Departments of Medicine and Cellular and Molecular Medicine and 3Glycobiology Research and Training Center, Howard Hughes Medical Institute, University of California San Diego, La Jolla, CA 92093-0687, USA
Received on October 27, 1999; revised on January 18, 2000; accepted on January 28, 2000.
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Abstract |
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Key words: glycan/mice/glycosyltransferase/NMR
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Introduction |
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N-Glycans are grouped into high mannose, complex, and hybrid types (Furukawa and Kobata, 1992; Varki and Freeze, 1994
; Stanley and Ioffe, 1995
), with ß-GlcNAc branches in complex N-glycans giving di- or multi-antennary units (Schachter, 1991
). Vertebrate O-glycans include seven or more different core structures (Schachter and Brockhausen, 1992
), and are often found in clusters on polypeptides called mucins (Verma and Davidson, 1994
; Devine and McKenzie, 1992
; Rose, 1992
; Strous and Dekker, 1992
). Cells may also contain lipid-linked oligosaccharide precursors from the N-glycan and GPI-anchor biosynthesis pathways (Ferguson, 1992
; Furukawa and Kobata, 1992
; Burda and Aebi, 1999
). Neutral and acidic GSLs can have a variety of extensions arising from the Glc-Cer or Gal-Cer core regions (Hakomori, 1990
; Zeller and Marchase, 1992
; Sandhoff and Klein, 1994
; Karlsson, 1995
). While core regions are unique for each class, elongation can involve similar outer chains. For example, N- and O-glycans and GSLs often carry subterminal Galß14GlcNAcß1- (so-called LacNAc) units, which can sometimes be repeated (polylactosamines), or less commonly, Galß13GlcNAcß1- or GalNAcß14GlcNAcß1- (so-called LacdiNAc) units (Smith et al., 1992
; Baenziger, 1996
). Some of these units are capped by sialic acid (Sia), Fuc,
-Gal, or ß-GlcA (Chan et al., 1991
; Jungalwala, 1994
; Varki and Freeze, 1994
). Further diversity arises from modifications like sulfation (Smith et al., 1992
; Hooper et al., 1996
) and variations of Sia structure (Troy, 1992
; Varki, 1992
; Rutishauser, 1996
; Kelm and Schauer, 1997
). GPI-anchors can also carry various side chain substituents, including phosphoethanolamine units, Man, GalNAc, or Gal residues, or even sialylated LacNAc units (Ferguson, 1992
). The outer regions of proteoglycans (Margolis and Margolis, 1993
; Hascall et al., 1994
; Salmivirta et al., 1996
) are unbranched GAG chains, which are polymers of a disaccharide with a hexosamine and a uronic acid (GlcA or IdoA), or in the case of KS, Gal. With the exception of HA, such GAG disaccharides can be O-sulfated at various positions. In HS, some GlcNAc residues are N-de-acetylated or N-sulfated (Salmivirta et al., 1996
).
Since glycans are involved in interactions with the environment, other cells or bioeffectors (Rademacher et al., 1988; Ferguson, 1992
; Varki, 1993
; Hakomori, 1990
; Schnaar, 1994
; Stanley and Ioffe, 1995
; Baenziger, 1996
; Crocker and Feizi, 1996
; Gahmberg and Tolvanen, 1996
; Rutishauser, 1996
; Dennis et al., 1999
; Reuter and Gabius, 1999
), their isolation and structural characterization are of great interest. However, there is limited information about the glycan repertoire of whole cells, tissues, and physiological fluids. Indeed, most reported structures of vertebrate N- and O-linked glycans have been from readily accessible sources such as mucins, plasma glycoproteins or erythrocytes. Recently, intact mammalian tissues such as brain and lung have been submitted to total N-glycan release, aiming to generate "tissue oligosaccharide libraries" (Wing et al., 1992
; Norgard-Sumnicht et al., 1995
; Fujimoto et al., 1999
). In two instances (Wing et al., 1992
; Norgard-Sumnicht et al., 1995
), such libraries included many unexplained anionic molecules. Thus, the oligosaccharide repertoire of mammalian organs may be even more extensive than summarized above. Investigators who study intact tissues typically focus on a specific class of glycans, and methods for their isolation and purification usually discard the other classes (Kobata and Furukawa, 1992
; Hascall et al., 1994
; Rudd and Dwek, 1997
; Geyer and Geyer, 1998
). In some situations, it would be desirable to isolate all glycan chains of all major groups of glycoconjugates in parallel. Examples are mice (Marth, 1994
) or cell lines (Esko, 1991
; Stanley, 1992
) with genetically engineered defects in glycosylation. To compare such mutants to the wild-type situation we have developed a "Glycan Isolation Protocol" for the isolation and fractionation of all major classes of glycans from vertebrate cells or tissues, and a novel nano-NMR approach to analyzing complex glycan mixtures. These approaches have been applied here to analyze tissues from two types of mice with genetically induced changes in glycosylation.
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Results and discussion |
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Mixtures of 2 to 3 glycans have been previously examined by NMR for full structural characterization (see, for example, Spellman et al., 1989, 1991; Watson et al., 1994
), but only when complete separation had not been possible. The larger the number of component glycans in a mixture, the less information can be gained about each individual component. On the other hand, global structural information about the presence of certain epitopes and their relative ratios in a mixture of glycans should be attainable from the spectra of mixtures. For example, we reasoned that it should be possible to obtain partial structural information from 1H-NMR spectra of whole complex mixtures of N- and O-glycans, particularly in cases where the purpose is to compare two closely related glycoprotein/glycopeptide samples. To deal with the issue of limited amounts of glycan samples, we used nano-1H-NMR spectroscopy (at 500 MHz) which we have shown previously (Manzi et al., 1995
) to be capable of improving sensitivity up to 10-fold over conventional, 5 mm probe NMR at the same magnetic field strength. To test the concept, we initially studied bovine fetuin, a well-known glycoprotein with at least 30 structurally unique N- and O-glycan chains that have been extensively studied by many laboratories using diverse analytical methods (Baenziger and Fiete, 1979
; Nilsson et al., 1979
; Takasaki and Kobata, 1986
; Green et al., 1988
; Hardy and Townsend, 1988
; Cumming et al., 1989
; Hermentin et al., 1994
; Ishii-Karakasa et al., 1997
; Kotani and Takasaki, 1997
; Chen et al., 1998
; Mechref and Novotny, 1998
). We obtained whole mixtures of N- and O-glycans from fetuin (Sigma) via automated hydrazinolysis in the N- and O-mode, followed by re-N-acetylation and clean-up. Starting from 2 mg of fetuin, the typical yield was ~100 µg of mixed N- and O-glycans. Figure 1 shows the spectrum obtained when this glycan mixture was analyzed by nano-probe 1H-NMR spectroscopy at 500 MHz. The presence and relative abundance of certain structural elements could be assigned from the structural reporter group signals that remained individually observable, despite the complexity of the mixture. The following structural features could be confidently assigned: (1) the overall ratio of Sia
23Gal versus Sia
26Gal structural elements was determined to be 2:1, by integration of the triplets corresponding to H3ax of
23 and
26 Sia, at
1.80 and 1.72, respectively, and independently of the H3eq signals at
2.76 and 2.67, respectively; (2) the ratio of di-antennary versus tri-antennary N-glycans was estimated to be 1:3, based on the relative intensities of the Man H2 signals at
4.25 and 4.21, respectively; (3) Fuc, in either
16 or
13 linkage to GlcNAc residues or
12 linkage to Gal residues was undetectable, by virtue of the absence of Fuc CH3 signals in the 1.17<
<1.28 region; (4) Neu5Gc was not present, as judged from the absence of the typical, sharp CH2 singlet at
4.114.12 (see below); and finally, (5) the apparent ratio of N- to O-glycans was found to be 3:1, based on integration of the H1 doublets of the
-anomers of the reducing-end GlcNAc and GalNAc residues at
5.18 and 5.21, respectively. (To reconcile this with the theoretical ratio of 1:1, it is not sufficient to just take into account that the ratios of
:ß anomers for N- and O-glycans are 67:33 and 55:45, respectively (Herlant-Peers et al., 1981
; Spellman et al., 1991
); it is likely that the relative yield of intact O-glycans in the automated hydrazinolysis procedure was lower than that of the N-glycans). On the other hand, the spectrum did not give unambiguous evidence regarding the occurrence of the Neu5Ac
26(Galß13)GlcNAc structural element, which is known to be present in a small proportion of the triantennary N-glycans (Green et al., 1988
; Cumming et al., 1989
); nor was it possible to distinguish between Sia
23Galß13 and Sia
23Galß14 elements, or between Sia
26Gal and Sia
26GalNAc units. The NMR parameters for each of the aforementioned elements are known to be unique (Vliegenthart et al., 1982
; Bernard et al., 1983
; Lecat et al., 1984
; Green et al., 1988
), yet their differences are apparently too subtle to be observable in the spectrum of this mixture. Nonetheless, the data indicate that, at the level of glycan complexity present in a glycoprotein like fetuin, it is possible to study a whole mixture of N- and O-glycans by 1H-NMR spectroscopy and obtain substantial structural information.
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The Glycan Isolation Protocol described here comes close to satisfying these criteria. The overall scheme is outlined in Figure 2, and described in detail under Materials and methods. It involves the initial extraction of GSLs and other glycolipids (along with phospholipids and sterols), SDS-mediated solubilization and subsequent proteolysis of denatured glycoproteins and proteoglycans, recovery of GPI-anchors as lipid-linked glycopeptides, and finally, the separation of N- and O-glycan containing glycopeptides from high-charge GAG-containing glycopeptides. Glycans from each fraction can subsequently be released and profiled, and selected components of each can be subjected to detailed analysis. Along the way, fractions containing low-molecular-weight molecules like monosaccharides, sugar nucleotides, free oligosaccharides, and small glycopeptides can be saved separately. Certain variations and optional extensions of the protocol are feasible (see Figure 3). As described below, the approach was validated using a set of radiolabeled standards representing each of the major classes of glycans to be separated from each other. First, we will briefly outline the rationale for the major decisions taken in setting up the approach.
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Separating protein- or lipid-bound glycans from soluble glycans.
Cells and body fluids contain pools of monosaccharides, sugar phosphates and sugar nucleotides and occasionally, free glycans. Such small molecules are best removed or separated from protein-bound glycans prior to protease treatment, either by dialysis using a large molecular weight cut-off (MWCO) membrane, or by membrane ultrafiltration. We found no difference between conventional dialysis and ultrafiltration on membrane cartridges for elimination of small molecules, or for the subsequent separation of small glycopeptides from the larger species (see below). Ultrafiltration is advantageous as the initial step when analyzing biological fluids that contain free oligosaccharides (e.g., milk) allowing them to be recovered in a reasonable volume for further fractionation and analysis. Likewise, during isolation of small O-type glycopeptides after the proteolysis step, it is convenient to have them recovered in the small volume obtained by ultrafiltration. If recovery of either of these low-molecular-weight fractions is not of interest, conventional dialysis is simpler, albeit with greater risk of accidental sample loss.
Approaches for glycopeptide production. To obtain reliable separations based on intrinsic properties of the glycans, the size of attached peptide needs to be minimized. Initial experiments using mouse brain or kidney as carriers for radiolabeled standards indicated similar effectiveness of Proteinase K and Pronase, as long as SDS was used to ensure complete solubilization. Recombinant Proteinase K was adopted since, unlike Pronase, it has no contaminating enzymatic activities. In the absence of SDS, complete solubilization of the proteins denatured by organic extraction was difficult. Also, while recovery and distribution of N- and O-glycans from a standard glycoprotein ([3H-sialyl]fetuin) was good even without SDS, radiolabeled GPI-anchor glycopeptides and mucin-type glycopeptides were recovered in the wrong fractions (data not shown). The poor recovery of GPI-anchor glycopeptides in the acidic organic extract is probably because attached proteins could not be completely digested without SDS denaturation.
Essentially complete solubilization of the delipidated samples was observed with 1% SDS for all cells and tissues studied. Furthermore, SDS could be effectively removed as a potassium salt precipitate after proteolysis. We did explore alternatives to SDS such as reduction-alkylation with dithiothreitol followed by iodoacetamide. While subsequent GPI extraction after proteolysis occurred at acceptable levels, the recovery of the 35S-labeled GAG-type glycopeptides was surprisingly reduced, evidently due to a ~20% loss of sulfate esters. Although this was not observed with dithiothreitol alone, it was not practical to maintain a reducing agent throughout the protocol (including the DEAE column elution). Also, random exposure to an oxidizing environment could allow artifactual disulfide bond formation between free thiols. Finally, the reducing agent could not be easily eliminated from the fraction containing the small O-type glycopeptides. For all these reasons, reduction alone or reduction-alkylation were not viable alternatives or adjuncts to denaturation of nonreduced proteins by SDS. Of course, reduction-alkylation could always be done on the isolated DEAE glycopeptide fractions of interest at the end, if this were necessary to optimize certain separations.
Recovery and distribution of sialic acids and other monosaccharides in different fractions obtained using the optimized protocol.
To demonstrate the feasibility and efficacy of the approach, we studied two types of tissues from the mouse: brain (a "soft" tissue, very rich in lipids) and kidney (a "hard" tissue, enriched in epithelial cells and extracellular matrix). The optimized protocol was applied to such samples, and aliquots obtained at each step (see Figure 2) were monitored for total Sia content (by the DMB-HPLC assay after saponification of O-acetyl esters and mild acid hydrolysis). Aliquots of the final fractions were also subjected to strong acid hydrolysis and studied for monosaccharide content by HPAEC-PAD (this was not feasible with some of the less pure intermediate fractions, because of interfering impurities). Representative results of these analyses are shown in Tables I and II. The distribution of Sias, neutral monosaccharides and hexosamines was generally appropriate for the predicted composition of the individual fractions. Because of the sensitivity of the DMB-HPLC assay and the lack of interference by other molecules, routine monitoring of Sia recovery was most useful to ascertain protocol reproducibility at different steps. Overall glycan recoveries from the starting homogenate ranged from 4585%, with improved recoveries typically seen after an operator had gained experience with the protocol.
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Recovery and distribution of standard glycoconjugates submitted to the optimized protocol. Bovine fetuin (which contains various kinds of sialylated O-glycans and N-glycans) was radiolabeled in the Sia side chains via mild periodate/NaB[3H]4 reduction, and then either subjected directly to automated hydrazinolysis for release of glycans, or mixed with unlabeled brain tissue homogenate and put through the optimized protocol, followed by automated hydrazinolysis of the glycopeptide fractions. As expected, essentially all of the glycans were recovered either in the second ultrafiltration (SLMW3, the small O-glycans, containing ~1/3 of the recovered radioactivity), or in the fraction eluted with 100 mM NaCl from DEAE (GP0100, comprising the remainder of the O-glycans and all the N-glycans, containing the remaining ~2/3 of the recovered radioactivity). The combined HPAEC profile of recovered glycans was similar to that of the starting material, indicating no major selective loss or structural change of any of the N- or O-glycans during the process (data not shown).
To directly monitor the recovery of individual classes of glycans in the presence of total tissue materials, 10,000 c.p.m. of radiolabeled standards representing each major class of glycan (see Materials and methods) were added to separate aliquots of the minced tissues (4070 mg wet weight brain/aliquot, 3560 mg wet weight kidney/aliquot), and the mixtures were submitted to the optimized protocol. As shown in Table III, the distribution of radioactivity indicates a reasonable recovery of the standards in the expected fractions, with relatively little cross-contamination (some differences in relative distribution do occur, depending upon whether the "carrier" tissue is brain or kidney). An exception was that a portion of the mucins were recovered in the GP1001000 fraction, instead of the GP0100 fraction. This is presumably because the clustered O-linked glycans on the mucins have a charge density similar to that of the GAGs (this problem can be partly alleviated by adding a 300 mM NaCl elution step prior to the 1 M NaCl step, see Figure 2, and below). The lowest yield was seen for the GPI anchors, where about ~50% of the starting material was found in the SLE fraction. However, this is not much worse than the yield obtained using the conventional protocol (extraction with Triton X-114) for isolating these glycans (~70% in our hands, data not shown). We also noted that the standard 3H-labeled GAGs derived from CHO cells (namely, CS and HS glycopeptides) underwent some degradation during the protocol. As shown in Table III, ~20% of the radioactivity was found in the PLMW10 fraction, instead of in the GP1001000 fraction as expected. This is not an artifact due to the quality of the standard or to fragmentation occurring during the homogenization (based on control data with pure standards, not shown). Thus, significant degradation had occurred during the short period of time after mixing the standard into the minced tissue, and prior to adding organic solvent (typically 510 min), presumably due to endogenous GAG-degrading enzymes. We have not pursued this matter further, but it indicates that endogenous glycan-degrading enzymes must be considered, especially at the early stages of the protocol.
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Contamination of the various fractions by other cellular constituents. Various low-molecular-weight components of cells (salts, nucleotides, amino acids, etc.) are recovered during the initial ultrafiltration/dialysis step and/or in the PLE fraction along with the monosaccharides, sugar nucleotides, and small free oligosaccharides. Very hydrophobic proteins (so-called "proteolipids") might be found in the PLE fraction. Except for regions carrying clustered O-linked chains, all remaining water-soluble polypeptides are completely digested by Proteinase K after boiling in SDS. Of course, small portions of peptide remain attached to the GPI-anchors and to the N- and O-glycans and to GAG chains. Most of the cellular phospholipids and neutral lipids are found in the initial organic extract, and the remainder are recovered in the second acidic organic extraction (as detected by HPTLC, data not shown). Fortuitously, all of the nucleic acids were recovered in the SLE (secondary lipid extract; see Figure 4), presumably because the acidification of the extraction mixture protonates the phosphodiester bonds in DNA and RNA. Regardless of the reason, the extraction of nucleic acids at this step assures that they do not contaminate the GAG chains, which are recovered later with a high salt elution from the DEAE column.
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Profiling of released oligosaccharides. Various profiling methods were used to monitor the success of the protocol (see Materials and methods). In the remainder of this paper, we will focus mainly on profiling the N- and O-glycans of mouse tissues. Optimization and automation of hydrazinolysis has allowed uniform and simultaneous release of both N- and O-linked glycans in acceptable yield (Patel et al., 1993). HPAEC is a suitable profiling strategy for such free N- and O-glycans derived from the low-charge (GP0-100) glycopeptide fraction, since even isomeric forms differing in only one linkage can be resolved from each other (Hardy and Townsend, 1994
). Indeed, as shown in Figure 5, the purity of the N- and O-glycans released from this fraction by automated hydrazinolysis is sufficient to obtain a clean HPAEC-PAD profile that is relatively reproducible from preparation to preparation. Also, different tissues give markedly different profiles of released oligosaccharides.
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Section 3. Application of the glycan isolation protocol to transgenic mice
Analysis of glycans from mice with a null mutation in the ST6Gal-I sialyltransferase. Following disruption of a gene encoding a specific glycosyltransferase in intact mice, the question arises if the predicted change in glycosylation does indeed occur in the genetically altered animal. The failure to find the predicted change in glycosylation in a particular tissue would indicate the presence of other enzymes capable of producing the same structure, while a complete loss of the pertinent structural element would prove that the gene deleted is the only one capable of biosynthesizing it in the tissue/cell type being examined. For example, the genetic disruption of the then only known ß-galactosyltransferase (Asano et al., 1997; Li et al., 1997
) did not result in elimination of all ß-Gal residues (Kotani et al., 1999
), because of the existence of several additional isoforms of this enzyme (Lo et al., 1998
). Furthermore, since most major glycoconjugate classes are synthesized in the Golgi-ER pathway and compete for the same sugar nucleotide pools, the question arises if unexpected changes occur in other classes of glycans. The protocol described above is presented as a first step towards addressing these issues.
ST6Gal-I (CMP-Sia:Galß14GlcNAc 26 sialyltransferase) is the only mammalian enzyme currently known to generate the Sia
26Gal linkage and its minimally required acceptor is Galß14GlcNAcß (Tsuji, 1996
). Despite the widespread constitutive or regulated expression of ST6Gal-I in various cell types (O'Hanlon et al., 1989
; Wang et al., 1989
; Jamieson et al., 1993
; Lo and Lau, 1996
) the phenotypic consequences of ST6Gal-I disruption in the mouse appeared to be limited to B cells, which also appeared to lose expression of the Sia
26Gal glycan structural element as determined by loss of binding by Sia specific lectins (Hennet et al., 1998
). It is conceptually possible that there are other ST6Gal enzymes in other tissues and cell types, transferases that could partly or fully compensate for the lack of ST6Gal-I expression. To ascertain the occurrence of glycans terminating in Sia
26Gal in tissues other than B-cells, we studied the GP0100 and GP100300 fractions derived from the liver, brain, and kidney of normal and ST6Gal-I null (homozygote and heterozygote) mice. Since these fractions contain many structurally distinct glycans, they were not amenable to fractionation and purification of each individual component. However, as shown in Figure 7, 1H-NMR analysis of the glycopeptide mixtures present in the GP0100 fractions of normal and mutant mouse liver indicated that the ST6Gal-I deficient mouse tissue lacks any detectable
26 linked Sia, whereas
23 and
26 linked Sia in the corresponding glycans from control tissues occur in the ratio of approximately 1:1. Not only do these fractions represent mixtures of many glycans (more than 50, as seen by HPAEC-PAD of these fractions after hydrazinolysis), they contain the glycans in peptide-bound form. Despite the added complication posed by the presence of amino acid signals in the 1H-NMR spectra, the relatively narrow line width and the characteristic patterns and well-defined positions of Sia H3ax and H3eq signals in the spectra enabled us to establish the presence of Sia
23Gal and Sia
26Gal units. Furthermore, it was possible to come to this conclusion with only ~200 g of the glycopeptide mixtures. Indeed, removal of the peptide portions by automated hydrazinolysis and sample clean-up gave glycan mixtures that did not give better quality spectra by 1H-NMR spectroscopy. Furthermore, the loss of glycan material during hydrazinolysis was ~50%, and the removal of 1H containing contaminants was apparently incomplete. The NMR spectra of the liver GP100300 fractions (not shown) revealed the same trend as those of the GP0100 fractions: no Sia
26 was detectable in the material from ST6Gal-I null mice, whereas the spectrum of the wild-type material showed a minor proportion (~5%) in
26 linkage. The 500 MHz 1H-NMR spectra of the GP0100 fractions from kidney and brain tissue (not shown) gave the same result as with liver. Taken together, these data indicate that ST6Gal-I is responsible for generating most or all of the Sia
26Gal residues on N- and O-glycans in these tissues of normal mice (the lower limit of sensitivity for detection of
26 linked Sia is 23% compared to the level of
23 linked Sia). Thus, direct 1H-NMR analysis of complex mixtures of glycans can be an adequate tool to assess changes in the levels of specific Sia units in sialyltransferase-null mouse tissues, and to measure the relative ratios of sialic acids in different types of linkages.
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The approach has some minor disadvantages and limitations. First, the whole process takes about one week, and involves many steps. However, up to eight samples can be processed in parallel, and there are large time gaps between steps, allowing the operator to pursue other activities in parallel. Second, the glycoproteins and proteoglycans are recovered as an SDS extract, and are therefore not suitable for isoelectric focusing or functional studies. However, prior to proteolysis, the extract is suitable for analysis by SDS-PAGE, and for antibody or lectin blotting studies. Third, some highly acidic GSLs may be recovered in the fraction meant to contain only GPI-anchor glycopeptides, and there is the potential for methyl esterification of sialic acids under these acidic conditions, in the presence of methanol. However, the fraction of such molecules is relatively small in most tissues, and other methods can be used to differentiate them from the GPI-anchors. Fourth, the use of exhaustive proteolysis limits the subsequent use of some N-glycanases which require some length of amino acids adjacent to the linkage region. Finally, the DEAE column gives incomplete separation of mucin glycopeptides from some GAG glycopeptides. However, as discussed earlier, a variety of nondegradative and degradative techniques can be used to achieve the desired separations.
Our immediate purpose in developing this approach was to study the outcome of genetic modulation of glycosyltransferases in mice. Given the rapid progress in identifying the genes encoding the glycosyltransferases, some might argue that it would be simpler to examine the expression pattern of their messenger RNAs as a means towards profiling glycosylation potential. However, there is now increasing evidence that expression of mRNA does not always correlate with the levels of a functional protein present in a given cell type (Page et al., 1999). In the case of glycosylation, even a direct measurement of glycosyltransferase activity is not sufficient. Unlike the synthesis of RNA and proteins, glycosylation is not exclusively template driven, and one cannot accurately predict the glycosylation phenotype of a given tissue or cell type from patterns of glycosyltransferase activity expression. For example, even though GlcNAcT-IV activity is barely detectable in rat liver, many of the major serum glycoproteins produced by the rat hepatocyte have multiantennary N-linked chains that include the ß14 branch synthesized by this enzyme (Schachter, 1991
). Likewise, the ratio of
23 to
26 linked sialic acids was only moderately altered in cytokine-activated endothelial cells, despite a >10-fold increase in activity of the sialyltransferase ST6Gal-I that attaches
26 linked sialic acids (Hanasaki et al., 1994
). Thus, to accurately reveal the glycosylation potential of a given tissue or cell type, there appears no viable alternative to the extraction and direct glycoprofiling of the expressed glycans.
Studies of nucleic acids and proteins can now be done at a whole cell or whole organ level, with gene-chip arrays and 2-D gel based proteomics (Page et al., 1999) providing a global overview of the expression of the genome and the status of the "proteome." Here we have made some early steps towards what might be eventually called "glycomics," i.e., elucidating the complete repertoire of glycan structures in a given cell-type or tissue. Obviously, much work is first needed to resolve the practical limitations in the protocol described here and in effectively profiling the resulting glycan fractions. It is possible that at least some of the steps could be automated. The approach might also be appropriately adapted or modified for other types of biological samples, e.g., insects, plants, and microbes. The potential applications of this approach are many, including the comparison of tissues between populations of a single species, between closely related species, between normal and disease states (e.g., cancer, inflammation), between cell lines with changes in glycosylation, in exploring genetic diseases of humans involving glycosylation and following genetic manipulation of glycosylation in intact cells or animals. We have demonstrated here two examples of the last situation. In each case, we were able to obtain the sought-after information simply by HPAEC-PAD profiling and/or nano-1H-NMR spectroscopy of whole mixtures of N- and O-glycans. In the first case (ST6Gal-I deficiency) we show an essentially complete absence of the enzyme product in the N- and O-glycopeptides from several tissues. In the other case (polypeptide GalNAcT-8 deficiency), we saw little loss of expression of mucin-type O-glycans, corroborating that there are several other enzymes capable of synthesizing the GalNAc-O-Ser/Thr linkage. The clear biological phenotype of the ST6Gal-I null mouse (Hennet et al., 1998
), and the lack of an obvious phenotype in the other case (Hennet et al., 1995
) now make more sense.
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Materials and methods |
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Radiolabeled standards
Radiolabeled variant surface glycoprotein labeled in the GPI-anchors by [3H]ethanolamine was a kind gift from Kojo Mensa-Wilmot (University of Georgia) (Mensa-Wilmot et al., 1994). Synthetic (O-GlcNAc-)YSDSPSTST (Reason et al., 1991
) with a ß-linked [6-3H]Gal residue attached to GlcNAc was kindly provided by Bradley Hayes and Gerald Hart (Johns Hopkins University). CMP-[9-3H]sialic acid and lactose were incubated with recombinant soluble
23 sialyltransferase (ST3Gal-III, kindly provided by Eric Sjoberg, Cytel Corp., San Diego) to enzymatically generate 3'[3H]sialyllactose, and the product was isolated by gel filtration essentially as described previously (Beyer et al., 1981
).
Fetuin was radiolabeled in its Sia moieties by mild periodate oxidation followed by reduction with NaB[3H]4 (Van Lenten and Ashwell, 1971). Briefly, bovine fetuin (100 µg) was dissolved in a minimal volume of freshly made 2 mM sodium metaperiodate in phosphate-buffered saline (PBS) and allowed to react on ice, in the dark, for 15 min. A 100-fold molar excess of glycerol was added, and incubation continued for 2 h. The oxidized fetuin was dialyzed (MWCO 1000) against water, recovered by lyophilization, dissolved in 1020 l 10 mM NaOH and a 4-fold molar excess of NaB[3H]4 in dimethyl formamide (10 µl) was added. After 13 h at RT, reduction was completed with a 20-fold molar excess of NaBH4. Excess reducing agent was quenched with acetone (10-fold molar excess relative to NaBH4) for 2 h at RT. The labeled fetuin was reisolated from the void volume of a Bio-Gel P-2 column eluted with 50 mM sodium acetate (pH 5.5), dialyzed (MWCO 1000) against 50 mM sodium acetate (pH 5.5) and then against distilled water. The sample was lyophilized and kept at 20°C until use. The uniform radiolabeling of all N- and O- sialyloligosaccharides was confirmed by releasing them via automated hydrazinolysis (see below), followed by HPAEC monitored by scintillation counting. The profile obtained was similar to that of larger amounts of unlabeled fetuin subjected to the same process and detected by PAD.
Disialoganglioside GD1a (Matreya) was radiolabeled in its Sia moieties as described above for fetuin, except that purification from by-products was done by repeated evaporation with acidified methanol, followed by reverse-phase chromatography on a Sep-Pak C18 cartridge. The sample was loaded in water, the cartridge was washed with water and methanol, and [3H]GD1a eluted with chloroform. Further purification was achieved by HPLC on an Iatrobead 6RS 8010 (10 µm) column (4.6 x 500 mm), eluted with a linear gradient consisting of chloroform/methanol/water from 53:42:5 to 48:42:10 (v/v) over 60 min. The double peak (corresponding to two different acyl chain lengths of the sphingosine moiety) was pooled, dried, dissolved in water, dialyzed against water (MWCO 3500) at 4°C overnight, lyophilized, and kept at 20°C until use.
Tritium and 35S-labeled HS- and CS-GAG glycopeptides were prepared by a modification of a previously described method (Bame and Esko, 1989). Briefly, CHO-K1 cell monolayers (4 P-100 plates) were metabolically radiolabeled with [6-3H]GlcN (100 µCi/plate) in glucose-depleted media (glucose at 0.1 g/l final10% of normal concentration) for 4 days, or with [35S]sulfate (100 µCi/plate) in sulfate-depleted media with normal glucose concentration (1 g/l), 10 mg/l of cysteine (1/10 of normal concentration), and 3 mg/l methionine (1/5 of normal concentration) (Norgard-Sumnicht and Varki, 1995
). Serum (10%) was present during the labeling (dialyzed in the case of the sulfate-depleted media). Labeled cells were washed three times with cold PBS, solubilized with 1 ml per plate of 100 mM NaOH at RT for 20 min, the extract was combined with the original labeling media, and the pH adjusted to 7.0. Proteinase K was added at a final concentration of 2 mg/ml and the mixture incubated at 50°C overnight. The samples were then diluted with water to a salt concentration of 100 mM or lower (checked with a Vapor Pressure Osmometer, 5500XR, Wescor, calibrated against standard solutions). The sample was applied to a 2 ml DEAE-Sephacel column and washed with 30 column volumes of 100 mM NaCl, 20 mM TrisHCl, pH 7.4. The HS- and CS-GAGs were eluted with 4 column volumes of 1.0 M NaCl, 20 mM TrisHCl, pH 7.4, and dialyzed against water in MWCO 3500 dialysis tubing.
Tritiated mucin was prepared from one P-100 plate of LS180 human colon carcinoma cells metabolically radiolabeled in Dulbeccos Modified Eagles Medium with 20% fetal calf serum for 3 days with 1 mCi of [6-3H]GlcN. The media containing shed mucins and GAGs was treated with a mixture of chondroitinase ABC (200 mU) and heparinase II (1.25 U) in 50 mM Tris acetate, 2.5 mM CaCl2, pH 6.9 overnight at 37°C. The sample was adjusted to 100 mM NaCl and then loaded onto a 2 ml Jacalin agarose column at 4°C, and the flow was stopped overnight. The column was then washed with 20 ml of 10 mM TrisHCl, 100 mM NaCl, 1 mM CaCl2, 1 mM MgCl2 (pH 7.5), and bound O-glycosylproteins eluted with 4 column volumes of 100 mM melibiose in the same buffer. The eluate was repeatedly dialyzed against water (MWCO 3500) at 4°C, lyophilized, dissolved in 100 µl of 100 mM TrisHCl buffer (pH 7.4) and treated with Proteinase K (final concentration 2 mg/ml) overnight at 50°C. After boiling for 10 min, mucin-type glycopeptides were fractionated on a Sephacryl S-200 column (10 ml) in 10 mM ammonium acetate. The largest mucin glycopeptides running in the void volume were pooled and used as a mucin standard.
Non-protein-bound GPI (GIPL) from Trypanosoma cruzi (Y-strain) (Carreira et al., 1996) was a kind gift from Lucia Mendonca-Previato (Universidade Federal do Rio de Janeiro, Brazil). The GIPL (200 µg) was treated with 20 mM metaperiodate in 100 mM sodium acetate buffer (pH 5.5) for 10 min on ice to oxidize between C-5 and C-6 of the galactofuranosyl moiety. The excess reagent was consumed by adding ethylene glycol. After 30 min, the reaction mixture was desalted by microdialysis (MWCO 1000) and dried before reducing with NaB[3H]4 (25 mCi) in 10 mM NaOH. The reaction was terminated with a 10-fold excess of unlabeled NaBH4, the excess reagent was consumed with glacial acetic acid, and methyl borate eliminated by repeated evaporation with acidified methanol. The radiolabeled GIPL was recovered by binding to a Sep-Pak cartridge and elution with chloroform/methanol.
Concurrent isolation of different classes of glycans from cells and tissues
A detailed Glycan Isolation Protocol for preparation of different classes of glycans from cells or tissues is described below. Samples are used fresh or immediately frozen upon collection and stored at 80°C until processed. As described in the companion paper (Norgard-Sumnicht et al., 2000) the protocol is also applicable to cultured cells, which are first pelleted and washed three times with ice-cold PBS to remove any serum components from the culture media. Body fluids (e.g., plasma), can also be processed according to the protocol, after partial concentration by lyophilization to obtain a protein concentration of up to 200 mg/ml. For convenience, the individual steps of the protocol are presented in sequential days. All procedures are carried out in glass tubes, or in the presence of detergent, until the samples are free of any lipid material. Lipid-containing fractions are stored in glass tubes, and other samples may be stored in plastic vials. Figure 2 outlines the overall approach, and also presents the nomenclature and abbreviations used to identify the individual fractions.
Day 1
After thawing and removal of loosely attached connective tissue, the weight of the tissue sample is determined (or the volume of the cell pellet is measured). Optimal starting amounts are ~250500 µg/ul. The tissue is finely minced, and the sample is transferred into a conical glass tube of appropriate volume.
Extraction of lipids. Lipids are extracted at RT in six sequential steps, with 20 volumes of chloroform/methanol (2:1, 1:1 and 1:2, v/v, each done twice), using a Polytron homogenizer (Brinkmann Instruments, Westbury, NY), applying 35 bursts of 515 s each, at 4050% of the maximum power, to ensure a uniform suspension at each step. After the first homogenization in chloroform/methanol 2:1 (v/v), an aliquot (2% of the total volume) of the "Total Homogenate" (TH) suspension may be set aside for protein, neutral/amino sugar and Sia analyses, or ß-counting (as appropriate), and stored at 20°C until analyzed (see "Options" section in Results and discussion). After each extraction step, the organic supernatant containing the lipid material is recovered by centrifugation at 1500 r.p.m. for 10 min and transferred with a glass (Pasteur) pipette into a 15-ml glass tube with a Teflon-lined screw cap. To remove any residual chloroform/methanol from the pellet (containing proteins, including glycoproteins and proteoglycans, and also nucleic acids), a final extraction step is done with 5 volumes of 95% ethanol. After removal of the ethanol, the final pellet is not allowed to dry out, but immediately hydrated in 0.5 ml of 1% (w/w) SDS in 100 mM TrisHCl (pH 7.4), and kept at 20°C overnight (except when the appearance of a non-pelletable, gel-like substance is observed; see "Options" section in Results and discussion for degradation of this gel by DNase-I). If cultured cells grown in a monolayer are being studied (see Norgard-Sumnicht et al., 2000, the following article), the extracellular matrix may be extracted from the culture plate with 1% SDS in 100 mM TrisHCl (pH 7.4), and added to the pellet obtained after the primary lipid extraction. Meanwhile, the organic extracts are combined and evaporated to dryness, either under vacuum or under a stream of nitrogen gas. The residue is dissolved in chloroform/methanol 2:1 (v/v) (~2 ml/100 mg of initial wet tissue or 2 ml/100 µl cell pellet) and the solution is stirred at 4°C overnight.
Day 2
Recovery of coextracted glycoproteins from the organic extract.
After stirring overnight, the organic extract is centrifuged at 1500 r.p.m. for 10 min, and the supernatant is transferred into a 15 ml glass tube with a Teflon-lined screw cap. The residue is washed with 95% ethanol, centrifuged once again, and the supernatant is pooled with the previous one. The combined organic extracts constitute the "Primary Lipid Extract" (PLE); after evaporation of the organic solvents, the PLE is stored in dry state at 20°C until further use (see "Options" section below).
Solubilization of glycoproteins and proteoglycans. The pellet left behind in the "recovery" step is promptly hydrated in a small volume of 1% SDS in 100 mM TrisHCl (pH 7.4), and combined with the main glycoprotein/proteoglycan containing fraction obtained on Day 1. The volume of the suspension is increased by addition of 1% SDS in 100 mM TrisHCl (pH 7.4), to 2 ml/100 mg of starting wet tissue. The sample is then boiled at 100°C for 1520 min to dissolve as much of the residue as possible. The tube is vortexed vigorously before and after heating, to ensure that no denatured (glyco-)protein material remains attached to the wall of the tube. The pH of the solution is verified to remain in the 7.07.5 range. The resulting denatured material is labeled the "Total Protein" (TP) fraction (see Figure 2). An aliquot (2%) of TP may be set aside for protein and carbohydrate analyses (see "Options" section).
Removal of small molecules. The denatured protein sample is centrifuged at 1500 r.p.m. for 15 min, to precipitate any insoluble material. The supernatant is removed for filtration, while the precipitate is washed with a small volume of 100 mM TrisHCl (pH 7.4), recentrifuged, with the secondary supernatant being used in the later stages of the filtration (the precipitate is saved for a following step). The supernatant is transferred into a 10,000 MWCO Centricon 10 or Centriprep 10 filtration unit (Amicon, Beverly, MA), chosen according to the wet weight of the starting tissue material (i.e., under 200 mg, and between 200 and 500 mg, respectively). For a typical TP solution with a volume of 15 ml, centrifugation is done at just under 3000 x g, in three steps of 40, 10 and 5 min, with collection of the filtrate (containing various types of low-molecular weight material) after each step. To maximize the efficiency of removal of the small molecules, the concentrated retentate is then diluted with 100 mM TrisHCl (pH 7.4) (and/or the secondary supernatant from the recentrifugation of the pellet; see above) to the maximum volume that the unit will hold, and subjected to repeated centrifugation. All filtrates are collected and pooled. The combined Centricon/Centriprep 10 run-through fraction (called PLMW10) contains sugar nucleotides, free monosaccharides, small oligosaccharides, and other cellular small molecules. PLMW10 is lyophilized and stored at 20°C. If the low-molecular-weight compounds are not of interest, a 12,000 MWCO dialysis tubing can be used as an alternative to the Centricon or Centriprep unit; dialysis against 400 volumes of 100 mM TrisHCl (pH 7.4) at 4°C overnight (followed by one additional dialysis for 4 h under the same conditions) will retain the glycoproteins/proteoglycans, free of small saccharides and sugar nucleotides.
Preparation of glycopeptides. The retentate in the Centricon/Centriprep (or the solution inside the dialysis tubing) is mixed with the precipitate left behind in the above centrifugation step of the TP solution in SDS and Tris buffer, and the total volume is brought back up with 100 mM TrisHCl (pH 7.4) to 2 ml/100 mg of wet tissue (since all of the originally added SDS is retained during ultrafiltration, this maintains the concentration of SDS at or below 1%); when using dialysis instead of a filtration unit, the volume typically recovered is a bit larger than 2 ml/100 mg wet tissue. An aliquot of the total protein extract may be saved at this point if it is desirable to study the intact glycoproteins/proteoglycans, or to use PNGases or endoglycosidases to specifically release N-glycans (see "Options" section below). The bulk of the solution is subjected to proteolytic digestion by adding 1/10th volume of Proteinase K (Gibco BRL, Gaithersburg, MD, 20 mg/ml in 50 mM TrisHCl, 2 mM calcium acetate, pH 8), to obtain a final concentration of ~2.0 mg/ml. Incubation is at 50°C overnight.
Day 3
A second aliquot of Proteinase K (at a final concentration of 2 mg/ml) is added in the morning of Day 3, and incubation continues for 8 h. The sample is then heated at 100°C for 15 min to inactivate Proteinase K, and subsequently cooled and centrifuged at 1500 r.p.m. for 10 min. If any insoluble material is left at this stage, the pellet may be saved and subjected to carbohydrate analysis (minor amounts of residue were obtained when extracting tissues with high matrix content such as the kidney, and compositional analysis revealed only traces of carbohydrate).
Day 4
Separation of O-GlcNAc-Ser/Thr and/or other small Ser/Thr-linked O-linked glycans from larger glycopeptides. The Pro- teinase K-digest supernatant is transferred into a 3000 MWCO Centriprep 3 or Centricon 3 unit and centrifuged at just under 3000 x g, in three steps (of 95, 35, and 10 min, respectively, for a volume of 15 ml) with removal of the filtrate after each step. The final retentate is diluted once more by adjusting the volume with 100 mM TrisHCl buffer (pH 7.4) to the original volume, and recentrifuged. The combined filtrates containing O-GlcNAc-Ser/Thr and/or other short Ser/Thr-linked oligosaccharide chains are lyophilized and stored at 20°C until analysis or further fractionation. This secondary low-molecular-weight fraction (SLMW3) is expected to also contain all released amino acids, including any modified amino acids such as tyrosine sulfate, and any small peptides having molecular weights of less than 3000. If none of the small glycopeptides are of interest, a 3000 MWCO dialysis tubing can be used as an alternative to the Centricon or Centriprep unit, dialyzing against 400 volumes of 100 mM TrisHCl (pH 7.4) at 4°C for at least 72 h.
Precipitation of SDS. The final retentate from the Centriprep/Centricon unit (or the dialysis bag) is transferred into a glass tube capable of withstanding centrifugation forces greater than 12,000g (e.g., a Corex No. 8441 tube). It is diluted with 100 mM TrisHCl (pH 7.4) to a volume of 23 ml. A saturated KCl solution (1% of the original volume of the SDS solution used for denaturation at the beginning of Day 2) is added and the solution is kept at 4°C overnight.
Day 5
The insoluble K-SDS is pelleted in the Corex tube by centrifugation at 10,000 r.p.m. for 20 min (~12,000 x g), and the supernatant is transferred into a clean glass tube.
Separation of GPI anchors. GPI-anchored glycopeptides and any remaining GSLs which failed to enter the PLE fraction (i.e., highly charged GSLs or GSLs originally trapped in the tissue matrix) are extracted from the aforementioned supernatant with chloroform/methanol/1 M HCl (65:35:1, v/v) using a volume equal to that of the sample. The phases are separated by centrifugation (at 1500 r.p.m. for 15 min at RT). The lower (organic) phase contains GPI-anchored glycopeptides and any remaining GSLs, and the upper (aqueous) phase contains all other glycopeptides. Depending on the absolute volume(s) of aqueous (and organic) solvent(s) used, i.e., on the salt concentration of the starting supernatant, an inter-phase emulsion appears more or less clearly observable during the extraction process; it is taken together with the upper phase and treated as part of the main aqueous phase. The pH of both phases is checked with pH paper, and adjusted to 7.4 if necessary (with 1020 µl aliquots of 1 M NaOH). The aqueous phase is transferred into another glass tube, and the organic extraction is repeated. The two organic phases are then pooled, constituting the Secondary Lipid Extract (SLE); it is dried and kept at 20°C until further analysis. It is noteworthy that this SLE fraction contains the nucleic acids in addition to GPI-anchored peptides (see below).
Days 56
Separation of high-charge GAG and mucin-type glycopeptides from N- and O-type glycopeptides. The aqueous phases from the previous step are pooled (the GPU fraction, Figure 2), diluted with an equal volume of water (to decrease the salt concentration to less than 100 mM), and then applied to a DEAE-Sephacel column equilibrated in 100 mM NaCl in 20 mM TrisHCl (pH 7.4) (1 ml of column volume per 100 mg wet weight of starting tissue or 100 l cell pellet) (Bame and Esko, 1989). The initial run-through is reapplied to the column, which is then eluted with 30 column volumes of the equilibration buffer. The total 100 mM NaCl eluate is collected; this fraction (GP0100) contains primarily the low-charge N- and O-type glycopeptides. Elution of the high-charge glycopeptides (mostly GAGs and clustered O-linked glycans from mucin regions resistant to the protease) is accomplished with 10 column volumes of 1 M NaCl in 20 mM TrisHCl (pH 7.4), resulting in the GP1001000 fraction. As discussed in the "Options" section (see Results and discussion), the latter step may be split into two stages: elution with 10 column volumes of 300 mM NaCl in 20 mM TrisHCl (pH 7.4) to selectively elute most of the mucin glycopeptides in GP100300, followed by a 1 M NaCl elution (as mentioned above) for collection of the GAG-type glycans in GP3001000.
Days 69
Desalting of glycopeptides. Salts are removed from the glycopeptides in fractions GP0100 and GP1001000 (c.q. GP100300 and GP3001000) by extensive dialysis against water at 4°C using 1000 MWCO tubing. If hydrazinolysis is planned, frequent changes of the water are required to achieve a final salt concentration of less than 5 nM. Samples are lyophilized and stored at 20°C until analysis.
Monitoring the fractionation process
Qualitative and quantitative recoveries for each step in the Glycan Isolation Protocol were monitored by analyzing aliquots for monosaccharide composition (by acid hydrolysis, followed by HPAEC-PAD), total Sia content (by the thiobarbituric acid colorimetric assay and/or by weak acid hydrolysis followed by DMB derivatization and HPLC analysis with fluorescence detection), total neutral sugar content (by the phenol/sulfuric acid assay), total protein content (by the Bio-Rad assay), the presence of peptides (by amino acid analysis), and (when applicable) radioactivity arising from internal standards. For the thiobarbituric acid, phenol/sulfuric acid and Bio-Rad assays, conventional spectrophotometric absorbance readings were replaced by analyzing 200 µl of the reaction mixture in a 96-well quartz plate, using a plate reader.
Monosaccharide composition analysis by high-pH anion-exchange chromatography with pulsed amperometric detection (HPAEC-PAD)
Aliquots of Glycan Isolation Protocol fractions were hydrolyzed with 2 M TFA (sequencing grade) at 100°C for 4 h, cooled down, dried in a Speed-Vac (Savant Instruments, Holbrook, NY), dissolved in water, and transferred into autosampler vials for injection onto a CarboPac PA-1 column (4 x 250 mm) (Dionex Corporation, Sunnyvale, CA). Elution was performed with sodium hydroxide (16 mM, isocratically) for neutral and amino monosaccharide composition analysis (or 2 mM sodium hydroxide, isocratically, for the specific purpose of separating xylose and mannose). For uronic acid analysis, samples were hydrolyzed for 6 h, under otherwise identical conditions. Elution of a uronic acid containing hydrolyzate on CarboPac PA-1 utilized 16 mM sodium hydroxide, isocratically for 24 min (as for neutral and amino monosaccharide analysis), followed by 100 mM sodium hydroxide with a gradient of sodium acetate, from 20 to 200 mM over 45 min, allowing the separation of the uronic acids. Calibration of retention times on the CarboPac PA-1 column and of PAD molar response factors was based on analysis of mixtures of monosaccharide standards exposed to the hydrolysis conditions detailed above.
Determination of total Sia content
Sias were released by hydrolysis after saponification of O-acetyl esters, derivatized with DMB and analyzed by reverse-phase HPLC on a TSK-Gel ODS-120T 5 µm column (4.6 mm x 25 cm) (Tosohaas, Montgomeryville, PA) as described (Manzi et al., 1990). DMB derivatives were eluted with acetonitrile/methanol/water (either isocratically, 9:7:84, v/v (Diaz et al., 1989
), or with a linear gradient from 7:7:86 to 11:7:82, v/v), at a flow rate of 0.9 ml/min for 40 min.
Release of N- and O-glycans from glycopeptides by automated hydrazinolysis
Since many inorganic anions and cations can interfere with hydrazinolysis, glycopeptide samples were extensively dialyzed (see Days 69) against water at 4°C using 1000 MWCO tubing. Salt-free samples (GPU, GP0100, GP100300) were transferred into clean glass reactor vials and lyophilized for at least 24 h at <50 millitorrs. The vials from the lyophilizer were immediately placed on the ports of an automated hydrazinolysis instrument (GlycoPrep 1000, Oxford GlycoSciences, U.K., up to 2 mg of starting material per vial). Operating conditions were selected for release of N- and O-glycans (hydrazine reaction at 95°C for 4 h) or only O-glycans (hydrazine reaction at 65°C for 5 h), as required. After the hydrazinolysis reaction and built-in purification (~1624 h), the released glycans were filtered through 0.5 µm PTFE filters (Oxford GlycoSciences) to remove silica gel particles, and lyophilized. The products were used as such for HPAEC-PAD glycan profiling (see below). However, prior to 1H NMR spectroscopy, further clean-up over an activated charcoal filter was necessary (see below).
HPTLC profiling of neutral GSLs and gangliosides
The PLE fraction (obtained in dry state at the end of Glycan Isolation Protocol Day 1) was dissolved in a minimal volume of chloroform/methanol 2:1 (v/v); methanol and water were then added to attain a final ratio chloroform/methanol/water of 2:43:55 (v/v). Any insoluble material was precipitated by centrifugation. The solution was loaded three times onto a prewashed Sep-Pak C18 cartridge, which was then washed with water (10 ml), and eluted with methanol (2 ml), chloroform/methanol 2:1 (v/v, 5 ml), and chloroform (5 ml) (Schnaar, 1994). The methanol and chloroform/methanol eluates were pooled and dried under a stream of nitrogen gas. Under these conditions, the methanol and chloroform/methanol eluates contained all GSLs, as judged from Sia and neutral/amino monosaccharide analyses. After evaporation of the solvents, the GSLs were profiled by HPTLC, as follows. Glass-coated Silica Gel-60 HPTLC plates (10 x 10 cm) (Merck; Darmstadt, Germany) were activated for 20 min at 110°C. An aliquot of the GSL sample (corresponding to 25 nmol Sia) was spotted on two different plates and developed in chloroform/methanol/0.02% aqueous CaCl2 (60:40:9, v/v, for optimal separation of gangliosides) and chloroform/methanol/water (10:10:3, v/v for neutral GSLs) (Schnaar and Needham, 1994
). Neutral and anionic GSLs were detected by spraying the plate with orcinol-sulfuric acid, while gangliosides were detected with resorcinol-HCl-Cu2+ (Schnaar and Needham, 1994
). Radiolabeled GSLs were detected by fluorography after spraying the HPTLC plate with En3Hance (DuPont-New England Nuclear, Boston, MA).
Release of glycans from GSLs by endoglycoceramidase
Prior to enzymatic release of the oligosaccharides, the PLE fraction was enriched in GSLs, either by chloroform/methanol extractions as described above (see HPLTC profiling), or by Folch partitioning (Smith, 1996). The latter procedure involved dissolving the PLE in chloroform/methanol 2:1 (v/v) (0.5 ml/100 mg tissue) in a glass tube, adding 0.1 M aqueous KCl (20% of the total volume), vortexing and centrifuging at 1500 r.p.m. for 15 min. The resulting upper (aqueous) phase was transferred into another glass tube, and the lower (organic) phase was extracted twice more with methanol/0.1 M aqueous KCl (1:1, v/v), under centrifugation at 1500 r.p.m. The upper phases, containing the GSLs with glycans consisting of 4 or more monosaccharide units, were pooled, washed with chloroform/methanol 2:1 (v/v), and eventually diluted with methanol/water (1:1, v/v). The compositions of the upper and lower phases were monitored by HPTLC and DMB Sia analysis (see above). After desalting over a prewashed Sep-Pak C18 cartridge (with salts being eluted by water, GSLs by chloroform/methanol 1:1 followed by chloroform/methanol/water 4:8:3), the GSL-containing solution was evaporated to dryness.
The GSLs, dissolved in 50 mM sodium acetate buffer (pH 5.0), were subjected to endoglycoceramidase digestion, in the presence of sodium cholate (at a final concentration of 0.75 mg/ml, thoroughly pre-mixed with the sodium acetate buffer), at 37°C for 48 h under toluene atmosphere (Ito and Yamagata, 1989; Miller-Podraza et al., 1993
). The progress of the digestion was monitored by HPTLC. The reaction mixture was extracted with 5 volumes of chloroform/methanol 2:1 (v/v). The phases were separated by centrifugation at 1500 r.p.m. for 15 min. The organic phase was washed twice with 3 volumes of water, and all aqueous phases were pooled. After washing once more with chloroform/methanol 2:1 (v/v), the aqueous phase was lyophilized. Desalting and removal of other noncarbohydrate contaminants was achieved by applying the sample (in 12 ml of water) to a GlycoClean H charcoal cartridge (Oxford GlycoSciences) (for details, see section on "NMR spectroscopy"). Essentially, after elution of non-carbohydrate contaminants by 5% acetonitrile/water, the glycans were eluted quantitatively by 50% acetonitrile/water and recovered in dry state by evaporation. The mixture of GSL-derived oligosaccharides was analyzed by 1H NMR spectroscopy and HPAEC-PAD profiling.
Oligosaccharide mapping by HPAEC-PAD
Aliquots of free oligosaccharides produced by hydrazinolysis or endoglycoceramidase digestion were analyzed by HPAEC-PAD (Hardy and Townsend, 1994) on a CarboPac PA-1 column (4 x 250 mm). A Dionex DX500 HPLC system equipped with UV and PAD detectors and an AS3500 ThermoSeparations autosampler were used; data acquisition and processing was controlled by Dionex PeakNet software (version 5.1, running under Windows 95 on an Intel Pentium MMX PC). Elution of glycan mixtures with 1 to 4 or 5 negative charges per molecule (i.e., typical anionic N- and O-glycans from glycoproteins/glycopeptides and oligosaccharides from gangliosides) was achieved using a 60 min linear gradient of sodium acetate (20250 mM from 5 to 65 min) with a constant concentration of sodium hydroxide (100 mM), and maintaining the 250 mM concentration of acetate for another 25 min. For separation of neutral oligosaccharides, a shallower linear gradient was employed (240 mM sodium acetate in 100 mM sodium hydroxide for 40 min). The column was calibrated with glycoprotein and glycolipid derived standards of known structure, run under the same conditions.
Analysis of GAG constituents among the high-charge glycopeptides
The presence and type of GAGs in the highest-charge DEAE fractions (GP1001000 or GP3001000) were assessed using a cocktail of GAG-degrading enzymes. Samples were dissolved in 50 mM Tris-acetate, 100 mM NaCl, and 2.5 mM CaCl2 (pH 6.9), incubated with keratanase II (100 mU), chondroitinase ABC (50 mU), chondroitinase AC (25 mU), and heparin lyase II (156 mU) at 37°C for 34 h, and the reaction mixture boiled for 15 min to inactivate the enzymes. A Superose-12 HR 10/30 FPLC column (Pharmacia, Uppsala, Sweden) was used to size both undigested and digested products. The column was run isocratically in 100 mM NaCl/20 mM MOPS (pH 7.4), containing 1 mM CaCl2, 1 mM MgCl2, and 0.02% sodium azide. A Pharmacia FPLC system (P-LKB-pump P-500; P-LKB-controller LCC-500 Plus) was used to elute the column at 0.4 ml/min flow rate. Fractions were collected directly into scintillation vials; 4 ml of scintillation fluid was added, and the radioactivity was determined in a ß-counter.
NMR spectroscopy of glycan mixtures
Oligosaccharide mixtures released from peptides by automated hydrazinolysis or from sphingolipids by endoglycoceramidase digestion (see above) were further purified over GlycoClean H charcoal cartridges (Oxford GlycoSciences). Briefly, GlycoClean H cartridges were prewashed with 1 M sodium hydroxide, water, 30% acetic acid and water (3 ml each), and then conditioned with 50% acetonitrile/water/0.1% TFA (3 ml) and 5% acetonitrile/water/0.1% TFA (6 ml). The glycan sample was applied (in less than 1 ml of aqueous solution), and salts and other hydrophilic contaminants washed off the cartridge with water (3 ml), followed by 5% acetonitrile/water/0.1% TFA (3 ml). Glycans were eluted with 50% acetonitrile/water/0.1% TFA (4 portions of 0.5 ml each) and recovered by evaporation, while contaminants remained bound to the charcoal. Specifically, this procedure effectively removed contaminants that would be detrimental to 1H-NMR analysis, namely, di-N-acetylhydrazine, a by-product of hydrazinolysis that is not removed by the GlycoPrep built-in automated clean-up procedure, and also sodium cholate and sodium acetate from endoglycoceramidase digests. Glycan samples were repeatedly exchanged in D2O (99.96%, Sigma/Aldrich, St. Louis, MO) with intermediate lyophilization, finally dissolved in 40 l of 99.996% D2O (Cambridge Isotope Laboratories, Andover, MA), and transferred into a 40 µl nano-cell (Varian, Palo Alto, CA). 1H-NMR spectra were recorded on a Varian Unity Inova 500 MHz spectrometer, equipped with a Varian 1H nano-NMR probe and controlled by a Sun Microsystems Sparc 5 computer, running VNMR software (version 5.3 B). NMR spectra were obtained in 100010,000 scans using presaturation of the HDO resonance by a low-power transmitter pulse, at spin rates of 1.52.0 kHz. Line broadening (by 0.20.5 Hz) of the spectra was applied in data processing before Fourier transformation. Chemical shifts are given relative to 4,4-dimethyl-4-silapentane-1-sulfonate (DSS); they were typically measured relative to the residual free acetate peak ( 1.908 p.p.m. at 2230°C and pD 68).
Options, variations, and extensions of the glycan isolation protocol (see also Figure 3)
1. Early removal of DNA.
Tissues (and cells) rich in DNA can pose the following problem. At high concentrations, DNA presents itself as a gel which would not solubilize when boiling the residue from the organic extract in 1% SDS (day 2). This gel also interferes with the subsequent ultrafiltration step(s). The problem can be circumvented using DNase-I to degrade the DNA gel-like material before hydrating the protein pellet in SDS in TrisHCl at the end of Day 1. Optimization of this step is currently being pursued.
2. Subfractionation of GSLs. The GSLs in the PLE can be further purified by using various previously described methods (Hakomori and Siddiqui, 1974), including Folch partitioning, fractionation into gangliosides, GIPLs and neutral lipids by DEAE chromatography, etc. Note that the PLE also contains the bulk of the cellular cholesterol, sphingomyelin and phospholipids. If labile O-acyl groups and GIPLs are not of interest, the phospholipids can be destroyed by base hydrolysis (Hakomori and Siddiqui, 1974
).
3. Release of glycans from GSLs by endoglycoceramidase. GSL-specific endoglycoceramidases (Ito and Yamagata, 1989; Miller-Podraza et al., 1993
) can be used to release the oligosaccharide portion from GSLs (see Materials and methods). Once recovered, these glycans can be profiled or fractionated (with or without tagging), and structurally characterized, as indicated below for the N- and O-glycans.
4. Release of N-glycans from denatured glycoproteins by endoglycosidases.
N-glycans in the delipidated SDS-solubilized extract can be released from proteins by a variety of endoglycosidases (endoH, endoD, endoF13) or peptide:N-glycosidases (PNGaseF or PNGaseA) (Maley et al., 1989; Plummer and Tarentino, 1991
). Most of these enzymes can be used despite the presence of SDS, provided that the SDS concentration is appropriately adjusted and/or an appropriate ratio of non-ionic detergent is added (Maley et al., 1989
; Plummer and Tarentino, 1991
). The released oligosaccharides can be recovered by gel filtration or other methods.
5. Subfractionation of free oligosaccharides and sugar nucleotides. These molecules found in the first ultrafiltration (PLMW10) can be further fractionated by various techniques (Maley et al., 1989; Plummer and Tarentino, 1991
; Strecker et al., 1992
; Chaturvedi et al., 1997
). If quantitative recovery is important, it should be noted that a portion of these molecules can enter the PLE fraction, and need to be recovered by ultrafiltration or dialysis.
6. Recovery and analysis of small O-type glycopeptides. The O-linked GlcNAc and other small glycopeptides (including a portion of the mono- and di-sialylated glycopeptides) are recovered in the second ultrafiltration (SLMW3) and can be studied by methods such as galactosyltransferase-catalyzed labeling with UDP-[3H]Gal (Greis et al., 1996) followed by ß-elimination, or by mass spectrometry after separation from free amino acids and other proteolysis products.
7. Release of glycans from GPI-anchors. The SLE contains the bulk of the GPI anchors, with short residual peptides attached to the ethanolamine residue in their core structure. The GPI-anchors can be cleaved by GPI-specific phospholipases or the glycans can be released by de-acylation, nitrous acid deamination, and HF treatment (Norgard-Sumnicht et al., 2000, following article). The released glycans can be profiled, fractionated, or analyzed as needed (Ferguson, 1992
).
8. Subfractionation of DEAE-bound glycopeptides and oligosaccharides by charge characteristics. The high-charge fraction from the DEAE column (GP1001000) comprises a mixture of HA, mucin fragments resistant to further proteolysis, and KS, CS and HS glycopeptides. These components can be partially separated by selective salt elutions and/or pH shift elutions from DEAE (e.g., a 300 mM NaCl elution prior to the 1 M NaCl step will recover most mucin-type glycopeptides). If there is great complexity, gradient elution from a DEAE-HPLC column and/or electrophoretic techniques can be used to fractionate them on the basis of differing charge density.
9. Subfractionation of DEAE-bound glycopeptides or free oligosaccharides by lectin affinity chromatography. Affinity chromatography methods (e.g., jacalin sepharose for binding mucins, columns of heparin-binding proteins for certain fractions of HS) can also be useful to achieve further separations.
10. Degradative subfractionation of DEAE-bound glycopeptides and oligosaccharides. Each component within the GP1001000 DEAE fraction could also be recovered by an approach in which the other components are destroyed by specific enzymes. Most mucins could be eliminated by treating with sialidases, and then re-running the DEAE column (this might not work if the mucin is heavily sulfated). Alternatively, the mucins could be recovered intact by treating this fraction with a mixture of broad-spectrum GAG-degrading enzymes. If these degradative procedures are carried out in a sequential manner, the resulting GAG fragments could be isolated by gel filtration and analyzed to ascertain indirectly the general structure of the parent fractions (i.e., percentage of each type of GAG), by identifying the specific disaccharides contained in these fractions.
11. Release and fractionation of N- and O-glycans in the 100 mM NaCl DEAE eluate. The oligosaccharides can be released by manual or automated hydrazinolysis, and then radiolabeled or fluorescently tagged. Subsequent fractionation may employ a variety of techniques, including different types of HPLC and serial lectin affinity chromatography (Varki et al., 1996).
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2 To whom correspondence should be addressed at: CMM-East, Room 1065, UCSD School of Medicine, La Jolla, CA 920930687
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