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酪胺信号放大质谱(TSA-MS)比值鉴定核斑点蛋白。

Tyramide signal amplification mass spectrometry (TSA-MS) ratio identifies nuclear speckle proteins.

机构信息

Department of Cell and Developmental Biology, University of Illinois at Urbana-Champaign, Urbana, IL.

Proteome Exploration Laboratory, Department of Biology and Biological Engineering, Beckman Institute, California Institute of Technology, Pasadena, CA.

出版信息

J Cell Biol. 2020 Sep 7;219(9). doi: 10.1083/jcb.201910207.

Abstract

We present a simple ratio method to infer protein composition within cellular structures using proximity labeling approaches but compensating for the diffusion of free radicals. We used tyramide signal amplification (TSA) and label-free mass spectrometry (MS) to compare proteins in nuclear speckles versus centromeres. Our "TSA-MS ratio" approach successfully identified known nuclear speckle proteins. For example, 96% and 67% of proteins in the top 30 and 100 sorted proteins, respectively, are known nuclear speckle proteins, including proteins that we validated here as enriched in nuclear speckles. We show that MFAP1, among the top 20 in our list, forms droplets under certain circumstances and that MFAP1 expression levels modulate the size, stability, and dynamics of nuclear speckles. Localization of MFAP1 and its binding partner, PRPF38A, in droplet-like nuclear bodies precedes formation of nuclear speckles during telophase. Our results update older proteomic studies of nuclear speckles and should provide a useful reference dataset to guide future experimental dissection of nuclear speckle structure and function.

摘要

我们提出了一种简单的比率方法,用于推断使用邻近标记方法但补偿自由基扩散的细胞结构内的蛋白质组成。我们使用酪胺信号放大(TSA)和无标记质谱(MS)来比较核斑点与着丝粒之间的蛋白质。我们的“TSA-MS 比”方法成功地鉴定了已知的核斑点蛋白。例如,在排名前 30 和 100 的蛋白质中,分别有 96%和 67%的蛋白质是已知的核斑点蛋白,包括我们在此验证为富含核斑点的蛋白质。我们表明,在我们的列表中排名前 20 的 MFAP1 在某些情况下会形成液滴,并且 MFAP1 的表达水平调节核斑点的大小、稳定性和动力学。MFAP1 和其结合伴侣 PRPF38A 在核斑点形成之前,在类似于液滴的核体中定位。我们的结果更新了核斑点的旧蛋白质组学研究,应该为未来核斑点结构和功能的实验剖析提供有用的参考数据集。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c1e5/7480118/a2a62dcf3e3a/JCB_201910207_Fig1.jpg

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