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基于无标记蛋白质组学的下一代蛋白酶底物捕获技术

Next-Generation Trapping of Protease Substrates by Label-Free Proteomics.

作者信息

Lindemann Claudia, Thomanek Nikolas, Kuhlmann Katja, Meyer Helmut E, Marcus Katrin, Narberhaus Franz

机构信息

Medizinisches Proteom-Center, Ruhr-Universität Bochum, Bochum, Germany.

Lehrstuhl für Biologie der Mikroorganismen, Ruhr-Universität Bochum, Bochum, Germany.

出版信息

Methods Mol Biol. 2018;1841:189-206. doi: 10.1007/978-1-4939-8695-8_14.

Abstract

AAA proteases (ATPases associated with various cellular activities) shape the cellular protein pool in response to environmental conditions. A prerequisite for understanding the underlying recognition and degradation principles is the identification of as many protease substrates as possible. Most previous studies made use of inactive protease variants to trap substrates, which were identified by 2D-gel based proteomics. Since this method is known for limitations in the identification of low-abundant proteins or proteins with many transmembrane domains, we established a trapping approach that overcomes these limitations. We used a proteolytically inactive FtsH variant (FtsH) of Escherichia coli (E. coli) that is still able to bind and translocate substrates into the proteolytic chamber but no longer able to degrade proteins. Proteins associated with FtsH or FtsH (proteolytically active FtsH) were purified, concentrated by an 1D-short gel, and identified by LC-coupled mass spectrometry (LC-MS) followed by label-free quantification. The identification of four known FtsH substrates validated this approach and suggests that it is generally applicable to AAA proteases.

摘要

AAA蛋白酶(与多种细胞活动相关的ATP酶)可根据环境条件塑造细胞蛋白质库。理解其潜在识别和降解原理的一个前提是尽可能多地鉴定蛋白酶底物。以前的大多数研究利用无活性蛋白酶变体来捕获底物,这些底物通过基于二维凝胶的蛋白质组学进行鉴定。由于该方法在鉴定低丰度蛋白质或具有多个跨膜结构域的蛋白质方面存在局限性,我们建立了一种克服这些局限性的捕获方法。我们使用了大肠杆菌(E. coli)的一种蛋白水解无活性的FtsH变体(FtsH),它仍然能够结合底物并将其转运到蛋白水解腔室中,但不再能够降解蛋白质。与FtsH或FtsH(蛋白水解活性FtsH)相关的蛋白质被纯化,通过一维短凝胶浓缩,并通过液相色谱-质谱联用(LC-MS)进行鉴定,随后进行无标记定量。四种已知FtsH底物的鉴定验证了该方法,并表明它通常适用于AAA蛋白酶。

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