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基于 timsTOF SCP 的 diaPASEF 方法对蛋白质鉴定和定量的评估。

Evaluation of Protein Identification and Quantification by the diaPASEF Method on timsTOF SCP.

机构信息

Departments of Structural Biology and Developmental Neurobiology, St. Jude Children's Research Hospital, Memphis, Tennessee 38105, United States.

Center for Proteomics and Metabolomics, St. Jude Children's Research Hospital, Memphis, Tennessee 38105, United States.

出版信息

J Am Soc Mass Spectrom. 2024 Jun 5;35(6):1253-1260. doi: 10.1021/jasms.4c00067. Epub 2024 May 16.

Abstract

Accurate and precise quantification is crucial in modern proteomics, particularly in the context of exploring low-amount samples. While the innovative 4D-data-independent acquisition (DIA) quantitative proteomics facilitated by timsTOF mass spectrometers gives enhanced sensitivity and selectivity for protein identification, the diaPASEF (parallel accumulation-serial fragmentation combined with data-independent acquisition) parameters have not been systematically optimized, and a comprehensive evaluation of the quantification is currently lacking. In this study, we conducted a thorough optimization of key parameters on a timsTOF SCP instrument, including sample loading amount (50 ng), ramp/accumulation time (140 ms), isolation window width (20 /), and gradient time (60 min). To further improve the identification of proteins in low-amount samples, we utilized different column settings and introduced 0.02% -dodecyl-β-d-maltoside (DDM) in the sample reconstitution solution, resulting in a remarkable 19-fold increase in protein identification at the single-cell-equivalent level. Moreover, a comprehensive comparison of protein quantification using a tandem mass tag reporter (TMT-reporter), complement TMT ions (TMTc), and diaPASEF revealed a strong correlation between these methods. Both diaPASEF and TMTc have effectively addressed the issue of ratio compression, highlighting the diaPASEF method's effectiveness in achieving accurate quantification data compared to TMT reporter quantification. Additionally, an in-depth analysis of in-group variation positioned diaPASEF between the TMT-reporter and TMTc methods. Therefore, diaPASEF quantification on the timsTOF SCP instrument emerges as a precise and accurate methodology for quantitative proteomics, especially for samples with small amounts.

摘要

在现代蛋白质组学中,准确和精确的定量至关重要,特别是在探索低丰度样本的情况下。虽然 timsTOF 质谱仪支持的创新的 4D-数据非依赖性采集(DIA)定量蛋白质组学为蛋白质鉴定提供了更高的灵敏度和选择性,但 diaPASEF(平行累积-串联碎裂与数据非依赖性采集相结合)参数尚未得到系统优化,并且目前缺乏对定量的全面评估。在这项研究中,我们在 timsTOF SCP 仪器上对关键参数进行了彻底优化,包括样品加载量(50ng)、斜坡/累积时间(140ms)、隔离窗口宽度(20/)和梯度时间(60min)。为了进一步提高低丰度样品中蛋白质的鉴定能力,我们利用了不同的柱设置,并在样品重溶解决方案中引入了 0.02%-十二烷基-β-D-麦芽糖苷(DDM),从而使单细胞当量水平的蛋白质鉴定数量显著增加了 19 倍。此外,使用串联质量标签报告器(TMT-reporter)、补充 TMT 离子(TMTc)和 diaPASEF 对蛋白质定量进行了全面比较,结果表明这些方法之间具有很强的相关性。diaPASEF 和 TMTc 都有效地解决了比例压缩的问题,这突出了 diaPASEF 方法与 TMT reporter 定量相比,在实现准确定量数据方面的有效性。此外,对组内变异的深入分析将 diaPASEF 置于 TMT-reporter 和 TMTc 方法之间。因此,timsTOF SCP 仪器上的 diaPASEF 定量是一种精确而准确的定量蛋白质组学方法,特别是对于小量样本。

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