2 Unité Des Aspergillus, Institut Pasteur, 25 Rue Du Docteur Roux, 75724 Paris Cedex 15, France
3 Division of Biological Chemistry and Molecular Microbiology, School of Life Sciences, University of Dundee, Wellcome Trust Biocentre, Dow Street, Dundee DD1 5EH, United Kingdom
Received on May 30, 2002; revised on September 3, 2002; accepted on September 3, 2002
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Abstract |
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Key words: Aspergillus / glycoprotein / glycosylphosphatidylinositol
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Introduction |
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All protein-linked GPI anchors have a conserved core structure of ethanolamine-P-Man3GlcN-PI, and GPI biosynthetic pathways are also largely conserved between organisms. In fungi, structural and biosynthetic studies of GPI are mostly restricted to the model yeast S. cerevesiae. These GPI molecules have a glycan with mainly four mannose residues, Man1-2Man
1-2Man
1-6Man
1-4GlcN
1-6myo-inositol-1-PO4, although some contain an additional
1-2- or
1-3-linked reducing terminal mannose residue (Frankhauser et al., 1993
). The lipid part differs from mammalian cells with the presence of ceramide or hydroxy-fatty acid-containing diacylglycerol (Conzelmann et al., 1992
; Frankhauser et al., 1993
).
To analyze the structure of the mature GPI anchors of a filamentous fungi, we purified several GPI proteins of A. fumigatus, a human pathogen, and analyzed the lipid and glycan moieties of their anchors.
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Results |
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Analysis of PIs
PI moieties from partially purified GPI proteins were isolated from western blots on polyvinylidene difluoride (PVDF) membrane after nitrous acid deamination and butanol extractions. After purification on a silica column, PIs were characterized by negative ion electrospray mass spectrometry (ES-MS) and electrospray tandem mass spectrometry (ES-MS-MS) (Figure 2). The same data were obtained from all GPI-anchored proteins. The ES-MS spectra revealed one principal [M-H]- pseudomolecular ion at m/z 924 and three minor ions at m/z 910, 938, and 952. The fragmentation of each PI compound produced only two daughter ions at m/z 241 [inositol-1,2-cyclic phosphate]- and m/z 259 [inositol-monophosphate]-. The presence of these daughter ions and the absence of fatty acid carboxylate ions and/or 1-O-alkylglycerol-2,3-cyclic phosphate ions is characteristic of inositol-phosphoceramides (IPCs) (Treumann et al., 1998). From the measured mass of the main component (925 Da), we can deduce the molecular weight of the ceramide component (683 Da). By analogy with typical ceramide structures in yeasts and fungi (Frankhauser et al., 1993
; Lester and Dickson, 1993
), this suggests that the ceramide is made of a C18-phytosphingosine and a 2-monohydroxylated C24:0 fatty acid. The minor components that differ by 14 Da or 28 Da presumably reflect variability of the size of one or other of the aliphatic chains.
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Discussion |
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Gel1p is a member of a new family of GPI-anchored ß1-3 glucanosyltransferases involved in cell wall ß-glucan modeling (Mouyna et al., 2000a,b
). Ecm33p is a homolog of a putative yeast GPI-anchored protein thought to be involved in cell wall biosynthesis because
ECM33 mutants show hypersensitivity to zymolyase (endoß1-3glucanase), hygromycin B, and K1 killer toxin and have an altered glucose/mannose ratio (monosaccharides mainly found in the cell wall) (Caro et al., 1997
).
PhoAp, an acid phosphatase purified as two protein bands on sodium dodecyl sulfatepolyacrylamide gel electrophoresis (SDSPAGE) at 70 and 80 kDa, was identified by sequence homolgy to PhoAp from Penicillium chrysogenum and Aspergillus niger (Haas et al., 1992; Ehrlich et al., 1994
; Bernard et al., 2002
). This protein, with 46% sequence identity to the A. niger homolog, is the major GPI-anchored protein in the A. fumigatus membrane preparation. To date, PhoAp is the only protein in A. fumigatus found to be associated with the cell wall ß1-3 glucan as it is released with an endo-ß1-3 glucanase digestion. In Kluyveromyces marxianus cell wall ß1-3 glucanase digestion also released an acid phosphatase (Yoda et al., 2000
). Covalent linkage of GPI-anchored proteins to cell wall polymer has been mainly described in yeast, where ß1-6 glucan constitutes a bridge between protein and ß1-3 glucan, the main cell wall polysaccharide (Kapteyn et al., 1996
, 1999
; Kollar et al., 1997
). However, no chemical proof of the covalent cross-linking for GPI-anchored PhoAp to cell wall ß1-3 glucan has been established to date.
Based on our chemical and enzymatic analysis, we can suggest that the main GPI anchor structure in A. fumigatus is as shown in Figure 7. For all four proteins analyzed, the lipid part is exclusively IPC, most likely containing a C18-phytosphingosine long-chain base amide-linked to a monohydroxylated C24:0 fatty acid, as judged by its mass and by analogy with the S. cerevisiae structure. Inositol-phosphoceramides are common in yeast GPI structures and have also been described in Dictyostellium discoideum (Stadler et al., 1989; Haynes et al., 1993
), plants (Oxley and Bacic, 1999
), and trypanosomatid parasites (McConville and Ferguson, 1993
; Serrano et al., 1995
; Ferguson et al., 1999
). To date, IPCs have not been found in mammalian GPI structures. In fungi, IPCs are also found as free phospholipids and as mannosylated IPC containing 2-monohydroxylated long chain fatty acids (Lester and Dickson, 1993
). However, their biosynthesis seems to be independent from that of GPI anchors (Reggiori and Conzelmann, 1998
). The major glycan component of the A. fumigatus GPI anchors is Man
1-3Man
1-2Man
1-2Man
1-6Man
1-4GlcN (Man5GlcN), which conforms to the minimal Man
1-2Man
1-6Man
1-4GlcN (Man3GlcN) core GPI glycan structure common to all protein-linked (type 1) GPI structures (McConville and Ferguson, 1993
) and is identical to one of the two Man5GlcN glycoforms found in a minority of GPI structures in S. cerevisiae (Frankhauser et al., 1993
).
Although on-blot GPI glycan labeling and off-blot release methods have been described previously (Zitzmann and Ferguson, 1999; Zitzmann et al., 2000
), as have GPI PI-fraction analyzed by ES-MS and ES-MS-MS (Serrano et al., 1995
; Rudd et al., 1997
; Treumann et al., 1998
; Almeida et al., 2000
), this is the first report to describe a novel off-blot method for GPI PI-fraction isolation prior to ES-MS and ES-MS-MS analysis. Thus, the entire GPI structure analysis described in this article was performed on protein bands transferred to PVDF membrane. The approach was effective and sensitive. However, the aqueous Hydrofluoric acid (HF) dephosphorylation step, neccesary to release the 2-AB-labeled GPI glycan from the PVDF membrane-bound protein component, results in the loss of all ethanolamine phosphate substituents. Thus, the ethanolamine phosphate bridge to the protein C-terminus shown in Figure 7 is drawn by analogy with other known GPI anchor structures (Ferguson et al., 1999
). Whether or not the A. fumigatus GPI anchor has additional ethanolamine phosphate substituents on the first and second mannose residues, which are common in higher-eukaryote GPI anchors, is unknown. The absence of additional ethanolamine phosphate groups in mature GPI anchors of S. cerevisiae (Frankhauser et al., 1993
) has been questioned recently, and it appears that at least some mature yeast GPI anchors retain the additional ethanolamine phosphate groups that are added during GPI biosynthesis (Canivenc-Gansel et al., 1998
; Flury et al., 2000
).
We considered the possibility that the A. fumigatus GPI anchors might contain galactofuranose substituents because this sugar occurs linked to mannan chains with similarity to the GPI structure in A. fumigatus galactomannans (Latgé et al., 1994) and because it has been described in the N- and O-linked oligosaccharides of Aspergillus glycoproteins (Buitrago et al., unpublished data; Takayanagi et al., 1994
; Haido et al., 1998
; Wallis et al., 2001
). The acid-labile galactofuranose residues are known to be labile to the full 48% aqueous HF dephosphorylation conditions used in this study (Turco et al., 1989
). Therefore, a mild aqueous HF treatment (using 25% aqueous HF for 24 h, data not shown) that retains a substantial proportion of galactofuranose residues was also investigated. However, the amino-bonded phase HPLC profiles of 2-AB-labeled GPI glycans prepared in this way were identical to those shown in Figure 3, suggesting that galactofuranose is not a component of A. fumigatus GPI anchors. This is also in agreement with the lack of immunoreactivity of the five GPI-anchored proteins with a galactofuranose-specific mono-clonal antibodies (data not shown) (Stynen et al., 1992
).
The data provided here on the mature GPI anchor structures of A. fumigatus provide a framework for probing the pathway of GPI biosynthesis in A. fumigatus that is presently unknown. From a structural point of view, it seems likely that the A. fumigatus GPI pathway will be similar to that of S. cerevisiae in that the GPI glycans contain a minimum of four Man residues and the principal lipid is a ceramide instead of a glyceride.
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Materials and methods |
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Protein solubilization and purification
Membrane preparations (30 ml at 20 mg protein/ml) were centrifuged at 50,000xg for 40 min at 4°C. The membrane pellet was first resuspended with a Dounce homogenizer in 40 ml of 50 mM TrisHCl, 2 mM EDTA, 20% glycerol, pH 8.8, with 5 mM HgCl2, two anti-protease pastilles (Complete anti-protease cocktail, Roche, Meylan, France) for 10 min on ice. The mixture was made 2% (v/v) with respect to Triton X100 and mixed in the homogenizer to solubilize membrane proteins for 10 min. Insoluble material was removed by centrifugation (50,000xg for 40 min at 4°C). Soluble material was applied to a Q-Sepharose Fast Flow column (20x1.6 cm, Pharmacia, Orsay, France) equilibrated in 50 mM TrisHCl, 2 mM EDTA, 20% glycerol, pH 8.8, with 0.5 mM HgCl2, 0.05% Triton X100 at a flow rate of 20 ml/h. After washing the unbound compounds, proteins were eluted with an NaCl gradient (0600 mM, 300 ml) in the starting buffer. Proteins were detected with the BCA protein assay kit (Pierce, PerbioSciences, Bezons, France). Fractions from Q-Sepharose chromatography containing GPI proteins were pooled and dialyzed against 20 mM TrisHCl, 1 mM EDTA, pH 7.5, with 0.5 mM HgCl2, 0.05% Triton X100. Proteins were then applied onto an EMD-DEAE-650(S) column (Fractogel-Superformance 150x10 mm, Merck), equilibrated with the same buffer, at 1 ml/min. Bound proteins were eluted with a linear NaCl gradient (0400 mM over 60 min).
SDSPAGE and western blot
Protein samples were analyzed by SDSPAGE (Laemmli, 1970) using a 10% separating acrylamide gels. Protein bands were visualized by staining with Coomassie blue. Gel1p and PhoAp (acid phosphatase) were detected on western blot using specific mouse or rabbit antibodies (Mouyna et al., 2000a
; Bernard et al., 2002
). GPI proteins were detected with an antiserum directed against soluble form of variant surface glycoproteins of Trypanosoma brucei that recognize the CRD epitope formed by the action of (G)PI-PLC on GPI proteins (Zamze et al., 1988
). Protein samples (40 µl) were incubated with 10 µl 200 mM imidazole/acetic acid, pH 7.4, 5 mM dithiothreitol, and with or without 0.2% (v/v) PI-PLC from Bacillus thuringiensis (200300 U/ml, Glyko) for 2 h at 30°C. GPI proteins were subsequently visualized by western blot with the anti-CRD serum.
Isolation of PIs from GPI proteins
Protein samples (12 nmol) were separated by large-scale SDSPAGE, and proteins were transferred onto PVDF membrane and visualized with Ponceau Red staining. GPI proteins were cut out with a razor blade. PVDF membrane strips were washed in Eppendorf tubes with methanol and water. The samples were deaminated by submerging the blot strips in 200 µl of 300 mM sodium acetate, pH 4.0, and an equal volume of freshly prepared 1 M NaNO2 for 23 h at 37°C. The strips were washed three times with water, then PIs were extracted three times with 0.5 ml water-saturated butan-1-ol for 20 min with vortex agitation and for 10 min in an ultrasonic bath. The butanol phases were concentrated under vacuum, and the PIs were repartitioned between 200 µl each butan-1-ol and water. The butanol phase was re-extracted twice with 200 µl butanol-saturated water and dried. The PI extracts were purified by adsorption chromatography on a 100200 µl silica column (Kieselgel 60, 70230 mesh, Merck, Fontenay-sous-bois, France): PI extracts were dissolved in chloroform: methanol (4:1, v/v) and applied to the small silica column equilibrated in the same solvent. After extensive washing, the PIs were eluted with 10 column volumes of chloroform: methanol (1:4 v/v). The eluate was dried and redissolved in chloroform:methanol (2:3 v/v) immediately prior to ES-MS analysis.
Isolation of the GPI glycan moiety
Protein samples (around 0.5 nmol) were separated by SDSPAGE, transferred onto a PVDF membrane, and visualized with Ponceau Red. After cutting out the protein bands of interest, the labeling and release of GPI glycans was performed as previously described (Zitzmann and Ferguson, 1999; Zitzmann et al., 2000
). Briefly, samples were deaminated and the free reducing end 2,5-AHM residue thus formed was labeled by reductive amination with 2-AB (Signal Labeling Kit, Glyko, Bicester, UK). The 2-AB-labeled glycans were released from the protein (and thus from the PVDF membrane) by dephosphorylation with ice-cold 48% aqueous HF treatment for 3 days. The aqueous HF reagent was removed by freeze-drying (three times).
HPLC of 2-AB-labeled GPI glycans
2-AB-labeled GPI glycans were analyzed on an amino-bonded phase column (3 cmx2.1 mm, Kromasil, Hitchrom, Theale, UK) and detected with a Gilson (model 121) fluorescence detector. Oligosaccharides were separated using the following conditions: flow 0.2 ml/min; buffer A, 95% acetonitrile; buffer B, 15 mM ammonium acetate in 5% acetonitrile. Gradient: 05 min, isocratic (100% buffer A); 525 min, linear gradient (100% A, 0% B to 70% A, 30% B); 2570 min, linear gradient (70% A, 30% B to 30% A, 70% B). 2-AB-labeled GPI glycans isolated from several T. brucei variant surface glycoproteins were used as standards.
Enzymatic digestion of 2-AB-labeled GPI glycans
Enzymatic digestions were done with exo--mannosidase activities. Samples were dried and resuspended in 10 µl of 100 mM ammonium acetate buffer at the optimum pH of each respective enzyme: nonspecific
-mannosidase from jackbeans (0.5 mU, optimum pH 5.5, Calbiochem, Nottingham, UK),
1-2-mannosidase from Aspergillus saİto (2 µU, optimum pH 5.0, Glyko),
1-2,3-mannosidase from Xanthomonas manihotis (10 U, optimum pH 6.0 with 5 mM CaCl2, New England Biolabs, Hitchin, UK), or
1-6-mannosidase from Xanthomonas manihotis (10 U, optimum pH 5.0, New England Biolabs). Reactions (37°C, overnight) were stopped by addition of 60 µl of ethanol, dried under vacuum, dissolved in 6 µl of water, and analyzed by HPLC on the amino-bonded phase column, as already described.
Permethylation of 2-AB-labeled GPI glycans
Samples were dried, redissolved in 50 µl dimethylsulfoxide, and treated with 50 µl of a 120 mg/ml slurry of NaOH in dimethylsulfoxide (20 min). Two aliquots (10 µl) of methyl iodide were added at 10-min intervals. The reaction was quenched by the addition of 15 µl acetic acid, 0.25 ml chloroform, and 1 ml water. The lower chloroform phase was washed four times with 1 ml water, dried, and redissolved in 80% acetonitrile, 0.5 mM sodium acetate.
ES-MS
PI samples were introduced into the electrospray source of a Micromass Quatro triple-quadrupole mass spectrometer at 6 µl/min in chloroform:methanol (2:3, v/v). Negative ion ES-MS spectra were recorded with a capillary voltage of 3.0 kV and a cone voltage of 50 V. Negative daughter ion ES-MS-MS spectra of [M-H]- pseudomolecular ions of PIs were recorded with argon as the collision gas (2.5x10-3 Torr) and 60 V collision energy.
Native 2-AB-labeled GPI glycans were introduced into the nano-electrospray source of a Micromass Q-Tof2 mass spectrometer via a nanotip in 50% acetonitrile, 1% formic acid. Positive ion ES-MS and ES-MS-MS spectra were recorded with a tip voltage of 950 V and cone voltage of 40 V. The collision energy for ES-MS-MS was 40 V.
Permethylated 2-AB-labeled GPI glycans were introduced into the nano-electrospray source of a Micromass Q-Tof2 mass spectrometer via a nanotip in 80% acetonitrile, 0.5 mM sodium acetate. Positive ion ES-MS and ES-MS-MS spectra were recorded with a tip voltage of 950 V and cone voltage of 40 V. The collision energy for ES-MS-MS was 80 V.
Peptide analysis
Coomassie bluestained GPI protein bands, isolated by SDSPAGE, were excised from the gel. In-gel digests were done with bovine trypsin. Samples were desalted, and peptide masses were analyzed by MALDI-TOF MS (Shevchenko et al., 1996). In addition, internal peptides obtained by reverse-phase HPLC after tryptic digestion were sequenced on an Edman microsequencer (Applied Biosystem 470 gas-phase sequencer) following the procedure described in Beauvais et al. (1997)
. Analyses were performed by J. D'Alayer (Laboratoire de microsequencage, Institut Pasteur, Paris). MALDI-TOF and Edman sequencing data were matched against the NCBInr and the Genome Therapeutics Corporation Pathogenome databases using the MS-Fit and MS-Edman programs (assembled into the Protein Prospector package, Baker, and Clauser), respectively. These protein identifications were performed by J. M. Bruneau (Aventis-Hoechst Marion Roussel, Romainville, France).
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Acknowledgements |
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1 To whom correspondence should be addressed; e-mail: tfontain{at}pasteur.fr
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Abbreviations |
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References |
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