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MS-Based Allotype-Specific Analysis of Polyclonal IgG-Fc N-Glycosylation
by
Domínguez-Vega, Elena
, Falck, David
, Sénard, Thomas
, de Taeye, Steven W.
, Rispens, Theo
, Gargano, Andrea F. G.
, Somsen, Govert W.
, Wuhrer, Manfred
, Vidarsson, Gestur
in
Allotypes
/ Amino acids
/ Antibodies
/ Capillary electrophoresis
/ Chromatography
/ Chromatography, Liquid
/ Data Analysis
/ Electrophoresis, Capillary
/ Enzymes
/ fragment crystallizable
/ Glycoproteins
/ Glycosylation
/ Humans
/ Immune system
/ Immunoglobulin Allotypes - immunology
/ Immunoglobulin Fc Fragments - chemistry
/ Immunoglobulin Fc Fragments - metabolism
/ Immunoglobulin G
/ Immunoglobulin G - chemistry
/ Immunoglobulin G - immunology
/ Immunoglobulin G - isolation & purification
/ Immunoglobulin G - metabolism
/ Immunology
/ Liquid chromatography
/ mass spectrometry
/ Mass Spectrometry - methods
/ Mass spectroscopy
/ N-glycosylation
/ Oxidation
/ Plasma
/ Post-translation
/ post-translational modifications
/ Protein Processing, Post-Translational
/ Proteins
/ Workflow
2020
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MS-Based Allotype-Specific Analysis of Polyclonal IgG-Fc N-Glycosylation
by
Domínguez-Vega, Elena
, Falck, David
, Sénard, Thomas
, de Taeye, Steven W.
, Rispens, Theo
, Gargano, Andrea F. G.
, Somsen, Govert W.
, Wuhrer, Manfred
, Vidarsson, Gestur
in
Allotypes
/ Amino acids
/ Antibodies
/ Capillary electrophoresis
/ Chromatography
/ Chromatography, Liquid
/ Data Analysis
/ Electrophoresis, Capillary
/ Enzymes
/ fragment crystallizable
/ Glycoproteins
/ Glycosylation
/ Humans
/ Immune system
/ Immunoglobulin Allotypes - immunology
/ Immunoglobulin Fc Fragments - chemistry
/ Immunoglobulin Fc Fragments - metabolism
/ Immunoglobulin G
/ Immunoglobulin G - chemistry
/ Immunoglobulin G - immunology
/ Immunoglobulin G - isolation & purification
/ Immunoglobulin G - metabolism
/ Immunology
/ Liquid chromatography
/ mass spectrometry
/ Mass Spectrometry - methods
/ Mass spectroscopy
/ N-glycosylation
/ Oxidation
/ Plasma
/ Post-translation
/ post-translational modifications
/ Protein Processing, Post-Translational
/ Proteins
/ Workflow
2020
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MS-Based Allotype-Specific Analysis of Polyclonal IgG-Fc N-Glycosylation
by
Domínguez-Vega, Elena
, Falck, David
, Sénard, Thomas
, de Taeye, Steven W.
, Rispens, Theo
, Gargano, Andrea F. G.
, Somsen, Govert W.
, Wuhrer, Manfred
, Vidarsson, Gestur
in
Allotypes
/ Amino acids
/ Antibodies
/ Capillary electrophoresis
/ Chromatography
/ Chromatography, Liquid
/ Data Analysis
/ Electrophoresis, Capillary
/ Enzymes
/ fragment crystallizable
/ Glycoproteins
/ Glycosylation
/ Humans
/ Immune system
/ Immunoglobulin Allotypes - immunology
/ Immunoglobulin Fc Fragments - chemistry
/ Immunoglobulin Fc Fragments - metabolism
/ Immunoglobulin G
/ Immunoglobulin G - chemistry
/ Immunoglobulin G - immunology
/ Immunoglobulin G - isolation & purification
/ Immunoglobulin G - metabolism
/ Immunology
/ Liquid chromatography
/ mass spectrometry
/ Mass Spectrometry - methods
/ Mass spectroscopy
/ N-glycosylation
/ Oxidation
/ Plasma
/ Post-translation
/ post-translational modifications
/ Protein Processing, Post-Translational
/ Proteins
/ Workflow
2020
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MS-Based Allotype-Specific Analysis of Polyclonal IgG-Fc N-Glycosylation
Journal Article
MS-Based Allotype-Specific Analysis of Polyclonal IgG-Fc N-Glycosylation
2020
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Overview
Current approaches to study glycosylation of polyclonal human immunoglobulins G (IgG) usually imply protein digestion or glycan release. While these approaches allow in-depth characterization, they also result in a loss of valuable information regarding certain subclasses, allotypes and co-occuring post-translational modifications (PTMs). Unfortunately, the high variability of polyclonal IgGs makes their intact mass spectrometry (MS) analysis extremely challenging. We propose here a middle-up strategy for the analysis of the intact fragment crystallizable (Fc) region of human plasma IgGs, with the aim of acquiring integrated information of the
-glycosylation and other PTMs of subclasses and allotypes. Human plasma IgG was isolated using Fc-specific beads followed by an on-bead C
2 domain digestion with the enzyme IdeS. The obtained mixture of Fc subunits was analyzed by capillary electrophoresis (CE) and hydrophilic interaction liquid chromatography (HILIC) hyphenated with MS. CE-MS provided separation of different IgG-subclasses and allotypes, while HILIC-MS allowed resolution of the different glycoforms and their oxidized variants. The orthogonality of these techniques was key to reliably assign Fc allotypes. Five individual donors were analyzed using this approach. Heterozygosis was observed in all the analyzed donors resulting in a total of 12 allotypes identified. The assignments were further confirmed using recombinant monoclonal IgG allotypes as standards. While the glycosylation patterns were similar within allotypes of the same subclass, clear differences were observed between IgG subclasses and donors, highlighting the relevance of the proposed approach. In a single analysis, glycosylation levels specific for each allotype, relative abundances of subclasses and information on co-occurring modifications are obtained. This middle-up method represents an important step toward a comprehensive analysis of immunoglobulin G-Fc variants.
Publisher
Frontiers Media SA,Frontiers Media S.A
Subject
/ Enzymes
/ Humans
/ Immunoglobulin Allotypes - immunology
/ Immunoglobulin Fc Fragments - chemistry
/ Immunoglobulin Fc Fragments - metabolism
/ Immunoglobulin G - chemistry
/ Immunoglobulin G - immunology
/ Immunoglobulin G - isolation & purification
/ Immunoglobulin G - metabolism
/ Plasma
/ post-translational modifications
/ Protein Processing, Post-Translational
/ Proteins
/ Workflow
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