Perspective on the potential of tandem-ion mobility /mass spectrometry methods for structural proteomics applications.

Tyler C Cropley, Mengqi Chai, Fanny C Liu, Christian Bleiholder
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Abstract

Cellular processes are usually carried out collectively by the entirety of all proteins present in a biological cell, i.e. the proteome. Mass spectrometry-based methods have proven particularly successful in identifying and quantifying the constituent proteins of proteomes, including different molecular forms of a protein. Nevertheless, protein sequences alone do not reveal the function or dysfunction of the identified proteins. A straightforward way to assign function or dysfunction to proteins is characterization of their structures and dynamics. However, a method capable to characterize detailed structures of proteins and protein complexes in a large-scale, systematic manner within the context of cellular processes does not yet exist. Here, we discuss the potential of tandem-ion mobility / mass spectrometry (tandem-IM/MS) methods to provide such ability. We highlight the capability of these methods using two case studies on the protein systems ubiquitin and avidin using the tandem-TIMS/MS technology developed in our laboratory and discuss these results in the context of other developments in the broader field of tandem-IM/MS.

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串联离子迁移/质谱法在结构蛋白质组学应用中的潜力展望。
细胞过程通常是由生物细胞中存在的所有蛋白质集体进行的,即蛋白质组。基于质谱的方法已被证明在鉴定和定量蛋白质组的组成蛋白(包括蛋白质的不同分子形式)方面特别成功。然而,蛋白质序列本身并不能揭示所鉴定蛋白质的功能或功能障碍。一种直接的方法来分配功能或功能障碍的蛋白质是表征其结构和动力学。然而,在细胞过程的背景下,能够以大规模、系统的方式表征蛋白质和蛋白质复合物的详细结构的方法尚不存在。在这里,我们讨论了串联离子迁移率/质谱(串联im /MS)方法提供这种能力的潜力。我们利用实验室开发的串联tims /MS技术对蛋白质系统泛素和亲和素进行了两个案例研究,强调了这些方法的能力,并在串联im /MS更广泛领域的其他发展背景下讨论了这些结果。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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