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VIP36的糖结合特性,一种作为货物受体发挥作用的细胞内动物凝集素。

Sugar-binding properties of VIP36, an intracellular animal lectin operating as a cargo receptor.

作者信息

Kamiya Yukiko, Yamaguchi Yoshiki, Takahashi Noriko, Arata Yoichiro, Kasai Ken-Ichi, Ihara Yoshito, Matsuo Ichiro, Ito Yukishige, Yamamoto Kazuo, Kato Koichi

机构信息

Graduate School of Pharmaceutical Sciences, Nagoya City University, 3-1 Tanabe-dori, Mizuho-ku, Nagoya 467-8603, Japan.

出版信息

J Biol Chem. 2005 Nov 4;280(44):37178-82. doi: 10.1074/jbc.M505757200. Epub 2005 Aug 29.

DOI:10.1074/jbc.M505757200
PMID:16129679
Abstract

The vesicular integral protein of 36 kDa (VIP36) is an intracellular animal lectin that acts as a putative cargo receptor, which recycles between the Golgi and the endoplasmic reticulum. Although it is known that VIP36 interacts with glycoproteins carrying high mannose-type oligosaccharides, detailed analyses of the sugar-binding specificity that discriminates isomeric oligosaccharide structures have not yet been performed. In the present study, we have analyzed, using the frontal affinity chromatography (FAC) method, the sugar-binding properties of a recombinant carbohydrate recognition domain of VIP36 (VIP36-CRD). For this purpose, a pyridylaminated sugar library, consisting of 21 kinds of oligosaccharides, including isomeric structures, was prepared and subjected to FAC analyses. The FAC data have shown that glucosylation and trimming of the D1 mannosyl branch interfere with the binding of VIP36-CRD. VIP36-CRD exhibits a bell-shaped pH dependence of sugar binding with an optimal pH value of approximately 6.5. By inspection of the specificity and optimal pH value of the sugar binding of VIP36 and its subcellular localization, together with the organellar pH, we suggest that VIP36 binds glycoproteins that retain the intact D1 mannosyl branch in the cis-Golgi network and recycles to the endoplasmic reticulum where, due to higher pH, it releases its cargos, thereby contributing to the quality control of glycoproteins.

摘要

36kDa囊泡整合蛋白(VIP36)是一种细胞内动物凝集素,作为一种假定的货物受体,在高尔基体和内质网之间循环。尽管已知VIP36与携带高甘露糖型寡糖的糖蛋白相互作用,但尚未对区分异构寡糖结构的糖结合特异性进行详细分析。在本研究中,我们使用前沿亲和色谱(FAC)方法分析了VIP36重组碳水化合物识别结构域(VIP36-CRD)的糖结合特性。为此,制备了一个由21种寡糖组成的包括异构结构的吡啶氨基化糖库,并进行FAC分析。FAC数据表明,D1甘露糖基分支的糖基化和修剪会干扰VIP36-CRD的结合。VIP36-CRD表现出糖结合的钟形pH依赖性,最佳pH值约为6.5。通过检查VIP36糖结合的特异性和最佳pH值及其亚细胞定位,结合细胞器pH值,我们认为VIP36结合在顺式高尔基体网络中保留完整D1甘露糖基分支的糖蛋白,并循环回到内质网,在那里由于pH值较高,它会释放其货物,从而有助于糖蛋白的质量控制。

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