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通过优化内部片段生成和分配,将自上而下质谱序列覆盖率提高一个数量级。

Increasing Top-Down Mass Spectrometry Sequence Coverage by an Order of Magnitude through Optimized Internal Fragment Generation and Assignment.

机构信息

Department of Chemistry and Chemical Biology, Northeastern University, Boston, Massachusetts 02115, United States.

Barnett Institute for Chemical and Biological Analysis, Northeastern University, Boston, Massachusetts 02115, United States.

出版信息

Anal Chem. 2021 Apr 27;93(16):6355-6362. doi: 10.1021/acs.analchem.0c04670. Epub 2021 Apr 12.

DOI:10.1021/acs.analchem.0c04670
PMID:33844516
Abstract

A major limitation of intact protein fragmentation is the lack of sequence coverage within proteins' interiors. We show that collisionally activated dissociation (CAD) produces extensive internal fragmentation within proteins' interiors that fill the existing gaps in sequence coverage, including disulfide loop regions that cannot be characterized using terminal fragments. A barrier to the adoption of internal fragments is the lack of methods for their generation and assignment. To provide these, we explore the effects of protein size, mass accuracy, internal fragment size, CAD activation energy, and data preprocessing upon the production and identification of internal fragments. We also identify and mitigate the major source of ambiguity in internal fragment identification, which we term "frameshift ambiguity." Such ambiguity results from sequences containing any "middle" portion surrounded by the same composition on both termini, which upon fragmentation can produce two internal fragments of identical mass, yet out of frame by one or more amino acids (e.g., TRAIT producing TRAI or RAIT). We show that such instances permit the a priori assignment of the middle sequence portion. This insight and our optimized methods permit the unambiguous assignment of greater than 97% of internal fragments using only the accurate mass. We show that any remaining ambiguity in internal fragment assignment can be removed by consideration of fragmentation propensities or by (pseudo)-MS. Applying these methods resulted in a 10-fold and 43-fold expanded number of identified ions, and a concomitant 7- and 16-fold increase in fragmentation sites, respectively, for native and reduced forms of a disease-associated SOD1 variant.

摘要

完整蛋白质片段化的一个主要限制是缺乏蛋白质内部的序列覆盖。我们表明,碰撞激活解离(CAD)在蛋白质内部产生广泛的内部片段化,填补了序列覆盖的现有空白,包括不能使用末端片段进行特征描述的二硫键环区域。采用内部片段的一个障碍是缺乏生成和分配它们的方法。为了提供这些方法,我们探索了蛋白质大小、质量精度、内部片段大小、CAD 激活能以及数据预处理对内部片段的生成和鉴定的影响。我们还确定并减轻了内部片段鉴定中的主要歧义源,我们称之为“移码歧义”。这种歧义源于序列中包含任何“中间”部分,该部分在两端都具有相同的组成,在片段化后可以产生两个质量相同但却相差一个或多个氨基酸的内部片段(例如,TRAI 产生 TRAI 或 RAIT)。我们表明,这种情况允许对中间序列部分进行先验分配。这种洞察力和我们优化的方法允许仅使用准确质量对超过 97%的内部片段进行明确分配。我们表明,通过考虑片段化倾向或(伪)MS,可以消除内部片段分配中的任何剩余歧义。应用这些方法分别导致天然和还原形式的疾病相关 SOD1 变体的鉴定离子数量增加了 10 倍和 43 倍,分别增加了 7 倍和 16 倍。

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