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质膜的亲和纯化

Affinity purification of plasma membranes.

作者信息

deBlaquiere J, Burgess A W

机构信息

Ludwig Institute for Cancer Research, Melbourne Tumour Biology Branch, Melbourne, Australia.

出版信息

J Biomol Tech. 1999 Jun;10(2):64-71.

Abstract

The interaction of biotin and avidin was used to affinity purify plasma membranes for use in in vitro studies of the epidermal growth factor (EGF) receptor and other cell-surface molecules. Biotinylated mouse fibroblasts were homogenized and plasma membranes purified using immobilized monomeric avidin. Capturing the membranes on the solid-phase support facilitated buffer exchange, protein analysis, and assay of receptor function. Electron microscopy and enzyme analysis showed that the plasma membranes obtained were of significantly improved purity when compared with crude membrane preparations. In particular, contamination with other cellular membranes, such as endoplasmic reticulum, mitochondria, lysosomes, and Golgi, is reduced considerably in the purified biotinylated membrane preparations. By titrating the level of biotinylation of whole cells, we identified a level of biotinylation that produces a high yield of pure cell-surface membranes but does not interfere with ligand activation of the EGF receptor protein (as determined by in vitro autophosphorylation assays).This method produces highly purified fibroblast plasma membranes quickly and with reasonable yield using standard laboratory equipment and should be easily adapted to suit experiments involving the activation of other cell surface molecules, signal transduction pathways initiated from the cell surface, and proteome analysis of plasma membranes from a wide variety of cells.

摘要

利用生物素与抗生物素蛋白的相互作用对质膜进行亲和纯化,以用于表皮生长因子(EGF)受体及其他细胞表面分子的体外研究。将生物素化的小鼠成纤维细胞匀浆,并用固定化的单体抗生物素蛋白纯化质膜。在固相载体上捕获膜有助于缓冲液交换、蛋白质分析及受体功能检测。电子显微镜和酶分析表明,与粗制膜制剂相比,所获得的质膜纯度显著提高。特别是,在纯化的生物素化膜制剂中,内质网、线粒体、溶酶体和高尔基体等其他细胞膜的污染大幅减少。通过滴定全细胞的生物素化水平,我们确定了一个生物素化水平,该水平能产生高产量的纯细胞表面膜,但不会干扰EGF受体蛋白的配体激活(通过体外自磷酸化测定确定)。该方法使用标准实验室设备能快速产生高度纯化的成纤维细胞质膜,且产量合理,应易于适用于涉及其他细胞表面分子激活、从细胞表面起始的信号转导途径以及多种细胞质膜蛋白质组分析的实验。

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