), forVT-FITC, CD13-PE, CD14-PE, and CD45-TRITC staining,respectively.

Isolation of PMNs
Twenty milliliters of EDTA or heparin blood of 8 healthy adult donors and of 2 children was obtained for the isolation ofPMNs. Blood was directly put on ice. Blood was mixed with 15 mLof PBS and put into a 50-mL tube. The blood was underlayed usingFicoll 1.077 g/mL. The cells were centrifuged 20 minutes at 200gat 4°C in a Sorvall centrifuge. The pellet contained PMNs anderythrocytes. Erythrocytes were lysed using ammonium chlorideor FACS lysing solution, and PMNs were washed twice with PBS containing1% bovine serum albumin (BSA). PMNs were resuspended in PBS orRPMI medium containing 1% of human serum and stored at 4°C for< 1 hour until use. The population PMNs was more than 95% pureas measured by an H₃-analyser (Technicon,Bayer).

Flow cytometric analysis after isolation of different cell types
Pooled PMNs as described above were used. Blood was mixed with PBS and cells were separated using Ficoll. The interphase wascollected for studying binding to lymphocytes and monocytes separately.The pellet contained PMNs and erythrocytes. The pellet was resuspendedin 20 mL PBS. Subsequently, Ficoll 1.077 g/mL was used to separatePMNs from erythrocytes. To make sure that the different cell populationswere more than 95% pure, cell populations were analyzed by anH₃-analyzer. Different cell types were incubated with 0.5 µL VT-FITC(1 mg/mL) on ice for 20 minutes. Cells were then washed twicewith PBS/1%BSA and centrifuged at 200g for 5 minutes. Cells wereresuspended in 500 µL of 0.5% paraformaldehyde. Binding of VT-FITCwas measured using flow cytometry. Experiments were repeated forthe different cell types, using an incubation time of 3hours.

Results were confirmed by using direct immunofluorescence and incubation of the different cell populations separately with¹²⁵I-VT-1 (seebelow).

Binding of VT-FITC to lipoproteins
To examine the binding between VT and lipoproteins, lipoproteins were isolated by ultracentrifugation and a precipitationmethod.²⁷ Very low-density lipoproteins (VLDLs), high-densitylipoproteins (HDLs), or low-density lipoproteins (LDLs) were incubatedwith VT-FITC during 3 hours on ice. After the incubation, lipoprotein-depletedserum was added. The solution was mixed thoroughly and incubatedfor 10 minutes. Subsequently, a precipitation solution was added,followed by centrifugation. After centrifugation, binding of VT-FITCwas determined by fluorescence spectrometry. Experiments wererepeated, using an incubation time of 1 hour or 20 minutes todetermine whether binding of VT to lipoproteins occurred aftera similar incubation period as needed forPMNs.

Binding of ¹²⁵I-VT-1 to human PMNs
VT-1 was labeled with Na-¹²⁵I according to the Iodogen procedure.²⁸ After isolation of PMNs from EDTA blood, PMNs were washedtwice with PBS and were then resuspended in Hanks balanced saltsolution (HBSS) containing 1% human serum albumin (Central Laboratoryof the Red Cross, Amsterdam, The Netherlands) at 0°C. Subsequently,0.5 × 10⁶ PMNs/250 µL were incubated for 3 hours with ¹²⁵I-VT-1 in different concentrations, ranging from 0.3 up to 70nmol/L. To determine nonspecific binding, unlabeled VT-1 in 25-foldexcess was added parallel with ¹²⁵I-VT-1. After incubation, the free fraction of ¹²⁵I-VT-1 was separated from the fraction of ¹²⁵I-VT-1 bound to the PMNs, using Ficoll 1.077 g/mL. PMNs were thenwashed with Hanks balanced salt solution/1% human serum albuminand centrifuged at 200g for 10 minutes. Cell-associated ¹²⁵I-VT-1 was determined in a gamma-counter. All determinations weredone in duplicate. Binding data were analyzed, using the methodof Scatchard.²⁹

Thin layer chromatography of neutral glycolipids extracted from PMNs
PMNs were isolated as described before. They were washed twice with PBS and subsequently resuspended in 0.5 mL of PBS. Next,glycolipids of the cells were extracted and separated as describedby Lingwood et al.³⁰ For the extraction of neutral glycolipids,1 mol/L NaCl was used instead of water to receive maximal yield.After separation of the neutral glycolipids, the TLC plate wascoated with polyisobutylmetacrylate, blocked overnight with 1%PBS/Tweenand incubated with ¹²⁵I-VT-1 in 1% albumin and 0.05% Tween-20 in PBS.²⁶ After washing,the binding of ¹²⁵I-VT-1 was analyzed, using a Fuji BAS 1000 phosphor-imager.

Human glomerular microvascular endothelial cells
Human glomerular microvascular endothelial cells (GMVECs) were isolated and cultured on gelatin-coated dishes as describedby van Setten et al.²⁶ Cells were characterized by indirectimmunofluorescence microscopy, using antibodies against von Willebrandfactor, PECAM-1, and VE-cadherin. No immunoreactivity was observedwith antigens against $alpha$ -smooth muscle actin or cytokeratin 20,indicating that there was no contamination with mesangial or epithelialcells. GMVECs were cultured in 24-well plates to perform experimentsand used between passage 6 and 10. They were used 5 days afterreaching confluence and stimulated for 24 hours with 10 ng/mLtumor necrosis factor $alpha$ (TNF- $alpha$ ), ifindicated.

Transfer of VT from PMNs to endothelium in vitro
After isolation, PMNs were washed twice with PBS and were then resuspended in medium M199 containing 20% fetal calf serum.PMNs were incubated with a monoclonal antibody, CD16-PE, to excludethe possibility that PMNs interfere with FACS analysis. Subsequently,different amounts of PMNs, varying between 0.5 and 2.0 × 10⁶ PMNs were incubated with 0.5 µL VT-FITC on ice during 30 minutes.After that, PMNs were washed twice with medium M199. NonstimulatedGMVECs and TNF- $alpha$ -stimulated GMVECs were incubated on ice for 4hours with 0.5-2.0 × 10⁶ PMNs loaded with VT-FITC. As control, GMVECs were also incubatedalone with VT-FITC, PMNs, or with medium containing 10% fetalcalf serum. After the incubation period, GMVECs were washed 3times with M199. GMVECs were detached with trypsin treatment andcentrifuged for 5 minutes at 200g at 4°C. Cells were washed withPBS, then resuspended in 500 µL 0.5% paraformaldehyde, and transferredinto a tube suitable for FACSanalysis.

Measurement of protein synthesis
GMVECs were cultured in 24-well plates and were used 5 days after reaching confluence. GMVECs stimulated by TNF- $alpha$ (10 ng/mL)and nonstimulated GMVECs were incubated with 10⁶ PMNs at 37°C for 24 hours. PMNs were preloaded with VT in differentconcentrations, ranging from 0.1 nmol/L to 10 nmol/L VT and washed2 times before adding to the GMVECs. PMNs not preincubated withVT were used as control. Protein synthesis was determined by assayingthe incorporation of ³H-leucine in newly synthesized proteins as described previously.²⁶

Statistics
All results of measuring protein synthesis are expressed as mean ± SEM. Changes with respect to control values were analyzedby using an unpaired Student t test. Values in which P $<=$ .05 wereregarded assignificant.

  Results

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Binding of VT in blood
Incubation of whole blood with VT-FITC after 20 minutes showed almost complete binding of VT to PMNs (Figure 1C and 1D), independentof blood group or age of the donor. Binding was completely blockedby pre-incubation of blood with unlabeled VT-1 for 20 minutes(data not shown). More than 90% of PMNs were positive, and allother cell types were negative. Control blood, incubated withan immunoglobulin (Ig)G antibody conjugated with FITC, showedno staining (Figure 1A and 1B). Selective binding of VT-FITC wasalso demonstrated by direct immunofluorescence studies (Figure2). Only PMNs bound VT-FITC.

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Fig 1. Binding of VT-FITC to PMNs in whole blood was demonstrated by flow cytometric analysis. (A, B) Flow cytometric analysis of control blood (incubated with IgG-FITC alone) before addition of VT-FITC. (C, D) Analysis after 20-minute incubation with 0.5 µL VT-FITC (1 mg/mL) exclusive binding to PMNs was found. L indicates lymphocytes; M, monocytes; P, PMNs. The experiment is representative for duplicate determinations in 10 experiments with blood of different donors.

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Fig 2. Direct immunofluorescence of binding of VT-FITC to PMNs. Whole blood was incubated with CD13-PE (A), a specific marker for PMNs, and with VT-FITC (B) on ice for 20 minutes. PMNs were the cells that had bound VT-FITC. No other components of blood were positive for binding VT-FITC.

To substantiate that PMNs were the only cells binding VT in blood, VT-FITC binding to purified erythrocytes, monocytes, andplatelets was also studied. Erythrocytes were incubated, and bindingwas analyzed using FACS analysis and direct immunofluorescence.No binding of VT-FITC to erythrocytes was observed independentof the P blood group (8 donors). No significant binding of VT-FITCto nonstimulated monocytes was observed (6 donors). Lymphocytesand thrombocytes (3 different donors) also did not bind VT-FITCin ourconditions.

Lingwood²³^,²⁴ suggested that lipoproteins may bind glycolipids, such as Gb3, and that VT may be cotransported by lipoproteinsin a piggyback way. LDL and HDL preparations were incubated separatelywith VT-FITC on ice for 3 hours. No significant binding was observed.This experiment was repeated with incubation times of 20 minutesand 1 hour. Again, no binding was found (data not shown). Similarly,no binding of ¹²⁵I-VT to these preparations was found. From these data, we concludethat VT only significantly binds to PMNs in whole blood and notto other components, such as erythrocytes, lymphocytes, monocytes,andlipoproteins.

Analysis VT binding to PMNs
To evaluate whether high-affinity binding sites were involved in the binding of VT to PMNs, the binding of ¹²⁵I-VT-1 to PMNs was determined. Figure 3A shows that the bindingof ¹²⁵I-VT-1 is saturable and specific. After incubation with a 25-foldexcess of unlabeled VT-1, binding with ¹²⁵I-VT-1 decreased more than 95%. Scatchard plot analysis (Figure3B) showed that nonstimulated PMNs have 2.1 × 10⁵ binding sites with a high affinity for VT (K_d = 10⁸ mol/L). This affinity is 100-fold less than what we and others¹⁰^,²⁶consistently found for VT-1 binding to Gb3 in human vein and GMVECs.To confirm that VT remained exposed on the surface, ¹²⁵I-VT-1 was bound to PMNs (30 minutes, 37°C), and, after 3 washings,the VT-loaded PMNs were incubated for 2.5 hours at 37°C in mediumsupplemented with 10% fetal calf serum and 100 U/mL aprotinin.After removal of the serum-containing medium, treatment of thesePMNs for 10 minutes by trypsin/EDTA released 95% of the ¹²⁵I-VT-1 associated with the cells. This indicates that the VT-1remained available at the cell surface.

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Fig 3. PMNs of 2 different donors were used to determine binding of ¹²⁵I-VT-1 to PMNs. (A) PMNs were incubated with increasing concentrations of ¹²⁵I-VT-1 (0.3 to 70 nmol/L) at 4°C for 3 hours ( $black-triangle$ ). Nonspecific binding ( $bullet$ ) was determined in the presence of 25-fold excess of unlabeled VT-1. (B) Shows the result of Scatchard plot analysis.

To investigate whether Gb3 or a different neutral glycolipid was responsible for binding of VT, thin layer chromatography(TLC) of neutral glycolipids extracted from nonstimulated PMNswas performed and compared with those of TNF- $alpha$ -stimulated GMVECsand LPS-stimulated monocytes. Thin layer chromatograms were incubatedwith radiolabeled VT-1 and washed thoroughly. The bound ¹²⁵I-VT-1 was detected with the use of a phosphor-imager (Figure4). ¹²⁵I-VT-1 strongly bound to the Gb3 in the standard neutral glycolipidpreparation (lane D) and the TNF- $alpha$ -treated neutral glycolipidextract of GMVECs (lane B). Two other bands binding ¹²⁵I-VT-1 just below the globotetraosylceramide (Gb4) were foundin glycolipid extractions of monocytes (lane C) and in smalleramounts in those of GMVECs. Nonstimulated PMNs showed 2 smallbands with a Rf value just below the Gb4 but distinct from thatobserved for monocytes. This pattern was consistently found with4 different neutral glycolipid extracts of PMNs obtained from4 different donors.

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Fig 4. ¹²⁵I-VT-1 binding to neutral glycolipid extracts from human PMNs, GMVECs, and monocytes. Glycolipids were extracted and separated as described in "Materials and methods." Binding of ¹²⁵I-VT-1 was visualized, using a phosphor-imager. (A) Glycolipid extract of 30 million PMNs of 1 representative donor. (B) Neutral glycolipid extraction of TNF- $alpha$ -treated GMVECs. (C) Glycolipid extract of monocytes stimulated with LPS (1 ng/mL). (D) Standard mixture of neutral glycolipids, 2 µg of each glycolipid. Standard of neutral glycolipids was stained with orcinol. (Gb3, globotriaosylceramide; Gb4, globotetraosylceramide; and Gb5, Forssman pentasaccharide).

Transfer of VT from PMNs to GMVECs
To investigate if VT-1 could be transferred from PMNs to GMVECs, we incubated nonstimulated and TNF- $alpha$ -stimulated GMVECs withPMNs that had bound VT-FITC at 0°C.

PMNs were previously incubated on ice with CD16-PE, a specific monoclonal antibody for PMNs, to prevent interference of PMNsby FACS analysis. After an incubation time of 3 hours on ice,GMVECs were washed carefully 3 times with PBS. Subsequently, GMVECswere detached and analyzed by flow cytometry. No PMNs were retainedby nonstimulated GMVECs (as revealed by FACS analysis after stainingwith CD16-PE; Figure 5A and 5C). GMVECs were negative for CD16-PEstaining (Figure 5C). However, TNF- $alpha$ -stimulated GMVECs retaineda small percentage of the PMNs added (ranging between 2.8% and3.6%) (Figure 5B). The population of PMNs was gated (indicatedby the area P in Figure 5B), which allowed simultaneous analysisof PMNs and GMVECs. The population of gated PMNs was positivefor CD-16-PE (Figure 5E) and distinct from the CD-16-PE-negativeGMVECs (Figure 5D). The differentiation between PMNs and GMVECsby gating permitted us to investigate if a transfer of VT-FITCfrom PMNs to GMVECs had occurred. After the 3-hour incubationperiod, 30% of the stimulated GMVECs had bound VT-FITC (Figure5G). Nonstimulated GMVECs did not bind any VT-FITC (Figure 5F).When IgG-FITC was incubated with GMVECs, no binding occurred.This excludes nonspecific binding of FITC to these cells. Ligandpassing of VT-FITC from PMNs to GMVECs was further confirmed bythe fact that no VT-FITC could be demonstrated on PMNs that wereremoved after the 3-hour incubation period on GMVECs on ice. Furthermore,PMNs that were CD16-PE positive and still adhering to endothelialcells (2.8%-3.6% of total PMNs added) were negative for VT-FITCbinding (Figure 5H). No uptake of VT-FITC by PMNs occurred duringthe incubation period.

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Fig 5. The transfer of VT-1-FITC bound to PMNs to human GMVECs was studied by flow cytometry. Panels A, C, and F: FACS analysis of nonstimulated GMVECs incubated for 4 hours with PMNs loaded with VT-FITC on ice. (A) Forward scatter and side scatter of nonstimulated GMVECs are shown. (C) No positive staining for CD16-PE was observed, indicating that all PMNs were removed by washing the monolayers. (F) Nonstimulated GMVECs did not bind any VT-FITC after incubation with VT-FITC-loaded PMNs. Panels B, D, E, G, and H: TNF- $alpha$ -stimulated GMVECs retained 2.8%-3.6% of PMNs (present in the gated area P in panel B) after 4 hours of incubation and washing of the monolayers. (D, E) PMNs were distinguished from GMVEC using CD16-PE; panel D represents all cells, whereas panel E reflects the gated area. (G) TNF- $alpha$ -treated GMVECs incubated with VT-FITC-loaded PMNs were able to bind 30%-50% of VT-FITC after the incubation period of 4 hours (all cells minus the gated area P). (H) PMNs showed no positive staining for VT-FITC, indicating that ligand passing of VT-FITC from PMNs to GMVECs had occurred.

GMVEC damage by ligand passing of VT from PMNs
Similar experiments were performed at 37°C. Unlabeled VT-1 bound to PMNs was used to study whether the transfer of VT-1 fromPMNs to GMVECs caused a biological effect. In TNF- $alpha$ -stimulatedGMVECs, both VT-binding PMNs and VT alone caused severe cytotoxityduring a 24-hour period, whereas PMNs alone had no effect (Figure6). The exposure of nonstimulated GMVECs to VT-binding PMNs alsocaused considerable cell death (30%-40%), whereas exposure ofVT-1 or PMNs alone had no effect. Comparable toxicities were observedwhen the VT-binding PMNs were washed 3 times and first incubatedfor 2.5 hours at 37°C (to mimic a circulation time before reachingthe target tissue) before they were washed again and transferredto the endothelial cells (data not shown).

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Fig 6. Phase-contrast microscopy of human GMVECs. Magnification × 50, except for (B) (magnification × 100). (A) Represents control GMVECs. (B) Shows the result of GMVECs incubated with PMNs for 24 hours. No change of morphology was observed. When cells were incubated with PMNs loaded with VT-1, cell death was observed after 24-hour incubation (C). (D) Represents control TNF- $alpha$ -treated GMVECs. The effect of PMNs loaded with VT-1 was also studied on TNF- $alpha$ -treated GMVECs (E) and compared with the effect of VT-1 on TNF- $alpha$ -treated GMVECs (F). In both conditions, equal amounts of cell death were observed.

Because VT exerts its cytotoxic effects by inhibiting protein synthesis, we quantified the effect of VT-preloaded PMNs onthe viability of GMVECs by determining the overall protein synthesis(from the incorporation of ³H-leucine in newly synthesized proteins). No effect on proteinsynthesis was observed when stimulated or nonstimulated GMVECswere incubated with PMNs. However, when nonstimulated and TNF- $alpha$ -stimulatedGMVECs were incubated with VT-preloaded PMNs, inhibition of proteinsynthesis (30% ± 15% and 60% ± 25%, respectively) was observed(Figure 7).

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Fig 7. Measurement of protein synthesis by incorporation of ³H-leucine in newly synthesized proteins. (A) Nonstimulated GMVECs incubated with VT-1 loaded PMNs showed during 24-hour incubation a reduction of protein synthesis. (B) GMVECs prestimulated for 24 hours with TNF- $alpha$ (10 ng/mL) showed strong inhibition during incubation with VT-1 alone or after incubation with VT-1 preloaded PMNs. Similar results were obtained from 5 different donors for GMVECs. Results are expressed as ± SEM. Statistical analysis was performed, using unpaired Student t test. P values smaller than .05 were considered to be significant. * P < 0.05 as compared to nonstimulated GMVECs (A) and TNF- $alpha$ -prestimulated GMVECs (B).

  Discussion

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

In this study, we demonstrate that VT-1 binds almost exclusively to nonstimulated PMNs in whole blood. Only 20 minutes ofincubation was sufficient to bind VT-1 to PMNs for more than 90%.No binding to other components of blood was observed, not evenwhen incubation time was prolonged to 3 hours. The K_d of the high-affinityreceptor for VT on PMNs is 100-fold less than that found for thefunctional receptor for VT, Gb3, on GMVECs. In line with thisdifference in affinity of VT, we found transfer of VT from PMNsto GMVECs and subsequent inhibition of protein synthesis and celldeath.

Several suggestions have been made to explain the transfer of VT from the intestine to the kidney. Bizan et al¹⁸ describedthat erythrocytes could bind VT, depending on their P blood groupphenotype. Robson et al¹⁹ as well as Taylor et al²⁰ suggestedthat there was an association between the outcome of the (D+)HUS and P blood group. However, other investigators could notdemonstrate a protective effect of the P1 blood group in HUS.We also could not find VT binding to erythrocytes in whole bloodof the 2 donors with P1 blood group in our study. However, wecannot exclude yet that local variations exist in P1 blood group-bindingproteins causing VT-binding in some people. Cooling et al²²indicated that, in particular, small and older platelets, obtainedby apheresis, contain small amounts of Gb3 and can bind VT. Ina whole blood environment, we did not observe any significantbinding of ¹²⁵I-VT-1 and VT-FITC to platelets (8 subjects studied). Therefore,the relative contribution of platelets to the transport of VTin plasma appears insignificant as compared with PMNs. Lingwood²³^,²⁴suggested that lipoproteins might be responsible for transportingVT. However, in the present study, we could not find binding ofVT to human LDL, VLDL, or HDL, thus excluding this possibility.In line with our previous observation that purified human monocytesonly bind VT significantly after activation by LPS,²¹ we foundno VT binding to monocytes in whole blood. On the contrary, VTbinding occurred exclusively to PMNs, independent of blood groupsor age of the donor. These data lead to the conclusion that PMNsare a good candidate for transporting VT in the systemic circulationto target organs in adults as well as inchildren.

The rapid binding of VT to PMNs can explain why VT is usually not detectable in blood plasma.³¹ After binding the VT, PMNsare able to transport the VT to target organs and transfer theVT to endothelial cells in vitro. Stimulating the GMVECs withinflammatory mediators, such as TNF- $alpha$ or LPS, induces the VT receptorGb3 on the cell surface.²⁶^,³² As expected, transfer of VT-1from PMNs to endothelium increased when GMVECs were previouslystimulated with TNF- $alpha$ . We demonstrate in this study that one typeof binding site is involved in VT-1 binding on PMNs and that thisbinding site is different from the Gb3 receptor found on endothelialcells. It is uncertain whether the VT receptor on PMNs representsa glycolipid, because VT-1 binding to PMNs was highly sensitiveto trypsin treatment. In contrast to the classical VT receptor,Gb3, the VT receptor found on PMNs does not result in VT internalization.The lower K_d for the receptor on PMNs than for Gb3 allows transferof VT from PMNs to endothelial cells. Within 24 hours, this transferwas accompanied by biological effects, especially inhibition ofprotein synthesis and cell death. Interestingly, we observed thatsuch biological effects not only affected cells that were prestimulatedwith TNF- $alpha$ but also in nonstimulated GMVECs that were incubatedwith VT-binding PMNs. These data indicate that PMNs not only canbind VT in the circulation but also can transfer it to targetcells that express the VT-receptorGb3.

That PMNs may play a seminal role in pathogenesis of HUS has been suggested many times. First, the number of PMNs is elevatedin HUS. It has been suggested that the number of PMNs is a predictivefactor for the outcome of the disease.^33-35 In addition, Taylorand colleagues³⁶^,³⁷ showed that there was an increased numberof PMNs in autopsy material of diarrhea-associated patients withHUS. Furthermore, Fitzpatrick et al³⁸^,³⁹ described that PMNsof HUS patients were activated and that, in HUS patients, levelsof elastase and IL-8 were elevated. These results were confirmedby other investigators,⁴⁰ and they suggested that PMNs may damagethe endothelium through release of the intracellular components,such as elastase.³⁸^,³⁹^,⁴¹ Finally, Morigi et al⁴² describedthat VT-1 increased PMNs adhesion to the endothelium under flowconditions by up-regulating adhesive proteins. The binding ofPMNs to the endothelium was reduced by blocking of E-selectin,ICAM-1, and VCAM-1 with respective antibodies. The adhesion ofPMNs to the endothelium was enhanced by pre-exposure of the endothelialcells by TNF- $alpha$ . These investigators found that VT-1 was able toinhibit the process of rolling that normally precedes adhesionof cells to the endothelium. In line with these findings is thatPMNs of HUS patients adhere more avidly to endothelial cells thanPMNs of healthy control subjects.⁴¹^,⁴³ All these results togetherindicate that PMNs play an important role in pathogenesis of HUS.Our data show a new and crucial aspect of the involvement of PMNsin (D+) HUS, namely the specific binding and transport of VT toPMNs in whole blood. Additional studies are needed to evaluatewhether the binding of VT to PMNs causes a metabolic effect inPMNs themselves. In this respect, it is of interest to note that,in a recent study,⁴⁴ the induction of superoxide productionin PMNs by Shiga toxin-1 wasdescribed.

In conclusion, our study demonstrates an additional role of PMNs in the pathogenesis of HUS and strongly suggests that PMNsare the cells that transport the VT from intestine to endothelium.This transport is facilitated by a receptor that has a 100-foldlower affinity than the high-affinity receptor (Gb3) that is expressedon GMVECs after exposure to TNF- $alpha$ . PMNs loaded with VT displaya direct cytotoxic effect to the endothelium of the kidney invitro by inhibition of protein synthesis. The occurrence of VT-1binding to PMNs in vivo and ligand passing of VT and PMNs hasto be demonstrated in future studies. We believe that this observationis important in understanding the pathogenesis of (D+) HUS andopens perspectives for futuretreatment.

  Footnotes

Submitted August 3, 1999; accepted January 25, 2000.

Supported by grant 97.1645 from the Dutch KidneyFoundation.

Reprints: Victor W. M. van Hinsbergh, Gaubius Laboratory, TNO-PG, Zer-nikedreef 9, PO Box 2215, 2301 CE Leiden, TheNetherlands; e-mail: VWM.vanHinsbergh{at}pg.tno.nl.

The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

  References

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

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  Copyright © 2000 by American Society of Hematology         Online ISSN: 1528-0020





	Copyright © 2000 by American Society of Hematology Online ISSN: 1528-0020