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通过高分辨率质谱应用的多重数据独立采集(MSX-DIA)提高了组蛋白肽分析的定量质量。

Multiplexed data independent acquisition (MSX-DIA) applied by high resolution mass spectrometry improves quantification quality for the analysis of histone peptides.

作者信息

Sidoli Simone, Fujiwara Rina, Garcia Benjamin A

机构信息

Epigenetics Program, Department of Biochemistry and Biophysics, Perelman School of Medicine, University of Pennsylvania, Philadelphia, PA, USA.

出版信息

Proteomics. 2016 Aug;16(15-16):2095-105. doi: 10.1002/pmic.201500527. Epub 2016 Jun 8.

Abstract

We present the MS-based application of the innovative, although scarcely exploited, multiplexed data-independent acquisition (MSX-DIA) for the analysis of histone PTMs. Histones are golden standard for complexity in MS based proteomics, due to their large number of combinatorial modifications, leading to isobaric peptides after proteolytic digestion. DIA has, thus, gained popularity for the purpose as it allows for MS/MS-based quantification without upfront assay development. In this work, we evaluated the performance of traditional DIA versus MSX-DIA in terms of MS/MS spectra quality, instrument scan rate and quantification precision using histones from HeLa cells. We used an MS/MS isolation window of 10 and 6 m/z for DIA and MSX-DIA, respectively. Four MS/MS scans were multiplexed for MSX-DIA. Despite MSX-DIA was programmed to perform two-fold more MS/MS events than traditional DIA, it acquired on average ∼5% more full MS scans, indicating even faster scan rate. Results highlighted an overall decrease of background ion signals using MSX-DIA, and we illustrated specific examples where peptides of different precursor masses were co-fragmented by DIA but not MSX-DIA. Taken together, MSX-DIA proved thus to be a more favorable method for histone analysis in data independent mode.

摘要

我们展示了基于质谱(MS)的创新型多重数据非依赖型采集(MSX-DIA)在组蛋白翻译后修饰(PTM)分析中的应用,尽管该方法尚未得到充分利用。由于组蛋白存在大量组合修饰,在蛋白水解消化后会产生等压肽段,因此在基于MS的蛋白质组学中,组蛋白是复杂度的黄金标准。因此,DIA因其无需预先进行分析方法开发即可实现基于MS/MS的定量分析而受到欢迎。在这项工作中,我们使用来自HeLa细胞的组蛋白,从MS/MS谱图质量、仪器扫描速率和定量精度方面评估了传统DIA与MSX-DIA的性能。我们分别为DIA和MSX-DIA使用了10 m/z和6 m/z的MS/MS隔离窗口。MSX-DIA对四次MS/MS扫描进行了复用。尽管MSX-DIA被设置为比传统DIA多执行两倍的MS/MS事件,但它平均采集的全MS扫描多了约5%,这表明其扫描速率更快。结果突出显示了使用MSX-DIA时背景离子信号总体上有所降低,并且我们举例说明了不同前体质量的肽段在DIA中会共同碎裂而在MSX-DIA中不会的具体情况。综上所述,MSX-DIA在数据非依赖模式下被证明是一种更适合组蛋白分析的方法。

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