Your search keyword '"printed glycan array"' showing total 17 results

1. Specificity of widely used lectins as probed with oligosaccharide and plant polysaccharide arrays

Author

Shilova, Nadezhda V., Galanina, Oxana E., Polyakova, Svetlana M., Nokel, Alexey Yu., Pazynina, Galina V., Golovchenko, Victoria V., Patova, Olga A., Mikshina, Polina V., Gorshkova, Tatayana A., and Bovin, Nicolai V.

Published

2024

2. Specificity of viscumin revised. As probed with a printed glycan array.

Author

Shilova, Nadezhda, Bovin, Nicolai, Maltseva, Diana, Polyakova, Svetlana, Sablina, Marina, Niwa, Hideaki, Zakharova, Galina, Raygorodskaya, Maria, Bufeeva, Lyuba, Belyi, Yury, Hushpulian, Dmitry, and Tonevitsky, Alexander

Subjects

*GLYCANS, *PROTEIN structure, *ANTINEOPLASTIC agents, *GANGLIOSIDES, *PLANT lectins, *MOIETIES (Chemistry)

Abstract

Viscumin, a lectin used in anti-cancer therapy, was originally considered as βGal recognizing protein; later, an ability to bind 6′-sialyl N-acetyllactosamine (6′SLN) terminated gangliosides was found. Here we probed viscumin with a printed glycan array (PGA) containing a large number of mammalian sulfated glycans, and found a strong binding to glycans with 6-O-SuGal moiety as lactose, N-acetyllactosamine (LN), di-N-acetyllactosamine (LacdiNAc), and even 6- O -SuGalNAcα (but not SiaTn). Also, the ability to bind some of αGal terminated glycans, including Galα1-3Galβ1-4GlcNAc, was observed. Unexpectedly, only weak interaction was detected with parent neutral β-galactosides including LN-LN-LN and branched (LN) 2 LN oligolactosamines; in the light of these data, one should not confidently classify viscumin as a β-galactoside-binding lectin. Carrying out PGA in the presence of neutral or sulfated/sialylated glycan, together with sequential elution from lactose-sepharose and consideration of the protein structure, lead to the conclusion that two glycan-binding sites of viscumin have different specificities, one of which prefers charged sulfated and sialylated moieties. • Viscumin specificity is broader than what was commonly believed to be galactose-ended glycans. • Two glycan-binding sites of viscumin have different specificities. • Viscumin has high affinity to glycans with 6-O-SuGal moiety. [ABSTRACT FROM AUTHOR]

Published

2022

3. Synthesis of disaccharides for the study of human blood antibodies capable of recognizing the inner Glcβ1-3GalNAc disaccharide fragment of bacterial polysaccharides.

Author

Pazynina, Galina V., Tsygankova, Svetlana V., Obukhova, Polina S., Shilova, Nadezhda V., Paramonov, Alexander S., Chizhov, Alexander O., Knirel, Yuriy A., and Bovin, Nicolai V.

Subjects

*DISACCHARIDES, *HUMAN experimentation, *IMMUNOGLOBULINS, *POLYSACCHARIDES

Abstract

[Display omitted] Disaccharides with the terminal Glcβ1-3 motif were synthesized as probes for studying human blood antibodies. An antibody isolated using Glcβ1-3GalNAcα–Sepharose was found to bind the inner part of the polysaccharide [–4GlcA6LThr3Acβ1-6Galβ1-6 Glcβ1-3GalNAc6Acβ 1–] n as evidenced by the use of a printed glycan array and inhibition assays. [ABSTRACT FROM AUTHOR]

Published

2023

4. Specificity profile of αGal antibodies in αGalT KO mice as probed with comprehensive printed glycan array: Comparison with human anti‐Galili antibodies.

Author

Dobrochaeva, Kira, Khasbiullina, Nailya, Shilova, Nadezhda, Knirel, Yuriy, Obukhova, Polina, Nokel, Alexey, Kunetskiy, Roman, Tsygankova, Svetlana, Bello‐Gil, Daniel, Costa, Cristina, Mañez, Rafael, and Bovin, Nicolai

Subjects

*BLOOD groups, *IMMUNOGLOBULINS, *IMMUNE system, *LABORATORY mice, *IMMUNOGLOBULIN G

Abstract

Background: The α1,3‐galactosyltransferase gene‐knockout (GalT KO) mice are able to produce natural anti‐αGal antibodies apparently without any specific immunization. GalT KO mice are commonly used as a model immunological system for studying anti‐αGal responses to Gal‐positive xenografts in human. In this study, we compared the specificity of mouse and human αGal antibodies to realize the adequacy of the murine model. Methods: Using hapten‐specific affinity chromatography antibodies against Galα1‐3Galβ1‐4GlcNAcβ epitope were isolated from both human and GalT KO mice blood sera. Specificity of isolated antibodies was determined using a printed glycan array (PGA) containing 400 mammalian glycans and 200 bacterial polysaccharides. Results: The quantity of isolated specific anti‐Galα antibodies corresponds to a content of <0.2% of total Ig, which is an order of magnitude lower than that generally assumed for both human and murine peripheral blood immunoglobulin, with a high predominance of IgM over IgG (95% vs 5%). Analysis using a printed glycan array has demonstrated that (a) antibodies from both species bind not only the Galα1‐3Galβ1‐4GlcNAcβ epitope, but also unrelated glycans; (b) particularly, for human (but not mouse) antibodies the best binders appear to be bacterial polysaccharides; (c) the profile of mouse antibodies is broader, it is noteworthy that they recognize a variety of human blood group B epitopes and even glycans without the α‐galactosyl residue. Conclusions: We believe that the mouse model should be used cautiously in xenotransplantation experiments when the fine epitope specificity of antibodies is critical. [ABSTRACT FROM AUTHOR]

Published

2021

5. Improved spot morphology for printed glycan arrays

Author

Navakouski Maksim, Shilova Nadezhda, Khasbiullina Nailya, Feofanov Alexey, Pudova Elena, Chen Kowa, Blixt Ola, and Bovin Nicolai

Subjects

printed glycan array, spots morphology, glycans, microarray, lab-on-chip, Biology (General), QH301-705.5

Abstract

Despite considerable success studying glycan-binding proteins using printed glycan arrays (PGAs), unambiguous quantitation of spot intensities by fluorescent readers remains a challenge. The main obstacles are the varying spot shape and size and in-spot fluorescence distribution caused by uneven drying of the printed drops. Two methods have been suggested for solving this problem: using polymeric glycoconjugates, which makes it possible to equalize the physicochemical properties (hydrophobicity, charge, and size) of different glycans, and applying a glycan solution on a slide coated with a thin oil mask, which hinders evaporation of the drop. Both approaches yield spots with similar sizes and an even distribution of the signal across the spot and are likely to be useful for improving the prints of other classes of molecules.

Published

2018

6. Natural Antibodies Against Sialoglycans

Author

Shilova, Nadezhda, Huflejt, Margaret E., Vuskovic, Marko, Obukhova, Polina, Navakouski, Maksim, Khasbiullina, Nailya, Pazynina, Galina, Galanina, Oxana, Bazhenov, Alexey, Bovin, Nicolai, Bayley, Hagan, Series editor, Houk, Kendall N., Series editor, Hughes, Greg, Series editor, Hunter, Christopher A., Series editor, Ishihara, Kazuaki, Series editor, Krische, Michael J, Series editor, Lehn, J.-M., Series editor, Luque, Rafael, Series editor, Olivucci, Massimo, Series editor, Siegel, Jay S., Series editor, Thiem, Joachim, Series editor, Venturi, Margherita, Series editor, Wong, Chi-Huey, Series editor, Wong, Henry N.C., Series editor, You, Shu-Li, Series editor, Wing-Wah Yam, Vivian, Series editor, Gerardy-Schahn, Rita, Delannoy, Philippe, and von Itzstein, Mark

Published

2015

7. The Formation of Glycan-Specific Natural Antibodies Repertoire in GalT-KO Mice Is Determined by Gut Microbiota

Author

Daniel Bello-Gil, Christophe Audebert, Sara Olivera-Ardid, Magdiel Pérez-Cruz, Gaël Even, Nailya Khasbiullina, Nausicaa Gantois, Nadezhda Shilova, Sophie Merlin, Cristina Costa, Nicolai Bovin, and Rafael Mañez

Subjects

GalT-KO mice, gut microbiota, metagenetic high-throughput sequencing, 16S rRNA gene, natural anti-glycan antibodies, printed glycan array, Immunologic diseases. Allergy, RC581-607

Abstract

Gut commensal bacteria are known to have a significant role in regulating the innate and adaptive immune homeostasis. Alterations in the intestinal microbial composition have been associated with several disease states, including autoimmune and inflammatory conditions. However, it is not entirely clear how commensal gut microbiota modulate and contribute to the systemic immunity, and whether circulating elements of the host immune system could regulate the microbiome. Thus, we have studied the diversity and abundance of specific taxons in the gut microbiota of inbred GalT-KO mice during 7 months of animal life by metagenetic high-throughput sequencing (16S rRNA gene, variable regions V3–V5). The repertoire of glycan-specific natural antibodies, obtained by printed glycan array technology, was then associated with the microbial diversity for each animal by metagenome-wide association studies (MWAS). Our data show that the orders clostridiales (most abundant), bacteriodales, lactobacillales, and deferribacterales may be associated with the development of the final repertoire of natural anti-glycan antibodies in GalT-KO mice. The main changes in microbiota diversity (month-2 and month-3) were related to important changes in levels and repertoire of natural anti-glycan antibodies in these mice. Additionally, significant positive and negative associations were found between the gut microbiota and the pattern of specific anti-glycan antibodies. Regarding individual features, the gut microbiota and the corresponding repertoire of natural anti-glycan antibodies showed differences among the examined animals. We also found redundancy in different taxa associated with the development of specific anti-glycan antibodies. Differences in microbial diversity did not, therefore, necessarily influence the overall functional output of the gut microbiome of GalT-KO mice. In summary, the repertoire of natural anti-carbohydrate antibodies may be partially determined by the continuous antigenic stimulation produced by the gut bacterial population of each GalT-KO mouse. Small differences in gut microbiota diversity could determine different repertoire and levels of natural anti-glycan antibodies and consequently might induce different immune responses to pathogens or other potential threats.

Published

2019

8. The Formation of Glycan-Specific Natural Antibodies Repertoire in GalT-KO Mice Is Determined by Gut Microbiota.

Author

Bello-Gil, Daniel, Audebert, Christophe, Olivera-Ardid, Sara, Pérez-Cruz, Magdiel, Even, Gaël, Khasbiullina, Nailya, Gantois, Nausicaa, Shilova, Nadezhda, Merlin, Sophie, Costa, Cristina, Bovin, Nicolai, and Mañez, Rafael

Subjects

IMMUNOGLOBULINS, GUT microbiome, GLYCANS, RIBOSOMAL RNA, MICROBIAL diversity

Abstract

Gut commensal bacteria are known to have a significant role in regulating the innate and adaptive immune homeostasis. Alterations in the intestinal microbial composition have been associated with several disease states, including autoimmune and inflammatory conditions. However, it is not entirely clear how commensal gut microbiota modulate and contribute to the systemic immunity, and whether circulating elements of the host immune system could regulate the microbiome. Thus, we have studied the diversity and abundance of specific taxons in the gut microbiota of inbred GalT-KO mice during 7 months of animal life by metagenetic high-throughput sequencing (16S rRNA gene, variable regions V3–V5). The repertoire of glycan-specific natural antibodies, obtained by printed glycan array technology, was then associated with the microbial diversity for each animal by metagenome-wide association studies (MWAS). Our data show that the orders clostridiales (most abundant), bacteriodales, lactobacillales , and deferribacterales may be associated with the development of the final repertoire of natural anti-glycan antibodies in GalT-KO mice. The main changes in microbiota diversity (month-2 and month-3) were related to important changes in levels and repertoire of natural anti-glycan antibodies in these mice. Additionally, significant positive and negative associations were found between the gut microbiota and the pattern of specific anti-glycan antibodies. Regarding individual features, the gut microbiota and the corresponding repertoire of natural anti-glycan antibodies showed differences among the examined animals. We also found redundancy in different taxa associated with the development of specific anti-glycan antibodies. Differences in microbial diversity did not, therefore, necessarily influence the overall functional output of the gut microbiome of GalT-KO mice. In summary, the repertoire of natural anti-carbohydrate antibodies may be partially determined by the continuous antigenic stimulation produced by the gut bacterial population of each GalT-KO mouse. Small differences in gut microbiota diversity could determine different repertoire and levels of natural anti-glycan antibodies and consequently might induce different immune responses to pathogens or other potential threats. [ABSTRACT FROM AUTHOR]

Published

2019

9. Human antibodies eluted from ligand-free Sepharose capable of binding bacterial polysaccharides and sulfated glycans.

Author

Dobrochaeva, K.L., Khasbiullina, N.R., Shilova, N.V., Obukhova, P.S., Knirel, Yu.A., Nokel, A.Yu., and Bovin, N.V.

Subjects

*SEPHAROSE, *POLYSACCHARIDES, *GLYCAN analysis, *GLYCAN structure, *BLOOD proteins

Abstract

Highlights • Human blood contains antibodies capable of binding to glycan-ligand-free Sepharose. • 'Anti-Sepharose' antibodies bind bacterial polysaccharides and sulfated glycans. • β- d -Gal seems to be a mimotope for α- l -Rha containing polysaccharides. • Part of antibodies recognize spatial rather than linear epitopes in polysaccharides. Abstract Sepharose matrix without immobilized ligands binds antibodies from human blood serum or immunoglobulin preparations. The eluted antibodies bind bacterial polysaccharides having no structural similarity to agarose (Sepharose is a cross-linked polysaccharide agarose) with a high affinity. It is concluded that the identified antibodies are capable of recognizing spatial rather than linear epitopes of bacterial polysaccharides. This side activity of Sepharose matrix should be taken into account in isolating target antibodies and other proteins from human blood. [ABSTRACT FROM AUTHOR]

Published

2019

10. Human Natural Antibodies Recognizing Glycan Galβ1-3GlcNAc (LeC)

Author

Kira Dobrochaeva, Nailya Khasbiullina, Nadezhda Shilova, Nadezhda Antipova, Polina Obukhova, Oxana Galanina, Mikhail Gorbach, Inna Popova, Sergey Khaidukov, Natalia Grishchenko, Nikolai Tupitsyn, Jacques Le Pendu, and Nicolai Bovin

Subjects

breast cancer, cancer-associated antibodies, LeC antigen, natural anti-glycan antibodies, printed glycan array, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

The level of human natural antibodies of immunoglobulin M isotype against LeC in patients with breast cancer is lower than in healthy women. The epitope specificity of these antibodies has been characterized using a printed glycan array and enzyme-linked immunosorbent assay (ELISA), the antibodies being isolated from donors’ blood using LeC-Sepharose (LeC is Galβ1-3GlcNAcβ). The isolated antibodies recognize the disaccharide but do not bind to glycans terminated with LeC, which implies the impossibility of binding to regular glycoproteins of non-malignant cells. The avidity (as dissociation constant value) of antibodies probed with a multivalent disaccharide is 10−9 M; the nanomolar level indicates that the concentration is sufficient for physiological binding to the cognate antigen. Testing of several breast cancer cell lines showed the strongest binding to ZR 75-1. Interestingly, only 7% of the cells were positive in a monolayer with a low density, increasing up to 96% at highest density. The enhanced interaction (instead of the expected inhibition) of antibodies with ZR 75-1 cells in the presence of Galβ1-3GlcNAcβ disaccharide, indicates that the target epitope of anti-LeC antibodies is a molecular pattern with a carbohydrate constituent rather than a glycan.

Published

2020

11. Human tandem-repeat-type galectins bind bacterial non-βGal polysaccharides.

Author

Knirel, Yu., Gabius, H.-J., Blixt, O., Rapoport, E., Khasbiullina, N., Shilova, N., and Bovin, N.

Abstract

Galectins are multifunctional effectors, for example acting as regulators of cell growth via protein-glycan interactions. The observation of capacity to kill bacteria for two tandem-repeat-type galectins, which target histo-blood epitopes toward this end (Stowell et al. Nat. Med. 16:295-301, ), prompted us to establish an array with bacterial polysaccharides. We addressed the question whether sugar determinants other than β-galactosides may be docking sites, using human galectins-4, -8, and -9. Positive controls with histo-blood group ABH-epitopes and the E. coli 086 polysaccharide ascertained the suitability of the set-up. Significant signal generation, depending on type of galectin and polysacchride, was obtained. Presence of cognate β-galactoside-related epitopes within a polysaccharide chain or its branch will not automatically establish binding properties, and structural constellations lacking galactosides, like rhamnan, were found to be active. These data establish the array as valuable screening tool, giving direction to further functional and structural studies. [ABSTRACT FROM AUTHOR]

Published

2014

12. Repertoire of human natural anti-glycan immunoglobulins. Do we have auto-antibodies?

Author

Bovin, Nicolai, Obukhova, Polina, Shilova, Nadezhda, Rapoport, Evgenia, Popova, Inna, Navakouski, Maksim, Unverzagt, Carlo, Vuskovic, Marko, and Huflejt, Margaret

Subjects

*GLYCANS, *AUTOANTIBODIES, *EPITOPES, *BLOOD serum analysis, *GLYCOLIPIDS, *ENZYME-linked immunosorbent assay, *IMMUNOGLOBULINS

Abstract

Abstract: Background: Profiling of donor''s antibodies using glycan arrays demonstrated presence of antibodies capable of binding to >100 mammalian glycans or their fragments. For example, relatively high binding to Galα1-4Galβ1-4GlcNAc (P1), Galα1-4Galβ1-4Glc (Pk), Galβ1-3GlcNAc (Lec), 4-O-SuGalβ1-4GlcNAc, and GalNAcα1-3GalNAc (Fs) was found in all tested individuals. Affinity isolation using hapten-specific chromatography in combination with epitope mapping revealed their glycotopes. Notably, a significant part of the antibodies was capable of recognizing a fragment of larger glycans, for example, -Galβ1-4Glc of glycolipids, or Fucα1-3GlcNAc motif of LeX/LeY antigens. Their epitope specificity did not vary between different healthy individuals. Nominally, all the mentioned immunoglobulins could be classified as auto-antibodies. Methods: In this work we re-evaluated results published earlier and analyzed new data to address the question why autologous antibodies found in healthy individuals do not cause severe auto-immune reactions. Results: In all cases the presumably “auto” antibodies were found to bind short fragments “subtracted” from larger glycans whereas recognition of the same fragment in the context of the whole natural chain was completely abolished. Thus, in spite of numerous formally positive signals observed on the printed glycan array, we are yet unable to identify in blood serum of healthy individuals true auto-antibodies capable of binding carbohydrate chains in their naturally occurring form. General significance: The identified natural anti-glycan antibodies were found to be specific, high-titer and population conservative immunoglobulins — all of this suggesting as yet unknown biological role(s) of the studied proteins. This article is part of a Special Issue entitled Glycoproteomics. [Copyright &y& Elsevier]

Published

2012

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

Author

Shilova, Nadezhda, Navakouski, Maxim, Khasbiullina, Nailya, Blixt, Ola, and Bovin, Nicolai

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. [ABSTRACT FROM AUTHOR]

Published

2012

14. Anti-carbohydrate antibodies of normal sera: Findings, surprises and challenges

Author

Huflejt, Margaret E., Vuskovic, Marko, Vasiliu, Daniela, Xu, Hongyu, Obukhova, Polina, Shilova, Nadezhda, Tuzikov, Alexander, Galanina, Oxana, Arun, Banu, Lu, Karen, and Bovin, Nicolai

Subjects

*AUTOANTIBODIES, *BLOOD testing, *GLYCOPROTEINS, *GLYCOLIPIDS, *OLIGOSACCHARIDES, *CARBOHYDRATES in the body, *MOLECULAR immunology

Abstract

Abstract: We have used microchip format glycan array to characterize the individual carbohydrate recognition patterns by antibodies (Ab) in sera of 106 healthy donors. The glycan library included blood group antigens and other most frequent terminal oligosaccharides and their cores of mammalian N- and O-linked glycoproteins and glycolipids, tumor-associated carbohydrate antigens, and common components of bacterial/pathogenic polysaccharides and lipopolysaccharides, totally 205 glycans. The serum Ab interacted with at least 50 normal human glyco-motifs. Apart from expected blood group-, xeno- (heterophil) and infection-related binding activities, we observed a number of new and unexpected features. The surprising, relatively high antibody binding was found to the blood group P1 and Pk trisaccharides and H(type 2) trisaccharide. Novel and very high binding activities have been observed towards Galβ1-3GlcNAc (LeC) related glycans, especially 3′-O-Su-LeC, and towards 4′-O-sulfated lactosamine. Relatively high and uniform Ab binding to GalNAcα1-3Gal disaccharide demonstrated absence of correlation with fucosylated blood group A GalNAcα1-3(Fucα1-2)Gal antigen—similarly to well known relationship between Galα1-3Gal and true, fucosylated blood group B Galα1-3(Fucα1-2)Gal antigen. The binding intensity to Galα1-3Galβ1-4GlcNAc xenoantigen was shown to be rather modest. Absence or very low Ab binding was found against oligosialic acid, sialooligosaccharides except SiaTn, type 2 backbone glycans such as Ley, and biantennary N-chain as well as its truncated forms, i.e. without terminal Sia, SiaGal, and SiaGalGlcNAc motifs. We have also found that Ab are capable of recognizing the short inner core typical for glycolipids (–Galβ1-4Glc) and glycoproteins (–GalNAcα) as a fragment of bigger glycans. [Copyright &y& Elsevier]

Published

2009

15. Improved spot morphology for printed glycan arrays

Author

Navakouski, Maksim, Shilova, Nadezhda, Khasbiullina, Nailya, Feofanov, Alexey, Pudova, Elena, Chen, Kowa, Blixt, Klas Ola, Bovin, Nicolai, Navakouski, Maksim, Shilova, Nadezhda, Khasbiullina, Nailya, Feofanov, Alexey, Pudova, Elena, Chen, Kowa, Blixt, Klas Ola, and Bovin, Nicolai

Published

2018

16. Human Natural Antibodies Recognizing Glycan Galβ1-3GlcNAc (LeC).

Author

Dobrochaeva, Kira, Khasbiullina, Nailya, Shilova, Nadezhda, Antipova, Nadezhda, Obukhova, Polina, Galanina, Oxana, Gorbach, Mikhail, Popova, Inna, Khaidukov, Sergey, Grishchenko, Natalia, Tupitsyn, Nikolai, Pendu, Jacques Le, and Bovin, Nicolai

Subjects

*GLYCANS, *IMMUNOGLOBULINS, *IMMUNOGLOBULIN M, *ENZYME-linked immunosorbent assay, *CANCER cells, *GLYCOPROTEINS

Abstract

The level of human natural antibodies of immunoglobulin M isotype against LeC in patients with breast cancer is lower than in healthy women. The epitope specificity of these antibodies has been characterized using a printed glycan array and enzyme-linked immunosorbent assay (ELISA), the antibodies being isolated from donors' blood using LeC-Sepharose (LeC is Galβ1-3GlcNAcβ). The isolated antibodies recognize the disaccharide but do not bind to glycans terminated with LeC, which implies the impossibility of binding to regular glycoproteins of non-malignant cells. The avidity (as dissociation constant value) of antibodies probed with a multivalent disaccharide is 10−9 M; the nanomolar level indicates that the concentration is sufficient for physiological binding to the cognate antigen. Testing of several breast cancer cell lines showed the strongest binding to ZR 75-1. Interestingly, only 7% of the cells were positive in a monolayer with a low density, increasing up to 96% at highest density. The enhanced interaction (instead of the expected inhibition) of antibodies with ZR 75-1 cells in the presence of Galβ1-3GlcNAcβ disaccharide, indicates that the target epitope of anti-LeC antibodies is a molecular pattern with a carbohydrate constituent rather than a glycan. [ABSTRACT FROM AUTHOR]

Published

2020

17. Improved spot morphology for printed glycan arrays.

Author

Maksim N, Nadezhda S, Nailya K, Alexey F, Elena P, Kowa C, Ola B, and Nicolai B

Subjects

Animals, Antibodies immunology, Bioprinting methods, Fluorescence, Fluorescent Dyes chemistry, Humans, Hydrophobic and Hydrophilic Interactions, Microarray Analysis methods, Polysaccharides immunology, Bioprinting instrumentation, Glycoconjugates chemistry, Lab-On-A-Chip Devices, Microarray Analysis instrumentation, Polymers chemistry, Polysaccharides chemistry

Abstract

Despite considerable success studying glycan-binding proteins using printed glycan arrays (PGAs), unambiguous quantitation of spot intensities by fluorescent readers remains a challenge. The main obstacles are the varying spot shape and size and in-spot fluorescence distribution caused by uneven drying of the printed drops. Two methods have been suggested for solving this problem: using polymeric glycoconjugates, which makes it possible to equalize the physicochemical properties (hydrophobicity, charge, and size) of different glycans, and applying a glycan solution on a slide coated with a thin oil mask, which hinders evaporation of the drop. Both approaches yield spots with similar sizes and an even distribution of the signal across the spot and are likely to be useful for improving the prints of other classes of molecules.

Published

2018