利用混合 PRM/DIA 同时进行靶向和发现驱动的临床蛋白质分型分析

IF 2.8 3区 医学 Q2 BIOCHEMICAL RESEARCH METHODS Clinical proteomics Pub Date : 2024-04-02 DOI:10.1186/s12014-024-09478-5
Sandra Goetze, Audrey van Drogen, Jonas B. Albinus, Kyle L. Fort, Tejas Gandhi, Damiano Robbiani, Véronique Laforte, Lukas Reiter, Mitchell P. Levesque, Yue Xuan, Bernd Wollscheid
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引用次数: 0

摘要

临床样本具有不可替代性,将其转化为可搜索和可重复使用的数字生物库,对于开展具有统计学意义的回顾性和综合性研究至关重要。目前,主要采用独立于数据的采集策略来全面数字化临床样本群。然而,DIA 的灵敏度有限,这就是为什么通常还要通过平行反应监测对选定的候选标记物进行有针对性的测量。在此,我们将最近共同开发的混合 PRM/DIA 技术作为一种新的智能数据采集策略,在蛋白型水平上对罕见临床样本进行全面数字化。通过智能触发多重并行反应监测(MSxPRM),结合使用 DIA 对临床生物样本进行发现驱动的数字化,混合 PRM/DIA 技术提高了当前临床关注的一组特定分析物的测量灵敏度。重标记参考肽被用作 MSxPRM 和内源性肽监测的触发器。我们首先在临床环境中对混合 PRM/DIA 进行了评估,评估对象为从 64 个注释的人类蛋白质组中筛选出的 185 种肿瘤相关抗原蛋白型肽。结果表明,即使在接近检测限的低浓度条件下,检测内源性肽的重现性和灵敏度也得到了提高。结果表明,多达 179 次的 MSxPRM 扫描不会影响 DIA 的整体性能。接下来,我们将混合 PRM/DIA 应用于生物库黑色素瘤样本的综合数字化,使用了一组 30 种 AQUA 肽,针对黑色素瘤患者分子肿瘤委员会评估中相关的 28 种候选生物标记物。在 DIA 检测到的约 6500 个蛋白质组中,选定的候选标记物(如 UFO、CDK4、NF1 和 PMEL)可通过 MSxPRM 扫描进行一致的定量监测,为支持未来的临床决策提供了更多信心。将 PRM 和 DIA 测量结合起来提供了一种新策略,可以灵敏、可重复地检测分子肿瘤委员会目前正在讨论的患者的蛋白质标记物,并有机会发现新的候选生物标记物。
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Simultaneous targeted and discovery-driven clinical proteotyping using hybrid-PRM/DIA
Clinical samples are irreplaceable, and their transformation into searchable and reusable digital biobanks is critical for conducting statistically empowered retrospective and integrative research studies. Currently, mainly data-independent acquisition strategies are employed to digitize clinical sample cohorts comprehensively. However, the sensitivity of DIA is limited, which is why selected marker candidates are often additionally measured targeted by parallel reaction monitoring. Here, we applied the recently co-developed hybrid-PRM/DIA technology as a new intelligent data acquisition strategy that allows for the comprehensive digitization of rare clinical samples at the proteotype level. Hybrid-PRM/DIA enables enhanced measurement sensitivity for a specific set of analytes of current clinical interest by the intelligent triggering of multiplexed parallel reaction monitoring (MSxPRM) in combination with the discovery-driven digitization of the clinical biospecimen using DIA. Heavy-labeled reference peptides were utilized as triggers for MSxPRM and monitoring of endogenous peptides. We first evaluated hybrid-PRM/DIA in a clinical context on a pool of 185 selected proteotypic peptides for tumor-associated antigens derived from 64 annotated human protein groups. We demonstrated improved reproducibility and sensitivity for the detection of endogenous peptides, even at lower concentrations near the detection limit. Up to 179 MSxPRM scans were shown not to affect the overall DIA performance. Next, we applied hybrid-PRM/DIA for the integrated digitization of biobanked melanoma samples using a set of 30 AQUA peptides against 28 biomarker candidates with relevance in molecular tumor board evaluations of melanoma patients. Within the DIA-detected approximately 6500 protein groups, the selected marker candidates such as UFO, CDK4, NF1, and PMEL could be monitored consistently and quantitatively using MSxPRM scans, providing additional confidence for supporting future clinical decision-making. Combining PRM and DIA measurements provides a new strategy for the sensitive and reproducible detection of protein markers from patients currently being discussed in molecular tumor boards in combination with the opportunity to discover new biomarker candidates.
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来源期刊
Clinical proteomics
Clinical proteomics BIOCHEMICAL RESEARCH METHODS-
CiteScore
5.80
自引率
2.60%
发文量
37
审稿时长
17 weeks
期刊介绍: Clinical Proteomics encompasses all aspects of translational proteomics. Special emphasis will be placed on the application of proteomic technology to all aspects of clinical research and molecular medicine. The journal is committed to rapid scientific review and timely publication of submitted manuscripts.
期刊最新文献
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