Literature DB >> 9356147

beta-Elimination of O-glycans from glycoproteins transferred to immobilon P membranes: method and some applications.

M Duk1, M Ugorski, E Lisowska.   

Abstract

Selective beta-elimination of O-glycans from glycoproteins transferred from electrophoretic gels onto Immobilon P membranes is described. The experiments were performed with erythrocyte membrane proteins, in which glycophorins are the major poly-O-glycosylated components, and with lysates of human colon cancer cells CX-1.1. Lectins and monoclonal antibodies against peptidic, glycopeptidic, and carbohydrate epitopes were used to examine the effect of degradation. Experiments with erythrocyte membrane proteins showed that after heating the blots in 0.055 M NaOH for 16 h at 40 degrees C the O-glycans of glycophorins were undetectable, while N-glycans and peptidic epitopes of proteins were detected with unchanged or even increased intensity compared to untreated blots. The method was used to show that most protein-linked sialyl-Lea epitopes present on CX-1.1 cancer cells are located on O-glycosidic chains. Moreover, beta-elimination on the blots allows examination of the dependence of peptidic epitopes on O-glycosylation. This was shown using monoclonal antibodies specific for blood group M- or N-related epitopes of glycophorin A (GPA). Most of these antibodies recognize glycopeptidic epitopes dependent on O-glycosylation and, therefore, they did not detect GPA on NaOH-treated blots. Some less frequent anti-M antibodies cross-reacting with the rare GPA variant of Mg type are specific for a peptidic epitope which is unrelated to the MN blood group-specific amino acid sequence in unglycosylated peptides, but is recognized in GPA-M only in the glycosylated antigen. These antibodies, which showed specificity for GPA-M on untreated blots, detected GPA-M, GPA-N, and glycophorin B on NaOH-treated blots. Copyright 1997 Academic Press.

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Year:  1997        PMID: 9356147     DOI: 10.1006/abio.1997.9994

Source DB:  PubMed          Journal:  Anal Biochem        ISSN: 0003-2697            Impact factor:   3.365


  14 in total

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3.  Detection and analysis of proteins modified by O-linked N-acetylglucosamine.

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Journal:  Curr Protoc Mol Biol       Date:  2011-07

4.  The Arabidopsis O-linked N-acetylglucosamine transferase SPINDLY interacts with class I TCPs to facilitate cytokinin responses in leaves and flowers.

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5.  Identification and origin of N-linked β-D-N-acetylglucosamine monosaccharide modifications on Arabidopsis proteins.

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6.  Glucose deprivation-induced increase in protein O-GlcNAcylation in cardiomyocytes is calcium-dependent.

Authors:  Luyun Zou; Xiaoyuan Zhu-Mauldin; Richard B Marchase; Andrew J Paterson; Jian Liu; Qinglin Yang; John C Chatham
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8.  Characterization of the specificity of O-GlcNAc reactive antibodies under conditions of starvation and stress.

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Review 9.  Lectins as tools in glycoconjugate research.

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Journal:  Glycoconj J       Date:  2009-11       Impact factor: 2.916

10.  Beta-1,2 oligomannose adhesin epitopes are widely distributed over the different families of Candida albicans cell wall mannoproteins and are associated through both N- and O-glycosylation processes.

Authors:  Chantal Fradin; Marie Christine Slomianny; Céline Mille; Annick Masset; Raymond Robert; Boualem Sendid; Joachim F Ernst; Jean Claude Michalski; Daniel Poulain
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