From the Institute of Biochemistry, University of Giessen, D-35392
Giessen, Germany and Department of Immunology and Cell
Biology, Research Center Borstel, D-23845 Borstel, Germany
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ABSTRACT |
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The isolated
neutral glycosphingolipid fraction from the pig parasitic nematode,
Ascaris suum, was fractionated by silica gel chromatography
to yield a neutral and a zwitterionic glycosphingolipid fraction, the
latter of which mainly contained two zwitterionic glycosphingolipids
termed components A and C. Preliminary chemical characterization with
hydrofluoric acid treatment and immunochemical characterization with a
phosphocholine-specific monoclonal antibody indicated that both
components contained phosphodiester substitutions: phosphocholine for
component A, and phosphocholine and phosphoethanolamine for component
C. Both components were biologically active in inducing human
peripheral blood mononuclear cells to release the inflammatory monokines tumor necrosis factor , interleukin 1, and interleukin 6. Component A was the more bioactive molecule, and its biological activity was abolished on removal of the phosphocholine substituent by
hydrofluoric acid. The glycosphingolipid components were structurally analyzed by matrix-assisted laser desorption/ionization
time-of-flight mass spectrometry, liquid secondary ion mass
spectrometry, methylation analysis, 1H NMR spectroscopy,
exoglycosidase cleavage, and ceramide analysis. Their chemical
structures were elucidated to be (see Structure I below),
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The carbohydrate moiety oligosaccharide core was characterized as belonging to the arthro series of protostomial glycosphingolipids. The ceramide moiety was distinguished by (R)-2-hydroxytetracosanoic acid as the dominant fatty acid species and by the C17 iso-branched sphingosine and sphinganine bases, 15-methylhexadecasphing-4-enine and 15-methylhexadecasphinganine, respectively.
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INTRODUCTION |
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Analyses of the immunoreactivity between neutral fraction glycolipids derived from various species of parasitic nematodes have indicated a high degree of serological cross-reactivity (1, 2). The structural basis for this immunological cross-reactivity between parasitic nematodes at the level of glycolipids is at present unknown. Structural studies on the neutral fraction glycosphingolipids from adults of the porcine parasitic nematode Ascaris suum have revealed that the identified arthro series oligosaccharide chain was not immunogenic, i.e. did not exhibit immunoreactivity toward infection sera from A. suum-infected mice (2, 3). However, a zwitterionic glycosphingolipid fraction was also isolated from A. suum that demonstrated a phosphodiester sidechain as a structural modification of possibly phosphocholine (PC)1 and phosphoethanolamine (PE). In addition, these zwitterionic glycolipids were immunogenic/antigenic, i.e. exhibited immunoreactivity toward infection sera from A. suum-infected mice (2).
PC-containing macromolecules have been regularly detected in the extracts of numerous species of parasitic nematodes by immunological means (4-9). Structurally, this moiety has been found bound to N- and O-linked glycans of glycoproteins, although the exact structure of the PC-oligosaccharide linkage is at present unknown (10). The biological significance of PC glycans in the host parasite relationship revolves around their immunomodulatory activity (11) such that the frequent observation of host T-cell hyporesponsiveness to filarial nematode infection (12) may involve PC because of its ability to block T- and B-cell antigen-specific proliferation (13, 14).
Little is known as to the biological activity of glycolipids, in
general, and parasitic helminth-derived glycolipids, in particular, as
regards their putative modulation of the host immune response via the
cytokine network. Gangliosides have been found to be inhibitory in
terms of cytokine synthesis and release (15), whereas neutral glycosphingolipids of the cestode Echinococcus
multilocularis inhibited the production of interleukin 2 (IL-2)
(16). Because of the physico-chemical similarity between
glycosphingolipids and lipopolysaccharides (LPS) of Gram-negative
bacteria and the induction by the latter of bioactive protein mediators
in the host, i.e. cytokines, responsible for the effects of
endotoxemia (17), a comparative study was performed by Krziwon et
al. (18) on the ability of the former to stimulate the production
of inflammation-associated cytokines. An atypical, zwitterionic
glycosphingolipid (as regards the linkage of the glucuronic acid
residue to the ceramide moiety and the presence of nonacetylated
glucosamine) from the LPS-negative, Gram-negative bacterium
Sphingomonas paucimobilis induced the synthesis and release
of the human mononuclear cell-derived, inflammation-associated cytokines tumor necrosis factor (TNF-
), IL-1, and IL-6 but with
approximately 10,000-fold less activity than LPS, in this respect.
We report here on the structures and biological activity of two
immunoreactive, zwitterionic fraction glycosphingolipids from A. suum in terms of their ability to stimulate the production of the
human mononuclear cell-derived, inflammation-associated cytokines
TNF-, IL-1, and IL-6.
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EXPERIMENTAL PROCEDURES |
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Materials--
Undamaged, washed adult male and female worms
were collected from the local abattoir and stored at 70 °C until
further use. LPS from Salmonella friedenau was kindly
donated by H. Brade (Borstel Research Institute).
Preparations--
Worms (800 g wet weight) were pulverized at
20 °C in a precooled Waring blendor and lyophilized. Glycolipids
were isolated and purified as described previously (3). In short,
glycolipids were extracted with chloroform/methanol/water 10:10:1 (by
vol), chloroform, methanol, 0.8 M aqueous sodium acetate
30:60:8 (by vol), and 2-propanol, n-hexane, water 55:20:25
(by vol) and evaporated to dryness. To remove most of the contaminating
triglycerides, the residue was treated with acetone at 4 °C for
2 h. Neutral (N-/Nz-) and acidic glycosphingolipids were separated
by DEAE-Sephadex A-25 column chromatography (Pharmacia). The column was
equilibrated with and the sample taken up in chloroform/methanol/water
30:60:8 (by vol). N-/Nz- glycosphingolipids were obtained in the
flow-through, and the acidic glycosphingolipids were eluted with
chloroform, methanol, aqueous 0.8 M sodium acetate 30:60:8
(by vol). Neutral (N-) and zwitterionic (Nz-) glycolipid fractions were
further fractionated on a silica gel60 column (Merck).
Homogeneous, zwitterionic components A and C were obtained by isocratic
elution with chloroform/methanol/water 10:10:2.5 (by vol) from a silica
gel60 column (1 × 50 cm, 70-250 mesh; Merck).
Bioassay Determination of Released Cytokines--
The isolated
Nz-glycosphingolipids, component A and C, and ceramide pentahexoside
(CPH) derived from component A by HF treatment (see below) were
subjected to sterile distilled water dialysis to remove potential cell
culture-perturbing contaminants and traces of organic solvents. After
Speed-Vac lyophilization, the glycosphingolipids were resuspended at 1 mg/ml in sterile distilled water, sonicated, and stored at 20 °C
until further use. As a positive control, S. friedenau-derived LPS was solubilized in pyrogen-free
phosphate-buffered saline at 1 mg/ml, neutralized with triethylamine,
sonicated, and stored at 4 °C until further use.
High Performance Thin-layer Chromatography (HPTLC)-- For HPTLC separation, HPTLC silica gel60 plates (Merck) were used. Glycolipids were dissolved at 2 µg/µl in chloroform/methanol/water 10:10:3 (by vol). For reproducibility, HPTLC was performed according to Nores et al. (22). Chloroform/methanol/water 10:10:3 (by vol) was used as the running solvent. For two-dimensional HPTLC, chloroform, methanol, 2% aqueous ammonia 10:10:3 (by vol) was employed as the second direction-running solvent. Glycosphingolipids were visualized using I2 vapor and/or by spraying the plates with orcinol/sulfuric acid (carbohydrate-positive compounds) or ninhydrin (free amino groups) and heating. For immunostaining, the developed HPTLC plates were fixed with polyisobutylmethylacrylate (Röhm & Haas, Darmstadt, Germany), blocked with phosphate-buffered saline and bovine serum albumin, and incubated with the phosphocholine-specific monoclonal antibody TEPC-15 (Sigma) overnight at 4 °C, as described elsewhere (1). Peroxidase-coupled anti-mouse Ig (Dako Diagnostics, Hamburg, Germany) was used as the secondary antibody.
Matrix-assisted Laser Desorption/Ionization Time-of-flight Mass
Spectrometry (MALDI-TOF-MS)--
MALDI-TOF-MS data were obtained using
a Vision 2000 instrument (Finnigan MAT, Bremen, Germany) operating in
the positive-ion reflectron and linear modes. Ions were formed by a
pulsed, ultraviolet laser beam (nitrogen laser, = 337 nm). The
matrix used was 2,5-dihydroxybenzoic acid (Sigma) at 10 g/liter in
0.1% aqueous trifluoroacetic acid/acetonitrile 1:2 (by vol).
Liquid Secondary-ion Mass Spectrometry (LSIMS)-- LSIMS was carried out with a MAT 900 mass spectrometer (Finnigan MAT) equipped with a cesium gun, which was operated at an emission current of 2-3 µA. Mass spectra were recorded at an acceleration potential of 5 kV with a resolution of approximately 3,000 and were acquired using a DEC 2100 data system. Spectra of native, peracetylated, or permethylated glycosphingolipids were recorded in the positive-ion mode using 3-nitrobenzyl alcohol (Aldrich) as matrix.
NMR Spectroscopy--
The 1H NMR spectra were
recorded at 333 K on a Bruker DRX 600 spectrometer with
deuterium-exchanged samples (0.9 mg each) for solutions in
Me2SO-d6 (99.96%; Aldrich)
containing 2% (by vol) 2H2O (99.96%; Aldrich)
using the 1H signal of dimethyl
sulfoxide-d5 (H 2.49) as internal
reference. All one- and two-dimensional NMR experiments like
two-dimensional correlation spectroscopy (COSY) and two- and three-step
related coherence transfer (RCT-1 and -2), were performed using
standard Bruker software (XWINNMR, Version 1.3).
HF Treatment-- Nz-glycosphingolipids (native or permethylated) were dried in a stream of nitrogen and incubated for 24 h at 4 °C with 50-200 µl of HF (48%; Fluka, Neu-Ulm, Germany). Excess was removed in a stream of nitrogen at room temperature.
Endoglycoceramidase Cleavage-- Nz-glycosphingolipids were resuspended in 100 µl of 50 mM sodium acetate buffer, pH 5.0, containing 1 g/liter sodium taurodeoxycholate, and 0.5 milliunits of endoglycoceramidase (Sigma) were added. After incubation at 37 °C for 24 h, another 0.5 milliunits of enzyme were added. The reaction was stopped after 48 h by adding 400 µl of H2O and 400 µl of water-saturated n-butanol for phase separation of the reaction products.
Pyridylamination-- Nz-oligosaccharides obtained by endoglycoceramidase cleavage were reductively pyridylaminated (23) and the pyridylaminated oligosaccharides were separated by amino-phase HPLC, as described previously (24).
Exoglycosidase Treatment--
Pyridylaminated oligosaccharides
were cleaved after obligatory HF treatment with either
-D-galactosidase (EC 3.2.1.22) from coffee beans
(Boehringer Mannheim),
N-acetyl-
-D-hexosaminidase (EC 3.2.1.52) from
jack beans (Sigma), or
-D-mannosidase (EC 3.2.1.25) from
Helix pomatia (Oxford Glycosystems, Abingdon, UK). For
cleavage, the dried oligosaccharides were taken up in 50 µl of 50 mM sodium citrate, pH 4.0, and incubated at 37 °C for
24 h with 50 milliunits of
-galactosidase, 166 milliunits of
-N-acetylhexosaminidase, and 25 milliunits of
-mannosidase, respectively.
Methylation Analysis-- Nz-glycosphingolipids (20 µg) were permethylated both before or after HF treatment and hydrolyzed (25). Partially methylated alditol acetates obtained after sodium borohydride reduction and peracetylation were analyzed by capillary GLC/MS using the instrumentation and microtechniques described elsewhere (26).
Peracetylation-- Nz-glycosphingolipids were peracetylated with acetic acid/trifluoroacetic anhydride 1:2 (by vol) for 10 min at room temperature (27).
Identification of Zwitterionic Substituents-- Phosphocholine was released by HF treatment of Nz-glycosphingolipid components A and C. Liberated choline residues were derivatized with pentafluoropropionic acid anhydride (Supelco, Deisenhofen, Germany) and analyzed by LSIMS. Ethanolamine was identified as its 9-fluorenylmethoxycarbonyl-derivative by HPLC (28) after HF treatment of component C.
N-Methylation of Phosphoethanolamine-- Nz-glycosphingolipid component C was treated with 200 µl of 750 mM aqueous sodium carbonate containing 20 µl of methyl iodide for 2 h at 50 °C (29, 30), and thereafter, desalted on a reverse-phase cartridge (31).
Ceramide Analysis--
For fatty acid analysis,
Nz-glycosphingolipids (1-10 nmol) were hydrolyzed according to Gaver
and Sweeley (32). The resultant fatty acid methyl esters were analyzed
by capillary GLC/MS using the instrumentation described previously
(26). For the separation of fatty acid species, a fused silica
capillary column (DB1, 0.25 mm internal diameter, 60 m; ICT, Bad
Homburg, Germany) was used. The column temperature was increased from
80 °C at 7 °C/min to a final temperature of 320 °C and held
isothermally for 10 min. Spectra were recorded either after chemical
ionization (CI-MS) with ammonia or electron-impact ionization (EI-MS)
at an electron energy of 2.4033 × 1017 J or
1.1215 × 10
17 J, respectively. For determination of
the absolute configuration at C-2 of the contained hydroxy fatty acids,
they were converted to the corresponding
(R)-phenylethylamides and trifluoroacetylated as described
previously (3). Sphingoid bases were analyzed after conversion to the
corresponding fatty acids by periodate and periodate/permanganate
oxidation as their methyl and picolinyl esters as described elsewhere
(3).
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RESULTS |
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Isolation of Zwitterionic Components A and C-- Glycosphingolipids were separated into a neutral and acidic fraction by anion-exchange column chromatography. Two-dimensional HPTLC of the resultant neutral fraction indicated the presence of two groups of glycosphingolipids: N-neutral, Nz-neutral zwitterionic glycosphingolipids (see Fig. 1). For isolation of the two main zwitterionic components A and C, the neutral fraction was subfractionated into a neutral and neutral zwitterionic fraction by silica gel column chromatography. A further silica gel column chromatography yielded four fractions designed as components A, B1, B2, and C. The fractions B1 and B2 represent nonhomogeneous, minor zwitterionic components and will not be discussed further in this publication.
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Chemical and Immunochemical Characterization-- The two zwitterionic components A and C were separated on HPTLC by chloroform/methanol/water 10:10:3 (by vol) as running solvent. Both components gave positive reactions on incubation with iodine vapor, spraying with orcinol/sulfuric acid, and molybdate reagent (organic phosphate groups). HPTLC-immunostaining with the phosphocholine-specific monoclonal antibody TEPC-15 is shown in Fig. 2. Due to the approximately 50-fold higher sensitivity of HPTLC-immunostaining, additional, minor species of components A and C resulting from heterogeneities in their lipid moieties were also visualized. The component C also reacted with ninhydrin, indicating the presence of a free amino group. HF treatment of the zwitterionic compounds yielded glycosphingolipids with migration properties on HPTLC similar to CPH, which showed no reaction with TEPC-15 or ninhydrin. Choline was identified after HF treatment of the components A and C by derivatization with pentafluoropropionic acid anhydride and analysis by LSIMS, yielding a molecular ion [M]+ at m/z 250. Ethanolamine was identified after HF treatment of compound C as its 9-fluorenylmethoxycarbonyl derivative by HPLC and co-chromatography with the standard (data not shown).
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Zwitterionic Component A- and C-induced Monokine
Production--
Since we consider A. suum merely as a model
for the human parasitic nematode Ascaris lumbricoides, all
in vitro procedures were performed with human and not
porcine PBMC. The zwitterionic components A and C and the component
A-derived CPH were assayed as to their biological activity in inducing
the inflammatory monokines TNF-, IL-1, and IL-6 because of the
postulated similarities in physico-chemical properties and biological
activity between glycosphingolipids and LPS. Components A and C, but
not ceramide pentasaccharide, were shown to be biologically active in
terms of a dose-dependant response in the release of TNF-
, IL-1,
and IL-6 (see Fig. 3). For IL-1 and IL-6,
this dose dependence of cytokine release was evident up to and
including 1000 ng/ml component A, with the apparent presumption that
higher concentrations were inhibitory at the cellular level. Of the two
zwitterionic glycolipids tested, component A was the more bioactive in
inducing the monokines TNF-
and IL-1; component A and to a lesser
extent component C were also capable of inducing low levels of IL-6
activity as demonstrated in three separate experiments (data not
shown). The apparent inconsistency in concentration levels measured was
due to the inherent between-experiment variability of the bioassay
system with different human donors.
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Structural Analysis of Zwitterionic Components A and C-- For structural analysis, the zwitterionic components A and C were subjected to MALDI-TOF-MS, LSIMS, methylation analysis, and exoglycosidase digestion. The results of MALDI-TOF-MS and LSIMS are summarized in Table I and methylation data in Table II.
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DISCUSSION |
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A slowly emerging chemical characteristic of invertebrate glycoconjugates (glycolipids, glycoproteins) is their frequent substitution by electrically neutral but amphoteric moieties. The diversity of zwitterionic glycoconjugates among the various phyla of the Invertebrata would point to their biological importance, but as yet, unknown functional significance. A major post-translational modification of parasitic helminth antigens is apparently PC. This antigenic determinant has been detected in nematodes (5, 8, 34, 35), in trematodes, including Schistosoma mansoni (9), and in the cestode Bothriocephalus scorpii (36). In fact, the frequency of serological cross-reactivity between cestodes, trematodes and, in particular, nematodes (37) may be accounted for by the broad distribution of PC-bearing molecules. The (macro)molecular location of the PC moiety is in most cases unknown, but at least in the excretory/secretory product (ES-62) of the adult filarial nematode, Acanthocheilonema viteae, it is attached to the protein backbone via an N-linked glycan (38).
Zwitterionic glycosphingolipids have been structurally characterized from various members of the invertebrate phyla, including identification of the monosaccharide-amphoteric moiety in the Sarcomastigophora (Flagellata) as Man-phosphoethanolamine (39), in the Annelida as Gal-phosphocholine (40-44), in the Arthropoda (Crustacea) as Glc-phosphonoethanolamine (45), in the Arthropoda (Insecta) as GlcNAc-phosphoethanolamine (33, 46, 47), in the Mollusca (freshwater Bivalvia) as Man-phosphoethanolamine (48), in the Mollusca (marine Gastropoda) as Gal-phosphonoethanolamine (49, 50), and in the Nematoda (Ascaridida) as GlcNAc-phosphocholine and Man-phosphoethanolamine (Ref. 3 and this publication).
Localization of zwitterionic substituents such as phosphocholine or
phosphoethanolamine was performed by HF treatment, both before or after
permethylation and subsequent hydrolysis, reduction, and peracetylation
(in the range of 10 µg of glycosphingolipid). The alkali instability
of the phosphoethanolamine substituent, however, requires selective
N-methylation before the permethylation procedure.
MALDI-TOF-MS analysis of the zwitterionic glycolipids revealed a
characteristic fragmentation in the reflectron mode, probably due to
the loss of choline (M 87) and ethanolamine (M-45),
respectively, by metastable decay, which was not detectable in the
linear mode. A similar fragmentation pattern has been observed in LSIMS
after permethylation, whereas the peracetylated structures were found
to be stable. This idiosyncratic fragmentation behavior may help to
detect and identify zwitterionic substituents by mass spectrometry.
Structural elucidation of the two major, zwitterionic glycosphingolipids (components A and C) of the porcine, parasitic nematode A. suum has shown their common pentasaccharide core to belong to the arthro-carbohydrate series (as originally isolated from glycosphingolipids of the blowflies Calliphora vicina and Lucilia caesar). The amphoteric substituent PC is linked to C-6 of the third monosaccharide in the oligosaccharide chain, GlcNAc, of component A, and, uniquely, the amphoteric substituents PE and PC are simultaneously linked to C-6 of the second and the third monosaccharide in the oligosaccharide chain, Man and GlcNAc, respectively, in component C. Component C, therefore, represents the first member of the glycosphingolipids to carry two zwitterionic substituents. The carbohydrate and ceramide moieties of the two zwitterionic glycosphingolipids correspond to the recently elucidated arthropentaosyl ceramide of A. suum. (3) Therefore, we have assumed that the biosynthetic pathway of the former involves zwitterionic substitution of the latter, either at the level of CPH or incomplete oligosaccharide cores.
The 1H-NMR data obtained for both glycosphingolipids A and
C were found to be structurally closely related to that identified in a
pentaglycosyl phosphoglycosphingolipid (Nz5a) isolated from the blowfly
C. vicina Meigen (51). Comparing the glycosphingolipid Nz5a
of the blowfly C. vicina Meigen and compound A described here, both belong to the arthro series, and only three structural differences were observed: (i) a terminal -GalNAcV
instead of
-GalV, (ii) the terminal sugar
(
-GalNAcV) being (1
4)-linked in Nz5a and
-GalV being (1
3)-linked in compound A, and (iii)
2-aminoethyl phosphate instead of a phosphocholine substituent in
position 6 of GlcNAcIII. The biological properties of
the glycosphingolipid Nz5a, however, were not investigated.
Glycosphingolipids have been shown to be immunomodulatory molecules
that suppress cells of the immune system, both in vivo and
in vitro. Thus, gangliosides inhibit the in vitro
proliferative response of various classes of activated immune cells
such as T- and B-lymphocytes, macrophages, and natural killer cells
(52). However, the molecular mechanism(s) underlying the
immunosuppressive activity of glycosphingolipids are incompletely
understood but include the direct interaction of ganglioside micelles
with IL-2 and IL-4 in the modulation of
IL-2-/IL-4-dependent processes (53) and the interference of
monocytes at the level of antigen presentation (54). The
immunomodulation of T-lymphocyte activation in vivo and
in vitro, observed in the case of Trypanosoma
cruzi glycoinositol phospholipids, can be directly related to the
ceramide moiety of the molecule (55). A functional resemblance of LPS
to glycosphingolipids has been proposed and reinforced by the ability
of the former to mimic the second messenger ceramide in TNF-- and
IL-1-stimulated cells (56, 57). Since there is no structural similarity
between these two classes of lipid molecules, it may be assumed that
this coincidence of biological activity is based on similar
physico-chemical properties. The ability of A. suum
zwitterionic components A and C to induce the human PBMC inflammatory
cytokines of TNF-
, IL-1, and IL-6 provides a further example for the
parallelism between LPS and glycosphingolipid biological activity.
Interestingly, the zwitterionic glycosphingolipids of A. suum stimulated rather than suppressed human PBMC production of
the cytokines TNF- and IL-6 in a concentration range similar to that of LPS stimulation, whereas these molecules were at least a factor 100-fold less potent than LPS in the stimulation of IL-1. In general, component C was less active than component A. When compared with LPS
with respect to the amount of cytokine induced, component A was as
active in the stimulation of TNF-
but was decreasingly active in the
sequence of IL-1 and IL-6. The expression of the inflammatory response
cytokines TNF-
, IL-1, and IL-6 is usually considered to be
concomitant (58). Until concrete data are available, there are at least
two plausible explanations for the detection of the anomalous,
nonconcomitant levels of these cytokines induced by the A. suum-derived zwitterionic glycosphingolipids under study. First,
kinetic studies of LPS- and zwitterionic glycosphingolipid-induced inflammatory cytokine expression demonstrated maximal activity in the
temporal sequence of TNF-
and IL-1 at approximately the same time
point and prior to that of IL-6 (18, 19). The fixed-point determination
of cytokine release in the assay used in this study at 8 h of
incubation introduces an experimental artifact whereby TNF-
and IL-1
approach their maximal levels of activity, whereas IL-6 induction is
suboptimal at this time point. Secondly, it is known that activation of
monocytes by LPS is a receptor-mediated process that is transduced by
the cell surface molecule CD 14 (59). The mechanism by which the
A. suum-derived zwitterionic glycosphingolipids induce
cytokine production is, however, unknown. It may be postulated that
they act in a direct way by replacing intracellular lipid second
messengers such as ceramide. Therefore, a different pattern of
cytokines released by activated monocytes may be due to different
mechanisms of activation.
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ACKNOWLEDGEMENTS |
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The authors wish to express special recognition to Ina Goroncy, Borstel Research Institute, Department of Immunology and Cell Biology for the implementation and ultimate success of the monokine bioassay experiments. We also thank Peter Kaese, Werner Mink, and Siegfried Kühnhardt for methylation, GLC/MS, and LSIMS analyses and Ulrich Zähringer (Department of Immunochemistry, Research Center Borstel, Borstel) for performing the NMR analysis.
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FOOTNOTES |
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* This project was supported by the Deutsche Forschungsgemeinschaft (SFB 535 and Graduiertenkolleg Molecular Biology and Pharmacology) and by the Bundesministerium für Bildung, Wissenschaft, Forschung und Technologie Grant 01 KI 9471.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
§ To whom correspondence should be addressed: Biochemisches Institut am Klinikum der Universität, Friedrichstrasse 24, D-35392 Giessen, Germany. Tel.: +49-641-99-47400; Fax: +49-641-99-47409; E-mail: Rudolf.Geyer{at}biochemie.med.uni-giessen.de.
1 The abbreviations used are: PC, phosphocholine; PE, phosphoethanolamine; CPH, ceramide pentahexoside; HPTLC, high-performance thin-layer chromatography; IL, interleukin; LPS, lipopolysaccharide; LSIMS, liquid secondary-ion mass spectrometry; MALDI-TOF-MS, matrix-assisted laser desorption/ionization time-of-flight mass spectrometry; N-glycolipid, neutral glycolipid; Nz-glycolipid, zwitterionic glycolipid; PBMC, peripheral blood mononuclear cells; TNF, tumor necrosis factor; HPLC, high performance liquid chromatography; GLC, gas-liquid chromatography; Hex, hexose; HexNAc, N-acetylhexosamine.
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REFERENCES |
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