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串联亲和纯化常用标签组合。

Commonly used tag combinations for tandem affinity purification.

机构信息

Department of Anesthesiology, David Geffen School of Medicine, 650 Charles E. Young Drive, University of California, Los Angeles, Los Angeles, CA 90095, USA.

出版信息

Biotechnol Appl Biochem. 2010 Feb 15;55(2):73-83. doi: 10.1042/BA20090273.

Abstract

TAP (tandem affinity purification) allows rapid and clean isolation of a tagged protein along with its interacting partners from cell lysates. Initially developed in yeast, the TAP method has subsequently been adapted to other cells and organisms. In combination with MS analysis, this method has become an indispensable tool for systematic identification of target-associated protein complexes. The key feature of TAP is the use of a dual-affinity tag, which is fused to the protein of interest. The original TAP tag consisted of two IgG-binding units of Protein A of Staphylococcus aureus and the calmodulin-binding peptide. As the technique has been widely exploited, a number of alternative TAP tags based on other affinity handles have been developed. The present review gives an overview of the various tag combinations for TAP with a highlight on those alternatives that result in improved yields or unique features. The information provided should assist in the selection and development of TAP tags for specific applications.

摘要

TAP(串联亲和纯化)允许从细胞裂解物中快速、干净地分离标记蛋白及其相互作用的伙伴。该方法最初在酵母中开发,随后已被改编用于其他细胞和生物。与 MS 分析相结合,该方法已成为系统鉴定靶标相关蛋白复合物的不可或缺的工具。TAP 的关键特征是使用双亲和标签,该标签融合到感兴趣的蛋白质上。原始的 TAP 标签由金黄色葡萄球菌的两个 IgG 结合单位的蛋白 A 和钙调蛋白结合肽组成。随着该技术的广泛开发,已经开发了许多基于其他亲和处理的替代 TAP 标签。本综述概述了 TAP 的各种标签组合,并重点介绍了那些可提高产量或具有独特特性的替代标签。提供的信息应有助于选择和开发特定应用的 TAP 标签。

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