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从软体动物贝壳形成液中分离出的具有内部岩藻糖分支到 GlcA 和 GlcN 残基的异常 N-聚糖结构。

Anomalous N-glycan structures with an internal fucose branched to GlcA and GlcN residues isolated from a mollusk shell-forming fluid.

机构信息

Glycomics Center, University of New Hampshire , 35 Colovos Road, Durham, New Hampshire 03824, United States.

出版信息

J Proteome Res. 2013 Oct 4;12(10):4547-55. doi: 10.1021/pr4006734. Epub 2013 Sep 17.

Abstract

This report describes the structural details of a unique N-linked valence epitope on the major protein within the extrapallial (EP) fluid of the mollusk, Mytilus edulis. Fluids from this area are considered to be responsible for shell expansion by a self-assembly process that provides an organic framework for the growth of CaCO3 crystals. Previous reports from our laboratories have described the purification and amino acid sequence of this EP protein, which was found to be a glycoprotein (EPG) of approximately 28 KDa with 14.3% carbohydrate on a single N-linked consensus site. Described herein is the de novo sequence of the major glycan and its glycomers. The sequence was determined by ion trap sequential mass spectrometry (ITMS(n)) resolving structure by tracking precursor-product relationships through successive rounds of collision induced disassociation (CID), thereby spatially resolving linkage and branching details within the confines of the ion trap. Three major glycomers were detected, each possessing a 6-linked fucosylated N-linked core. Two glycans possessed four and five identical antennae, while the third possessed four antennas, but with an additional methylfucose 2-linked to the glucuronic acid moiety, forming a pentasaccharide. The tetrasaccharide structure was: 4-O-methyl-GlcA(1-4)[GlcNAc(1-3)]Fuc(1-4)GlcNAc, while the pentasaccharide was shown to be as follows: mono-O-methyl-Fuc(1-2)-4-O-methyl-GlcA(1-4)[GlcNAc(1-3)]Fuc(1-4)GlcNAc. Samples were differentially deuteriomethylated (CD3/CH3) to localize indigenous methylation, further analyzed by high resolution mass spectrometry (HRMS) to confirm monomer compositions, and finally gas chromatography mass spectrometry (GC-MS) to assign structural and stereoisomers. The interfacial shell surface location of this major extrapallial glycoprotein, its calcium and heavy metal binding properties and unique structure suggests a probable role in shell formation and possibly metal ion detoxification. A closely related terminal tetrasaccharide structure has been reported in spermatozoan glycolipids of freshwater bivalves.

摘要

本报告描述了贻贝外套膜(EP)液体内主要蛋白上独特的 N 连接价表位的结构细节。该区域的液体被认为通过自组装过程负责贝壳扩张,为 CaCO3 晶体的生长提供有机框架。我们实验室之前的报告描述了这种 EP 蛋白的纯化和氨基酸序列,发现它是一种糖蛋白(EPG),分子量约为 28 kDa,在单个 N 连接保守位点上有 14.3%的碳水化合物。本文描述了主要聚糖及其糖基的从头序列。该序列通过离子阱顺序质谱(ITMS(n))确定,通过在连续的碰撞诱导解离(CID)循环中跟踪前体-产物关系来解析结构,从而在离子阱的限制范围内空间解析连接和分支细节。检测到三种主要糖基,每个都具有 6 连接的岩藻糖基化 N 连接核心。两种聚糖具有四个和五个相同的触角,而第三种聚糖具有四个触角,但在葡萄糖醛酸部分上额外连接了一个甲基岩藻糖,形成五糖。四糖结构为:4-O-甲基-GlcA(1-4)[GlcNAc(1-3)]Fuc(1-4)GlcNAc,而五糖结构如下所示:单-O-甲基-Fuc(1-2)-4-O-甲基-GlcA(1-4)[GlcNAc(1-3)]Fuc(1-4)GlcNAc。样品进行了差示氘甲基化(CD3/CH3)以定位内源性甲基化,然后通过高分辨率质谱(HRMS)进一步分析以确认单体组成,最后通过气相色谱质谱(GC-MS)分配结构和立体异构体。这种主要的外套膜糖蛋白在界面贝壳表面的位置、其钙和重金属结合特性以及独特的结构表明它可能在贝壳形成和可能的金属离子解毒中发挥作用。在淡水双壳类动物的精子糖脂中已经报道了密切相关的末端四糖结构。

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