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一种膜糖蛋白Sec12p,是酵母中蛋白质从内质网运输到高尔基体所必需的。

A membrane glycoprotein, Sec12p, required for protein transport from the endoplasmic reticulum to the Golgi apparatus in yeast.

作者信息

Nakano A, Brada D, Schekman R

机构信息

Department of Biochemistry, University of California, Berkeley 94720.

出版信息

J Cell Biol. 1988 Sep;107(3):851-63. doi: 10.1083/jcb.107.3.851.

Abstract

SEC12, a gene that is required for secretory, membrane, and vacuolar proteins to be transported from the endoplasmic reticulum to the Golgi apparatus, has been cloned from a genomic library by complementation of a sec12 ts mutation. Genetic analysis has shown that the cloned gene integrates at the SEC12 locus and that a null mutation at the locus is lethal. The DNA sequence predicts a protein of 471 amino acids containing a hydrophobic stretch of 19 amino acids near the COOH terminus. To characterize the gene product (Sec12p) in detail, a lacZ-SEC12 gene fusion has been constructed and a polyclonal antibody raised against the hybrid protein. The antibody recognizes Sec12p as a approximately 70-kD protein that sediments in a mixed membrane fraction that includes endoplasmic reticulum. Sec12p is not removed from the membrane fraction by treatment at high pH and high salt and is not degraded by exogenous protease unless detergent is present. Glycosylation of Sec12p during biogenesis is indicated by an electrophoretic mobility shift of the protein that is influenced by tunicamycin and by imposition of an independent secretory pathway block. We suggest that Sec12p is an integral membrane glycoprotein with a prominent domain that faces the cytoplasm where it functions to promote protein transport to the Golgi apparatus. In the process of transport, Sec12p itself may migrate to the Golgi apparatus and function in subsequent transport events.

摘要

SEC12是一个基因,分泌蛋白、膜蛋白和液泡蛋白从内质网运输到高尔基体需要该基因。通过对sec12温度敏感突变进行互补,已从基因组文库中克隆出该基因。遗传分析表明,克隆的基因整合在SEC12位点,该位点的无效突变是致死的。DNA序列预测该蛋白有471个氨基酸,在COOH末端附近有一段19个氨基酸的疏水序列。为了详细表征该基因产物(Sec12p),构建了一个lacZ-SEC12基因融合体,并制备了针对该杂交蛋白的多克隆抗体。该抗体识别Sec12p为一种约70-kD的蛋白,它沉淀在包括内质网的混合膜组分中。Sec12p在高pH和高盐条件下处理后不会从膜组分中去除,除非存在去污剂,否则不会被外源蛋白酶降解。衣霉素和独立分泌途径阻断对蛋白质电泳迁移率的影响表明,Sec12p在生物合成过程中发生了糖基化。我们认为,Sec12p是一种整合膜糖蛋白,具有一个突出的面向细胞质的结构域,其功能是促进蛋白质向高尔基体的运输。在运输过程中,Sec12p本身可能迁移到高尔基体,并在随后的运输事件中发挥作用。

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