Your search keyword '"Blixt, Ola"' showing total 533 results

201. Additional file 4 of Autoantibodies to aberrantly glycosylated MUC1 in early stage breast cancer are associated with a better prognosis

Author

Blixt, Ola, Bueti, Deanna, Burford, Brian, Allen, Diane, Julien, Sylvain, Hollingsworth, Michael, Gammerman, Alex, Fentiman, Ian, Taylor-Papadimitriou, Joyce, and Burchell, Joy M

Subjects

3. Good health

Abstract

Additional file 4: Supplementary Figure 3. Clinical characteristics of the 395 breast cancer patients who donated sera for the study. Time to metastasis of the breast cancer cohort related to clinical tumour size, lymph nodes positivity, age at diagnosis and tumour grade. (PDF 170 KB)

202. Additional file 11 of Autoantibodies to aberrantly glycosylated MUC1 in early stage breast cancer are associated with a better prognosis

Author

Blixt, Ola, Bueti, Deanna, Burford, Brian, Allen, Diane, Julien, Sylvain, Hollingsworth, Michael, Gammerman, Alex, Fentiman, Ian, Taylor-Papadimitriou, Joyce, and Burchell, Joy M

Subjects

Data_FILES, 3. Good health

Abstract

Authors’ original file for figure 6

203. Additional file 5 of Autoantibodies to aberrantly glycosylated MUC1 in early stage breast cancer are associated with a better prognosis

Author

Blixt, Ola, Bueti, Deanna, Burford, Brian, Allen, Diane, Julien, Sylvain, Hollingsworth, Michael, Gammerman, Alex, Fentiman, Ian, Taylor-Papadimitriou, Joyce, and Burchell, Joy M

Subjects

skin and connective tissue diseases, 3. Good health

Abstract

Additional file 5: Supplementary Figure 4. Expression of B3GNT6 in breast cancers. qRT-PCR of B3GNT6 in 58 primary breast cancers. (PDF 86 KB)

204. Additional file of Autoantibodies to aberrantly glycosylated MUC1 in early stage breast cancer are associated with a better prognosis

Author

Blixt, Ola, Bueti, Deanna, Burford, Brian, Allen, Diane, Julien, Sylvain, Hollingsworth, Michael, Gammerman, Alex, Fentiman, Ian, Taylor-Papadimitriou, Joyce, and Burchell, Joy M

Subjects

carbohydrates (lipids), lipids (amino acids, peptides, and proteins), skin and connective tissue diseases, neoplasms, digestive system diseases, 3. Good health

Abstract

Additional file of Autoantibodies to aberrantly glycosylated MUC1 in early stage breast cancer are associated with a better prognosis

205. Additional file 7 of Autoantibodies to aberrantly glycosylated MUC1 in early stage breast cancer are associated with a better prognosis

Author

Blixt, Ola, Bueti, Deanna, Burford, Brian, Allen, Diane, Julien, Sylvain, Hollingsworth, Michael, Gammerman, Alex, Fentiman, Ian, Taylor-Papadimitriou, Joyce, and Burchell, Joy M

Subjects

Data_FILES, 3. Good health

Abstract

Authors’ original file for figure 2

206. Additional file 1 of Autoantibodies to aberrantly glycosylated MUC1 in early stage breast cancer are associated with a better prognosis

Author

Blixt, Ola, Bueti, Deanna, Burford, Brian, Allen, Diane, Julien, Sylvain, Hollingsworth, Michael, Gammerman, Alex, Fentiman, Ian, Taylor-Papadimitriou, Joyce, and Burchell, Joy M

Subjects

3. Good health

Abstract

Additional file 1: Supplementary Table 1. Description of MUC1 glycoforms printed onto the slides. Table describing the glycopeptides printed onto the microarrays used to screen the large cohorts. (PDF 52 KB)

207. Host range of influenza A virus H1 to H16 in dabbling vs. diving ducks based on tissue and receptor binding studies

Author

Verhagen, Josanne H., Eriksson, Per, Leijten, Lonneke, Blixt, Ola, Ellström, Patrik, Olsen, Björn, Kuiken, Thijs, Waldenström, Jonas, Verhagen, Josanne H., Eriksson, Per, Leijten, Lonneke, Blixt, Ola, Ellström, Patrik, Olsen, Björn, Kuiken, Thijs, and Waldenström, Jonas

208. Assessing the interspecies transmission mechanisms of influenza A viruses

Author

Naguib, Mahmoud M., Eriksson, Per, Jax, Elinor, Nilsson, Jonas, Sihlbom, Carina, Olsson, Britt-Marie, Verhagen, Josanne H., Wille, Michelle, Waldenström, Jonas, Blixt, Ola, Larson, Göran, Kraus, Robert H.S., Lundkvist, Åke, Olsen, Björn, Järhult, Josef D., Ellström, Patrik, Naguib, Mahmoud M., Eriksson, Per, Jax, Elinor, Nilsson, Jonas, Sihlbom, Carina, Olsson, Britt-Marie, Verhagen, Josanne H., Wille, Michelle, Waldenström, Jonas, Blixt, Ola, Larson, Göran, Kraus, Robert H.S., Lundkvist, Åke, Olsen, Björn, Järhult, Josef D., and Ellström, Patrik

209. Clinical isolates of Helicobacter pylori demonstrates alternative BabA-mediated adherence to human gastric mucosa

Author

Henriksson, Sara, Mendez, Melissa, Bugaytsova, Jeanna, Brännström, Kristoffer, Nordén, Jenny, Berg, Douglas E, Blixt, Ola, Teneberg, Susann, Borén, Thomas, Henriksson, Sara, Mendez, Melissa, Bugaytsova, Jeanna, Brännström, Kristoffer, Nordén, Jenny, Berg, Douglas E, Blixt, Ola, Teneberg, Susann, and Borén, Thomas

Abstract

Helicobacter pylori infection is life-long and can cause peptic ulcer disease and gastric cancer. The H. pylori BabA adhesin binds the ABO/Leb blood group (bg) antigens (Leb), which mediates attachment to the gastric epithelium. The prevalence of ABO binding is high worldwide and also in northern Europe. However, prevalence is reduced by 50% in Germany and is further reduced in Spain and Portugal. An inventory of strains from different European populations resulted in strains with high level of BabA expression but very little or no binding to Leb. The majority of such strains could not bind to human gastric mucosa in vitro. We further characterized a Spanish isolates, strain 812, that binds only weakly to soluble Leb-conjugate but still adheres firmly to gastric mucosa indicative of that it might bind to an alternative set of receptor. Receptor analysis by glycan arrays revealed higher binding of strain 812 to ALeb and Bleb glycans than to Leb, indicating that BabA from strain 812 has shifted its binding epitope somewhat away from the central Fuca1.2Gal bg domain and closer to the very terminal bg A and B determinants, i.e. GalNAca1.3Gal (bgA) or the Gala1.3Gal (bgB). By a colony screening approach we identified a subpopulation of 812 clones adapted for stronger Leb binding. Such affinity shifts comes from replacement of distinguishing amino acids by mechanisms of recombination with a BabA-related outer membrane protein.

210. Characterization of avian influenza virus attachment patterns to human and pig tissues.

Author

Eriksson, Per, Lindskog, Cecilia, Engholm, Ebbe, Blixt, Ola, Waldenström, Jonas, Munster, Vincent, Lundkvist, Åke, Olsen, Björn, Jourdain, Elsa, and Ellström, Patrik

Abstract

Wild birds of Anseriformes and Charadriiformes are natural reservoirs of influenza A viruses (IAVs). Occasionally, IAVs transmit and adapt to mammalian hosts, and are maintained as epidemic strains in their new hosts. Viral adaptions to mammalian hosts include altered receptor preference of host epithelial sialylated oligosaccharides from terminal α2,3-linked sialic acid (SA) towards α2,6-linked SA. However, α2,3-linked SA has been found in human respiratory tract epithelium, and human infections by avian IAVs (AIVs) have been reported. To further explore the attachment properties of AIVs, four AIVs of different subtypes were investigated on human and pig tissues using virus histochemistry. Additionally, glycan array analysis was performed for further characterization of IAVs’ receptor structure tropism. Generally, AIV attachment was more abundant to human tissues than to pig tissues. The attachment pattern was very strong to human conjunctiva and upper respiratory tract, but variable to the lower respiratory tract. AIVs mainly attached to α2,3-linked SA, but also to combinations of α2,3- and α2,6-linked SA. The low attachment of these AIV isolates to pig tissues, but high attachment to human tissues, addresses the question whether AIVs in general require passage through pigs to obtain adaptions towards mammalian receptor structures. [ABSTRACT FROM AUTHOR]

Published

2018

211. Antibody Recognition of a Carbohydrate Epitope: A Template for HIV Vaccine Design.

Author

Scanlan, Chris, Calarese, Daniel, Lee, Hing-Ken, Blixt, Ola, Wong, Chi-Huey, Wilson, Ian, Burton, Dennis, Dwek, Raymond, and Rudd, Pauline

Published

2005

212. Editorial.

Author

Blixt, Ola

Published

2008

213. Arraying glycomics: a novel bi-functional spacer for one-step microscale derivatization of free reducing glycans.

Author

Bohorov, Ognian, Andersson-Sand, Hillevi, Hoffmann, Julia, and Blixt, Ola

Abstract

Glycan array development is limited by the complexity of efficiently generating derivatives of free reducing glycans with primary amines or other functional groups. A novel bi-functional spacer with selective reactivity toward the free glycan and a second functionality, a primary amine, was synthesized. We demonstrated an efficient one-step derivatization of various glycans including naturally isolated N-glycans, O-glycans, milk oligosaccharides, and bacterial polysaccharides in microgram scale. No protecting group manipulations or activation of the anomeric center was required. To demonstrate its utility for glycan microarray fabrication, we compared glycans with different amine-spacers for incorporation onto an amine-reactive glass surface. Our study results revealed that glycans conjugated with this bi-functional linker were effectively printed and detected with various lectins and antibodies. [ABSTRACT FROM PUBLISHER]

Published

2006

214. Identification of Ligand Specificities for Glycan-Binding Proteins Using Glycan Arrays.

Author

Alvarez, Richard A. and Blixt, Ola

Abstract

An abstract of the article "Identification of Ligand Specificities for Glycan-Binding Proteins Using Glycan Arrays," by Richard A. Alvarez and Ola Blixt is presented.

Published

2006

215. Chemoenzymatic Synthesis of Glycan Libraries.

Author

Blixt, Ola and Razi, Nahid

Abstract

An abstract of the article "Chemoenzymatic Synthesis of Glycan Libraries," by Ola Blixt and Nahid Razi is presented.

Published

2006

216. Synthesis of Sugar Arrays in Microtiter Plate.

Author

Fazio, Fabio, Bryan, Marian C., Blixt, Ola, Paulson, James C., and Wong, Chi-Huey

Subjects

*RING formation (Chemistry), *ALKYNES, *AZIDES

Abstract

Studies the synthesis of sugar arrays in microtiter plate. Standard conditions for the construction of the triazole ring; Copper-catalyzed regiospecific 1,3-cyclo-addition between terminal alkynes and azides; Advantages of thermal formation.

Published

2002

217. Reversible derivatization of sugars with carbobenzyloxy groups and use of the derivatives in solution-phase enzymatic oligosaccharide synthesis.

Author

Norberg, Thomas, Kallin, Elisabet, and Blixt, Ola

Subjects

*DERIVATIZATION, *SUGARS, *TRANSFER hydrogenation, *SOLID phase extraction, *CATALYTIC hydrogenation, *CATALYTIC hydrolysis

Abstract

Simple protocols for attaching and detaching carbobenzyloxy (Cbz) groups at the reducing end of sugars was developed. Briefly, lactose was converted into its glycosylamine, which was then acylated with carbobenzyloxy chloride in high overall yield. The obtained lactose Cbz derivative was used in sequential glycosylations using glycosyltransferases and nucleotide sugars in aqueous buffers. Isolation of the reaction products after each step was by simple C-18 solid-phase extraction. The Cbz group was removed by catalytic hydrogenolysis or catalytic transfer hydrogenation followed by in situ glycosylamine hydrolysis. In this way, a trisaccharide (GlcNAc-lactose), a human milk tetrasaccharide (LNnT), and a human milk pentasaccharide (LNFPIII) were prepared in a simple and efficient way. [Display omitted] • Reducing-end oligosaccharides were derivatized with an N-carbobenzyloxy (Cbz) group to form Cbz-oligosaccharides. • Simple Cbz oligosacchardes were enzymatically extended in several steps to form larger oligosaccharides. • Cbz oligosaccharides were easily separated from aqueous reaction mixtures by C18 solid-phase extraction. • Cbz oligosaccharides were easily converted back to reducing-end oligosaccharides. [ABSTRACT FROM AUTHOR]

Published

2021

218. Host Range of Influenza A Virus H1 to H16 in Eurasian Ducks Based on Tissue and Receptor Binding Studies.

Author

Verhagen, Josanne H., Eriksson, Per, Leijten, Lonneke, Blixt, Ola, Olsen, Björn, Waldenström, Jonas, Ellström, Patrik, and Kuiken, Thijs

Subjects

*INFLUENZA viruses, *INFLUENZA A virus, *MALLARD, *DUCK plague, *GLYCAN structure, *AVIAN anatomy, *OVERLAY dentures

Abstract

Dabbling and diving ducks partly occupy shared habitats but have been reported to play different roles in wildlife infectious disease dynamics. Influenza A virus (IAV) epidemiology in wild birds has been based primarily on surveillance programs focused on dabbling duck species, particularly mallard (Anas platyrhynchos). Surveillance in Eurasia has shown that in mallards, some subtypes are commonly (H1 to H7 and H10), intermediately (H8, H9, H11, and H12), or rarely (H13 to H16) detected, contributing to discussions on virus host range and reservoir competence. An alternative to surveillance in determining IAV host range is to study virus attachment as a determinant for infection. Here, we investigated the attachment patterns of all avian IAV subtypes (H1 to H16) to the respiratory and intestinal tracts of four dabbling duck species (Mareca and Anas spp.), two diving duck species (Aythya spp.), and chicken, as well as to a panel of 65 synthetic glycan structures. We found that IAV subtypes generally showed abundant attachment to colon of the Anas duck species, mallard, and Eurasian teal (Anas crecca), supporting the fecal-oral transmission route in these species. The reported glycan attachment profile did not explain the virus attachment patterns to tissues but showed significant attachment of duck-originated viruses to fucosylated glycan structures and H7 virus tropism for Neu5Gc-LN. Our results suggest that Anas ducks play an important role in the ecology and epidemiology of IAV. Further knowledge on virus tissue attachment, receptor distribution, and receptor binding specificity is necessary to understand the mechanisms underlying host range and epidemiology of IAV. [ABSTRACT FROM AUTHOR]

Published

2021

219. Structural characterization of an unprecedented lectin-like antitumoral anti-MUC1 antibody.

Author

Macías-León, Javier, Bermejo, Iris A., Asín, Alicia, García-García, Ana, Compañón, Ismael, Jiménez-Moreno, Ester, Coelho, Helena, Mangini, Vincenzo, Albuquerque, Inês S., Marcelo, Filipa, Asensio, Juan L., Bernardes, Gonçalo J. L., Joshi, Hiren J., Fiammengo, Roberto, Blixt, Ola, Hurtado-Guerrero, Ramón, and Corzana, Francisco

Subjects

*ANTI-antibodies, *CANCER vaccines, *LECTINS

Abstract

The molecular basis of antibody 5E5, which recognizes the entire GalNAc unit as a primary epitope is disclosed. The antibody's contacts with the peptide are mostly limited to two residues, allowing it to show some degree of promiscuity. These findings open the door to the chemical design of peptide-mimetics for developing efficient anti-cancer vaccines and diagnostic tools. [ABSTRACT FROM AUTHOR]

Published

2020

220. Specificity of human natural antibodies referred to as anti-Tn.

Author

Dobrochaeva, Kira, Khasbiullina, Nailya, Shilova, Nadezhda, Antipova, Nadezhda, Obukhova, Polina, Ovchinnikova, Tatiana, Galanina, Oxana, Blixt, Ola, Kunz, Horst, Filatov, Alexander, Knirel, Yuriy, LePendu, Jacques, Khaidukov, Sergey, and Bovin, Nicolai

Subjects

*GLYCANS, *IMMUNOGLOBULINS, *AMINO acid sequence, *IMMUNOGLOBULIN M, *OLIGOSACCHARIDES, *AFFINITY chromatography, *GLYCOPROTEINS

Abstract

• Isolated on GalNAcα-Sepharose human antibodies bind to GalNAcα glycopeptides weakly. • Bacterial polysaccharides lacking any GalNAcα structural motif are able to bind the antibodies. • The antibodies recognize a dis- rather than a canonical continuous epitope. To understand the role of human natural IgM known as antibodies against the carbohydrate epitope Tn, the antibodies were isolated using GalNAcα−Sepharose affinity chromatography, and their specificity was profiled using microarrays (a glycan array printed with oligosaccharides and bacterial polysaccharides, as well as a glycopeptide array), flow cytometry, and inhibition ELISA. The antibodies bound a restricted number of GalNAcα-terminated oligosaccharides better than the parent monosaccharide, e.g., 6-O-Su-GalNAcα and GalNAcα1−3Galβ1−3(4)GlcNAcβ. The binding with several bacterial polysaccharides that have no structural resemblance to the affinity ligand GalNAcα was quite unexpected. Given that GalNAcα is considered the key fragment of the Tn antigen, it is surprising that these antibodies bind weakly GalNAcα−OSer and do not bind a wide variety of GalNAcα−OSer/Thr-containing mucin glycopeptides. At the same time, we have observed specific binding to cells having Tn-positive glycoproteins containing similar glycopeptide motifs in a conformationally rigid macromolecule. Thus, specific recognition of the Tn antigen apparently requires that the naturally occurring "anti-Tn" IgM recognize a complex epitope comprising the GalNAcα as an essential component and a fairly long amino acid sequence where the amino acids adjacent to GalNAcα do not contact the antibody paratope; i.e., the antibodies recognize a spatial epitope or a molecular pattern rather than a classical continuous sequence. In addition, we have not found any increase in the binding of natural antibodies when GalNAcα residues were clustered. These results may help in further development of anticancer vaccines based on synthetic Tn constructs. [ABSTRACT FROM AUTHOR]

Published

2020

221. A novel monoclonal antibody to a defined peptide epitope in MUC16.

Author

Marcos-Silva, Lara, Ricardo, Sara, Chen, Kowa, Blixt, Ola, Arigi, Emma, Pereira, Daniela, Høgdall, Estrid, Mandel, Ulla, Bennett, Eric P., Vakhrushev, Sergey Y., David, Leonor, and Clausen, Henrik

Subjects

*MONOCLONAL antibodies, *EPITOPES, *TUMOR markers, *MUCINS, *GENETIC overexpression, *PEPTIDES

Abstract

The MUC16 mucin is overexpressed and aberrantly glycosylated in ovarian carcinomas. Immunodetection of circulating MUC16 is one of the most used cancer biomarker assays, but existing antibodies toMUC16 fail to distinguish normal and aberrant cancer glycoforms. Although all antibodies reactwith the tandem-repeat region, their epitopes appear to be conformational dependent and not definable by a short peptide. Aberrant glycoforms of MUC16 may constitute promising targets for diagnostic and immunotherapeutic intervention, and it is important to develop well-defined immunogens for induction of potent MUC16 immunity. Here, we developed a MUC16 vaccine based on a 1.7TR (264 aa) expressed in Escherichia coli and in vitro enzymatically glycosylated to generate the aberrant cancer- associated glycoform Tn. This vaccine elicited a potent serum IgG response in mice and we identified two major immunodominant linear peptide epitopes within the tandem repeat. We developed one monoclonal antibody, 5E11, reactive with a minimum epitope with the sequence FNTTER. This sequence contains potential N- and O-glycosylation sites and, interestingly, glycosylation blocked binding of 5E11. In immunochemistry of ovarian benign and cancer lesions, 5E11 showed similar reactivity as traditional MUC16 antibodies, suggesting that the epitope is not efficiently glycosylated. The study provides a vaccine design and immunodominant MUC16 TR epitopes. [ABSTRACT FROM AUTHOR]

Published

2015

222. RIFINs are adhesins implicated in severe Plasmodium falciparum malaria.

Author

Goel, Suchi, Palmkvist, Mia, Moll, Kirsten, Joannin, Nicolas, Lara, Patricia, R Akhouri, Reetesh, Moradi, Nasim, Öjemalm, Karin, Westman, Mattias, Angeletti, Davide, Kjellin, Hanna, Lehtiö, Janne, Blixt, Ola, Ideström, Lars, Gahmberg, Carl G, Storry, Jill R, Hult, Annika K, Olsson, Martin L, von Heijne, Gunnar, and Nilsson, IngMarie

Subjects

*MALARIA, *PLASMODIUM falciparum, *POLYPEPTIDES, *MICROBIAL adhesion, *BLOOD group antigens, *POLYMERASE chain reaction

Abstract

Rosetting is a virulent Plasmodium falciparum phenomenon associated with severe malaria. Here we demonstrate that P. falciparum-encoded repetitive interspersed families of polypeptides (RIFINs) are expressed on the surface of infected red blood cells (iRBCs), where they bind to RBCs-preferentially of blood group A-to form large rosettes and mediate microvascular binding of iRBCs. We suggest that RIFINs have a fundamental role in the development of severe malaria and thereby contribute to the varying global distribution of ABO blood groups in the human population. [ABSTRACT FROM AUTHOR]

Published

2015

223. Amplified suspension magnetic bead-based assay for sensitive detection of anti-glycan antibodies as potential cancer biomarkers.

Author

Blšákova, Anna, Květoň, Filip, Lorencová, Lenka, Blixt, Ola, Vikartovská, Alica, Kasak, Peter, and Tkac, Jan

Subjects

*MAGNETIC suspension, *GLYCANS, *TUMOR markers, *ENERGY dispersive X-ray spectroscopy, *SURFACE plasmon resonance, *IMMUNOGLOBULINS

Abstract

The development of a novel SUspension Magnetic-Bead-based Assay (SUMBA) for the detection of antibodies against aberrant glycans (AGA) as potential cancer biomarkers is presented here. The SUMBA method was extensively optimised by choosing proper commercially available AGA able to specifically, and with high affinity, recognise aberrant glycans, which were attached to the protein backbone working as a molecular scaffold (a glycoconjugate). The whole SUMBA was optimised using several analytical techniques such as Surface Plasmon Resonance and Energy Dispersive X-ray Spectroscopy. Additionally, the SUMBA method was extensively optimised for signal enhancement. With all steps optimised, we were able to detect AGA ultrasensitively with a limit of detection of 0.45 pM. Moreover, AGA could be detected in serum samples with a recovery index in the range of 98%–104%. SUMBA applied for detection of anti-glycan antibodies in serum samples. [Display omitted] • Application of magnetic beads modified with aberrant glycans for enrichment of AGA. • Use of polyHRP for signal enhancement. • A direct comparison of magnetic bead-based assay to ELISA method of detection. • LOD of 450 fM and recovery index of 98–104% for detection of anti-Tn AGA in serum sample. [ABSTRACT FROM AUTHOR]

Published

2022

224. Large-scale chemoenzymatic synthesis of blood group and tumor-associated poly-N-acetyllactosamine antigens

Author

Vasiliu, Daniela, Razi, Nahid, Zhang, Yingning, Jacobsen, Nathan, Allin, Kirk, Liu, Xiaofei, Hoffmann, Julia, Bohorov, Ognian, and Blixt, Ola

Subjects

*GLYCOPROTEINS, *GLYCOCONJUGATES, *BLOOD, *PROTEINS

Abstract

Abstract: Poly-N-acetyllactosamines (pLNs) are common terminal sugars of many N- and O-linked glycan structures present in glycoproteins and glycolipids. Utilizing various glycosyltransferases, we developed new and efficient chemoenzymatic methods for the synthesis of pLNs in gram-scale. Specifically, the use of sialyltransferases and fucosyltransferases enabled us to synthesize and purify 24 blood group and tumor-associated pLN derivatives with α-(2→3)- and α-(2→6)-linked sialic acid, as well as with α-(1→2)- and α-(1→3)-linked fucose. All synthesized derivatives were linked to a short 2-azidoethyl spacer for further modification. [Copyright &y& Elsevier]

Published

2006

225. Glycan Array Screening Reveals a Candidate Ligand for SigIec-8.

Author

Bochner, Bruce S., Alvarez, Richard A., Mehta, Padmaja, Bovin, Nicolai V., Blixt, Ola, White, John R., and Schnaar, Ronald L.

Subjects

*SIALIC acids, *LECTINS, *EOSINOPHILS, *BASOPHILS, *MAST cells, *GLYCOSIDES, *STREPTAVIDIN

Abstract

Sialic acid-binding immunoglobulin-like lectin 8 (Siglec-8) is selectively expressed on human eosinophils, basophils, and mast cells, where it regulates their function and survival. Previous studies demonstrated sialic acid-dependent binding of Siglec-8 but failed to reveal significant substructure specificity or high affinity of that binding. To test a broader range of potential ligands, a Siglec-8-Ig chimeric protein was tested for binding to 172 different glycan structures immobilized as biotinylated glycosides on a 384-well streptavidin-coated plate. Of these, ∼40 structures were sialylated. Among these, avid binding was detected to a single defined glycan, NeuAcα2-3(6-O-sulfo)Galβ1-4[Fucα13]GlcNAc, also referred to in the literature as 6'-sulfosLex. Notably, neither unsulfated sLex (NeuAcα23Galβ1-4[Fucα1-3]GlcNAc) nor an isomer with the sulfate on the 6-position of the GlcNAc residue (6-sulfosLex, NeuAcα2-3Galβ1-4[Fucα1-3](6-O-sulfo)GlcNAc) supported detectable binding. Subsequent secondary screening was performed using surface plasmon resonance. Biotin glycosides immobilized on streptavidin biosensor chips were exposed to Siglec-8-Ig in solution. Whereas surfaces derivatized with sLex and 6-sulfo-sLex failed to support detectable Siglec-8 binding, 6'-sulfosLex supported significant binding with a Kd of 2.3 µM. In a separate test of binding specificity, aminopropyl glycosides were covalently immobilized at different concentrations on activated (N-hydroxysuccinimidyl) glass surfaces (Schott-Nexterion Slide H). Subsequent exposure to Siglec-8-Ig precomplexed with fluorescein isothiocyanate anti-human Fc resulted in fluorescent signals at immobilized concentrations of 6'-sulfo-sLex of < 5 pmol/spot. In contrast, sLex and 6-sulfo-sLex did not support any Siglec-8 binding at the highest concentration tested (300 pmol/spot). We conclude that Siglec-8 binds preferentially to the sLex structure bearing an additional sulfate ester on the galactose 6-hydroxyl. [ABSTRACT FROM AUTHOR]

Published

2005

226. Synthesis of deoxy and acylamino derivatives of lactose and use of these for probing the active site of Neisseria meningitidis N-acetylglucosaminyltransferase

Author

Westerlind, Ulrika, Hagback, Per, Tidbäck, Björn, Wiik, Lotta, Blixt, Ola, Razi, Nahid, and Norberg, Thomas

Published

2005

227. Phage-Display Selection of a Human Single-Chain Fv Antibody Highly Specific for Melanoma and Breast Cancer Cells Using a Chemoenzymatically Synthesized G[SUBM3]-Carbohydrate Antigen.

Author

Lee, Kyung Joo, Mao, Shenlan, Chengzao Sun, Changshou Gao, Blixt, Ola, Arrues, Sandra, Hom, Louis G., Kaufmann, Gunnar F., Hoffman, Timothy Z., Coyle, Avery R., Paulson, James, Felding-Habermann, Brunhilde, and Janda, Kim D.

Subjects

*GLYCOSPHINGOLIPIDS, *CANCER treatment, *EPITOPES, *THERAPEUTICS

Abstract

Overexpression of the cell-surface glycosphingolipid G[SUBM3] is associated with a number of different cancers, including those of the skin, colon, breast, and lung. Antibodies against the G[SUBM3] epitope have potential application as therapeutic agents in the treatment of these cancers. We describe the chemoenzymatic synthesis of two G[SUBM3]-derived reagents and their use in the panning of a phage-displayed human single-chain Fv (scFv) antibody library derived from the blood of cancer patients. Three scFv-phage clones, GM3A6, GM3AS, and GM3A15, were selected for recombinant expression and were characterized using BIAcore and flow cytometry. BIAcore measurements using the purified, soluble scFvs yielded dissociation constants (K[SUBd]) ranging from 4.2 × 10[SUP-7] to 2.1× 1[SUP-5] M. Flow cytometry was used to evaluate the ability of each scFv to discriminate between normal human cells (human dermal fibroblast, HDFa), melanoma cells (HMV-1, M21, and C-8161), and breast cancer cells (BCM-1, BCM-2, and BMS). GM3A6 displayed cross-reactivity with normal cells, as well as tumor cells, and GM3A15 possessed little or no binding activity toward any of the cell lines tested. However, GM3A8 bound to five of the six tumor cell lines and showed no measurable reactivity against the HDFa cells. Hence, we have demonstrated that a synthetic G[SUBM3] panning reagent can be used to isolate a fully human scFv that is highly specific for native G[SUBM3] on the surface of tumor cells. The result is a significant step toward effective immunotherapies for the treatment of cancer. [ABSTRACT FROM AUTHOR]

Published

2002

228. Differential recognition of influenza A virus H1N1 neuraminidase by DNA vaccine-induced antibodies in pigs and ferrets.

Author

Tingstedt JL, Stephen C, Risinger C, Blixt O, Gunalan V, Johansen IS, Fomsgaard A, Polacek C, and Lassaunière R

Subjects

Animals, Swine, Humans, Ferrets, Neuraminidase genetics, Antibodies, Viral, Vaccines, DNA, Influenza A Virus, H1N1 Subtype, Influenza A Virus, H7N1 Subtype, Influenza, Human, Influenza Vaccines

Abstract

Neuraminidase (NA) accounts for approximately 10-20% of the total glycoproteins on the surface of influenza viruses. It cleaves sialic acids on glycoproteins, which facilitates virus entry into the airways by cleaving heavily glycosylated mucins in mucus and the release of progeny virus from the surface of infected cells. These functions make NA an attractive vaccine target. To inform rational vaccine design, we define the functionality of influenza DNA vaccine-induced NA-specific antibodies relative to antigenic sites in pigs and ferrets challenged with a vaccine-homologous A/California/7/2009(H1N1)pdm09 strain. Sera collected pre-vaccination, post-vaccination and post-challenge were analyzed for antibody-mediated inhibition of NA activity using a recombinant H7N1 CA09 virus. Antigenic sites were further identified with linear and conformational peptide microarrays spanning the full NA of A/California/04/2009(H1N1)pdm09. Vaccine-induced NA-specific antibodies inhibited the enzymatic function of NA in both animal models. The antibodies target critical sites of NA such as the enzymatic site, second sialic binding site and framework residues, shown here by high-resolution epitope mapping. New possible antigenic sites were identified that potentially block the catalytic activity of NA, including an epitope recognized solely in pigs and ferrets with neuraminidase inhibition, which could be a key antigenic site affecting NA function. These findings show that our influenza DNA vaccine candidate induces NA-specific antibodies that target known critical sites, and new potential antigenic sites of NA, inhibiting the catalytic activity of NA., Competing Interests: AF is co-inventor on a patent application covering an influenza DNA vaccine; all rights to the vaccine have been assigned to Statens Serum Institut SSI, a Danish national not-for-profit governmental public health institute. The remaining authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2023 Tingstedt, Stephen, Risinger, Blixt, Gunalan, Johansen, Fomsgaard, Polacek and Lassaunière.)

Published

2023

229. Targeting a Tumor-Specific Epitope on Podocalyxin Increases Survival in Human Tumor Preclinical Models.

Author

Canals Hernaez D, Hughes MR, Li Y, Mainero Rocca I, Dean P, Brassard J, Bell EM, Samudio I, Mes-Masson AM, Narimatsu Y, Clausen H, Blixt O, Roskelley CD, and McNagny KM

Abstract

Podocalyxin (Podxl) is a CD34-related cell surface sialomucin that is normally highly expressed by adult vascular endothelia and kidney podocytes where it plays a key role in blocking adhesion. Importantly, it is also frequently upregulated on a wide array of human tumors and its expression often correlates with poor prognosis. We previously showed that, in xenograft studies, Podxl plays a key role in metastatic disease by making tumor initiating cells more mobile and invasive. Recently, we developed a novel antibody, PODO447, which shows exquisite specificity for a tumor-restricted glycoform of Podxl but does not react with Podxl expressed by normal adult tissue. Here we utilized an array of glycosylation defective cell lines to further define the PODO447 reactive epitope and reveal it as an O-linked core 1 glycan presented in the context of the Podxl peptide backbone. Further, we show that when coupled to monomethyl auristatin E (MMAE) toxic payload, PODO447 functions as a highly specific and effective antibody drug conjugate (ADC) in killing ovarian, pancreatic, glioblastoma and leukemia cell lines in vitro . Finally, we demonstrate PODO447-ADCs are highly effective in targeting human pancreatic and ovarian tumors in xenografted NSG and Nude mouse models. These data reveal PODO447-ADCs as exquisitely tumor-specific and highly efficacious immunotherapeutic reagents for the targeting of human tumors. Thus, PODO447 exhibits the appropriate characteristics for further development as a targeted clinical immunotherapy., Competing Interests: The authors DC, MH, PD, IS, OB, KM, CR are inventors of a pending patent application on PODO447 and methods of using the same (US20180296673A1). MH, KM and CR are inventors of a pending patent application on PODO83 and methods of using the same (US20190367606A1). KM and CR possess an awarded patent on podocalyxin as a prognostic marker in cancer (US9309323B2). The remaining authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2022 Canals Hernaez, Hughes, Li, Mainero Rocca, Dean, Brassard, Bell, Samudio, Mes-Masson, Narimatsu, Clausen, Blixt, Roskelley and McNagny.)

Published

2022

230. Engineering the Ligand Specificity of the Human Galectin-1 by Incorporation of Tryptophan Analogues.

Author

Tobola F, Lepšík M, Zia SR, Leffler H, Nilsson UJ, Blixt O, Imberty A, and Wiltschi B

Subjects

Binding Sites, Galectins metabolism, Humans, Ligands, Oligosaccharides chemistry, Galectin 1 chemistry, Tryptophan

Abstract

Galectin-1 is a β-galactoside-binding lectin with manifold biological functions. A single tryptophan residue (W68) in its carbohydrate binding site plays a major role in ligand binding and is highly conserved among galectins. To fine tune galectin-1 specificity, we introduced several non-canonical tryptophan analogues at this position of human galectin-1 and analyzed the resulting variants using glycan microarrays. Two variants containing 7-azatryptophan and 7-fluorotryptophan showed a reduced affinity for 3'-sulfated oligosaccharides. Their interaction with different ligands was further analyzed by fluorescence polarization competition assay. Using molecular modeling we provide structural clues that the change in affinities comes from modulated interactions and solvation patterns. Thus, we show that the introduction of subtle atomic mutations in the ligand binding site of galectin-1 is an attractive approach for fine-tuning its interactions with different ligands., (© 2022 Wiley-VCH GmbH.)

Published

2022

231. PODO447: a novel antibody to a tumor-restricted epitope on the cancer antigen podocalyxin.

Author

Canals Hernaez D, Hughes MR, Dean P, Bergqvist P, Samudio I, Blixt O, Wiedemeyer K, Li Y, Bond C, Cruz E, Köbel M, Gilks B, Roskelley CD, and McNagny KM

Subjects

Animals, Antibodies, Monoclonal pharmacology, Biomarkers, Tumor immunology, CHO Cells, Cell Line, Tumor, Cricetulus, Epitopes immunology, Female, HEK293 Cells, Humans, Ovarian Neoplasms therapy, Rabbits, Antibodies, Monoclonal immunology, Ovarian Neoplasms immunology, Sialoglycoproteins immunology

Abstract

Background: The success of new targeted cancer therapies has been dependent on the identification of tumor-specific antigens. Podocalyxin (Podxl) is upregulated on tumors with high metastatic index and its presence is associated with poor outcome, thus emerging as an important prognostic and theragnostic marker in several human cancers. Moreover, in human tumor xenograft models, Podxl expression promotes tumor growth and metastasis. Although a promising target for immunotherapy, the expression of Podxl on normal vascular endothelia and kidney podocytes could hamper efforts to therapeutically target this molecule. Since pathways regulating post-translational modifications are frequently perturbed in cancer cells, we sought to produce novel anti-Podxl antibodies (Abs) that selectively recognize tumor-restricted glycoepitopes on the extracellular mucin domain of Podxl., Methods: Splenic B cells were isolated from rabbits immunized with a Podxl-expressing human tumor cell line. Abs from these B cells were screened for potent reactivity to Podxl + neoplastic cell lines but not Podxl + primary endothelial cells. Transcripts encoding heavy and light chain variable regions from promising B cells were cloned and expressed as recombinant proteins. Tumor specificity was assessed using primary normal tissue and an ovarian cancer tissue microarray (TMA). Mapping of the tumor-restricted epitope was performed using enzyme-treated human tumor cell lines and a glycan array., Results: One mAb (PODO447) showed strong reactivity with a variety of Podxl+ tumor cell lines but not with normal primary human tissue including Podxl+ kidney podocytes and most vascular endothelia. Screening of an ovarian carcinoma TMA (219 cases) revealed PODO447 reactivity with the majority of tumors, including 65% of the high-grade serous histotype. Subsequent biochemical analyses determined that PODO447 reacts with a highly unusual terminal N-acetylgalactosamine beta-1 (GalNAcβ1) motif predominantly found on the Podxl protein core. Finally, Ab-drug conjugates showed specific efficacy in killing tumor cells in vitro ., Conclusions: We have generated a novel and exquisitely tumor-restricted mAb, PODO447, that recognizes a glycoepitope on Podxl expressed at high levels by a variety of tumors including the majority of life-threatening high-grade serous ovarian tumors. Thus, tumor-restricted PODO447 exhibits the appropriate specificity for further development as a targeted immunotherapy., Competing Interests: Competing interests: The authors are inventors of a pending patent application on PODO447 and methods of using the same (US20180296673A1). MRH, PB, IS, CBG, KM and CR are inventors of a pending patent application on PODO83 and methods of using the same (US20190367606A1). KM and CR possess an awarded patent on podocalyxin as a prognostic marker in cancer (US9309323B2)., (© Author(s) (or their employer(s)) 2020. Re-use permitted under CC BY-NC. No commercial re-use. See rights and permissions. Published by BMJ.)

Published

2020

232. Evaluation of Sialyl-Lactotetra as a Marker for Epithelial Ovarian Tumors.

Author

Barone A, Linder A, Mateoiu C, Köster Larsen R, Blixt O, Teneberg S, and Sundfeldt K

Abstract

Ovarian carcinoma is a heterogeneous disease with distinct molecular and histological profiles, ranging from low grade atypia to highly aggressive tumors associated with a poor prognosis. In the present study, glycosphingolipids were isolated from human high-grade serous ovarian carcinoma, whereby the novel stem cell marker Sialyl-lactotetra (S-Lc 4 ) was characterized in two out of three cases. The presence and level of S-Lc 4 was further evaluated immunohistochemically in a cohort of patients with ovarian tumors ranging from benign lesions to high grade serous carcinoma ( n = 478). Its expression was assessed in association with tumor grade, stage, histology, and survival. The data showed that S-Lc 4 is most common and highly expressed in borderline type tumors and carcinomas with low levels of aggressiveness, such as mucinous, endometrioid, and low grade serous. Accordingly, S-Lc 4 -positivity was associated with better disease-free survival. The expression of S-Lc 4 was seemingly associated with lineage continuity and could be traced from premalignant lesions to carcinoma, suggesting inheritance by a stem cell lineage that gives rise to generally indolent tumors., (Copyright © 2020 Barone, Linder, Mateoiu, Köster Larsen, Blixt, Teneberg and Sundfeldt.)

Published

2020

233. Intra-tumour IgA1 is common in cancer and is correlated with poor prognosis in bladder cancer.

Author

Welinder C, Jirström K, Lehn S, Nodin B, Marko-Varga G, Blixt O, Danielsson L, and Jansson B

Abstract

A high frequency of IgA1-positive tumour cells was found in tissue micro-arrays of oesophagus, colon, testis, lung, breast, bladder and ovarian cancer. IgA1 was observed in the cytoplasm and the plasma membrane. A correlation was found between intra-tumour IgA1 and poor overall survival in a large cohort of bladder cancer patients (n = 99, p = 0.011, log-rank test). The number of IgA1-positive tumour cells was also found to be higher in female than male bladder cancer patients. The presence of IgA1 was confirmed in formalin-fixed paraffin-embedded ovarian carcinoma samples using LC-MS/MS analysis. Uptake of IgA1 was also observed in breast cancer and melanoma cell lines when cultivated in the presence of serum from healthy individuals, indicating a possible origin of the IgA1 antibodies in cancer cells.

Published

2016

234. Cytotoxic activity against human neuroblastoma and melanoma cells mediated by IgM antibodies derived from peripheral blood of healthy donors.

Author

Devarapu SK, Mamidi S, Plöger F, Dill O, Blixt O, Kirschfink M, and Schwartz-Albiez R

Subjects

Biomarkers, Tumor immunology, Cell Line, Tumor, Epitopes immunology, Gangliosides immunology, Healthy Volunteers, Humans, Immunoglobulin M blood, Antibody-Dependent Cell Cytotoxicity, Immunoglobulin M immunology, Melanoma immunology, Neuroblastoma immunology

Abstract

A small percentage of healthy donors identified in the Western population carry antibodies in their peripheral blood which convey cytotoxic activity against certain human melanoma and neuroblastoma cell lines. We measured the cytotoxic activity of sera and plasmas from healthy donors on the human neuroblastoma cell line Kelly and various melanoma cell lines. Antibodies of IgM isotype, presumably belonging to the class of naturally occurring antibodies, exerted cytotoxic activity in a complement-dependent fashion. Apart from complement-dependent tumor cell lysis, we observed C3 opsonization in all tumor cell lines upon treatment with cytotoxic plasmas. Cell lines tested primarily expressed membrane complement regulatory proteins (mCRP) CD46, CD55 and CD59 to various extents. Blocking of mCRPs by monoclonal antibodies enhanced cell lysis and opsonization, though some melanoma cells remained resistant to complement attack. Epitopes recognized by cytotoxic antibodies were represented by gangliosides such as GD2 and GD3, as evidenced by cellular sialidase pretreatment and enhanced expression of distinct gangliosides. It remains to be clarified why only a small fraction of healthy persons carry these antitumor cytotoxic antibodies., (© 2016 UICC.)

Published

2016

235. Arraying the post-translational glycoproteome (PTG).

Author

Blixt O and Westerlind U

Subjects

Epitopes metabolism, Glycopeptides analysis, Glycosylation, Humans, Proteome metabolism, Glycomics methods, Protein Processing, Post-Translational, Proteome chemistry

Abstract

Glycosylation is chemically the most complex post-translational modification of proteins and therefore understanding the structural and biological implications of post-translational glycosylation is a major challenge. The need for rapid and reliable investigations of protein-glycan interaction events and the substantial efforts required to synthesize glycans and glycopeptides with a variety of structures has called for the development of miniaturized analytical techniques. In the last decade, glycan and glycopeptide microarrays have enabled high-throughput analysis of diverse protein-glycan interactions. Evaluations of enzyme activities and substrate specificities, characterization of glycan binding proteins, mapping of antibody epitopes, detection of autoantibodies and serodiagnosis are typically conducted on microarrays. The most significant developments in synthesis, immobilization and applications of glycopeptide microarrays are covered in this review., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published

2014

236. Synthesis of O-glycopeptides and construction of glycopeptide microarrays.

Author

Blixt O and Cló E

Subjects

Amino Acids chemistry, Fluorenes chemistry, Glycopeptides chemistry, Polysaccharides chemistry, Glycopeptides chemical synthesis, Protein Array Analysis methods, Solid-Phase Synthesis Techniques methods

Abstract

O-glycosylation of proteins is an important modification which affects biological function and immunity. In this chapter, we provide protocols for efficient solid-phase O-glycopeptide synthesis (SPGPS) and protocols for the construction of glycopeptide microarray chips for screening applications. This will be exemplified for mucin-type glycopeptides and the construction of glycopeptide microarrays. To this end, the protocols provided are particularly suited for small-scale robotic parallel synthesis. N-Terminal amine capping of deletion peptides during synthesis stands out as vital to this strategy. It allows for direct on-slide enrichment of the full-length target product and thereby bypasses tedious isolation and purification procedures.

Published

2013

237. Printed glycan array: antibodies as probed in undiluted serum and effects of dilution.

Author

Shilova N, Navakouski M, Khasbiullina N, Blixt O, and Bovin N

Subjects

Animals, Carbohydrate Sequence, Goats, Humans, Protein Binding, Immunoglobulin G blood, Immunoglobulin M blood, Polysaccharides immunology, Protein Array Analysis methods, Serum immunology

Abstract

Using printed glycan array (PGA) we compared the results of antibody profiling in undiluted, moderately (1:15) and highly (1:100) diluted human blood serum. Undiluted serum is suitable for studying blood as a tissue in its native state, whereas to study the serum of newborns or small animals one usually has to dilute the starting material in order to have sufficient volume for PGA experimentation. The PGA used in this study allows for the use of whole serum without modifications to the protocol, and the background is surprisingly low. Antibodies profiles observed in undiluted serum versus 1:15 dilution were similar, with only a limited number of new signals identified in the undiluted serum. However, unexpected irregularities were found when IgG and IgM are measured separately, namely, at a 1:15 dilution more intensive IgG signals for many glycans are observed. We believe that in conditions of moderate dilution IgG and IgM antibodies can compete with each other for antigen and as a result, the higher affinity anti-glycan IgGs give rise to more intense signals. Therefore depending on the purpose, different dilutions of serum will be optimal: in competitive 1:15 conditions the observed IgG/IgM ratio corresponds to their titer, whereas at 1:100 dilution the measured ratio corresponds to real molar concentration of IgG and IgM.

Published

2012

238. Analysis of Tn antigenicity with a panel of new IgM and IgG1 monoclonal antibodies raised against leukemic cells.

Author

Blixt O, Lavrova OI, Mazurov DV, Cló E, Kracun SK, Bovin NV, and Filatov AV

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal, Murine-Derived biosynthesis, Antigens, CD immunology, Binding, Competitive, Humans, Immunoglobulin G biosynthesis, Immunoglobulin M biosynthesis, Jurkat Cells, Leukemia, Membrane Glycoproteins immunology, Mice, Molecular Chaperones biosynthesis, Molecular Sequence Data, Mucin-1 immunology, Peptide Fragments immunology, Protein Binding, Recombinant Proteins biosynthesis, Antibodies, Monoclonal, Murine-Derived chemistry, Antibody Specificity, Antigens, Tumor-Associated, Carbohydrate immunology, Immunoglobulin G chemistry, Immunoglobulin M chemistry

Abstract

CD175 or Tn antigen is a carbohydrate moiety of N-acetylgalactosamine (GalNAc)α1-O- linked to the residue of amino acid serine or threonine in a polypeptide chain. Despite the chemical simplicity of the Tn antigen, its antigenic structure is considered to be complex and the clear determinants of Tn antigenicity remain poorly understood. As a consequence, a broad variety of anti-Tn monoclonal antibodies (mAbs) have been generated. To further investigate the nature and complexity of the Tn antigen, we generated seven different anti-Tn mAbs of IgM and IgG classes raised against human Jurkat T cells, which are Tn-positive due to the low activity of T-synthase and mutation in specific chaperone Cosmc. The binding analysis of anti-Tn mAbs with the array of synthetic saccharides, glycopeptides and O-glycoproteins revealed unexpected differences in specificities of anti-Tn mAbs. IgM mAbs bound the terminal GalNAc residue of the Tn antigen irrespective of the peptide context or with low selectivity to the glycoproteins. In contrast, IgG mAbs recognized the Tn antigen in the context of a specific peptide motif. Particularly, JA3 mAb reacted to the GSPP or GSPAPP, and JA5 mAb recognized specifically the GSP motif (glycosylation sites are underlined). The major O-glycan carrier proteins CD43 and CD162 and isoforms of CD45 expressed on Jurkat cells were precipitated by anti-Tn mAbs with different affinities. In summary, our data suggest that Tn antigen-Ab binding capacity is determined by the peptide context of the Tn antigen, antigenic specificity of the Ab and class of the immunoglobulin. The newly generated anti-Tn IgG mAbs with the strong specificity to glycoprotein CD43 can be particularly interesting for the application in leukemia diagnostics and therapy.

Published

2012

239. Design of a covalently bonded glycosphingolipid microarray.

Author

Arigi E, Blixt O, Buschard K, Clausen H, and Levery SB

Subjects

Amidohydrolases metabolism, Antibodies, Monoclonal analysis, Antibodies, Monoclonal metabolism, Antibody Specificity, Cell Membrane chemistry, Cholera Toxin analysis, Cholera Toxin metabolism, Molecular Structure, Peanut Agglutinin analysis, Peanut Agglutinin metabolism, Protein Binding, Glycomics methods, Glycosphingolipids analysis, Glycosphingolipids chemistry, Microarray Analysis methods

Abstract

Glycosphingolipids (GSLs) are well known ubiquitous constituents of all eukaryotic cell membranes, yet their normal biological functions are not fully understood. As with other glycoconjugates and saccharides, solid phase display on microarrays potentially provides an effective platform for in vitro study of their functional interactions. However, with few exceptions, the most widely used microarray platforms display only the glycan moiety of GSLs, which not only ignores potential modulating effects of the lipid aglycone, but inherently limits the scope of application, excluding, for example, the major classes of plant and fungal GSLs. In this work, a prototype "universal" GSL-based covalent microarray has been designed, and preliminary evaluation of its potential utility in assaying protein-GSL binding interactions investigated. An essential step in development involved the enzymatic release of the fatty acyl moiety of the ceramide aglycone of selected mammalian GSLs with sphingolipid N-deacylase (SCDase). Derivatization of the free amino group of a typical lyso-GSL, lyso-G(M1), with a prototype linker assembled from succinimidyl-[(N-maleimidopropionamido)-diethyleneglycol] ester and 2-mercaptoethylamine, was also tested. Underivatized or linker-derivatized lyso-GSL were then immobilized on N-hydroxysuccinimide- or epoxide-activated glass microarray slides and probed with carbohydrate binding proteins of known or partially known specificities (i.e., cholera toxin B-chain; peanut agglutinin, a monoclonal antibody to sulfatide, Sulph 1; and a polyclonal antiserum reactive to asialo-G(M2)). Preliminary evaluation of the method indicated successful immobilization of the GSLs, and selective binding of test probes. The potential utility of this methodology for designing covalent microarrays that incorporate GSLs for serodiagnosis is discussed.

Published

2012

240. Seromic profiling of colorectal cancer patients with novel glycopeptide microarray.

Author

Pedersen JW, Blixt O, Bennett EP, Tarp MA, Dar I, Mandel U, Poulsen SS, Pedersen AE, Rasmussen S, Jess P, Clausen H, and Wandall HH

Subjects

Antibodies, Monoclonal immunology, Autoantibodies immunology, Biomarkers, Tumor immunology, Case-Control Studies, Colorectal Neoplasms diagnosis, Colorectal Neoplasms immunology, Enzyme-Linked Immunosorbent Assay, Epitopes analysis, Female, Glycopeptides immunology, Glycosylation, Humans, Immunoenzyme Techniques, Male, Middle Aged, Mucins immunology, Prognosis, Protein Processing, Post-Translational, Recombinant Proteins immunology, Recombinant Proteins metabolism, Biomarkers, Tumor analysis, Colorectal Neoplasms blood, Glycopeptides blood, Mucins blood, Protein Array Analysis

Abstract

Cancer-associated autoantibodies hold promise as sensitive biomarkers for early detection of cancer. Aberrant post-translational variants of proteins are likely to induce autoantibodies, and changes in O-linked glycosylation represent one of the most important cancer-associated post-translational modifications (PTMs). Short aberrant O-glycans on proteins may introduce novel glycopeptide epitopes that can elicit autoantibodies because of lack of tolerance. Technical barriers, however, have hampered detection of such glycopeptide-specific autoantibodies. Here, we have constructed an expanded glycopeptide array displaying a comprehensive library of glycopeptides and glycoproteins derived from a panel of human mucins (MUC1, MUC2, MUC4, MUC5AC, MUC6 and MUC7) known to have altered glycosylation and expression in cancer. Seromic profiling of patients with colorectal cancer identified cancer-associated autoantibodies to a set of aberrant glycopeptides derived from MUC1 and MUC4. The cumulative sensitivity of the array analysis was 79% with a specificity of 92%. The most prevalent of the identified autoantibody targets were validated as authentic cancer immunogens by showing expression of the epitopes in cancer using novel monoclonal antibodies. Our study provides evidence for the value of glycopeptides and other PTM-peptide arrays in diagnostic measures., (Copyright © 2011 UICC.)

Published

2011

241. Characterization of an immunodominant cancer-specific O-glycopeptide epitope in murine podoplanin (OTS8).

Author

Steentoft C, Schjoldager KT, Cló E, Mandel U, Levery SB, Pedersen JW, Jensen K, Blixt O, and Clausen H

Subjects

Amino Acid Sequence, Animals, Antibody Specificity immunology, Enzyme-Linked Immunosorbent Assay, Glycopeptides chemistry, Glycosylation, Humans, Immunoglobulin G immunology, Mice, Molecular Sequence Data, Protein Array Analysis, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Glycopeptides immunology, Immunodominant Epitopes chemistry, Immunodominant Epitopes immunology, Membrane Glycoproteins chemistry, Membrane Glycoproteins immunology, Neoplasms chemistry, Neoplasms immunology

Abstract

Auto-antibodies induced by cancer represent promising sensitive biomarkers and probes to identify immunotherapeutic targets without immunological tolerance. Surprisingly few epitopes for such auto-antibodies have been identified to date. Recently, a cancer-specific syngeneic murine monoclonal antibody 237, developed to a spontaneous murine fibrosarcoma, was shown to be directed to murine podoplanin (OTS8) with truncated Tn O-glycans. Our understanding of such cancer-specific auto-antibodies to truncated glycoforms of glycoproteins is limited. Here we have investigated immunogenicity of a chemoenzymatically produced Tn-glycopeptide derived from the putative murine podoplanin O-glycopeptide epitope. We found that the Tn O-glycopeptide was highly immunogenic in mice and produced a Tn-glycoform specific response with no reactivity against unglycosylated peptides or the O-glycopeptide with extended O-glycan (STn and T glycoforms). The immunodominant epitope was strictly dependent on the peptide sequence, required Tn at a specific single Thr residue (Thr(77)), and antibodies to the epitope were not found in naive mice. We further tested a Tn O-glycopeptide library derived from human podoplanin by microarray analysis and demonstrated that the epitope was not conserved in man. We also tested human cancer sera for potential auto-antibodies to similar epitopes, but did not detect such antibodies to the Tn-library of podoplanin. The reagents and methods developed will be valuable for further studies of the nature and timing of induction of auto-antibodies to distinct O-glycopeptide epitopes induced by cancer. The results demonstrate that truncated O-glycopeptides constitute highly distinct antibody epitopes with great potential as targets for biomarkers and immunotherapeutics.

Published

2010

242. Contemporary North American influenza H7 viruses possess human receptor specificity: Implications for virus transmissibility.

Author

Belser JA, Blixt O, Chen LM, Pappas C, Maines TR, Van Hoeven N, Donis R, Busch J, McBride R, Paulson JC, Katz JM, and Tumpey TM

Subjects

Animals, Disease Models, Animal, Ferrets virology, Hemagglutination Tests, Humans, Influenza A Virus, H7N7 Subtype chemistry, Influenza A Virus, H7N7 Subtype physiology, Male, Microarray Analysis, N-Acetylneuraminic Acid analysis, Polysaccharides analysis, Poultry virology, Virus Replication, Influenza A Virus, H7N7 Subtype pathogenicity, Influenza in Birds transmission, Influenza, Human transmission, Receptors, Virus physiology, Virus Attachment

Abstract

Avian H7 influenza viruses from both the Eurasian and North American lineage have caused outbreaks in poultry since 2002, with confirmed human infection occurring during outbreaks in The Netherlands, British Columbia, and the United Kingdom. The majority of H7 infections have resulted in self-limiting conjunctivitis, whereas probable human-to-human transmission has been rare. Here, we used glycan microarray technology to determine the receptor-binding preference of Eurasian and North American lineage H7 influenza viruses and their transmissibility in the ferret model. We found that highly pathogenic H7N7 viruses from The Netherlands in 2003 maintained the classic avian-binding preference for alpha2-3-linked sialic acids (SA) and are not readily transmissible in ferrets, as observed previously for highly pathogenic H5N1 viruses. However, H7N3 viruses isolated from Canada in 2004 and H7N2 viruses from the northeastern United States isolated in 2002-2003 possessed an HA with increased affinity toward alpha2-6-linked SA, the linkage type found prominently on human tracheal epithelial cells. We identified a low pathogenic H7N2 virus isolated from a man in New York in 2003, A/NY/107/03, which replicated efficiently in the upper respiratory tract of ferrets and was capable of transmission in this species by direct contact. These results indicate that H7 influenza viruses from the North American lineage have acquired sialic acid-binding properties that more closely resemble those of human influenza viruses and have the potential to spread to naïve animals.

Published

2008

243. Glycan microarrays for screening sialyltransferase specificities.

Author

Blixt O, Allin K, Bohorov O, Liu X, Andersson-Sand H, Hoffmann J, and Razi N

Subjects

Animals, Cell Line, Glycomics methods, Humans, Rats, Substrate Specificity, Swine, Microarray Analysis methods, Polysaccharides analysis, Polysaccharides metabolism, Sialyltransferases metabolism

Abstract

Here we demonstrate that glycan microarrays can be used for high-throughput acceptor specificity screening of various recombinant sialyltransferases. Cytidine-5'-monophospho-N-acetylneuraminic acid (CMP-Neu5Ac) was biotinylated at position 9 of N-acetylneuraminic acid (Neu5Ac) by chemoenzymatic synthesis generating CMP-9Biot-Neu5Ac. The activated sugar nucleotide was used as donor substrate for various mammalian sialyltranferases which transferred biotinylated sialic acids simultaneously onto glycan acceptors immobilized onto a microarray glass slide. Biotinylated glycans detected with fluorescein-streptavidin conjugate to generate a specificity profile for each enzyme both confirming previously known specificities and reveal additional specificity information. Human alpha2,6sialyltransferase-I (hST6Gal-I) also sialylates chitobiose structures (GlcNAcbeta1-4GlcNAc)(n) including N-glycans, rat alpha2,3sialyltransferase (rST3Gal-III) tolerates fucosylated acceptors such as Lewis(a), human alpha2,3sialyltransferase-IV (hST3Gal-IV) broadly sialylates oligosaccharides of types 1-4 and porcine alpha2,3sialyltransferase-I (pST3Gal-I) sialylates ganglio-oligosaccharides and core 2 O-glycans in our array system. Several of these sialyltransferases perform a substitution reaction and exchange a sialylated acceptor with a biotinylated sialic acid but are restricted to the most specific acceptor substrates. Thus, this method allows for a rapid generation of enzyme specificity information and can be used towards synthesis of new carbohydrate compounds and expand the glycan array compound library.

Published

2008

244. Biocompatible carbon nanotubes generated by functionalization with glycodendrimers.

Author

Wu P, Chen X, Hu N, Tam UC, Blixt O, Zettl A, and Bertozzi CR

Subjects

Hydroxy Acids, Molecular Structure, Propionates chemistry, Biocompatible Materials chemistry, Dendrimers chemistry, Glycogen chemistry, Nanotubes, Carbon chemistry

Published

2008

245. Glycoarrays. Editorial.

Author

Blixt O

Subjects

Carbohydrates analysis, Glycomics methods

Published

2008

246. Surface plasmon resonance imaging for real-time, label-free analysis of protein interactions with carbohydrate microarrays.

Author

Karamanska R, Clarke J, Blixt O, Macrae JI, Zhang JQ, Crocker PR, Laurent N, Wright A, Flitsch SL, Russell DA, and Field RA

Subjects

Biotinylation, Protein Binding, Time Factors, Carbohydrate Metabolism, Carbohydrates analysis, Glycomics methods, Microarray Analysis methods, Proteins analysis, Proteins metabolism, Surface Plasmon Resonance methods

Abstract

Plant lectin recognition of glycans was evaluated by SPR imaging using a model array of N-biotinylated aminoethyl glycosides of beta-D-glucose (negative control), alpha-D: -mannose (conA-responsive), beta-D-galactose (RCA(120)-responsive) and N-acetyl-beta-D-: glucosamine (WGA-responsive) printed onto neutravidin-coated gold chips. Selective recognition of the cognate ligand was observed when RCA(120) was passed over the array surface. Limited or no binding was observed for the non-cognate ligands. SPR imaging of an array of 40 sialylated and unsialylated glycans established the binding preference of hSiglec7 for alpha2-8-linked disialic acid structures over alpha2-6-sialyl-LacNAcs, which in turn were recognized and bound with greater affinity than alpha2-3-sialyl-LacNAcs. Affinity binding data could be obtained with as little as 10-20 microg of lectin per experiment. The SPR imaging technique was also able to establish selective binding to the preferred glycan ligand when analyzing crude culture supernatant containing 10-20 microg of recombinant hSiglec7-Fc. Our results show that SPR imaging provides results that are in agreement with those obtained from fluorescence based carbohydrate arrays but with the added advantage of label-free analysis.

Published

2008

247. Pathogen specific carbohydrate antigen microarrays: a chip for detection of Salmonella O-antigen specific antibodies.

Author

Blixt O, Hoffmann J, Svenson S, and Norberg T

Subjects

Animals, Glycomics, Health, Humans, Indicator Dilution Techniques, Molecular Structure, Rabbits, Salmonella Infections blood, Salmonella Infections immunology, Sensitivity and Specificity, Antibodies, Bacterial immunology, Antibody Specificity, Microarray Analysis methods, O Antigens immunology, Salmonella immunology

Abstract

A Salmonella O-antigen microarray was developed by covalent coupling of oligosaccharide antigens specific for serogroups Salmonella enterica sv. Paratyphi (group A), Typhimurium (group B) and Enteritidis (group D). Antibodies were correctly detected in sera from patients with culture verified salmonellosis. High serogroup-specificity was seen with the disaccharide antigens. With the larger antigens, containing the backbone sequence Manalpha1-2Rhaalpha1-2Gal (MRG), common backbone-specific antibodies (O-antigen 12) were also detected. This is "proof of principle" that pathogen-specific carbohydrate antigen microarrays constitute a novel technology for rapid and specific serological diagnosis in either individual patients or larger sero-epidemiological and vaccine studies.

Published

2008

248. Glycan microarray technologies: tools to survey host specificity of influenza viruses.

Author

Stevens J, Blixt O, Paulson JC, and Wilson IA

Subjects

Animals, Birds, Carbohydrate Conformation, Carbohydrate Sequence, Disease Outbreaks veterinary, Hemagglutinin Glycoproteins, Influenza Virus genetics, Hemagglutinin Glycoproteins, Influenza Virus metabolism, Humans, Influenza in Birds virology, Microarray Analysis instrumentation, Microarray Analysis veterinary, Polysaccharides chemistry, Species Specificity, Hemagglutinin Glycoproteins, Influenza Virus chemistry, Influenza A Virus, H5N1 Subtype metabolism, Microarray Analysis methods, Polysaccharides metabolism, Receptors, Virus chemistry, Receptors, Virus metabolism

Abstract

New technologies are urgently required for rapid surveillance of the current H5N1 avian influenza A outbreaks to gauge the potential for adaptation of the virus to the human population, a crucial step in the emergence of pandemic influenza virus strains. Owing to the species-specific nature of the interaction between the virus and host glycans, attention has recently focused on novel glycan array technologies that can rapidly assess virus receptor specificity and the potential emergence of human-adapted H5N1 viruses.

Published

2006

249. Structure and receptor specificity of the hemagglutinin from an H5N1 influenza virus.

Author

Stevens J, Blixt O, Tumpey TM, Taubenberger JK, Paulson JC, and Wilson IA

Subjects

Amino Acid Sequence, Amino Acid Substitution, Animals, Antigenic Variation, Binding Sites, Birds, Carbohydrate Conformation, Cloning, Molecular, Crystallography, X-Ray, Glycosylation, Hemagglutinin Glycoproteins, Influenza Virus genetics, Hemagglutinin Glycoproteins, Influenza Virus immunology, Humans, Influenza A Virus, H5N1 Subtype genetics, Influenza A Virus, H5N1 Subtype metabolism, Lung virology, Models, Molecular, Molecular Sequence Data, Mutation, Polysaccharides metabolism, Protein Conformation, Protein Folding, Protein Structure, Tertiary, Receptors, Virus chemistry, Respiratory Mucosa virology, Sialic Acids chemistry, Sialic Acids metabolism, Species Specificity, Virulence, Hemagglutinin Glycoproteins, Influenza Virus chemistry, Hemagglutinin Glycoproteins, Influenza Virus metabolism, Influenza A Virus, H5N1 Subtype chemistry, Influenza A Virus, H5N1 Subtype pathogenicity, Receptors, Virus metabolism

Abstract

The hemagglutinin (HA) structure at 2.9 angstrom resolution, from a highly pathogenic Vietnamese H5N1 influenza virus, is more related to the 1918 and other human H1 HAs than to a 1997 duck H5 HA. Glycan microarray analysis of this Viet04 HA reveals an avian alpha2-3 sialic acid receptor binding preference. Introduction of mutations that can convert H1 serotype HAs to human alpha2-6 receptor specificity only enhanced or reduced affinity for avian-type receptors. However, mutations that can convert avian H2 and H3 HAs to human receptor specificity, when inserted onto the Viet04 H5 HA framework, permitted binding to a natural human alpha2-6 glycan, which suggests a path for this H5N1 virus to gain a foothold in the human population.

Published

2006

250. Chemoenzymatic synthesis of 2-azidoethyl-ganglio-oligosaccharides GD3, GT3, GM2, GD2, GT2, GM1, and GD1a.

Author

Blixt O, Vasiliu D, Allin K, Jacobsen N, Warnock D, Razi N, Paulson JC, Bernatchez S, Gilbert M, and Wakarchuk W

Subjects

Escherichia coli enzymology, G(M2) Ganglioside chemical synthesis, Galactosyltransferases metabolism, Lactosylceramides chemical synthesis, N-Acetylgalactosaminyltransferases metabolism, Sialyltransferases metabolism, Substrate Specificity, Gangliosides chemical synthesis

Abstract

We have synthesized several ganglio-oligosaccharide structures using glycosyltransferases from Campylobacter jejuni. The enzymes, alpha-(2-->3/8)-sialyltransferase (Cst-II), beta-(1-->4)-N-acetylgalactosaminyltransferase (CgtA), and beta-(1-->3)-galactosyltransferase (CgtB), were produced in large-scale fermentation from Escherichia coli and further characterized based on their acceptor specificities. 2-Azidoethyl-glycosides corresponding to the oligosaccharides of GD3 (alpha-D-Neup5Ac-(2-->8)-alpha-D-Neup5Ac-(2-->3)-beta-D-Galp-(1-->4)-beta-D-Glcp-), GT3 (alpha-D-Neup5Ac-(2-->8)-alpha-D-Neup5Ac-(2-->8)-alpha-D-Neup5Ac-(2-->3)-beta-D-Galp-(1-->4)-beta-D-Glcp-), GM2 (beta-D-GalpNAc-(1-->4)-[alpha-D-Neup5Ac-(2-->3)]-beta-D-Galp-(1-->4)-beta-D-Glcp-), GD2 (beta-D-GalpNAc-(1-->4)-[alpha-D-Neup5Ac-(2-->8)-alpha-D-Neup5Ac-(2-->3)]-beta-D-Galp-(1-->4)-beta-D-Glcp-), GT2 (beta-D-GalpNAc-(1-->4)-[alpha-D-Neup5Ac-(2-->8)-alpha-D-Neup5Ac-(2-->8)-alpha-D-Neup5Ac-(2-->3)]-beta-D-Galp-(1-->4)-beta-D-Glcp-), and GM1 (beta-D-Galp-(1-->3)-beta-D-GalpNAc-(1-->4)-[alpha-D-Neup5Ac-(2-->3)]-beta-D-Galp-(1-->4)-beta-D-Glcp-) were synthesized in high yields (gram-scale). In addition, a mammalian alpha-(2-->3)-sialyltransferase (ST3Gal I) was used to sialylate GM1 and generate GD1a (alpha-D-Neup5Ac-(2-->3)-beta-D-Galp-(1-->3)-beta-D-GalpNAc-(1-->4)-[alpha-D-Neup5Ac-(2-->3)]-beta-D-Galp-(1-->4)-beta-D-Glcp-) oligosaccharide. We also cloned and expressed a rat UDP-N-acetylglucosamine-4'epimerase (GalNAcE) in E. coli AD202 cells for cost saving in situ conversion of less expensive UDP-GlcNAc to UDP-GalNAc.

Published

2005