Abstract
Many of the functional proteins and lipids in HDL particles are potentially glycosylated yet very little is known about the glycoconjugates of HDL. In this study, HDL was isolated from plasma by sequential micro-ultracentrifugation, followed by glycoprotein and glycolipid analysis. N-glycans, glycopeptides, and gangliosides were extracted and purified followed by analysis with nano-HPLC-Chip Q-TOF MS and MS/MS. HDL particles were found to be highly sialylated. Most of the N-glycans (~90%) from HDL glycoproteins were sialylated with one or two neuraminic acids (Neu5Ac). The most abundant N-glycan was a biantennary complex type glycan with two sialic acids (Hexose5HexNAc4Neu5Ac2), and was found in multiple glycoproteins using site-specific glycosylation analysis. The observed O-glycans were all sialylated and most contained a core 1 structure with two Neu5Acs, including those that were associated with apolipoprotein CIII (ApoC-III) and fetuin A. GM3 (monosialoganglioside, NeuAc2-3Gal1-4Glc-Cer) and GD3 (disialoganglioside, NeuAc2-8NeuAc2-3Gal1-4Glc-Cer) were the major gangliosides in HDL. A 60% GM3 and 40% GD3 distribution was observed. Both GM3 and GD3 were composed of heterogeneous ceramide lipid tails, including d18:1/16:0 and d18:1/23:0. This report describes for the first time a glycomic approach for analyzing HDL, highlighting that HDL are highly sialylated particles.
Keywords: HDL, glycomics, glycoproteomics, gangliosides, sialylation, mass spectrometry
Introduction
HDL particles have been considered to be atheroprotective due to their role in reverse cholesterol transport, however, many other functions including toxin binding, antioxidant, anti-inflammatory, antiglycation, antithrombotic, and immunomodulatory functions have recently been described.[1] HDL particles are heterogeneous, and yet the molecular and functional bases behind the large degree of variability among the different classes and subclasses of HDL particles have not been established.[2] A key challenge facing the field of lipoprotein biology is that chemical, compositional, and structural changes can transform atheroprotective HDL into pro-atherogenic, pro-inflammatory particles.[3] Under inflammatory conditions HDL particles are ineffective at reverse cholesterol transport despite high plasma HDL concentrations.[4] The anti-oxidant function of HDL –protection of LDL from oxidation– is impaired in heart disease patients.[5] Dysfunctional HDL with impaired anti-oxidant and endothelial protection are found in type 2 diabetes patients.[6] HDL from patients with cardiovascular disorders are compositionally different from those of healthy individuals.[7, 8] In addition, the antimicrobial, anti-inflammatory, antiglycation, antithrombotic, and immunomodulatory functions of HDL and how these are modified by HDL composition are poorly understood.
As complex multi-molecular aggregates, many of the functional proteins and lipids in HDL are potentially glycosylated. Yet, very little is known about these glycoconjugates of HDL. There is evidence that ApoA-I, A-II, C-I, C-II, and C-III are all glycosylated.[9] Glycosylation of ApoA may be important for the secretion of HDL from the liver[10], and may influence its association/dissociation properties to HDL particles: sialylated ApoA-II associated only with HDL3 whereas non-sialylated ApoA-II associated with HDL of all sizes.[11] Desialylation of ApoE is associated with hepatic steatosis.[12] ApoE Leiden, an aberrantly glycosylated variant of ApoE, shows defective binding to the LDL receptor.[13] Decreased sialic acid in cerebrospinal fluid ApoE was found with aging, and was associated with smaller lipoprotein particle sizes, which may be involved in the formation of amyloid plaque.[14] Loss of sialic acid α2,6-Neu5Ac containing structures in ApoC-III was found in lung cancer patients.[15] Serum amyloid A (SAA), which is released in response to acute phase immune reaction circulates primarily as a constituent of HDL particles.[16] An N-glycosylated form of SAA that is distinct from acute phase SAA has been described.[17] These data suggest important as yet not fully characterized mechanistic links between the glycosylation of HDL-associated glyocoproteins and HDL function. However, the glycosylation of the HDL proteome has not been characterized.
Gangliosides are glycolipids containing sialic acids in their carbohydrate moieties. Bacterial toxins display a heterogeneous specificity of binding to their glycolipid receptors.[18] For example, lactosylceramide and ganglioside GM3 bind several enterotoxigenic strains of E. Coli.[19] Twenty-five percent of serum gangliosides were reported to be associated with HDL in human serum, with a different compositional profile for HDL compared with other circulating lipoproteins (e.g. VLDL and LDL) and serum.[20] However, only limited information is available on the occurrence of these ganglioside species in plasma HDL, and whether and how they vary with disease.
Studies of the HDL proteome have uncovered an array of 110 proteins that are thought to be associated with HDL particles. In fact, it is now thought that different subsets of HDL particles, separated in different ways – ultracentrifugation, electrophoretic migration, immunoaffinity chromatography, size exclusion chromatography, and others – are characterized by different proteomes.[21] However, although the proteins that associate with HDL have been identified and for some of these proteins the glycosylation has been characterized independently, to date, there have been no direct investigations of the overall glycome of HDL.
In this article we describe an analytical strategy that is detailed and quantitative, comprehensively examining the glycan structures on glycoproteins and glycolipids of HDL. Previously, no adequate methods to determine HDL glycan diversity as a whole in a clinically relevant manner existed. Methods for elucidating the complete HDL glycome using a combination of nanoflow liquid chromatography and high performance mass spectrometry for the simultaneous identification and quantification of glycoconjugates in HDL particles are described. On the basis of the glycosylation discovered we propose a new model for HDL as a class of highly sialylated particles.
Experimental Procedures
A comprehensive glycome analysis work-flow is summarized in Figure 1 and described below.
HDL Isolation
Fasting (12 hr) blood samples were obtained from a healthy study participant as part of an ongoing approved protocol to collect fasting plasma from healthy subjects for methods development. Briefly, healthy subjects are recruited on the University of California Davis campus by flyering and announcements at seminars. Subjects are screened for basic eligibility criteria (healthy, able to give blood, and not taking any medications) and provide written informed consent to participate in the study. The Institutional Review Board of the University of California Davis approved the study protocol. The study was conducted according to the principles expressed in the Declaration of Helsinki.
Preparation of HDL was performed by a sequential micro-ultracentrifugation method described by Brousseau et al.[22] with slight modifications. Blood was collected from the antecubital vein into EDTA evacuated tubes, centrifuged immediately (1,300 ×g, 10 min, 4°C), portioned into aliquots, and stored at –80 °C until analyzed. Three thawed replicate plasma samples (0.8ml each as triplicates) were gently overlaid on the KBr solution to avoid the introduction of air. To isolate the combined VLDL and LDL fractions, potassium bromide (KBr) solution (1.1 ml, d = 1.084 g/ml) was transferred into cone-top polyallomer tubes up to the 1.9ml neckline. Ultracentrifugation was performed using a Sorvall RC M120 GX equipped with a S120-AT2 fixed-angle rotor (Thermo Scientific, Waltham, MA, USA) for 2.5 h, 8°C, 435,680 ×g. By this procedure the combined VLDL and LDL fractions with a density lower than 1.060 g/mL were removed from the top of the tubes (0.9 ml) by aspiration using a gel-loading pipette (Rainin, Oakland, CA, USA). The remaining infranate (1.0 ml) was transferred into new cone-top polyallomer tubes. To isolate the HDL fraction, the transferred infranate was overlaid with 0.9ml of KBr solution (d = 1.34 g/ml) and ultracentrifugation was performed (3 hr, 8°C, 435,680 ×g). The HDL fraction (1.2 g/ml-1.063) was identified as the top 0.6ml layer found at the top of the tubes. The HDL fraction was collected from the top of the tube (0.6 ml) and desalted using an Amicon dialysis membrane with a molecular weight cut-off of 3,000 (Millipore, Billerica, MA, USA) in nanopure water (18 Ω), prior to being dried down and reconstituted with 300 μL water.
Density solutions of KBr, at d = 1.084 g/ml and 1.34 g/ml were made weekly and adjusted and verified by measurement using the Densito 30PX portable densitometer (Mettler Toledo, Columbus, OH, USA). Thirteen replicates of plasma samples isolated from fasted and fed healthy human subjects were measured by the Densito 30PX to verify the density of plasma. The mean ± SEM density of the plasma samples was 1.027 ± 0.0005 g/ml.
Glycoprotein Analysis
Tryptic Digestion
100 μL of 50 mM ammonium bicarbonate solution was added to 10 μL isolated HDL, followed by reducing with 5 μL of 550 mM dithiothreitol (DTT) with incubation for 50 min at 60 °C. 10 μL of 450 mM iodoacetamide (IAA) was then added and carboxymethylation was performed by incubation for 20 min at room temperature in dark. Reduced and carboxymethylated HDL was digested using Sequencing Grade Modified Trypsin (Promega, Madison, WI, USA) 2 μL (1 μg/μL) in 100 μL of 50 mM ammonium bicarbonate buffer , for 16 hr at 37 °C. The digests were purified on a reverse-phase cleanup C18 pipette tip (Agilent Technology, Wilmington, DE, USA). The C18 zip-tip was preconditioned successively with acetonitrile (150 μL, 10 times) and water (150 μL, 10 times). The tryptic digest was loaded on to the zip-tip by pipetting 20 times up and down and then washed with water (150 μL) for 10 times. HDL tryptic peptides were eluted with 0.05% formic acid (FA) in 80% acetonitrile (ACN) in water (v/v) (200 μL, 20 times extractions), dried down, and then reconstituted in 20 μL nanopure water.
N-linked Glycan Release and Purification
N-linked glycans were released from 60 μL HDL in 200 μL 100mM ammonia bicarbonate buffer using endoglycosidase PNGase F (New England Biolabs, Ipswich, MA, USA) (2 μL) for 10 min under microwave condition (power 20 W, temperature 60 °C). The released N-glycans were cleaned up via solid phase extraction (SPE) using graphitized carbon cartridges (Grace Davison Discovery Sciences, Deerfield, IL, USA). The glycan digest was loaded on preconditioned graphitized carbon cartridges then washed with 6 mL nanopure water. N-glycans were eluted with 6 mL 0.05% Trifluoroacetic acid (TFA) in 40% ACN in water (v/v), dried down, prior to reconstituted in 20 μL nanopure water for MS analysis.
Pronase Digestion and Glycopeptide Cleanup
100 μg Pronase E was covalently coupled to cyanogen bromide (CNBr) activated sepharose beads (Sigma-Aldrich, St. Louis, MO, USA) via coupling chemistry and as earlier reported in our laboratory.[23-26] 100 μL isolated HDL was added to the Pronase-beads and incubated at 37 °C for 18 h. Pronase would normally digest the glycoproteins to glycopeptides with peptide portion 1-20 amino acids. The glycopeptide digest was desalted and enriched via SPE procedure using graphitized carbon cartridges. Similar as N-glycan cleanup procedure, followed by conditioning the cartridges using acetonitrile and water and loading the digest mix, a clean mixture of glycopeptides were eluted in 9 mL 0.05% Trifluoroacetic acid (TFA) in 40% ACN in water (v/v), dried down, and then reconstituted in 20 μL nanopure water prior to MS analysis.
Ganglioside Analysis
Extraction of Gangliosides
100 μL isolated HDL was mixed with 1 mL water, 2.7 mL methanol and 1.3 mL chloroform and the mixture was shaken vigorously for 5 seconds. After centrifugation at 3,000 g for 5 min, 0.5 mL of water was added for the phase separation. The supernatant was collected. The bottom organic layer was re-extracted using 5 mL of 3:4:8 water/chloroform/methanol (v:v:v) and mixed, and then the supernatants were pooled and dried.
A C8 SPE cartridge (Supelco, Bellefonte, PA, USA) was conditioned with 6mL of 1:1 isopropanol/methanol (v/v) and 1:1 methanol/water (v/v). The sample was diluted with 1mL of 1:1 methanol/water (v/v) and applied on the SPE cartridge. The cartridge was washed with the 9mL of 1:1 methanol/water (v/v) solution to ensure removal of all polar compounds. The gangliosides were eluted by washing 9mL of 1:1 isopropanol/methanol (v/v), and the eluant was evaporated to dryness. The purified sample was stored at −80 °C until analysis.
Instrumentation
A nano-HPLC-Chip Q-TOF instrument using the Agilent 1200 series microwell-plate autosampler (maintained at 6 °C by the thermostat), capillary pump, nano pump, HPLC-Chip interface, and the Agilent 6520 Q-TOF MS (Agilent Technologies, Inc., Santa Clara, CA) was used in this study.
For the tryptic peptide and the ganglioside analyses, a reverse-phase nano-HPLC Chip (G4240-62001, Agilent Technologies, Inc., Santa Clara, CA) with a 40 nL enrichment column and 43 × 0.075 mm ID analytical column was used. The column was packed with ZORBAX C18 (5 μm pore size) stationary phase. The mobile phase for tryptic peptides consisted of 0.1% formic acid in 3% ACN in water (v/v) as solvent A, and 0.1% formic acid in 90% ACN in water (v/v) as solvent B. The mobile phases used for gangliosides were water (solvent C) and 15% isopropanol in methanol (v/v) (solvent D), with both containing 20 mM ammonium acetate and 0.1% acetic acid. The nano pump gradient was performed on the analytical column to separate the tryptic peptides with a flow rate at 0.4 μL /min and the gangliosides with 0.3 μL /min. The peptides were eluted in 45 min with the following gradient: 0% B (0.00-2.50 min); 0 to 16% B (2.50-20.00 min); 16 to 44% B (20.00-30.00 min); 44 to 100% B (30.00-35.00 min) and 100% B (35.00 -45.00 min). The gradient used for gangliosides separation was as follows: 70% of D (0.00-1.00 min); 70 to 80% D (1.00-3.00 min); 80 to 100% D (3.00-40.00 min) and 100% D (40.00-45.00 min). The working samples were dissolved in water/methanol (1:1, v/v).
For the N-glycan and the pronase glycopeptide analysis, an Agilent 6210 HPLC Chip II with a 40 nL enrichment column and 43 × 0.075 mm ID analytical column both packed with porous graphitized carbon stationary phase was used. The mobile phase consisted of 0.1% formic acid in 3% ACN in water as solvent A and 0.1% formic acid in 90% ACN in water (v/v) as solvent B. The nano pump gradient was performed on the analytical column to separate the N-glycans and glycopeptides with a flow rate at 0.4 μL /min. The samples were eluted in 45 min with the following gradient: 0% B (0.00-2.50 min); 0 to 16% B (2.50-20.00 min); 16 to 44% B (20.00-30.00 min); 44 to 100% B (30.00-35.00 min) and 100% B (35.00-45.00 min).
The Agilent 6520 Q-TOF MS was operated in the positive ion mode for MS and MS/MS modes for the tryptic peptides, N-glycans, and pronase glycopeptides. The recorded mass ranges were m/z 500-3,000 for MS only and m/z 50-3,000 for MS/MS. Acquisition rates were 0.63 spectra/s for both MS and MS/MS. For gangliosides, MS was operated in the negative and MS/MS was operated in both positive and negative modes. The recorded mass ranges were m/z 500-2,500 for MS only and m/z 50-1,500 for MS/MS. The drying gas temperature was set at 325 °C with a flow rate of 4 L/min. All mass spectra were internally calibrated using the G1969-85000 ESI tuning mix (Agilent Technologies, Inc., Santa Clara, CA), with reference masses at m/z 922.010, and 1,521.971 in the positive ion mode, at m/z 680.036 and 1279.995 for negative mode.
In MS/MS mode, generally, the collision energies for the tryptic peptides, N-glycans, and pronase glycopeptides were calculated as:
For gangliosides, the data dependent MS/MS analysis was performed with collision energies set at 40V for the negative mode and 80V for the positive mode.
Data Analysis
All tryptic MS/MS data were analyzed using X! Tandem (www.thegpm.org). Trypsin digesion would help ID the HDL associated proteins. X! Tandem was set up to search the Swissprot human complete proteome set database. X! Tandem was searched with a fragment ion mass tolerance of 80 ppm and a parent ion tolerance of 100 ppm. Iodoacetamide derivative of cysteine was specified in X! Tandem as a fixed modification. Deamidation of asparagine and glutamine, oxidation of methionine and tryptophan were specified in X! Tandem as variable modifications
Data analyses for N-glycans, glycopeptides and gangliosides were performed with the MassHunter Qualitative Analysis software ver. B.03.01 (Agilent Technologies, Inc., Santa Clara, CA).
For the N-glycan analysis, within a 20 ppm accurate mass criterion molecular Feature Extraction (MFE) was performed through a mode of the “Find by Molecular Feature” function for non-targeted profiling. The deconvoluted glycan mass, retention time, and the abundance were extracted. The glycan compositions were assigned based on the accurate mass and the corresponding MS/MS data.
Glycopeptide assignments were achieved by the combination of the tandem MS information and the accurate glycopeptide precursor ion mass via in-house software GP Finder. The mass list of the glycopeptides precursor ions was analyzed with accurate mass, protein sequence, biological filters of glycans, and a MS tolerance level (≤20 ppm). The tandem mass spectra were then taken into account for further inspection with glycan and peptide fragmentation patterns with a mass tolerance for fragment ions (≤80 ppm). The unique significance of GP Finder is to use false discovery rate by generating a decoy library to the scoring system and to serve as a more reliable means of making assignments.
For gangliosides, MFE was performed to generate a peak list (m/z, retention time and peak area) taking all ions into account exceeding 1,000 counts. Focused post-processing precursor ion scan analysis was performed through a mode of the “Find by Auto MS/MS”. The NeuAc ions (m/z 290.095) were the fragment ions used to determine the precursor ion masses representing gangliosides.
Results and Discussion
HDL particles remain poorly characterized due to their size, complexity, dynamic nature and large degree of diversity in composition and function. Enabling technologies that can be used to comprehensively analyze these biologically important particles are needed. In particular, very little is known about the biological functions related to the glycosylated components of HDL. This deficiency in understanding the glycobiology of HDL may be critically important since early published evidence indicates that both glycoproteins and glycolipids associated with HDL and their variation in glycosylation patterns may be either mechanistically involved or diagnostic of HDL functions. In this study HDL particles isolated from healthy human plasma were comprehensively examined for their glycan structures and the results lead to a compelling new model of HDL as a class of highly sialylated particles.
Proteomics Analysis
Tryptic peptides were digested from HDL fractions isolated by ultracentrifugation. After high-performance liquid chromatography (HPLC) separation via reversed phase C18 column, the peptides were analyzed by tandem MS. Following database search, 17 proteins were identified shown in Supplemental Table S1 from one replicate as an example. The base −10 log of the expectation that any particular protein assignment was made at random was lower than −2. ApoA-I was observed as the major protein. In humans, about 60% of the protein content in HDL is represented by ApoA-I.[27] Other apoproteins were present, including Apo C-II, C-III, D, E, and M, which are typical minor apoproteins associated with HDL. On the other hand, ApoB-100, the major constituent of VLDL and LDL, was not present. Other proteins known to be associated with HDL were also observed, including acute phase response proteins such as SAA, liver secreted proteins such as alpha-2-HS-glycoprotein (fetuin A), and the key mediators of the complement system C3 inhibitor.[28-31] The proteins associated with HDL isolated from healthy human plasma in this study have all been suggested as HDL-associated proteins in previous studies.[32-35] These results confirmed our HDL isolation approach, and provided a list of proteins for site-specific glycosylation analysis.
Glycans from HDL compositionally profiled by Nano-LC MS
The N-glycans were released using the protocol described in experimental procedures. Analyses were done from the isolated HDL triplicates. The glycan profile of HDL is illustrated with one of the triplicates (Figure 2). The depicted glycan structures were based on biological precedence and their correct masses, however, isomers are putative.[36] HPLC-microchip packed with a PGC stationary phase was used to separate glycans with high sensitivity and reproducibility.[37-40] The total ion chromatogram (TIC) from the raw LC/MS data was separated into a number of extracted compound chromatograms (ECCs). The extractor algorithm was based on the expected charge carriers, potential neutral mass losses, and a predicted isotopic distribution. Each peak represents one compound eluting at certain retention time with the detected m/z, which enables the assignments of glycan composition.
The most abundant glycan (including isomers) was a biantennary complex type glycan with two sialic acids (Hexose5HexNAc4Neu5Ac2). Perhaps not surprisingly, these glycans are also the most abundant in blood.[36] In this regard, HDL-associated proteins are similar to other abundant glycoproteins in blood.[41] Two abundant isomers were observed eluting at retention times 23 min and 25 min. Most of the glycans (90%) from HDL glycoproteins were sialylated with one or two Neu5Ac(s). Ion intensities were measured in the MS mode based on the protonated molecular ion in positive mode (Table 1). Following the most abundant glycan with two Neu5Ac, a complex type biantennary glycan with one Neu5Ac was shown in a high intensity eluting at 17 min – 20 min including four observed isomers. Our group reported glycans with sialic acids retain longer with PGC.[39] Here we also observed that the sole addition of an acidic NeuAc residue increased the retention time by nearly 5 min.
Table 1.
Retention time (min) |
Measured m/z |
Charge state |
Mass error (ppm) |
Hexose | HexNAc | Fucose | NeuAc | Ion Intensity (counts) |
---|---|---|---|---|---|---|---|---|
24.839 | 1112.403 | 2 | 3.57 | 5 | 4 | 0 | 2 | 6091078 |
23.541 | 1112.402 | 2 | 2.94 | 5 | 4 | 0 | 2 | 4906932 |
19.915 | 966.8551 | 2 | 4.13 | 5 | 4 | 0 | 1 | 1196125 |
18.466 | 966.8576 | 2 | 6.78 | 5 | 4 | 0 | 1 | 797081 |
22.675 | 966.8543 | 2 | 3.37 | 5 | 4 | 0 | 1 | 129647 |
17.355 | 966.8556 | 2 | 4.65 | 5 | 4 | 0 | 1 | 78041 |
17.725 | 865.3141 | 2 | 3.12 | 5 | 3 | 0 | 1 | 171480 |
16.31 | 865.3134 | 2 | 2.38 | 5 | 3 | 0 | 1 | 47271 |
24.524 | 1039.883 | 2 | 2.91 | 5 | 4 | 1 | 1 | 141126 |
22.706 | 1039.883 | 2 | 2.99 | 5 | 4 | 1 | 1 | 95666 |
23.434 | 1039.884 | 2 | 3.92 | 5 | 4 | 1 | 1 | 41850 |
20.862 | 1039.878 | 2 | −1.68 | 5 | 4 | 1 | 1 | 19297 |
17.857 | 894.3368 | 2 | 4.97 | 5 | 4 | 1 | 0 | 140215 |
16.374 | 894.3332 | 2 | 0.98 | 5 | 4 | 1 | 0 | 58633 |
15.169 | 821.3112 | 2 | 9.56 | 5 | 4 | 0 | 0 | 93233 |
13.997 | 821.3069 | 2 | 4.31 | 5 | 4 | 0 | 0 | 43677 |
25.483 | 1185.427 | 2 | −0.37 | 5 | 4 | 1 | 2 | 62932 |
19.253 | 784.2855 | 2 | 0.65 | 4 | 3 | 0 | 1 | 55095 |
16.874 | 813.3067 | 2 | 0.92 | 4 | 4 | 1 | 0 | 53118 |
19.206 | 885.8271 | 2 | 2.78 | 4 | 4 | 0 | 1 | 48338 |
17.746 | 885.8248 | 2 | 0.15 | 4 | 4 | 0 | 1 | 24690 |
12.726 | 942.3367 | 2 | 7.5 | 9 | 2 | 0 | 0 | 38575 |
11.579 | 942.3349 | 2 | 5.58 | 9 | 2 | 0 | 0 | 16327 |
23.563 | 1258.465 | 2 | 6.4 | 5 | 4 | 2 | 2 | 37927 |
21.401 | 1076.901 | 2 | 2.33 | 6 | 5 | 1 | 0 | 30048 |
24.534 | 1294.957 | 2 | −5.19 | 6 | 5 | 0 | 2 | 25651 |
16.092 | 732.2802 | 2 | 0.95 | 3 | 4 | 1 | 0 | 22085 |
Sialic acid, mostly found as a terminal component of glycoproteins and glycolipids on the outer surface of cells, is involved in cellular secretions.[42] Sialic acid participates in multiple and diverse cellular events, such as acting as an antirecognition agent by shielding recognition sites[42-44] and conversely by being a biological recognition site as a ligand for multiple molecules.[45, 46] Sialic acid is anionic and therefore likely contributes to HDL’s negative charge. Previously it has been shown that the addition of phosphatidylinositol, which increases HDL’s negative charge, blocked binding of HDL to hepatic lipase.[47] Other previous studies have also shown that the electronegativity of HDL affects its binding to cholesterol ester transfer protein and thus the exchange of cholesterol esters with LDL.[48] The sialylated glycans in HDL associated proteins may be involved in molecular and cellular interactions that affect the function of HDL. For example, sialic acid residues of ApoE may be essential for its recognition by HDL3 particles and further the binding to HDL3.[49] Interestingly, desialylation of lipoprotein-associated apoproteins was found to be associated with increased circulating neuraminidase excreted by Streptococcus pneumonia in patients with hemolytic uremic syndrome,[50] suggesting that bacterial infection may lead to desialylation of HDL particles in vivo.
In addition to complex type sialylated N-glycans, fucosylated N-glycans were present at relatively low abundances. High-mannose and hybrid type N-glycans were also observed, indicating the variety of N-glycans from HDL-associated proteins. The wide dynamic range of the detected N-glycans by the described method allows the evaluation of all types of oligosaccharides and further analyses of their biological functions.
Supplemental Figure S1 shows the overlaid ECCs of N-glycans from the three replicates. The separation of glycans and their profiles was similar, as the most abundant ones were observed as sialylated complex type eluting at 23 min-25 min. The method is considered reproducible with regard to the glycan composition assignments from these technical triplicates.
Site-specific analysis of HDL Glycoproteins
Glycopeptides were assigned based on a combination of the MS/MS data and the accurate precursor ion mass measurement. The advantage of non-specific digestion with pronase is the ability of the enzyme mixture to cleave the protein(s) into short peptides with typically one glycosylation site. Previous studies from our group on the analysis of non-specific digested glycopeptides with CID (collision-induced dissociation) experiments revealed detailed and comprehensive glycan compositional information for each glycopeptide (both N- and O-linked).23, 24 Glycosidic bond cleavages (B- and Y- type ions) were the major products as well as some minor peptide fragmentations.
Table 2 lists the pronase digested glycopeptides from HDL associated glycoproteins with their glycan composition, glycosylation site, protein ID, and intensity. The most abundant N-glycan (Hexose5HexNAc4Neu5Ac2) was found in multiple glycoproteins from the glycopeptide assignment. Here, all the identified proteins from the HDL were confirmed in triplicate experiments using X! Tendem and were used in the glycopeptide assignment search. A number of deconvoluted glycopeptide MS/MS spectra are shown as examples in Figure 3. Figure 3A represents the MS/MS spectrum for a triprotonated fetuin A glycopeptide containing this most abundant disialylated N-glycan. Particularly unique to glycopeptides containing sialylated glycans are B-type ions corresponding to neutral mass 291 Da (Neu5Ac), and neutral mass 273 Da (Neu5Ac–H2O). Mass peaks also include those observed as 203 Da, 365 Da, and 656 Da, which correspond to the neutral masses of HexNAc, (Hex+HexNAc), and (Hex+HexNAc+Neu5Ac). Due to the labile nature of sialic acid residues and their positions at the termini, the initial loss of sialic acid was commonly observed with the sialylated glycopeptides. Following the sequential neutral losses of monosaccharides of Neu5Ac, Hexose and HexNAc, the CID data revealed the mass peak 832 Da corresponding to glycopeptide (APLNDT+HexNAc). The presence of (peptide+HexNAc) is considered a valuable means for validating the assignment of glycopeptide particularly when analyzing complex protein mixtures.[51]
Table 2.
Retention Time (min) |
Measured m/z |
Charge state |
Mass Error (ppm) |
Hexose | HexNAc | Fucose | NeuAc | Protein | Sequence | site |
---|---|---|---|---|---|---|---|---|---|---|
24.893 | 967.7219 | 3 | 12.13 | 5 | 4 | 0 | 2 | HEMO | LPQPQN | 453 |
25.338 | 945.7015 | 3 | 1.61 | 5 | 4 | 0 | 2 | FETUA | APLNDT | 156 |
22.66 | 875.6656 | 3 | 11.12 | 5 | 4 | 0 | 2 | TRFE | SNVT | 630 |
21.539 | 865.9789 | 3 | 7.70 | 5 | 4 | 0 | 2 | FETUA | NGSN | 176 |
21.539 | 865.9789 | 3 | 7.70 | 5 | 4 | 0 | 2 | APO-H | GNNS | 163 |
21.205 | 856.3226 | 3 | 8.25 | 5 | 4 | 0 | 2 | KNG1 | QTN | 205 |
21.205 | 856.3226 | 3 | 13.68 | 5 | 4 | 0 | 2 | A1AT | GNAT | 271 |
17.342 | 851.6635 | 3 | 14.67 | 5 | 4 | 0 | 2 | FETUA | NKS | 432 |
23.225 | 851.3275 | 3 | 5.01 | 5 | 4 | 0 | 2 | A1AT | NLT | 107 |
17.54 | 822.6527 | 3 | 9.53 | 5 | 4 | 0 | 2 | ANGT | KN | 170 |
15.447 | 697.2652 | 3 | 17.33 | 5 | 4 | 1 | 0 | A1AT | NST | 70 |
15.447 | 697.2652 | 3 | 19.91 | 5 | 4 | 1 | 0 | ANGT | NST | 304 |
14.503 | 643.2539 | 3 | 4.78 | 4 | 4 | 1 | 0 | HEMO | NST | 246 |
16.925 | 728.6016 | 3 | 19.26 | 5 | 4 | 0 | 1 | ANGT | HN | 47 |
13.771 | 594.2537 | 2 | 0.93 | 1 | 1 | 0 | 1 | FETUA | VTSQP | 256 |
13.957 | 594.2637 | 2 | 12.90 | 1 | 1 | 0 | 1 | KNG1 | KTEGP | 542 |
14.090 | 572.243 | 2 | 6.96 | 1 | 1 | 0 | 1 | FETUA | QPSVG | 346 |
21.75 | 721.3209 | 2 | 8.46 | 1 | 1 | 0 | 1 | HEMO | SLAIATPL | 24 |
24.809 | 730.3203 | 2 | 6.19 | 1 | 1 | 0 | 2 | FETUA | VPTPV | 270 |
19.01 | 739.8152 | 2 | 14.86 | 1 | 1 | 0 | 2 | FETUA | VTSQP | 256 |
18.797 | 739.8152 | 2 | 1.976 | 1 | 1 | 0 | 2 | APOCIII | RPTSA | 94 |
18.717 | 584.7726 | 2 | 18.75 | 1 | 1 | 0 | 1 | FETUA | VPTPV | 270 |
26.005 | 830.3642 | 2 | 18.21 | 1 | 1 | 0 | 2 | FETUA | EAVPTPV | 270 |
Abbreviations: HEMO, hemopexin; FETUA, fetuin A; TRFE, serotransferrin; APO-H, apolipoprotein H; KNG1, kininogen-1; A1AT, alpha-1-antitrypsin; ANGT, Angiotensinogen; APOCIII, Apolipoprotein CIII
Pronase digestion simultanously enables site-specific analysis of both N- and O-glycans. In addition to the abundant N-glycans discussed previously, a number of O-glycopeptides were present attached with sialylated O-glycans (Table 2). The observed O-glycans associated with the HDL glycoproteins were all sialylated, comfirming that HDL particles are highly sialylated. Figure 3(B and C) revealed the deconvoluted MS/MS spectra for two diprotonated O-glycopeptides from ApoC-III and fetuin A, respectively. Most O-glycopeptides analyzed in the HDL mixture contained a core 1 type with two Neu5Acs.
Figure 4 shows the site heterogeneity of four glycoproteins from eight of the identified HDL associated glycoproteins as an example. Fetuin A is a multifunctional circulating liver-derived glycoprotein in serum and plasma.[52] Several studies have suggested that fetuin A may be critically important to cardiovascular health.[53-56] Both N- and O-glycans were observed at multiple glycosylation sites with fetuin A, all of which were sialylated (Figure 4A), which is consistent with the previous glycosylation analysis on the individual protein fetuin A.[57] The most abundant glycan (Hexose5HexNAc4Neu5Ac2) was disialylated and was found on most of the glycoproteins examined. It was present at ASN156 and ASN176 of fetuin A.
Angiotensinogen is a heterogeneous glycoprotein mainly produced by hepatocytes in plasma, which has a well-known role in blood pressure regulation in animals and humans.[58] It has previously been shown that the glycosylation of angiotensinogen may play a significant role in its functional heterogeneity.[59] Results of site heterogeneity of angiotensinogen are summarized in Figure 4B. Among the four potential N-glycosylation sites, three identified sites were occupied with N-glycans in this study. While two sites were observed associated with sialylated N-glycans, site ASN304 was attached with fucosylated N-glycans. Angiotensinogen was also found attached with the most abundant sialylated glycan (Hexose5HexNAc4Neu5Ac2) at ASN170.
Figure 4C details the glycan associated with Alpha-1B-glycoprotein (A1BG). A1BG is believed to be a member of the immunoglobulin family.[60]The mono-sialylated glycan (Hexose5HexNAc4Neu5Ac1) attached at ASN363 on A1BG.
The glycosylation of apolipoprotein C3 (Apo C3) was analyzed by a couple of groups, showing the distribution of O-glycans.[61, 62] The disialylated O-glycan at site Thr94 from ApoC-III is shown in Figure 4D. APO C3 inhibits lipoprotein lipase and hepatic lipase, thought to inhibit hepatic uptake of triglyceride-rich particles.[63] APO C3 was also recently found to be increased in HDL isolated from patients with both stable coronary artery disease and acute coronary syndrome as well as in hemodialysis patients.[64, 65]
In general, for the first time the site-specific glycosylation of these proteins in HDL particles has been described. Compared with previous disscussed glycan analysis, there were some glycans that were not observed in the glycopeptide analysis due to their low abundances as well as the potential short peptide length from pronase digestion. However, the functions they impart on HDL through their glycosylation, and whether alterations in their glycosylation as part of HDL particles is either causative or diagnostic in disease are unknown.
HDL gangliosides characterized by MS/MS
Gangliosides are another contributor of sialic acid in HDL. We applied a high resolution Q-TOF MS method with reverse-phase nanoHPLC separation for the analysis of human HDL gangliosides. The high mass accuracy of these instruments, along with the MS/MS capability made it possible to perform focused detection of ganglioside species in the polar lipid extract.[66] Post-processing precursor ion scans indicate the existence of gangliosides, which elute at certain retention times. Moreover, based on accurate mass, glycan information and ceramide composition were simultaneously obtained.
Figure 5 is representative of the extracted compound chromatograms (ECCs) of HDL gangliosides. The chromatogram reveals an elution pattern starting with gangliosides with shorter ceramide chains followed by those with longer ceramides. Examination of the profiles shows that GM3 (monosialoganglioside, NeuAc2-3Gal1-4Glc-Cer) and GD3 (disialoganglioside, NeuAc2-8NeuAc2-3Gal1-4Glc-Cer) were abundant ganglioside ions in HDL from healthy human plasma, in agreement with earlier studies.[67] Eight GM3 and four GD3 gangliosides were detected. A 60% GM3 and 40% GD3 distribution was observed, and ion intensities were measured in the MS mode based on the deprotonated molecular ion (Table 3). Interestingly, the composition of human aorta from patients who had died of myocardial infarction were found to have higher GD3 content in the aortic media versus the intima[68] and total ganglioside content was found to be lower in cells isolated from atherosclerotic compared with normal human aorta.[69] Gangliosides have even been found to stimulate lipoxygenase-mediated eicosanoid production in peripheral blood lymphocytes, and GD3 was more stimulatory compared with GM1 or GM3.[70] These previous reports suggest that ganglioside content and composition may have important biological implications in heart disease and its related mechanisms involving lipoproteins.
Table 3.
Retention time (min) |
Measured m/z |
Charge state |
Mass error (ppm) |
Structural Assignment |
Ion Intensity (counts) |
---|---|---|---|---|---|
12.9 | 1151.711 | −1 | −4.3 | GM3(d18:1/16:0) | 1120103 |
16.2 | 1179.732 | −1 | 4.2 | GM3(d16:1/20:0) or GM3 (d18:1/18:0) |
498901 |
19.7 | 1207.760 | −1 | 7.5 | GM3(d16:1/22:0) | 459570 |
21.4 | 1221.779 | −1 | 4.1 | GM3(d16:1/23:0) | 288025 |
22.9 | 1235.793 | −1 | 5.7 | GM3(d16:1/24:0) or GM3(d18:1/22:0) |
772085 |
24.3 | 1249.812 | −1 | 2.4 | GM3(d16:1/25:0) or GM3(d18:1/23:0) |
543404 |
25.8 | 1263.833 | −1 | −1.6 | GM3(d18:1/24:0) | 494824 |
26.7 | 1277.849 | −1 | −1.6 | GM3(d18:1/25:0) | 42591 |
20.2 | 755.935 | −2 | 1.3 | GD3(d16:1/23:0) | 455116 |
21.4 | 762.945 | −2 | −1.3 | GD3(d16:1/24:0) or GD3(d18:1/22:0) |
1006020 |
23.1 | 769.972 | −2 | 1.3 | GD3(d16:1/25:0) or GD3(d18:1/23:0) |
815475 |
24.7 | 776.960 | −2 | 0.0 | GD3(d18:1/24:0) | 523004 |
The analysis also revealed the composition of the major ceramide portion of GM3 and GD3 gangliosides. Both GM3 and GD3 were composed of heterogeneous ceramide lipid tails, including d18:1/16:0 and d18:1/23:0. Types of sphingoid bases and fatty acids in the backbones were determined with the use of 80V MS/MS. Fragments at m/z 264.269 and at m/z 236.238 indicated the existence of sphingoid bases d18:1 and d16:1, respectively. As an example, GM3 (d18:1/16:0) yields a diagnostic sialic acid fragment at m/z 290.09 in 40V negative mode MS/MS, while 80V positive mode MS/MS spectrum provides the ceramide information at m/z 520.49 and 264.27 (Supplemental Figure S2). The importance of the ceramide lipid tail compositional differences is currently poorly understood. For example, transmembrane anchored angiotensin converting enzyme, an enzyme important for blood pressure regulation, was found to associate only with C18 but not C16 sphingomyelin containing rafts.[71] A recent report showed that nascent HDL resemble lipid rafts suggesting the possibility that HDL have microheterogeneity with lipid raft-like portions of the phospholipid outer layer that recruit specific gangliosides and proteins to perform specific functions, just as occurs in plasma membrane lipid rafts.[72] The simultaneous identification of the glycan and ceramide will provide a clearer picture of the role of gangliosides in lipoprotein biology.
Conclusion
We have established analytical methods for profiling the glycome of HDL particles. the approach detailed here provides a simultaneous and detailed analysis of glycoproteins (both N-and O-glycan composition, as well as site-specific glycopeptide composition) and gangliosides (both the glycan and ceramide portion) that was previously not achievable. The methods developed in this study can be used for the analysis of other nanobioparticles including LDL, VLDL, and chylomicrons, as well as the various size subclasses of these major lipoprotein classes. This approach will have implications for elucidating a number of biological functions of HDL. With this method in place it is now possible to conduct an array of experiments and analyses of clinical samples to understand the important biological functions and diagnostic potential of HDL that are mediated by glycans.
Supplementary Material
Acknowledgement
The study was funded by grants from the National Institutes of Health (R01GM049077) and the University of California Discovery Program (BIO08-128504 and 09 GEB-02 NHB) the California Dairy Research Foundation.
Abbreviations
- HDL
high density lipoprotein
- LDL
low density lipoprotein
- VLDL
very low density lipoprotein
- APO
apoprotein
- HPLC
high-performance liquid chromatography
- Q-TOF
quadrupole time-of-flight
- CID
collision-induced dissociation
- SPE
solid phase extraction
- Hex
hexose
- HexNAc
N-acetylhexosamine
- Neu5Ac
neuraminic acid (sialic acid)
- Fuc
fucose
- GCC
graphitized carbon cartridge
- PNGase F
peptide N-glycosidase F
- ACN
acetonitrile
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