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人α1,3/4-岩藻糖基转移酶III-VII在复合糖型N-聚糖上LewisX和唾液酸化LewisX基序生物合成中的体内特异性。与人类β-微量蛋白一起进行的bhk-21细胞共表达研究。

In vivo specificity of human alpha1,3/4-fucosyltransferases III-VII in the biosynthesis of LewisX and Sialyl LewisX motifs on complex-type N-glycans. Coexpression studies from bhk-21 cells together with human beta-trace protein.

作者信息

Grabenhorst E, Nimtz M, Costa J, Conradt H S

机构信息

Protein Glycosylation, Gesellschaft für Biotechnologische Forschung mbH, D-38124 Braunschweig, Germany.

出版信息

J Biol Chem. 1998 Nov 20;273(47):30985-94. doi: 10.1074/jbc.273.47.30985.

DOI:10.1074/jbc.273.47.30985
PMID:9812995
Abstract

Each of the five human alpha1,3/4-fucosyltransferases (FT3 to FT7) has been stably expressed in BHK-21 cells together with human beta-trace protein (beta-TP) as a secretory reporter glycoprotein. In order to study their in vivo properties for the transfer of peripheral Fuc onto N-linked complex-type glycans, detailed structural analysis was performed on the purified glycoprotein. All fucosyltransferases were found to peripherally fucosylate 19-52% of the diantennary beta-TP N-glycans, and all enzymes were capable of synthesizing the sialyl LewisX (sLex) motif. However, each enzyme produced its own characteristic ratio of sLex/Lex antennae as follows: FT7 (only sLex), FT3 (14:1), FT5 (3:1), FT6 (1.1:1), and FT4 (1:7). Fucose transfer onto beta-TP N-glycans was low in FT3 cells (11% of total antennae), whereas the values for FT7, FT5, FT4, and FT6 cells were 21, 25, 35, and 47%, respectively. FT3, FT4, FT5, and FT7 transfer preponderantly one Fuc per diantennary N-glycan. FT4 preferentially synthesizes di-Lex on asialo diantennary N-glycans and mono-Lex with monosialo chains. In contrast, FT6 forms mostly alpha1,3-difucosylated chains with no, one, or two NeuAc residues. FT3, FT4, and FT6 were proteolytically cleaved and released into the culture medium in significant amounts, whereas FT7 and FT5 were found to be largely resistant toward proteolysis. Studies on engineered soluble variants of FT6 indicate that these forms do not significantly contribute to the in vivo fucose transfer activity of the enzyme when expressed at activity levels comparable to those obtained for the wild-type Golgi form of FT6 in the recombinant host cells.

摘要

五种人类α1,3/4-岩藻糖基转移酶(FT3至FT7)中的每一种都已与人类β-微量蛋白(β-TP)作为分泌型报告糖蛋白在BHK-21细胞中稳定表达。为了研究它们在体内将外周岩藻糖转移到N-连接复合型聚糖上的特性,对纯化的糖蛋白进行了详细的结构分析。发现所有岩藻糖基转移酶可使19-52%的二天线β-TP N-聚糖发生外周岩藻糖基化,并且所有酶都能够合成唾液酸化路易斯X(sLex)基序。然而,每种酶产生其自身特征性的sLex/Lex天线比例如下:FT7(仅sLex)、FT3(14:1)、FT5(3:1)、FT6(1.1:1)和FT4(1:7)。FT3细胞中β-TP N-聚糖上的岩藻糖转移率较低(占总天线的11%),而FT7、FT5、FT4和FT6细胞的值分别为21%、25%、35%和47%。FT3、FT4、FT5和FT7每个二天线N-聚糖主要转移一个岩藻糖。FT4优先在去唾液酸二天线N-聚糖上合成二Lex,在单唾液酸链上合成单Lex。相反,FT6主要形成具有零个、一个或两个NeuAc残基的α1,3-二岩藻糖基化链。FT3、FT4和FT6被蛋白水解切割并大量释放到培养基中,而FT7和FT5被发现对蛋白水解具有很大抗性。对FT6工程化可溶性变体的研究表明,当这些形式在重组宿主细胞中以与野生型高尔基体形式的FT6相当的活性水平表达时,它们对该酶的体内岩藻糖转移活性没有显著贡献。

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