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黑曲霉细胞膜的甘露糖基转移作用:内源性受体的甘露糖基化及产物的部分分析

Mannosyl transfer by membranes of Aspergillus niger: mannosylation of endogenous acceptors and partial analysis of the products.

作者信息

Rudick M J

出版信息

J Bacteriol. 1979 Jan;137(1):301-8. doi: 10.1128/jb.137.1.301-308.1979.

Abstract

A smooth membrane fraction of Aspergillus niger catalyzed the transfer of mannose from GDP-mannose to endogenous lipid and protein acceptors. The mannolipid was acidic, as judged by diethylaminoethyl-cellulose chromatography, and had a mobility similar to ficaprenyl phosphate on thin-layer chromatograms. Mannose transfer occurred optimally at pH 6.5 to 7.5 and required Mn(2+) for use of the protein as acceptor, but either Mn(2+) or Mg(2+) with the lipid as acceptor. Glycopeptides of the mannosylated protein ([(14)C]gly) and of an alpha-glucosidase (alpha-glu) secreted by the organism were produced by Pronase digestion and separation of the products on Sephadex G-25. Because ovalbumin has a carbohydrate composition similar to that of alpha-glu and because the carbohydrate structure of ovalbumin is known, ovalbumin glycopeptides (Ov) were similarly obtained and used as standards in determining carbohydrate structures. Oligosaccharide chains of [(14)C]gly, alpha-glu, and Ov were obtained by treatment of the respective glycopeptides with endo-beta-N-acetylglucosaminidase, reduction with NaBT(4), and concanavalin A-Sepharose chromatography. The (3)H-labeled oligosaccharides obtained were subjected to the following treatments: (i) digestion with alpha- and beta-mannosidases, (ii) Smith degradation, and (iii) acetolysis. Subsequently, changes in paper chromatographic mobilities were detected. Also, alpha-glu was permethylated, and the partially methylated alditol acetates were analyzed by gas-liquid chromatography. The resultant proposed structure shows that the oligosaccharide chain of alpha-glu is almost identical to that of an Ov chain, while [(14)C]gly has a structure which is probably the same as that of alpha-glu. It is suggested that the transferase(s) involved in [(14)C]gly synthesis in vitro may be responsible for glycosylation of secreted enzymes.

摘要

黑曲霉的一种光滑膜组分催化了甘露糖从GDP-甘露糖向内源脂质和蛋白质受体的转移。通过二乙氨基乙基纤维素色谱法判断,甘露糖脂呈酸性,在薄层色谱图上其迁移率与磷酸法卡普烯基酯相似。甘露糖转移在pH 6.5至7.5时最佳,以蛋白质作为受体时需要Mn(2+),但以脂质作为受体时Mn(2+)或Mg(2+)均可。经链霉蛋白酶消化并在葡聚糖G-25上分离产物,得到了该生物体分泌的甘露糖基化蛋白([(14)C]gly)和α-葡萄糖苷酶(α-glu)的糖肽。由于卵清蛋白的碳水化合物组成与α-glu相似,且卵清蛋白的碳水化合物结构已知,因此以类似方式获得了卵清蛋白糖肽(Ov),并将其用作确定碳水化合物结构的标准。通过用内切β-N-乙酰氨基葡萄糖苷酶处理相应的糖肽、用NaBT(4)还原以及伴刀豆球蛋白A-琼脂糖色谱法,得到了[(14)C]gly、α-glu和Ov的寡糖链。对得到的(3)H标记寡糖进行以下处理:(i)用α-和β-甘露糖苷酶消化,(ii)史密斯降解,(iii)乙酰解。随后,检测纸色谱迁移率的变化。此外,对α-glu进行全甲基化,并通过气相色谱分析部分甲基化的糖醇乙酸酯。所得的推测结构表明,α-glu的寡糖链与Ov链几乎相同,而[(14)C]gly的结构可能与α-glu相同。有人提出,体外参与[(14)C]gly合成的转移酶可能负责分泌酶的糖基化。

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