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重组核心蛋白聚糖结构域I的特性及其被糖胺聚糖和寡糖的取代

Characterization of recombinant perlecan domain I and its substitution by glycosaminoglycans and oligosaccharides.

作者信息

Costell M, Mann K, Yamada Y, Timpl R

机构信息

Max-Planck-Institut für Biochemie, Martinsried, Germany.

出版信息

Eur J Biochem. 1997 Jan 15;243(1-2):115-21. doi: 10.1111/j.1432-1033.1997.t01-1-00115.x.

Abstract

Recombinant mouse perlecan domain 1(173 residues) was produced in transfected embryonic kidney cells and purified from the culture medium on DEAE-cellulose. It was shown to be modified by glycosaminoglycans and could be partially separated into two protein pools which were either substituted with heparan sulfate (fragment IA) or, to a smaller extent (20%), with chondroitin/dermatan sulfate or a mixture of both glycosaminoglycans (fragment IB). The average molecular mass of the glycosaminoglycans was about 8-10 kDa and, thus, smaller than in tissue-derived perlecans. Sequence and carbohydrate analyses localized the heparan sulfate attachment site to three Ser residues within SGD consensus sequences. Furthermore, the N-terminal part of fragment IA contained six Thr/Ser residues substituted by branched galactosamine-containing oligosaccharides and an N-substituted Asn residue. Fragment I was also shown to contain unique immunological epitopes which are not dependent on glycosaminoglycans and are shared by tissue-derived perlecan. Circular dichroism demonstrated a distinct alpha helix (20%) and beta structure (60%) in fragment IA, consistent with predictions of a novel SEA protein module located in the C-terminal part of domain I.

摘要

重组小鼠核心蛋白聚糖结构域1(173个残基)在转染的胚胎肾细胞中产生,并在DEAE - 纤维素上从培养基中纯化。结果表明它被糖胺聚糖修饰,并且可以部分分离为两个蛋白池,一个被硫酸乙酰肝素取代(片段IA),另一个较小比例(20%)被硫酸软骨素/硫酸皮肤素或这两种糖胺聚糖的混合物取代(片段IB)。糖胺聚糖的平均分子量约为8 - 10 kDa,因此比组织来源的核心蛋白聚糖中的糖胺聚糖分子量小。序列和碳水化合物分析将硫酸乙酰肝素连接位点定位到SGD共有序列内的三个丝氨酸残基上。此外,片段IA的N端部分包含六个被含分支半乳糖胺的寡糖取代的苏氨酸/丝氨酸残基和一个N - 取代的天冬酰胺残基。片段I还显示含有独特的免疫表位,这些表位不依赖于糖胺聚糖,并且与组织来源的核心蛋白聚糖共有。圆二色性表明片段IA中存在明显的α螺旋(20%)和β结构(60%),这与位于结构域I C端部分的新型SEA蛋白模块的预测一致。

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