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稳定和瞬时蛋白质-蛋白质相互作用的分析。

Analysis of stable and transient protein-protein interactions.

作者信息

Byrum Stephanie, Smart Sherri K, Larson Signe, Tackett Alan J

机构信息

Department of Biochemistry and Molecular Biology, University of Arkansas for Medical Sciences, Little Rock, AR, USA.

出版信息

Methods Mol Biol. 2012;833:143-52. doi: 10.1007/978-1-61779-477-3_10.

Abstract

The assembly of proteins into defined complexes drives a plethora of cellular activities. These protein complexes often have a set of more stably interacting proteins as well as more unstable or transient interactions. Studying the in vivo components of these protein complexes is challenging as many of the techniques used for isolation result in the purification of only the most stable components and the transient interactions are lost. A technology called transient isotopic differentiation of interactions as random or targeted (transient I-DIRT) has been developed to identify these transiently interacting proteins as well as the stable interactions. Described here are the detailed methodological approaches used for a transient I-DIRT analysis of a multi-subunit complex, NuA3, that acetylates histone H3 and functions to activate gene transcription. Transcription is known to involve a concert of protein assemblies performing different activities on the chromatin/gene template, thus understanding the less stable or transient protein interactions with NuA3 will shed light onto the protein complexes that function synergistically, or antagonistically, to regulate gene transcription and chromatin remodeling.

摘要

蛋白质组装成特定的复合物驱动着大量的细胞活动。这些蛋白质复合物通常有一组相互作用更稳定的蛋白质,以及一些更不稳定或短暂的相互作用。研究这些蛋白质复合物的体内成分具有挑战性,因为许多用于分离的技术只能纯化出最稳定的成分,而短暂的相互作用则会丢失。一种名为随机或靶向相互作用的瞬时同位素分化技术(transient I-DIRT)已被开发出来,用于识别这些瞬时相互作用的蛋白质以及稳定的相互作用。本文描述了用于对多亚基复合物NuA3进行瞬时I-DIRT分析的详细方法,NuA3可使组蛋白H3乙酰化并激活基因转录。已知转录涉及在染色质/基因模板上执行不同活动的蛋白质组装协同作用,因此了解与NuA3不太稳定或短暂的蛋白质相互作用将有助于揭示协同或拮抗作用以调节基因转录和染色质重塑的蛋白质复合物。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ee02/3314026/8249d78ac7a6/nihms-364368-f0001.jpg

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