Your search keyword '"Adnan Halim"' showing total 24 results

1. Decision letter: POMK regulates dystroglycan function via LARGE1-mediated elongation of matriglycan

Author

Adnan Halim and James C. Paulson

Subjects

biology, Chemistry, Dystroglycan, biology.protein, Elongation, Function (biology), Cell biology

Published

2020

2. Characterizing the O-glycosylation landscape of human plasma, platelets, and endothelial cells

Author

Sergey Y. Vakhrushev, Hiren J. Joshi, Morten Hanefeld Dziegiel, Hans H. Wandall, Katrine T. Schjoldager, Sarah L. King, Anders Woetmann, Thomas Daugbjerg Madsen, and Adnan Halim

Subjects

0301 basic medicine, chemistry.chemical_classification, Glycan, Protease, Glycosylation, medicine.diagnostic_test, medicine.medical_treatment, Proteolysis, Protein domain, Hematology, Biology, Amino acid, carbohydrates (lipids), 03 medical and health sciences, chemistry.chemical_compound, 030104 developmental biology, Biochemistry, chemistry, Vascular Biology, biology.protein, medicine, Protein precursor, Glycoprotein

Abstract

The hemostatic system comprises platelet aggregation, coagulation, and fibrinolysis, and is critical to the maintenance of vascular integrity. Multiple studies indicate that glycans play important roles in the hemostatic system; however, most investigations have focused on N-glycans because of the complexity of O-glycan analysis. Here we performed the first systematic analysis of native-O-glycosylation using lectin affinity chromatography coupled to liquid chromatography mass spectrometry (LC-MS)/MS to determine the precise location of O-glycans in human plasma, platelets, and endothelial cells, which coordinately regulate hemostasis. We identified the hitherto largest O-glycoproteome from native tissue with a total of 649 glycoproteins and 1123 nonambiguous O-glycosites, demonstrating that O-glycosylation is a ubiquitous modification of extracellular proteins. Investigation of the general properties of O-glycosylation established that it is a heterogeneous modification, frequently occurring at low density within disordered regions in a cell-dependent manner. Using an unbiased screen to identify associations between O-glycosites and protein annotations we found that O-glycans were over-represented close (± 15 amino acids) to tandem repeat regions, protease cleavage sites, within propeptides, and located on a select group of protein domains. The importance of O-glycosites in proximity to proteolytic cleavage sites was further supported by in vitro peptide assays demonstrating that proteolysis of key hemostatic proteins can be inhibited by the presence of O-glycans. Collectively, these data illustrate the global properties of native O-glycosylation and provide the requisite roadmap for future biomarker and structure-function studies.

Published

2017

3. Multiple distinct O-Mannosylation pathways in eukaryotes

Author

Adnan Halim, Henrik Clausen, Hiren J. Joshi, Ida Signe Bohse Larsen, and Yoshiki Narimatsu

Subjects

Glycosylation, Protein domain, Biology, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Protein Domains, Structural Biology, Molecular Biology, Gene, 030304 developmental biology, Glycoproteins, Genetics, 0303 health sciences, Cadherin, fungi, Plexin, Eukaryota, Phenotype, Yeast, Glycoproteomics, Oxygen, chemistry, biology.protein, Mannose, 030217 neurology & neurosurgery

Abstract

Protein O-mannosylation (O-Man), originally discovered in yeast five decades ago, is an important post-translational modification (PTM) conserved from bacteria to humans, but not found in plants or nematodes. Until recently, the homologous family of ER-located protein O-mannosyl transferases (PMT1-7 in yeast; POMT1/POMT2 in humans), were the only known enzymes involved in directing O-Man biosynthesis in eukaryotes. However, recent studies demonstrate the existence of multiple distinct O-Man glycosylation pathways indicating that the genetic and biosynthetic regulation of O-Man in eukaryotes is more complex than previously envisioned. Introduction of sensitive glycoproteomics strategies provided an expansion of O-Man glycoproteomes in eukaryotes (yeast and mammalian cell lines) leading to the discovery of O-Man glycosylation on important mammalian cell adhesion (cadherin superfamily) and signaling (plexin family) macromolecules, and to the discovery of unique nucleocytoplasmic O-Man glycosylation in yeast. It is now evident that eukaryotes have multiple distinct O-Man glycosylation pathways including: i) the classical PMT1-7 and POMT1/POMT2 pathway conserved in all eukaryotes apart from plants; ii) a yet uncharacterized nucleocytoplasmic pathway only found in yeast; iii) an ER-located pathway directed by the TMTC1-4 genes found in metazoans and protists and primarily dedicated to the cadherin superfamily; and iv) a yet uncharacterized pathway found in metazoans primarily dedicated to plexins. O-Man glycosylation is thus emerging as a much more widespread and evolutionary diverse PTM with complex genetic and biosynthetic regulation. While deficiencies in the POMT1/POMT2 O-Man pathway underlie muscular dystrophies, the TMTC1-4 pathway appear to be involved in distinct congenital disorders with neurodevelopmental phenotypes. Here, we review and discuss the recent discoveries of the new non-classical O-Man glycosylation pathways, their substrates, functions and roles in disease.

Published

2018

4. A strategy for generating cancer-specific monoclonal antibodies to aberrant O-glycoproteins: identification of a novel dysadherin-Tn antibody

Author

Federico Battisti, Hans Schreiber, Sergey Y. Vakhrushev, Yoshiki Narimatsu, Hiren J. Joshi, Catharina Steentoft, Ulla Mandel, Julie Van Coillie, Thomas Daugbjerg Madsen, Diana Campos, Adnan Halim, and Max Fuhrmann

Subjects

medicine.drug_class, Monoclonal antibody, Biochemistry, Epitope, Metastasis, Regular Manuscripts, 03 medical and health sciences, Epitopes, Mice, Antigen, Cell Line, Tumor, Neoplasms, medicine, Animals, Humans, MUC1, 030304 developmental biology, Glycoproteins, 0303 health sciences, biology, 030302 biochemistry & molecular biology, Cancer, Antibodies, Monoclonal, medicine.disease, Chimeric antigen receptor, Cancer research, biology.protein, Antibody

Abstract

Successful application of potent antibody-based T-cell engaging immunotherapeutic strategies is currently limited mainly to hematological cancers. One major reason is the lack of well-characterized antigens on solid tumors with sufficient cancer specific expression. Aberrantly O-glycosylated proteins contain promising cancer-specific O-glycopeptide epitopes suitable for immunotherapeutic applications, but currently only few examples of such antibody epitopes have been identified. We previously showed that chimeric antigen receptor T-cells directed towards aberrantly O-glycosylated MUC1 can control malignant growth in a mouse model. Here, we present a discovery platform for the generation of cancer-specific monoclonal antibodies targeting aberrant O-glycoproteins. The strategy is based on cancer cell lines engineered to homogeneously express the truncated Tn O-glycoform, the so-called SimpleCells. We used SimpleCells of different cancer origin to elicit monoclonal antibodies with selectivity for aberrant O-glycoproteins. For validation we selected and characterized one monoclonal antibody (6C5) directed to a Tn-glycopeptide in dysadherin (FXYD5), known to be upregulated in cancer and promote metastasis. While dysadherin is widely expressed also in normal cells, we demonstrated that the 6C5 epitope is specifically expressed in cancer.

Published

2018

5. O-Linked Glycosylation of the Mucin Domain of the Herpes Simplex Virus Type 1-specific Glycoprotein gC-1 Is Temporally Regulated in a Seed-and-spread Manner

Author

Ulla Mandel, Göran Larson, Rickard Nordén, Eric P. Bennett, Adnan Halim, Jonas Nilsson, Kristina Nyström, and Sigvard Olofsson

Subjects

Glycan, Glycosylation, Glycobiology and Extracellular Matrices, Herpesvirus 1, Human, Biology, medicine.disease_cause, Biochemistry, Cell Line, chemistry.chemical_compound, Viral Envelope Proteins, parasitic diseases, Glycosyltransferase, medicine, Humans, Molecular Biology, chemistry.chemical_classification, Mucin, Herpes Simplex, Cell Biology, Sialyltransferases, Glycoproteomics, carbohydrates (lipids), Herpes simplex virus, chemistry, O-linked glycosylation, biology.protein, lipids (amino acids, peptides, and proteins), Glycoprotein

Abstract

The herpes simplex virus type 1 (HSV-1) glycoprotein gC-1, participating in viral receptor interactions and immunity interference, harbors a mucin-like domain with multiple clustered O-linked glycans. Using HSV-1-infected diploid human fibroblasts, an authentic target for HSV-1 infection, and a protein immunoaffinity procedure, we enriched fully glycosylated gC-1 and a series of its biosynthetic intermediates. This fraction was subjected to trypsin digestion and a LC-MS/MS glycoproteomics approach. In parallel, we characterized the expression patterns of the 20 isoforms of human GalNAc transferases responsible for initiation of O-linked glycosylation. The gC-1 O-glycosylation was regulated in an orderly manner initiated by synchronous addition of one GalNAc unit each to Thr-87 and Thr-91 and one GalNAc unit to either Thr-99 or Thr-101, forming a core glycopeptide for subsequent additions of in all 11 GalNAc residues to selected Ser and Thr residues of the Thr-76-Lys-107 stretch of the mucin domain. The expression patterns of GalNAc transferases in the infected cells suggested that initial additions of GalNAc were carried out by initiating GalNAc transferases, in particular GalNAc-T2, whereas subsequent GalNAc additions were carried out by followup transferases, in particular GalNAc-T10. Essentially all of the susceptible Ser or Thr residues had to acquire their GalNAc units before any elongation to longer O-linked glycans of the gC-1-associated GalNAc units was permitted. Because the GalNAc occupancy pattern is of relevance for receptor binding of gC-1, the data provide a model to delineate biosynthetic steps of O-linked glycosylation of the gC-1 mucin domain in HSV-1-infected target cells.

Published

2015

6. LC–MS/MS characterization of combined glycogenin-1 and glycogenin-2 enzymatic activities reveals their self-glucosylation preferences

Author

Ali-Reza Moslemi, Erik Larsson, Göran Larson, Jonas Nilsson, Anders Oldfors, Johanna Nilsson, and Adnan Halim

Subjects

Glycosylation, Glycogenin, Biophysics, Tandem mass spectrometry, Biochemistry, Catalysis, Gene Expression Regulation, Enzymologic, Substrate Specificity, Analytical Chemistry, chemistry.chemical_compound, Glucosyltransferases, Tandem Mass Spectrometry, Catalytic Domain, Glycosyltransferase, Humans, Glycogen synthase, Molecular Biology, Glycoproteins, chemistry.chemical_classification, biology, Glycogen, Chemistry, Enzyme Activation, carbohydrates (lipids), HEK293 Cells, Enzyme, biology.protein, Protein Processing, Post-Translational, Chromatography, Liquid

Abstract

Glycogen synthesis is initiated by self-glucosylation of the glycosyltransferases glycogenin-1 and -2 that, in the presence of UDP-glucose, form both the first glucose-O-tyrosine linkage, and then stepwise add a series of α1,4-linked glucoses to a growing chain of variable length. Glycogen-1 and -2 coexist in liver glycogen preparations where the proteins are known to form homodimers, and they also have been shown to interact with each other. In order to study how glycogenin-1 and -2 interactions may influence each other's glucosylations we setup a cell-free expression system for in vitro production and glucosylation of glycogenin-1 and -2 in various combinations, and used a mass spectrometry based workflow for the characterization and quantitation of tryptic glycopeptides originating from glycogenin-1 and -2. The analysis revealed that the self-glucosylation endpoint was the incorporation of 4-8 glucose units on Tyr 195 of glycogenin-1, but only 0-4 glucose units on Tyr-228 of glycogenin-2. The glucosylation of glycogenin-2 was enhanced to 2-4 glucose units by the co-presence of enzymatically active glycogenin-1. Glycogenin-2 was, however, unable to glucosylate inactive glycogenin-1, at least not an enzymatically inactivated Thr83Met glycogenin-1 mutant, recently identified in a patient with severe glycogen depletion.

Published

2014

7. An online nano-LC-ESI-FTICR-MS method for comprehensive characterization of endogenous fragments from amyloid β and amyloid precursor protein in human and cat cerebrospinal fluid

Author

Rita Persson, Annika Öhrfelt, Henrik Zetterberg, Göran Larson, Ann Brinkmalm, Jonas Nilsson, Ulla Rüetschi, Jan-Eric Månsson, Mikael K. Gustavsson, Niklas Mattsson, Adnan Halim, Johan Gobom, Charles H. Vite, Gunnar Brinkmalm, Erik Portelius, and Kaj Blennow

Subjects

chemistry.chemical_classification, Glycosylation, biology, Chemistry, P3 peptide, Peptide, Tandem mass spectrometry, Amino acid, chemistry.chemical_compound, Biochemistry, Amyloid precursor protein, biology.protein, Senile plaques, Peptide sequence, Spectroscopy

Abstract

Amyloid precursor protein (APP) is the precursor protein to amyloid β (Aβ), the main constituent of senile plaques in Alzheimer's disease (AD). Endogenous Aβ peptides reflect the APP processing, and greater knowledge of different APP degradation pathways is important to understand the mechanism underlying AD pathology. When one analyzes longer Aβ peptides by low-energy collision-induced dissociation tandem mass spectrometry (MS/MS), mainly long b-fragments are observed, limiting the possibility to determine variations such as amino acid variants or post-translational modifications (PTMs) within the N-terminal half of the peptide. However, by using electron capture dissociation (ECD), we obtained a more comprehensive sequence coverage for several APP/Aβ peptide species, thus enabling a deeper characterization of possible variants and PTMs. Abnormal APP/Aβ processing has also been described in the lysosomal storage disease Niemann-Pick type C and the major large animal used for studying this disease is cat. By ECD MS/MS, a substitution of Asp7 → Glu in cat Aβ was identified. Further, sialylated core 1 like O-glycans at Tyr10, recently discovered in human Aβ (a previously unknown glycosylation type), were identified also in cat cerebrospinal fluid (CSF). It is therefore likely that this unusual type of glycosylation is common for (at least) species belonging to the magnorder Boreoeutheria. We here describe a detailed characterization of endogenous APP/Aβ peptide species in CSF by using an online top-down MS-based method.

Published

2012

8. Molecular pathogenesis of a new glycogenosis caused by a glycogenin-1 mutation

Author

Ali-Reza Moslemi, Jonas Nilsson, Anders Oldfors, Johanna Nilsson, Anders Pedersen, Adnan Halim, and Göran Larson

Subjects

Glycogenin, Molecular Sequence Data, Glycogen debranching enzyme, chemistry.chemical_compound, Tandem Mass Spectrometry, Glycogen branching enzyme, medicine, Cell-free expression, Humans, Glycogen storage disease, Amino Acid Sequence, Threonine, Tyrosine, Glycogen synthase, Molecular Biology, DNA Primers, Glycoproteins, Mass spectrometry, Base Sequence, Cell-Free System, biology, Glycogen, medicine.disease, Molecular biology, Glucose, chemistry, Biochemistry, Glucosyltransferases, Mutation, Biocatalysis, Chromatography, Gel, biology.protein, Molecular Medicine, Chromatography, Liquid

Abstract

Glycogenin-1 initiates the glycogen synthesis in skeletal muscle by the autocatalytic formation of a short oligosaccharide at tyrosine 195. Glycogenin-1 catalyzes both the glucose-O-tyrosine linkage and the α1,4 glucosidic bonds linking the glucose molecules in the oligosaccharide. We recently described a patient with glycogen depletion in skeletal muscle as a result of a non-functional glycogenin-1. The patient carried a Thr83Met substitution in glycogenin-1. In this study we have investigated the importance of threonine 83 for the catalytic activity of glycogenin-1. Non-glucosylated glycogenin-1 constructs, with various amino acid substitutions in position 83 and 195, were expressed in a cell-free expression system and autoglucosylated in vitro. The autoglucosylation was analyzed by gel-shift on western blot, incorporation of radiolabeled UDP-14C-glucose and nano-liquid chromatography with tandem mass spectrometry (LC/MS/MS). We demonstrate that glycogenin-1 with the Thr83Met substitution is unable to form the glucose-O-tyrosine linkage at tyrosine 195 unless co-expressed with the catalytically active Tyr195Phe glycogenin-1. Our results explain the glycogen depletion in the patient expressing only Thr83Met glycogenin-1 and why heterozygous carriers without clinical symptoms show a small proportion of unglucosylated glycogenin-1.

Published

2012

9. The N-terminal domain of α-dystroglycan, released as a 38kDa protein, is increased in cerebrospinal fluid in patients with Lyme neuroborreliosis

Author

Henrik Anckarsäter, Rolf Anckarsäter, Göran Larson, Lars Hagberg, Henrik Zetterberg, Niklas Mattsson, Kaj Blennow, Camilla Hesse, Inger Johansson, Adnan Halim, Ammi Grahn, Ulf Andreasson, and Daniel Bremell

Subjects

Adult, Male, Central nervous system, Biophysics, Enzyme-Linked Immunosorbent Assay, Biochemistry, Dystroglycans, Cerebrospinal fluid, Extracellular, medicine, Dystroglycan, Humans, Lyme Neuroborreliosis, Molecular Biology, CSF albumin, Aged, biology, business.industry, Cell Biology, Middle Aged, medicine.disease, Protein Structure, Tertiary, medicine.anatomical_structure, Immunology, biology.protein, Female, business, Neuroborreliosis, Biomarkers

Abstract

α-Dystroglycan is an extracellular adhesion protein that is known to interact with different ligands. The interaction is thought to stabilize the integrity of the plasma membrane. The N-terminal part of α-dystroglycan may be proteolytically processed to generate a small 38 kDa protein (α-DG-N). The physiological significance of α-DG-N is unclear but has been suggested to be involved in nerve regeneration and myelination and to function as a potential biomarker for neurodegenerative and neuromuscular diseases. In this report we show that α-DG-N is released into different body fluids, such as lachrimal fluid, cerebrospinal fluid (CSF), urine and plasma. To investigate the significance of α-DG-N in CSF we examined the levels of α-DG-N and known neurodegenerative markers in CSF from patients diagnosed with Lyme neuroborreliosis (LNB) and healthy controls. In untreated acute phase LNB patients, 67% showed a significant increase of CSF α-DG-N compared to healthy controls. After treatment with antibiotics the CSF α-DG-N levels were normalized in the LNB patients.

Published

2011

10. Site-specific characterization of threonine, serine, and tyrosine glycosylations of amyloid precursor protein/amyloid β-peptides in human cerebrospinal fluid

Author

Ulla Rüetschi, Adnan Halim, Jonas Nilsson, Henrik Zetterberg, Göran Larson, Ann Westman-Brinkmalm, Kaj Blennow, Erik Portelius, and Gunnar Brinkmalm

Subjects

Proteomics, Threonine, Glycosylation, Molecular Sequence Data, Serine, Amyloid beta-Protein Precursor, chemistry.chemical_compound, Alzheimer Disease, Tandem Mass Spectrometry, Amyloid precursor protein, Humans, Amino Acid Sequence, Tyrosine, Peptide sequence, Amyloid beta-Peptides, Multidisciplinary, biology, P3 peptide, Biological Sciences, Molecular biology, Glycopeptide, Biochemistry, chemistry, biology.protein, Chromatography, Liquid

Abstract

The proteolytic processing of human amyloid precursor protein (APP) into shorter aggregating amyloid β (Aβ)-peptides, e.g., Aβ1-42, is considered a critical step in the pathogenesis of Alzheimer’s disease (AD). Although APP is a well-known membrane glycoprotein carrying both N- and O-glycans, nothing is known about the occurrence of released APP/Aβ glycopeptides in cerebrospinal fluid (CSF). We used the 6E10 antibody and immunopurified Aβ peptides and glycopeptides from CSF samples and then liquid chromatography—tandem mass spectrometry for structural analysis using collision-induced dissociation and electron capture dissociation. In addition to 33 unglycosylated APP/Aβ peptides, we identified 37 APP/Aβ glycopeptides with sialylated core 1 like O-glycans attached to Thr(−39, −21, −20, and −13), in a series of APP/Aβ X -15 glycopeptides, where X was −63, −57, −52, and −45, in relation to Asp1 of the Aβ sequence. Unexpectedly, we also identified a series of 27 glycopeptides, the Aβ1- X series, where X was 20 (DAEFRHDSGYEVHHQKLVFF), 19, 18, 17, 16, and 15, which were all uniquely glycosylated on Tyr10. The Tyr10 linked O-glycans were (Neu5Ac) 1-2 Hex(Neu5Ac)HexNAc- O - structures with the disialylated terminals occasionally O-acetylated or lactonized, indicating a terminal Neu5Acα2,8Neu5Ac linkage. We could not detect any glycosylation of the Aβ1-38/40/42 isoforms. We observed an increase of up to 2.5 times of Tyr10 glycosylated Aβ peptides in CSF in six AD patients compared to seven non-AD patients. APP/Aβ sialylated O-glycans, including that of a Tyr residue, the first in a mammalian protein, may modulate APP processing, inhibiting the amyloidogenic pathway associated with AD.

Published

2011

11. Differentiation of glycosphingolipid-derived glycan structural isomers by liquid chromatography/mass spectrometry

Author

Susann Teneberg, Adnan Halim, and Hasse Karlsson

Subjects

Spectrometry, Mass, Electrospray Ionization, Glycan, Erythrocytes, Resolution (mass spectrometry), Protein mass spectrometry, Swine, Electrospray ionization, Molecular Sequence Data, Mass spectrometry, Biochemistry, Glycosphingolipids, Sample preparation in mass spectrometry, Mice, chemistry.chemical_compound, Isomerism, Polysaccharides, Liquid chromatography–mass spectrometry, Animals, Humans, Cells, Cultured, Chromatography, High Pressure Liquid, Chromatography, Molecular Structure, biology, Dendritic Cells, Glycosphingolipid, Intestines, Mice, Inbred C57BL, Carbohydrate Sequence, chemistry, biology.protein

Abstract

Isolation and characterization of glycosphingolipids is of importance in many aspects of glycobiology, but is difficult to achieve due to the high degree of heterogeneity and isomerism present in these compounds. In this study, oligosaccharides obtained from non-acid glycosphingolipids by enzymatic digestion with endoglycoceramidase II of Rhodococcus sp. were analyzed by liquid chromatography/electrospray ionization mass spectrometry using graphitized carbon columns. Resolution of isomeric oligosaccharides was achieved, and the MS(2) analyses gave complete sequence information and allowed differentiation of linkage positions. Diagnostic cross-ring (0,2)A-type fragments have previously been described for GlcNAc substituted on C-4 and for 4-substituted Glc. Diagnostic cross-ring (0,2)A-type fragments were present in the MS(2) spectrum of the H type 2 (Fucalpha2Galbeta4GlcNAcbeta4Galbeta4Glc) pentasaccharide, but not in the MS(2) spectrum of H type 1 pentasaccharide (Fucalpha2Galbeta3GlcNAcbeta4Galbeta4Glc). Cross-ring (0,2)A-type fragments were also obtained from the 4-substituted Glc at the reducing end of the glycosphingolipid-derived oligosaccharides. Oligosaccharides of the globo-series (globotriaose (Galalpha4Galbeta4Glc) and globotetraose (GalNAcbeta3Galalpha4Galbeta4Glc)) and the isoglobo-series (isoglobotriaose (Galalpha3Galbeta4Glc) and isoglobotetraose (GalNAcbeta3Galalpha3Galbeta4Glc)) were also chromatographically resolved on the graphitized carbon column. Furthermore, diagnostic fragment ions from cross-ring (0,2)A-type cleavages were present in the MS(2) spectra of the globo-series oligosaccharides, having a Gal substituted on C-4. The applicability of this method on tissue-derived samples was demonstrated using a non-acid glycosphingolipid fraction from human gastric epithelium and a partially purified non-acid glycosphingolipid fraction from 8 x 10(7) bone marrow-derived mouse dendritic cells. Here, liquid chromatography/mass spectrometry of the oligosaccharides released by endoglycoceramidase allowed tentative identification of a number of glycosphingolipids ranging from tri- to nonaglycosylceramides.

Published

2010

12. A systematic study of modulation of ADAM-mediated ectodomain shedding by site-specific O-glycosylation

Author

Adnan Halim, Daniel J. Rader, Henrik Clausen, Katrine T. Schjoldager, Sumeet A. Khetarpal, and Christoffer K. Goth

Subjects

Lipopolysaccharides, Proteases, Cell signaling, Glycosylation, ADAM10, Blotting, Western, Molecular Sequence Data, Biology, Substrate Specificity, Genes, Reporter, Disintegrin, Animals, Humans, Amino Acid Sequence, Mice, Knockout, Multidisciplinary, Tumor Necrosis Factor-alpha, Glycopeptides, Hep G2 Cells, Biological Sciences, ADAM Proteins, Molecular biology, Protein Structure, Tertiary, carbohydrates (lipids), Crosstalk (biology), HEK293 Cells, Membrane protein, Ectodomain, Mutation, biology.protein, N-Acetylgalactosaminyltransferases, lipids (amino acids, peptides, and proteins)

Abstract

Regulated shedding of the ectodomain of cell membrane proteins by proteases is a common process that releases the extracellular domain from the cell and activates cell signaling. Ectodomain shedding occurs in the immediate extracellular juxtamembrane region, which is also where O-glycosylation is often found and examples of crosstalk between shedding and O-glycosylation have been reported. Here, we systematically investigated the potential of site-specific O-glycosylation mediated by distinct polypeptide GalNAc-transferase (GalNAc-T) isoforms to coregulate ectodomain shedding mediated by the A Disintegrin And Metalloproteinase (ADAM) subfamily of proteases and in particular ADAM17. We analyzed 25 membrane proteins that are known to undergo ADAM17 shedding and where the processing sites included Ser/Thr residues within ± 4 residues that could represent O-glycosites. We used in vitro GalNAc-T enzyme and ADAM cleavage assays to demonstrate that shedding of at least 12 of these proteins are potentially coregulated by O-glycosylation. Using TNF-α as an example, we confirmed that shedding mediated by ADAM17 is coregulated by O-glycosylation controlled by the GalNAc-T2 isoform both ex vivo in isogenic cell models and in vivo in mouse Galnt2 knockouts. The study provides compelling evidence for a wider role of site-specific O-glycosylation in ectodomain shedding.

Published

2015

13. Complex regulation of prolyl-4-hydroxylases impacts root hair expansion

Author

Christian Peter Poulsen, Cecilia Borassi, Rafael Andrade Buono, Eliana Marzol, Juan D. Salgado Salter, Henrik Vibe Scheller, Bent O. Petersen, Silvia Melina Velásquez, Naomi Geshi, José M. Estevez, Ken Matsuoka, Norberto D. Iusem, Javier Gloazzo Dorosz, Adiphol Dilokpimol, Ai Oikawa, Yukiko Ohsawa, Silvina Paola Denita Juárez, Marisa S. Otegui, Adnan Halim, Martiniano M. Ricardi, Silvina Mangano, and Svenning Rune Møller

Subjects

Enzymologic, Glycosylation, proline hydroxylation, enzymology, Plant Biology & Botany, Arabidopsis, Plant Biology, Plant Science, Root hair elongation, Root hair, Hydroxylation, Plant Roots, Prolyl Hydroxylases, Gene Expression Regulation, Enzymologic, root hairs, Cell wall, chemistry.chemical_compound, Gene Expression Regulation, Plant, Hydroxyproline/metabolism, protein targeting, Genetics, Arabidopsis thaliana, Tip growth, Plant Roots/enzymology, Extensin, Molecular Biology, Secretory pathway, biology, cell walls, Arabidopsis Proteins, Plant, biology.organism_classification, Cell biology, Hydroxyproline, Arabidopsis Proteins/genetics, Biochemistry, chemistry, Gene Expression Regulation, Arabidopsis/enzymology, Multigene Family, biology.protein, Prolyl Hydroxylases/genetics, Biochemistry and Cell Biology, cell expansion

Abstract

© 2015 The Author. Root hairs are single cells that develop by tip growth, a process shared with pollen tubes, axons, and fungal hyphae. However, structural plant cell walls impose constraints to accomplish tip growth. In addition to polysaccharides, plant cell walls are composed of hydroxyproline-rich glycoproteins (HRGPs), which include several groups of O-glycoproteins, including extensins (EXTs). Proline hydroxylation, an early post-translational modification (PTM) of HRGPs catalyzed by prolyl 4-hydroxylases (P4Hs), defines their subsequent O-glycosylation sites. In this work, our genetic analyses prove that P4H5, and to a lesser extent P4H2 and P4H13, are pivotal for root hair tip growth. Second, we demonstrate that P4H5 has in vitro preferred specificity for EXT substrates rather than for other HRGPs. Third, by P4H promoter and protein swapping approaches, we show that P4H2 and P4H13 have interchangeable functions but cannot replace P4H5. These three P4Hs are shown to be targeted to the secretory pathway, where P4H5 forms dimers with P4H2 and P4H13. Finally, we explore the impact of deficient proline hydroxylation on the cell wall architecture. Taken together, our results support a model in which correct peptidyl-proline hydroxylation on EXTs, and possibly in other HRGPs, is required for proper cell wall self-assembly and hence root hair elongation in Arabidopsis thaliana.

Published

2015

14. Glycoproteomic analysis of seven major allergenic proteins reveals novel post-translational modifications

Author

Carl Erik Olsen, Hans H. Wandall, Bent O. Petersen, Sergey Y. Vakhrushev, Jens Brimnes, Peter Adler Würtzen, Henrik Ipsen, Svenning Rune Møller, Caroline B. Madsen, Adnan Halim, Stephanie Brand, and Michael C. Carlsson

Subjects

Glycan, Allergy, medicine.medical_treatment, Computational biology, medicine.disease_cause, Orbitrap, Biochemistry, Mass Spectrometry, Analytical Chemistry, law.invention, Immune system, Allergen, Antigen, law, immune system diseases, Polysaccharides, medicine, otorhinolaryngologic diseases, Antigens, Dermatophagoides, Molecular Biology, Betula, Desensitization (medicine), Plant Proteins, House dust mite, biology, Chemistry, Research, food and beverages, Allergens, Antigens, Plant, biology.organism_classification, medicine.disease, respiratory tract diseases, Phleum, Immunology, biology.protein, Pollen, Protein Processing, Post-Translational

Abstract

Allergenic proteins such as grass pollen and house dust mite (HDM) proteins are known to trigger hypersensitivity reactions of the immune system, leading to what is commonly known as allergy. Key allergenic proteins including sequence variants have been identified but characterization of their post-translational modifications (PTMs) is still limited. Here, we present a detailed PTM(1) characterization of a series of the main and clinically relevant allergens used in allergy tests and vaccines. We employ Orbitrap-based mass spectrometry with complementary fragmentation techniques (HCD/ETD) for site-specific PTM characterization by bottom-up analysis. In addition, top-down mass spectrometry is utilized for targeted analysis of individual proteins, revealing hitherto unknown PTMs of HDM allergens. We demonstrate the presence of lysine-linked polyhexose glycans and asparagine-linked N-acetylhexosamine glycans on HDM allergens. Moreover, we identified more complex glycan structures than previously reported on the major grass pollen group 1 and 5 allergens, implicating important roles for carbohydrates in allergen recognition and response by the immune system. The new findings are important for understanding basic disease-causing mechanisms at the cellular level, which ultimately may pave the way for instigating novel approaches for targeted desensitization strategies and improved allergy vaccines.

Published

2014

15. Assignment of saccharide identities through analysis of oxonium ion fragmentation profiles in LC-MS/MS of glycopeptides

Author

Carina Sihlbom, Adnan Halim, Christian Pett, Göran Larson, Jonas Nilsson, Manuel Schorlemer, Ulla Rüetschi, Johan Lengqvist, Gunnar Brinkmalm, and Ulrika Westerlind

Subjects

Proteomics, Glycan, Glycosylation, Proteome, Stereochemistry, Molecular Sequence Data, Oligosaccharides, Mass spectrometry, Biochemistry, Onium Compounds, Fragmentation (mass spectrometry), Polysaccharides, Tandem Mass Spectrometry, Structural isomer, Amino Acid Sequence, biology, Molecular Structure, Chemistry, Glycopeptides, General Chemistry, Glycopeptide, Glycoproteomics, Carbohydrate Sequence, biology.protein, Ion trap, Oxonium ion, Chromatography, Liquid

Abstract

Protein glycosylation plays critical roles in the regulation of diverse biological processes, and determination of glycan structure-function relationships is important to better understand these events. However, characterization of glycan and glycopeptide structural isomers remains challenging and often relies on biosynthetic pathways being conserved. In glycoproteomic analysis with liquid chromatography-tandem mass spectrometry (LC-MS/MS) using collision-induced dissociation (CID), saccharide oxonium ions containing N-acetylhexosamine (HexNAc) residues are prominent. Through analysis of beam-type CID spectra and ion trap CID spectra of synthetic and natively derived N- and O-glycopeptides, we found that the fragmentation patterns of oxonium ions characteristically differ between glycopeptides terminally substituted with GalNAcα1-O-, GlcNAcβ1-O-, Galβ3GalNAcα1-O-, Galβ4GlcNAcβ-O-, and Galβ3GlcNAcβ-O- structures. The difference in the oxonium ion fragmentation profiles of such glycopeptides may thus be used to distinguish among these glycan structures and could be of importance in LC-MS/MS-based glycoproteomic studies.

Published

2014

16. Enrichment of glycopeptides for glycan structure and attachment site identification

Author

Ulla Rüetschi, Adnan Halim, Elisabet Carlsohn, Jonas Nilsson, Gunnar Brinkmalm, Camilla Hesse, and Göran Larson

Subjects

Proteomics, Glycan, Glycosylation, Tandem mass spectrometry, Biochemistry, chemistry.chemical_compound, Polysaccharides, Tandem Mass Spectrometry, Humans, Peptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase, Molecular Biology, Peptide sequence, Glycoproteins, chemistry.chemical_classification, biology, Glycopeptides, Cerebrospinal Fluid Proteins, Glycosidic bond, Cell Biology, Sialic acid, carbohydrates (lipids), chemistry, biology.protein, Glycoprotein, Biotechnology

Abstract

We present a method to enrich for glycoproteins from proteomic samples. Sialylated glycoproteins were selectively periodate-oxidized, captured on hydrazide beads, trypsinized and released by acid hydrolysis of sialic acid glycosidic bonds. Mass spectrometric fragment analysis allowed identification of glycan structures, and additional fragmentation of deglycosylated ions yielded peptide sequence information, which allowed glycan attachment site and protein identification. We identified 36 N-linked and 44 O-linked glycosylation sites on glycoproteins from human cerebrospinal fluid.

Published

2009

17. Interlaboratory Study on Differential Analysis of Protein Glycosylation by Mass Spectrometry: The ABRF Glycoprotein Research Multi-Institutional Study 2012

Author

Uwe Möginger, Carthene R. Bazemore-Walker, Lauren E. Ball, Benjamin F. Mann, Jan Mirco Schulz, Carina Sihlbom, David Horn, Eden P. Go, Jeffrey S. Rohrer, Lipika Basumallick, Gregory O. Staples, Manfred Wuhrer, Detlev Suckau, Jonas Nilsson, Wolfgang Jabs, Richard R. Drake, Deanna C. Hurum, Christian Neusüβ, Christopher W. Cairo, Bernd Meyer, Leena Valmu, F. Altmann, Petr Pompach, William R. Alley, Michael Blank, Nancy Leymarie, Yoshinao Wada, Adnan Halim, Mellisa Ly, Daniel Kolarich, Randy M. Whittal, Yetrib Hathout, Milos V. Novotny, Jennifer T. Aguilan, Rambod Daneshfar, Joseph Zaia, Svenja-Catharina Bunz, Paul J. Hensbergen, Morten Thaysen-Andersen, Kristy J. Brown, John F. Cipollo, Clemens Gruber, Yehia Mechref, Alexandra Ruthenbeck, Megan T. Watson, Anja Resemann, Yiying Zhu, Radoslav Goldman, Markus Windwarder, Chunxia Zou, Yanming An, Henning N. Behnken, Haixu Tang, Rosa Viner, Béla Reiz, Ulrike Schweiger-Hufnagel, Nicolle H. Packer, Heather Desaire, Paula J. Griffin, Kristina Marx, Miloslav Sanda, Ron Orlando, Göran Larson, Julius O. Nyalwidhe, Karen R. Jonscher, Mark E. McComb, and Ehwang Song

Subjects

Proteomics, Glycan, Glycosylation, Computational biology, Mass spectrometry, Bioinformatics, Biochemistry, Mass Spectrometry, Analytical Chemistry, Glycomics, chemistry.chemical_compound, Polysaccharides, Humans, Molecular Biology, Tumor marker, Glycoproteins, biology, Chemistry, Research, Reproducibility of Results, Prostate-Specific Antigen, Glycoproteomics, Prostate-specific antigen, biology.protein, Kallikreins, Laboratories, Chromatography, Liquid

Abstract

One of the principal goals of glycoprotein research is to correlate glycan structure and function. Such correlation is necessary in order for one to understand the mechanisms whereby glycoprotein structure elaborates the functions of myriad proteins. The accurate comparison of glycoforms and quantification of glycosites are essential steps in this direction. Mass spectrometry has emerged as a powerful analytical technique in the field of glycoprotein characterization. Its sensitivity, high dynamic range, and mass accuracy provide both quantitative and sequence/structural information. As part of the 2012 ABRF Glycoprotein Research Group study, we explored the use of mass spectrometry and ancillary methodologies to characterize the glycoforms of two sources of human prostate specific antigen (PSA). PSA is used as a tumor marker for prostate cancer, with increasing blood levels used to distinguish between normal and cancer states. The glycans on PSA are believed to be biantennary N-linked, and it has been observed that prostate cancer tissues and cell lines contain more antennae than their benign counterparts. Thus, the ability to quantify differences in glycosylation associated with cancer has the potential to positively impact the use of PSA as a biomarker. We studied standard peptide-based proteomics/glycomics methodologies, including LC-MS/MS for peptide/glycopeptide sequencing and label-free approaches for differential quantification. We performed an interlaboratory study to determine the ability of different laboratories to correctly characterize the differences between glycoforms from two different sources using mass spectrometry methods. We used clustering analysis and ancillary statistical data treatment on the data sets submitted by participating laboratories to obtain a consensus of the glycoforms and abundances. The results demonstrate the relative strengths and weaknesses of top-down glycoproteomics, bottom-up glycoproteomics, and glycomics methods.

Published

2013

18. Mining the O-mannose glycoproteome reveals cadherins as major O-mannosylated glycoproteins

Author

Henrik Clausen, Hiren J. Joshi, Malene Bech Vester-Christensen, Adnan Halim, Steven B. Levery, Sergey Y. Vakhrushev, Eric P. Bennett, and Catharina Steentoft

Subjects

chemistry.chemical_classification, Glycan, animal structures, Multidisciplinary, Glycosylation, biology, Cadherin, Cell adhesion molecule, Plexin, Mannose, Biological Sciences, Cell biology, carbohydrates (lipids), chemistry.chemical_compound, chemistry, biology.protein, Glycoprotein, Cell adhesion

Abstract

The metazoan O-mannose (O-Man) glycoproteome is largely unknown. It has been shown that up to 30% of brain O-glycans are of the O-Man type, but essentially only alpha-dystroglycan (α-DG) of the dystrophin–glycoprotein complex is well characterized as an O-Man glycoprotein. Defects in O-Man glycosylation underlie congenital muscular dystrophies and considerable efforts have been devoted to explore this O-glycoproteome without much success. Here, we used our SimpleCell strategy using nuclease-mediated gene editing of a human cell line (MDA-MB-231) to reduce the structural heterogeneity of O-Man glycans and to probe the O-Man glycoproteome. In this breast cancer cell line we found that O-Man glycosylation is primarily found on cadherins and plexins on β-strands in extracellular cadherin and Ig-like, plexin and transcription factor domains. The positions and evolutionary conservation of O-Man glycans in cadherins suggest that they play important functional roles for this large group of cell adhesion glycoproteins, which can now be addressed. The developed O-Man SimpleCell strategy is applicable to most types of cell lines and enables proteome-wide discovery of O-Man protein glycosylation.

Published

2013

19. LC-MS/MS characterization of O-glycosylation sites and glycan structures of human cerebrospinal fluid glycoproteins

Author

Göran Larson, Ulla Rüetschi, Adnan Halim, and Jonas Nilsson

Subjects

PNGase F, Threonine, Glycan, Spectrometry, Mass, Electrospray Ionization, Glycosylation, Molecular Sequence Data, Molecular Conformation, Tandem mass spectrometry, Biochemistry, Receptors, G-Protein-Coupled, Glycomics, chemistry.chemical_compound, Apolipoproteins E, Hemopexin, Polysaccharides, Serine, Humans, Peptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase, Trypsin, Amino Acid Sequence, Cerebrospinal Fluid, Glycoproteins, chemistry.chemical_classification, biology, Chemistry, Membrane Proteins, Receptor Protein-Tyrosine Kinases, General Chemistry, Glycopeptide, Sialic acid, carbohydrates (lipids), biology.protein, Glycoprotein, Chromatography, Liquid

Abstract

The GalNAc O-glycosylation on Ser/Thr residues of extracellular proteins has not been well characterized from a proteomics perspective. We previously reported a sialic acid capture-and-release protocol to enrich tryptic N- and O-glycopeptides from human cerebrospinal fluid glycoproteins using nano-LC-ESI-MS/MS with collision-induced dissociation (CID) for glycopeptide characterization. Here, we have introduced peptide N-glycosidase F (PNGase F) pretreatment of CSF samples to remove the N-glycans facilitating the selective characterization of O-glycopeptides and enabling the use of an automated CID-MS(2)/MS(3) search protocol for glycopeptide identification. We used electron-capture and -transfer dissociation (ECD/ETD) to pinpoint the glycosylation site(s) of the glycopeptides, identified as predominantly core-1-like HexHexNAc-O- structure attached to one to four Ser/Thr residues. We characterized 106 O-glycosylations and found Pro residues preferentially in the n - 1, n + 1, and/or n + 3 positions in relation to the Ser/Thr attachment site (n). The characterization of glycans and glycosylation sites in glycoproteins from human clinical samples provides a basis for future studies addressing the biological and diagnostic importance of specific protein glycosylations in relation to human disease.

Published

2012

20. Human urinary glycoproteomics; attachment site specific analysis of N- and O-linked glycosylations by CID and ECD

Author

Camilla Hesse, Göran Larson, Ulla Rüetschi, Adnan Halim, and Jonas Nilsson

Subjects

Male, Proteomics, Glycan, Glycosylation, Tandem mass spectrometry, Biochemistry, Analytical Chemistry, chemistry.chemical_compound, Tandem Mass Spectrometry, medicine, Humans, Molecular Biology, Glycoproteins, chemistry.chemical_classification, Electron-capture dissociation, biology, Research, Glycopeptides, Trypsin, Glycopeptide, N-Acetylneuraminic Acid, Glycoproteomics, chemistry, biology.protein, Glycoprotein, Dialysis, medicine.drug, Chromatography, Liquid

Abstract

Urine is a complex mixture of proteins and waste products and a challenging biological fluid for biomarker discovery. Previous proteomic studies have identified more than 2800 urinary proteins but analyses aimed at unraveling glycan structures and glycosylation sites of urinary glycoproteins are lacking. Glycoproteomic characterization remains difficult because of the complexity of glycan structures found mainly on asparagine (N-linked) or serine/threonine (O-linked) residues. We have developed a glycoproteomic approach that combines efficient purification of urinary glycoproteins/glycopeptides with complementary MS-fragmentation techniques for glycopeptide analysis. Starting from clinical sample size, we eliminated interfering urinary compounds by dialysis and concentrated the purified urinary proteins by lyophilization. Sialylated urinary glycoproteins were conjugated to a solid support by hydrazide chemistry and trypsin digested. Desialylated glycopeptides, released through mild acid hydrolysis, were characterized by tandem MS experiments utilizing collision induced dissociation (CID) and electron capture dissociation fragmentation techniques. In CID-MS(2), Hex(5)HexNAc(4)-N-Asn and HexHexNAc-O-Ser/Thr were typically observed, in agreement with known N-linked biantennary complex-type and O-linked core 1-like structures, respectively. Additional glycoforms for specific N- and O-linked glycopeptides were also identified, e.g. tetra-antennary N-glycans and fucosylated core 2-like O-glycans. Subsequent CID-MS(3), of selected fragment-ions from the CID-MS(2) analysis, generated peptide specific b- and y-ions that were used for peptide identification. In total, 58 N- and 63 O-linked glycopeptides from 53 glycoproteins were characterized with respect to glycan- and peptide sequences. The combination of CID and electron capture dissociation techniques allowed for the exact identification of Ser/Thr attachment site(s) for 40 of 57 putative O-glycosylation sites. We defined 29 O-glycosylation sites which have, to our knowledge, not been previously reported. This is the first study of human urinary glycoproteins where "intact" glycopeptides were studied, i.e. the presence of glycans and their attachment sites were proven without doubt.

Published

2011

21. Involvement of viral glycoprotein gC-1 in expression of the selectin ligand sialyl-Lewis X induced after infection with herpes simplex virus type 1

Author

Sigvard Olofsson, Göran Larson, Jonas Nilsson, Kristina Nyström, Rickard Nordén, Adnan Halim, Edward Trybala, and Beata Adamiak

Subjects

Microbiology (medical), Glycan, Fucosyltransferase, Glycosylation, Glycoconjugate, Lewis X Antigen, Herpesvirus 1, Human, medicine.disease_cause, Ligands, Pathology and Forensic Medicine, chemistry.chemical_compound, Viral Envelope Proteins, medicine, Immunology and Allergy, Humans, Sialyl Lewis X Antigen, chemistry.chemical_classification, biology, Mucin, Mucins, General Medicine, Fibroblasts, Fucosyltransferases, Molecular biology, Herpes simplex virus, Sialyl-Lewis X, chemistry, biology.protein, Glycoprotein, Selectin

Abstract

Several herpesviruses induce expression of the selectin receptor sialyl-Lewis X (sLe(x) ) by activating transcription of one or more of silent host FUT genes, each one encoding a fucosyltransferase that catalyses the rate-limiting step of sLe(x) synthesis. The aim here was to identify the identity of the glycoconjugate associated with sLe(x) glycoepitope in herpes simplex virus type 1 (HSV-1) infected human diploid fibroblasts, using immunofluorescence confocal microscopy. Cells infected with all tested HSV-1 strains analysed demonstrated bright sLe(x) fluorescence, except for two mutant viruses that were unable to induce proper expression of viral glycoprotein gC-1: One gC-1 null mutant and another mutant expressing gC-1 devoid of its major O-glycan-containing region (aa 33-116). The sLe(x) reactivity of HSV-1 infected cells was abolished by mild alkali treatment. Altogether the results indicated that the detectable sLe(x) was associated with O-linked glycans, situated in the mucin region of gC-1. No evidence for sLe(x) (i) in other HSV-1 glycoproteins with mucin domains such as gI-1 or (ii) in host cell glycoproteins/glycolipids was found. Thus, the mucin domain of HSV-1 gC-1 may support expression of selectin ligands such as sLe(x) and other larger O-linked glycans in cell types lacking endogenous mucin domain-containing glycoproteins, optimized for O-glycan expression, provided that the adequate host glycosyltransferase genes are activated.

Published

2011

22. Novel Leb-like Helicobacter pylori-binding glycosphingolipid created by the expression of human alpha-1,3/4-fucosyltransferase in FVB/N mouse stomach

Author

Susann Teneberg, Adnan Halim, Thomas Borén, Lennart Hammarström, Jonas Ångström, Anna Hultberg, Lena Rakhimova, and David Fagerberg

Subjects

Genetically modified mouse, Alpha (ethology), Mice, Transgenic, Biochemistry, Glycosphingolipids, Mass Spectrometry, chemistry.chemical_compound, Mice, medicine, Animals, Humans, Beta (finance), Glycoproteins, chemistry.chemical_classification, FVB/N Mouse, Binding Sites, biology, Helicobacter pylori, Stomach, Glycosphingolipid, Fucosyltransferases, Epithelium, carbohydrates (lipids), medicine.anatomical_structure, chemistry, Gastric Mucosa, biology.protein, lipids (amino acids, peptides, and proteins), Antibody, Glycoprotein

Abstract

The "Le(b) mouse" was established as a model for investigations of the molecular events following Le(b)-mediated adhesion of Helicobacter pylori to the gastric epithelium. By the expression of a human alpha-1,3/4-fucosyltransferase in the gastric pit cell lineage of FVB/N transgenic mice, a production of Le(b) glycoproteins in gastric pit and surface mucous cells was obtained in this "Le(b) mouse," as demonstrated by binding of monoclonal anti-Le(b) antibodies. To explore the effects of the human alpha-1,3/4-fucosyltransferase on glycosphingolipid structures, neutral glycosphingolipids were isolated from stomachs of transgenic alpha-1,3/4-fucosyltransferase-expressing mice. A glycosphingolipid recognized by BabA-expressing H. pylori was isolated and characterized by mass spectrometry and proton NMR as Fuc alpha 2Gal beta 3(Fuc alpha 4)GalNAc beta 4 Gal beta 4 Glc beta 1Cer, i.e., a novel Le(b)-like glycosphingolipid on a ganglio core. In addition, two other novel glycosphingolipids were isolated from the mouse stomach epithelium that were found to be nonbinding with regard to H. pylori. The first was a pentaglycosylceramide, GalNAc beta 3 Gal alpha 3(Fuc alpha 2)Gal beta 4 Glc beta 1Cer, in which the isoglobotetrasaccharide has been combined with Fuc alpha 2 to yield an isoglobotetraosylceramide with an internal blood group B determinant. The second one was an elongated fucosyl-gangliotetraosylceramide, GalNAc beta 3(Fuc alpha 2)Gal beta 3GalNAc beta 4Gal beta 4 Glc beta 1Cer.

Published

2008

23. Discovery of an O-mannosylation pathway selectively serving cadherins and protocadherins

Author

Henrik Clausen, Ida Signe Bohse Larsen, Kerry M. Goodman, Barry Honig, Lawrence Shapiro, Julia Brasch, Hiren J. Joshi, Adnan Halim, Sergey Y. Vakhrushev, Yoshiki Narimatsu, Lars Hansen, Lina Siukstaite, and O.J. Harrison

Subjects

0301 basic medicine, Glycan, animal structures, Glycosylation, Protocadherin, Mannose, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Humans, Multidisciplinary, biology, Cadherin, Cell adhesion molecule, HEK 293 cells, Glycosyltransferases, Membrane Proteins, Biological Sciences, Cadherins, carbohydrates (lipids), 030104 developmental biology, HEK293 Cells, chemistry, Biochemistry, Hepatocyte Growth Factor Receptor, Multigene Family, biology.protein, Carrier Proteins, 030217 neurology & neurosurgery

Abstract

The cadherin (cdh) superfamily of adhesion molecules carry O-linked mannose (O-Man) glycans at highly conserved sites localized to specific β-strands of their extracellular cdh (EC) domains. These O-Man glycans do not appear to be elongated like O-Man glycans found on α-dystroglycan (α-DG), and we recently demonstrated that initiation of cdh/protocadherin (pcdh) O-Man glycosylation is not dependent on the evolutionary conserved POMT1/POMT2 enzymes that initiate O-Man glycosylation on α-DG. Here, we used a CRISPR/Cas9 genetic dissection strategy combined with sensitive and quantitative O-Man glycoproteomics to identify a homologous family of four putative protein O-mannosyltransferases encoded by the TMTC1–4 genes, which were found to be imperative for cdh and pcdh O-Man glycosylation. KO of all four TMTC genes in HEK293 cells resulted in specific loss of cdh and pcdh O-Man glycosylation, whereas combined KO of TMTC1 and TMTC3 resulted in selective loss of O-Man glycans on specific β-strands of EC domains, suggesting that each isoenzyme serves a different function. In addition, O-Man glycosylation of IPT/TIG domains of plexins and hepatocyte growth factor receptor was not affected in TMTC KO cells, suggesting the existence of yet another O-Man glycosylation machinery. Our study demonstrates that regulation of O-mannosylation in higher eukaryotes is more complex than envisioned, and the discovery of the functions of TMTCs provide insight into cobblestone lissencephaly caused by deficiency in TMTC3.

24. Targeting the glycoproteome

Author

Göran Larson, Jonas Nilsson, Ammi Grahn, and Adnan Halim

Subjects

Glycan, Glycosylation, Proteome, Tandem mass spectrometry, Liquid chromatography, High resolution, Computational biology, Polypeptide chain, Glycopeptide, Models, Biological, Biochemistry, Mass Spectrometry, Article, chemistry.chemical_compound, Humans, Amino acid residue, Molecular Biology, Cells, Cultured, Glycoproteins, chemistry.chemical_classification, biology, Glycopeptides, Cell Biology, Glycoproteomics, Lectin affinity, chemistry, Enrichment, biology.protein, Glycoprotein, Hydrophobic and Hydrophilic Interactions, Attachment sites, Hydrazide chemistry, Chromatography, Liquid

Abstract

Despite numerous original publications describing the structural complexity of N- and O-linked glycans on glycoproteins, only very few answer the basic question of which particular glycans are linked to which amino acid residues along the polypeptide chain. Such structural information is of fundamental importance for understanding the biological roles of complex glycosylations as well as deciphering their non-template driven biosynthesis. This review focuses on presenting and commenting on recent strategies, specifically aimed at identifying the glycoproteome of cultured cells and biological samples, using targeted and global enrichment procedures and utilizing the high resolution power, high through-put capacity and complementary fragmentation techniques of tandem mass spectrometry. The goal is to give an update of this emerging field of protein and glyco-sciences and suggest routes to bridge the data gap between the two aspects of glycoprotein characteristics, i.e. glycan structures and their attachment sites.