The Effect of Glycosylation on the Antibody Recognition of a MUC2 Mucin Epitope

被引:12
|
作者
Uray, Katalin [1 ]
Mizuno, Mamoru [2 ]
Inazu, Toshiyuki [3 ,4 ]
Goto, Kohtaro [2 ]
Hudecz, Ferenc [1 ,5 ]
机构
[1] Eotvos Lorand Univ, Hungarian Acad Sci, Res Grp Peptide Chem, H-1518 Budapest, Hungary
[2] Noguchi Inst, Lab Glycoorgan Chem, Tokyo, Japan
[3] Tokai Univ, Sch Engn, Dept Appl Chem, Hiratsuka, Kanagawa 25912, Japan
[4] Tokai Univ, Inst Glycosci, Hiratsuka, Kanagawa 25912, Japan
[5] Eotvos Lorand Univ, Inst Chem, H-1518 Budapest, Hungary
关键词
MUC2; mucin; glycosylated peptides; antibody binding of epitope; INTESTINAL MUCIN; CORE EPITOPE; PEPTIDE;
D O I
10.1002/bip.22526
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
MUC2 glycoprotein, produced by the epithelium of the colon and built up mainly of repeat units of (1)PTTTPITTTTTVTPTPTPTGTQT(23), can be overexpressed or underglycosylated in gastrointestinal diseases, e. g. in case of colon carcinoma. We have been studying the epitope structure of the MUC2 by focusing on the repeat unit with the mucin peptide specific MAb 996 monoclonal antibody. This antibody recognizes the (18)PTGTQ(22) sequence as minimal, and (16)PTPTGTQ(22) as optimal epitope within the underglycosylated glycoprotein. In this article, we aim to clarify the effect of glycosylation of the epitope on MAb 996 antibody binding including its correlation with the secondary structure of the modified peptides: glycosylation in the epitope core and in the flank. For this we have prepared the (16)PTPTGTQ(22) peptide glycosylated with N-acetylgalactoseamine (Tn antigen) in position 17, 19, 21, or on all three threonines. The MAb 996 antibody binding properties of the peptides were characterized in competitive ELISA experiments, and their solution secondary structure was studied by circular dichroism spectroscopy in water and in the ordered structure promoting trifluoroethanol. Our results show that glycosylation in position 19 (peptide (PTPT)-P-16(GalNAca) GTQ(22)) resulted in enhanced antibody recognition and significantly altered secondary structure, while glycosylation in position 21 completely demolished the binding. These findings could be useful in determining the nature of antigen-antibody interaction, and perhaps designing synthetic peptide vaccines for tumor therapy. (C) 2014 Wiley Periodicals, Inc.
引用
收藏
页码:390 / 395
页数:6
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