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内质网相关蛋白质量控制与降解:内质网相关降解成分的全基因组筛选

Endoplasmic reticulum-associated protein quality control and degradation: genome-wide screen for ERAD components.

作者信息

Schäfer Antje, Wolf Dieter H

机构信息

Institut für Biochemie, Universität Stuttgart, Germany.

出版信息

Methods Mol Biol. 2005;301:289-92. doi: 10.1385/1-59259-895-1:289.

Abstract

In this chapter, a genetic approach is presented that leads to the isolation of mutants and to the identification of proteins involved in protein quality control and endoplasmic reticulum-associated degradation (ERAD). The method makes use of a genomic screen of a yeast deletion library (EUROSCARF). Transformation of each of the approx 5000 strains deleted in one nonvital gene each with a CPY* chimera containing CPY* C-terminally fused to a transmembrane domain and the cytosolic Leu2 protein (3-isopropylmalate dehydrogenase) constitutes the basic screening procedure. Because of a Leu2p deficiency in all deletion strains, cells can grow only when the CTL* chimera is present. As the CPY* module of CTL* will be recognized in ERAD-proficient cells, CTL* will be degraded and the strain is unable to grow. Therefore the absence of genes necessary for ER quality control and ERAD will allow cell growth and indicate the necessity of the respective gene for these processes.

摘要

在本章中,我们介绍了一种遗传学方法,该方法可用于分离突变体,并鉴定参与蛋白质质量控制和内质网相关降解(ERAD)的蛋白质。该方法利用酵母缺失文库(EUROSCARF)进行基因组筛选。将每个约5000个在一个非必需基因上缺失的菌株,分别用一种CPY嵌合体进行转化,该嵌合体的CPY在C末端与一个跨膜结构域和胞质Leu2蛋白(3-异丙基苹果酸脱氢酶)融合,这构成了基本的筛选程序。由于所有缺失菌株中都存在Leu2p缺陷,只有当CTL嵌合体存在时细胞才能生长。由于在ERAD功能正常的细胞中,CTL的CPY模块会被识别,CTL会被降解,菌株无法生长。因此,内质网质量控制和ERAD所需基因的缺失将允许细胞生长,并表明这些过程中相应基因的必要性。

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