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人重组α1,3/4-岩藻糖基转移酶不同长度构建体的受体特异性。用蛋白A替换岩藻糖基转移酶V的茎区和跨膜结构域可产生具有GDP-岩藻糖水解活性的酶。

Acceptor specificity of different length constructs of human recombinant alpha 1,3/4-fucosyltransferases. Replacement of the stem region and the transmembrane domain of fucosyltransferase V by protein A results in an enzyme with GDP-fucose hydrolyzing activity.

作者信息

de Vries T, Srnka C A, Palcic M M, Swiedler S J, van den Eijnden D H, Macher B A

机构信息

Department of Chemistry and Biochemistry, San Francisco State University, California 94132, USA.

出版信息

J Biol Chem. 1995 Apr 14;270(15):8712-22. doi: 10.1074/jbc.270.15.8712.

Abstract

The acceptor specificity of recombinant full-length, membrane-bound fucosyltransferases, expressed in COS-7 cells, and soluble, protein-A chimeric forms of alpha 1,3-fucosyltransferase (Fuc-T) III, Fuc-TIV, and Fuc-TV was analyzed toward a broad panel of oligosaccharide, glycolipid, and glycoprotein substrates. Our results on the full-length enzymes confirm and extend previous studies. However, chimeric Fuc-Ts showed increased activity toward glycoproteins, whereas chimeric Fuc-TIII and Fuc-TV had a decreased activity with glycosphingolipids, compared to the full-length enzymes. Unexpectedly, chimeric Fuc-TV exhibited a GDP-fucose hydrolyzing activity. In substrates with multiple acceptor sites, the preferred site of fucosylation was identified. Fuc-TIII and Fuc-TV catalyzed fucose transfer exclusively to OH-3 of glucose in lacto-N-neotetraose and lacto-N-tetraose, respectively, as was demonstrated by 1H NMR spectroscopy. Thin layer chromatography immunostaining revealed that FucT-IV preferred the distal GlcNAc residue in nLc6Cer, whereas Fuc-TV preferred the proximal Gl-cNAc residue. Incubation of Fuc-TIV or Fuc-TV with VI3NeuAcnLc6Cer resulted in products with the sialyl-LewisX epitope as well as the VIM-2 structure. To identify polar groups on acceptors that function in enzyme binding, deoxygenated substrate analogs were tested as acceptors. All three Fuc-Ts had an absolute requirement for a hydroxyl at C-6 of galactose in addition to the accepting hydroxyl at C-3 or C-4 of GlcNAc.

摘要

分析了在COS - 7细胞中表达的重组全长膜结合岩藻糖基转移酶以及α1,3 - 岩藻糖基转移酶(Fuc - T)III、Fuc - TIV和Fuc - TV的可溶性蛋白A嵌合形式对多种寡糖、糖脂和糖蛋白底物的受体特异性。我们对全长酶的研究结果证实并扩展了先前的研究。然而,与全长酶相比,嵌合Fuc - T对糖蛋白的活性增加,而嵌合Fuc - TIII和Fuc - TV对糖鞘脂的活性降低。出乎意料的是,嵌合Fuc - TV表现出GDP - 岩藻糖水解活性。在具有多个受体位点的底物中,确定了岩藻糖基化的优先位点。1H NMR光谱表明,Fuc - TIII和Fuc - TV分别仅将岩藻糖转移至乳糖 - N - 新四糖和乳糖 - N - 四糖中葡萄糖的OH - 3位。薄层色谱免疫染色显示,FucT - IV优先作用于nLc6Cer中远端的GlcNAc残基,而Fuc - TV优先作用于近端的Gl - cNAc残基。Fuc - TIV或Fuc - TV与VI3NeuAcnLc6Cer孵育产生具有唾液酸化路易斯X表位以及VIM - 2结构的产物。为了鉴定在酶结合中起作用的受体上的极性基团,测试了脱氧底物类似物作为受体。除了GlcNAc的C - 3或C - 4位的接受羟基外,所有三种Fuc - T对半乳糖C - 6位的羟基都有绝对需求。

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