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用于空间和时间控制蛋白质功能化的多价螯合剂。

Multivalent chelators for spatially and temporally controlled protein functionalization.

作者信息

You Changjiang, Piehler Jacob

机构信息

Department of Biology, University of Osnabrück, Barbarastr. 11, 49076, Osnabrück, Germany.

出版信息

Anal Bioanal Chem. 2014 May;406(14):3345-57. doi: 10.1007/s00216-014-7803-y. Epub 2014 Apr 26.

Abstract

Site-specific protein modification-e.g. for immobilization or labelling-is a key prerequisite for numerous bioanalytical applications. Although modification by use of short peptide tags is particularly attractive, efficient and bio-orthogonal systems are still lacking. Here, we review the application of multivalent chelators (MCH) for high-affinity yet reversible recognition of oligohistidine (His)-tagged proteins. MCH are based on multiple nitrilotriacetic acid (NTA) moieties grafted on to molecular scaffolds suitable for conjugation to surfaces, probes or other biomolecules. Reversible interaction with the His-tag is mediated via transition metal ions chelated by the NTA moieties. The small size and biochemical compatibility of these recognition units and the possibility of rapid dissociation of the interaction with His-tagged proteins despite sub-nanomolar binding affinity, enable distinct and versatile handling and modification of recombinant proteins. In this review, we briefly introduce the key principles and features of MCH-His-tag interactions and recapitulate the broad spectrum of bioanalytical applications with a focus on quantitative protein interaction analysis on micro or nano-patterned solid surfaces and specific protein labelling in living cells.

摘要

位点特异性蛋白质修饰(例如用于固定或标记)是众多生物分析应用的关键前提条件。尽管使用短肽标签进行修饰特别有吸引力,但仍缺乏高效且生物正交的系统。在此,我们综述了多价螯合剂(MCH)在高亲和力且可逆识别寡聚组氨酸(His)标签蛋白方面的应用。MCH基于多个接枝到适合与表面、探针或其他生物分子缀合的分子支架上的次氮基三乙酸(NTA)部分。与His标签的可逆相互作用是通过由NTA部分螯合的过渡金属离子介导的。这些识别单元的小尺寸和生化兼容性,以及尽管结合亲和力低于纳摩尔但与His标签蛋白的相互作用仍可能快速解离的特性,使得能够对重组蛋白进行独特且通用的处理和修饰。在本综述中,我们简要介绍了MCH-His标签相互作用的关键原理和特征,并概述了广泛的生物分析应用,重点是在微图案或纳米图案固体表面上的定量蛋白质相互作用分析以及活细胞中的特异性蛋白质标记。

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