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参与糖基磷脂酰肌醇锚定连接的内质网蛋白:无细胞体系中的光交联研究

Endoplasmic reticulum proteins involved in glycosylphosphatidylinositol-anchor attachment: photocrosslinking studies in a cell-free system.

作者信息

Vidugiriene J, Vainauskas S, Johnson A E, Menon A K

机构信息

Department of Biochemistry, University of Wisconsin, Madison, WI 53706, USA.

出版信息

Eur J Biochem. 2001 Apr;268(8):2290-300. doi: 10.1046/j.1432-1327.2001.02106.x.

DOI:10.1046/j.1432-1327.2001.02106.x
PMID:11298746
Abstract

Assembly of glycosylphosphatidylinositol (GPtdIns)-anchored proteins requires translocation of the nascent polypeptide chain across the endoplasmic reticulum (ER) membrane and replacement of the C-terminal signal sequence with a GPtdIns moiety. The anchoring reaction is carried out by an ER enzyme, GPtdIns transamidase. Genetic studies with yeast indicate that the transamidase consists of a dynamic complex of at least two subunits, Gaa1p and Gpi8p. To study the GPtdIns-anchoring reaction, we used a small reporter protein that becomes GPtdIns-anchored when the corresponding mRNA is translated in the presence of microsomes, in conjunction with site-specific photocrosslinking to identify ER membrane components that are proximal to the reporter during its conversion to a GPtdIns-anchored protein. We generated variants of the reporter protein such that upon in vitro translation in the presence of Nepsilon-(5-azido-2-nitrobenzoyl)-lysyl-tRNA, photoreactive lysine residues would be incorporated in the protein specifically near the GPtdIns-attachment site. We analyzed photoadducts resulting from UV irradiation of the samples. We show that proproteins can be crosslinked to the transamidase subunit Gpi8p, as well as to ER proteins of molecular mass approximately 60 kDa, approximately 70 kDa, and approximately 120 kDa. The identification of a photoadduct between a proprotein and Gpi8p provides the first direct evidence of an interaction between a proprotein substrate and one of the genetically identified transamidase subunits. The approximately 70-kDa protein that we identified may correspond to the other subunit Gaa1p, while the other proteins possibly represent additional, hitherto unidentified subunits of the mammalian GPtdIns transamidase complex.

摘要

糖基磷脂酰肌醇(GPtdIns)锚定蛋白的组装需要新生多肽链跨内质网(ER)膜转运,并将C端信号序列替换为GPtdIns部分。锚定反应由ER酶GPtdIns转酰胺酶进行。酵母的遗传学研究表明,转酰胺酶由至少两个亚基Gaa1p和Gpi8p组成的动态复合物构成。为了研究GPtdIns锚定反应,我们使用了一种小的报告蛋白,当相应的mRNA在微粒体存在下翻译时,该报告蛋白会被GPtdIns锚定,并结合位点特异性光交联来鉴定在报告蛋白转化为GPtdIns锚定蛋白过程中靠近报告蛋白的ER膜成分。我们生成了报告蛋白的变体,使得在Nε-(5-叠氮基-2-硝基苯甲酰基)-赖氨酰-tRNA存在下进行体外翻译时,光反应性赖氨酸残基将特异性地掺入靠近GPtdIns附着位点的蛋白中。我们分析了样品紫外线照射产生的光加合物。我们发现前体蛋白可以与转酰胺酶亚基Gpi8p以及分子量约为60 kDa、约70 kDa和约120 kDa的ER蛋白交联。前体蛋白与Gpi8p之间光加合物的鉴定提供了前体蛋白底物与遗传鉴定的转酰胺酶亚基之一之间相互作用的首个直接证据。我们鉴定出的约70 kDa蛋白可能对应于另一个亚基Gaa1p,而其他蛋白可能代表哺乳动物GPtdIns转酰胺酶复合物中迄今未鉴定的其他亚基。

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Efficient glycosylphosphatidylinositol (GPI) modification of membrane proteins requires a C-terminal anchoring signal of marginal hydrophobicity.
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