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对从卵巢癌患者腹水中纯化的半乳糖基转移酶合成的产物的表征。

Characterization of products synthesized by galactosyltransferase purified from the ascites of ovarian cancer patients.

作者信息

Chatterjee S K, Bhattacharya M, Barlow J J

出版信息

J Natl Cancer Inst. 1986 Oct;77(4):855-62.

PMID:2429004
Abstract

Galactosyltransferase purified from the ascites of ovarian cancer patients can use to an equal extent N-glycosidic glycoproteins, such as asialoagalactofetuin, and O-glycosidic mucin, such as asialo bovine submaxillary mucin (BSM), as acceptors. Thermal treatment and substrate competition experiments demonstrated that the same enzyme catalyzed the transfer of galactose to both types of acceptors. Alkaline borohydride treatment showed that, while the product with asialoagalactofetuin was totally resistant, about 90% of the product with asialo BSM was hydrolyzed by this treatment. Gel filtration of the released oligosaccharides on a calibrated Biogel P-2 column showed three peaks. One major oligosaccharide (O-2) of size 5.7 glucose U and two minor peaks (O-1 and O-3) of sizes 8.7 and 3.7 glucose U, respectively, were obtained. The oligosaccharides were doubly labeled, first by incubation with uridine-diphosphate [14C]galactose, followed by alkali treatment in the presence of [3H]borohydride. The doubly labeled oligosaccharides were separately purified by gel filtration and ion-exchange chromatography and digested with various exoglycosidases. The digested products were characterized by gel filtration and paper chromatography in three different systems. From these results, the structures of these oligosaccharides were computed as follows: O-1 = beta-galactosyl-beta-N-acetylglucosamine-galactosaminitol (sialic acid); O-2 = beta-galactose-beta-N-acetylglucosamine-galactosaminitol; O-3 = beta-galactose-galactosaminitol. These results suggest that the galactosyltransferase from the ascites of ovarian cancer patients catalyzes the transfer of galactose to N-acetylglucosamine, irrespective of whether it is a part of an N-glycan or an O-glycan.

摘要

从卵巢癌患者腹水中纯化得到的半乳糖基转移酶,对N-糖苷键连接的糖蛋白(如去唾液酸半乳糖胎球蛋白)和O-糖苷键连接的粘蛋白(如去唾液酸牛下颌粘蛋白(BSM))作为受体的利用程度相同。热处理和底物竞争实验表明,同一酶催化半乳糖向这两种类型受体的转移。碱性硼氢化物处理表明,虽然去唾液酸半乳糖胎球蛋白的产物完全抗水解,但去唾液酸BSM的产物约90%会被该处理水解。在经校准的Biogel P-2柱上对释放的寡糖进行凝胶过滤,显示出三个峰。分别得到了一个大小为5.7个葡萄糖单位的主要寡糖(O-2)和两个大小分别为8.7和3.7个葡萄糖单位的次要峰(O-1和O-3)。这些寡糖经过双重标记,首先与尿苷二磷酸[14C]半乳糖一起孵育,然后在[3H]硼氢化物存在下进行碱处理。通过凝胶过滤和离子交换色谱分别纯化双重标记的寡糖,并用各种外切糖苷酶进行消化。消化产物通过在三种不同系统中的凝胶过滤和纸色谱进行表征。根据这些结果,这些寡糖的结构计算如下:O-1 = β-半乳糖基-β-N-乙酰葡糖胺-半乳糖胺醇(唾液酸);O-2 = β-半乳糖-β-N-乙酰葡糖胺-半乳糖胺醇;O-3 = β-半乳糖-半乳糖胺醇。这些结果表明,来自卵巢癌患者腹水中的半乳糖基转移酶催化半乳糖向N-乙酰葡糖胺的转移,无论它是N-聚糖还是O-聚糖的一部分。

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J Natl Cancer Inst. 1986 Oct;77(4):855-62.
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