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多重三氟甲基和羟基自由基化学实现高分辨率蛋白质足迹分析。

Multiplex Trifluoromethyl and Hydroxyl Radical Chemistry Enables High-Resolution Protein Footprinting.

作者信息

Jain Rohit, Farquhar Erik R, Dhillon Nanak S, Jeon Nayeon, Chance Mark R, Kiselar Janna

机构信息

Center for Synchrotron Biosciences, Case Western Reserve University, School of Medicine, Cleveland, Ohio 44106, United States.

Center for Proteomics and Bioinformatics, Case Western Reserve University, School of Medicine, Cleveland, Ohio 44106, United States.

出版信息

Anal Chem. 2025 Jan 14;97(1):482-491. doi: 10.1021/acs.analchem.4c04610. Epub 2024 Dec 25.

DOI:10.1021/acs.analchem.4c04610
PMID:39720871
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11830425/
Abstract

Hydroxyl radical-based protein footprinting (HRPF) coupled with mass spectrometry is a valuable medium-resolution technique in structural biology, facilitating the assessment of protein structure and molecular-level interactions in solution conditions. In HRPF with X-rays (XFP), hydroxyl radicals generated by water radiolysis covalently label multiple amino acid (AA) side chains. However, HRPF technologies face challenges in achieving their full potential due to the broad (>10) dynamic range of AA reactivity with OH and difficulty in detecting slightly modified residues, most notably in peptides with highly reactive residues like methionine, or where all residues have low OH reactivities. To overcome this limitation, we developed a multiplex labeling chemistry that utilizes both CF radicals (CF) produced from a trifluoromethylation (TFM) reagent and OH radicals (OH), under controlled and optimized radiolysis doses generated by X-rays. We optimized the dual CF/OH chemistry using model peptides and proteins, thereby extending the existing OH labeling platform to incorporate simultaneous CF labeling. We labeled >50% of the protein sequence and >80% of protein solvent-accessible AAs via multiplex TFM labeling resulting in high-resolution footprinting, primarily by enhancing the labeling of AAs with low OH reactivity via the CF channel, while labeling moderate and highly OH-reactive AAs in both CF and OH channels. Moreover, the low reactivity of methionine with CF enabled the detection and quantification of additional AAs labeled by CF within methionine-containing peptides. Finally, we found that the solvent accessibility of protein AAs directly correlated with CF labeling, demonstrating that multiplex TFM labeling enables a high-resolution assessment of molecular interactions for enhanced HRPF.

摘要

基于羟基自由基的蛋白质足迹分析(HRPF)与质谱联用是结构生物学中一种有价值的中分辨率技术,有助于在溶液条件下评估蛋白质结构和分子水平的相互作用。在X射线介导的HRPF(XFP)中,水辐射分解产生的羟基自由基共价标记多个氨基酸(AA)侧链。然而,由于AA与OH的反应活性具有较宽(>10)的动态范围,且难以检测轻微修饰的残基,尤其是在含有高反应活性残基(如甲硫氨酸)的肽段中,或者所有残基的OH反应活性都较低的情况下,HRPF技术在充分发挥其潜力方面面临挑战。为克服这一限制,我们开发了一种多重标记化学方法,该方法在X射线产生的可控且优化的辐射分解剂量下,利用三氟甲基化(TFM)试剂产生的CF自由基(CF)和OH自由基(OH)。我们使用模型肽和蛋白质优化了双CF/OH化学方法,从而扩展了现有的OH标记平台,使其能够同时进行CF标记。通过多重TFM标记,我们标记了>50%的蛋白质序列和>80%的蛋白质溶剂可及AA,从而实现了高分辨率足迹分析,这主要是通过CF通道增强低OH反应活性AA的标记,同时在CF和OH通道中标记中等和高OH反应活性的AA。此外,甲硫氨酸与CF的低反应活性使得能够检测和定量含甲硫氨酸肽段中CF标记的其他AA。最后,我们发现蛋白质AA的溶剂可及性与CF标记直接相关,这表明多重TFM标记能够对分子相互作用进行高分辨率评估,从而增强HRPF。