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一种新的 MALDI FTICR MS 组织分析优化策略,用于基于实验设计和数据建模的非靶向代谢组学分析。

A new optimization strategy for MALDI FTICR MS tissue analysis for untargeted metabolomics using experimental design and data modeling.

机构信息

Normandie Univ, COBRA, UMR 6014 and FR 3038, Université de Rouen, INSA de Rouen, CNRS, IRCOF, 1 rue Tesnière, 76821, Mont-Saint-Aignan, Cedex, France.

Department of Metabolic Biochemistry, Rouen University Hospital, 76000, Rouen, France.

出版信息

Anal Bioanal Chem. 2019 Jul;411(17):3891-3903. doi: 10.1007/s00216-019-01863-6. Epub 2019 May 15.

Abstract

Ultra-high-resolution imaging mass spectrometry using matrix-assisted laser desorption ionization (MALDI) MS coupled to a Fourier transform ion cyclotron resonance (FTICR) mass analyzer is a powerful technique for the visualization of small molecule distribution within biological tissues. The FTICR MS provides ultra-high resolving power and mass accuracy that allows large molecular coverage and molecular formula assignments, both essential for untargeted metabolomics analysis. These performances require fine optimizations of the MALDI FTICR parameters. In this context, this study proposes a new strategy, using experimental design, for the optimization of ion transmission voltages and MALDI parameters, for tissue untargeted metabolomics analysis, in both positive and negative ionization modes. These experiments were conducted by assessing the effects of nine factors for ion transmission voltages and four factors for MALDI on the number of peaks, the weighted resolution, and the mean error within m/z 150-1000 mass range. For this purpose, fractional factorial designs were used with multiple linear regression (MLR) to evaluate factor effects and to optimize parameter values. The optimized values of ion transmission voltages (RF amplitude TOF, RF amplitude octopole, frequency transfer optic, RF frequency octopole, deflector plate, funnel 1, skimmer, funnel RF amplitude, time-of-flight, capillary exit), MALDI parameters (laser fluence, number of laser shots), and detection parameters (data size, number of scans) led to an increase of 32% and 18% of the number of peaks, an increase of 8% and 39% of the resolution, and a decrease of 56% and 34% of the mean error in positive and negative ionization modes, respectively. Graphical abstract.

摘要

利用基质辅助激光解吸电离(MALDI)与傅里叶变换离子回旋共振(FTICR)质谱联用的超高分辨率成像质谱(Ultra-high-resolution imaging mass spectrometry using matrix-assisted laser desorption ionization (MALDI) MS coupled to a Fourier transform ion cyclotron resonance (FTICR) mass analyzer)是一种用于可视化生物组织中小分子分布的强大技术。FTICR MS 提供了超高分辨率和质量精度,允许进行大分子量覆盖和分子公式分配,这两者都是无靶向代谢组学分析的关键。这些性能需要对 MALDI FTICR 参数进行精细优化。在这种情况下,本研究提出了一种新的策略,使用实验设计来优化离子传输电压和 MALDI 参数,以进行组织无靶向代谢组学分析,同时在正离子和负离子模式下进行。通过评估九个离子传输电压因素和四个 MALDI 因素对峰数、加权分辨率和 m/z 150-1000 质量范围内的平均误差的影响,进行了这些实验。为此,使用分因子设计和多元线性回归(MLR)来评估因素效应并优化参数值。优化后的离子传输电压值(RF 幅度 TOF、RF 幅度八极、频率转换光学、RF 频率八极、偏转板、1 号漏斗、滑流、漏斗 RF 幅度、飞行时间、毛细管出口)、MALDI 参数(激光能量密度、激光脉冲数)和检测参数(数据大小、扫描次数)的值,分别使正离子和负离子模式下的峰数增加了 32%和 18%,分辨率提高了 8%和 39%,平均误差降低了 56%和 34%。

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