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Glyco-Engineering

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Cover of 'Glyco-Engineering'

Table of Contents

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    Book Overview
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    Chapter 1 Current Approaches to Engineering N -Linked Protein Glycosylation in Bacteria
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    Chapter 2 Inverse Metabolic Engineering for Enhanced Glycoprotein Production in Escherichia coli
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    Chapter 3 GlycoSNAP: A High-Throughput Screening Methodology for Engineering Designer Glycosylation Enzymes
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    Chapter 4 Production of Glycoproteins with Asparagine-Linked N -Acetylglucosamine in Escherichia coli
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    Chapter 5 Glyco-engineering O-Antigen-Based Vaccines and Diagnostics in E. coli
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    Chapter 6 Progress in Yeast Glycosylation Engineering.
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    Chapter 7 Protein Production with a Pichia pastoris OCH1 Knockout Strain in Fed-Batch Mode.
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    Chapter 8 Engineering the Pichia pastoris N-Glycosylation Pathway Using the GlycoSwitch Technology
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    Chapter 9 Development of a Valuable Yeast Strain Using a Novel Mutagenesis Technique for the Effective Production of Therapeutic Glycoproteins.
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    Chapter 10 An Overview and History of Glyco-Engineering in Insect Expression Systems.
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    Chapter 11 Glyco-Engineering
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    Chapter 12 Glyco-Engineering
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    Chapter 13 Engineering N-Glycosylation Pathway in Insect Cells: Suppression of β-N-Acetylglucosaminidase and Expression of β-1,4-Galactosyltransferase.
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    Chapter 14 N-Glyco-Engineering in Plants: Update on Strategies and Major Achievements
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    Chapter 15 Glyco-Engineering
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    Chapter 16 Im“plant”ing of Mammalian Glycosyltransferase Gene into Plant Suspension-Cultured Cells Using Agrobacterium-Mediated Transformation
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    Chapter 17 Transient Glyco-Engineering of N. benthamiana Aiming at the Synthesis of Multi-antennary Sialylated Proteins
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    Chapter 18 Subcellular Targeting of Proteins Involved in Modification of Plant N- and O-Glycosylation
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    Chapter 19 Assembly of Multigene Constructs Using Golden Gate Cloning.
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    Chapter 20 Strategies for Engineering Protein N-Glycosylation Pathways in Mammalian Cells
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    Chapter 21 Glycan Remodeling with Processing Inhibitors and Lectin-Resistant Eukaryotic Cells
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    Chapter 22 Production of Highly Sialylated Recombinant Glycoproteins Using Ricinus communis Agglutinin-I-Resistant CHO Glycosylation Mutants
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    Chapter 23 Metabolic Glyco-Engineering in Eukaryotic Cells and Selected Applications
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    Chapter 24 Evaluation of Quenching and Extraction Methods for Nucleotide/Nucleotide Sugar Analysis
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    Chapter 25 Chemoenzymatic Glyco-engineering of Monoclonal Antibodies
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    Chapter 26 Chemical Polysialylation of Recombinant Human Proteins
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    Chapter 27 Site-Specific Glycosylation Profiling Using Liquid Chromatography-Tandem Mass Spectrometry (LC-MS)
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    Chapter 28 Mass Spectrometric Analysis of Oligo- and Polysialic Acids
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    Chapter 29 Isomer-Specific Analysis of Released N-Glycans by LC-ESI MS/MS with Porous Graphitized Carbon
Attention for Chapter 23: Metabolic Glyco-Engineering in Eukaryotic Cells and Selected Applications
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Chapter title
Metabolic Glyco-Engineering in Eukaryotic Cells and Selected Applications
Chapter number 23
Book title
Glyco-Engineering
Published in
Methods in molecular biology, January 2015
DOI 10.1007/978-1-4939-2760-9_23
Pubmed ID
Book ISBNs
978-1-4939-2759-3, 978-1-4939-2760-9
Authors

Friedrich Piller, Aline Mongis, Véronique Piller

Abstract

By metabolic glyco-engineering cellular glycoconjugates are modified through the incorporation of synthetic monosaccharides which are usually analogues of naturally present sugars. In order to get incorporated, the monosaccharides need to enter the cytoplasm and to be substrates for the enzymes necessary for their transformation into activated sugars, most often nucleotide sugars. These have to be substrates for glycosyltransferases which finally catalyze their incorporation into glycans. Such pathways are difficult to reconstitute in vitro and therefore new monosaccharide analogues have to be tested in tissue culture for their suitability in metabolic glyco-engineering. For this, glycosylation mutants are the most appropriate since they are unable to synthesize specific glycans but through the introduction of the monosaccharide analogues they may express some glycans at the cell surface with the unnatural sugar incorporated. The presence of those glycans can be easily and quantitatively detected by lectin binding or by chemical methods identifying specific sugars. Monosaccharide analogues can also block the pathways leading to sugar incorporation, thus inhibiting the synthesis of glycan structures which is also easily detectable at the cell surface by lectin labeling. The most useful and most frequently employed application of metabolic glyco-engineering is the introduction of reactive groups which can undergo bio-orthogonal click reactions for the efficient labeling of glycans at the surface of live cells.

Mendeley readers

Mendeley readers

The data shown below were compiled from readership statistics for 3 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 3 100%

Demographic breakdown

Readers by professional status Count As %
Researcher 1 33%
Unknown 2 67%
Readers by discipline Count As %
Engineering 1 33%
Unknown 2 67%