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由弗氏脾脏病灶形成病毒的红细胞增多症诱导株编码的糖蛋白52的碳水化合物结构。

Carbohydrate structure of glycoprotein 52 encoded by the polycythemia-inducing strain of Friend spleen focus-forming virus.

作者信息

Strube K H, Schott H H, Geyer R

机构信息

Biochemisches Institut der Justus-Liebig-Universität Giessen, Federal Republic of Germany.

出版信息

J Biol Chem. 1988 Mar 15;263(8):3762-71.

PMID:2831202
Abstract

The primary envelope (env) gene product of the polycythemia-inducing variant of Friend spleen focus-forming virus (F-SFFVP), representing a glycoprotein with an apparent Mr of 52,000 (gp52), was isolated from F-SFFVP-infected normal rat kidney cells metabolically labeled with [2-3H]mannose in the presence or absence of glucose. Structures of the oligosaccharides present were determined by micromethylation analysis, acetolysis, and digestion with exoglycosidases. Gp52 radiolabeled in the presence of glucose contains solely oligomannosidic glycans comprising 6 to 9 mannose residues (Man6-9GlcNAc2), some of which carry additional glucose. The structures of the glycans found reflect the typical intermediates of oligosaccharide processing. The glycosylation of gp52 isolated from glucose-deprived cells (-Glc), however, is characterized by increased amounts of Man5-7 species comprising other structural isomers. Only gp52 (-Glc) glycans are, in part, further processed yielding incomplete complex-type oligosaccharides. Our results demonstrate that the limited post-translational processing of the primary F-SFFVP env gene product is neither due to aberrant trimming of its oligomannosidic glycans nor due to transfer of immature lipid-linked oligosaccharide-intermediates as observed in glucose-starved cells.

摘要

从多血症诱导型弗氏脾脏灶形成病毒(F-SFFVP)的主要包膜(env)基因产物中分离出一种糖蛋白,其表观分子量为52,000(gp52)。该病毒感染正常大鼠肾细胞,在有或没有葡萄糖存在的情况下用[2-³H]甘露糖进行代谢标记。通过微甲基化分析、乙酰解和外切糖苷酶消化来确定所存在的寡糖结构。在有葡萄糖存在的情况下进行放射性标记的gp52仅含有由6至9个甘露糖残基组成的寡甘露糖聚糖(Man6-9GlcNAc2),其中一些还带有额外的葡萄糖。所发现的聚糖结构反映了寡糖加工的典型中间体。然而,从缺乏葡萄糖的细胞(-Glc)中分离出的gp52的糖基化特征是含有其他结构异构体的Man5-7种类的量增加。只有gp52(-Glc)聚糖部分会进一步加工产生不完全的复合型寡糖。我们的结果表明,F-SFFVP主要env基因产物有限的翻译后加工既不是由于其寡甘露糖聚糖的异常修剪,也不是由于在葡萄糖饥饿细胞中观察到的未成熟脂质连接寡糖中间体的转移。

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