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Ultra-high resolution MALDI-FTICR-MSI analysis of intact proteins in mouse and human pancreas tissue

机译:超高分辨率MALDI-FTICR-MSI分析小鼠和人胰腺组织中的完整蛋白质分析

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摘要

Matrix assisted laser desorption/ionization mass spectrometry imaging (MALDI-MSI) of intact proteins is mostly performed using time-of-flight (TOF) based mass spectrometers, operated in linear mode. Linear MALDI-TOF systems provide limited mass resolving power and mass accuracy, which complicates assigning identities to the peaks in the MSI datasets. In this work we report ultra-high mass resolution MALDI-MSI based on 15T Fourier transform ion cyclotron resonance (FTICR) mass spectrometry for the analysis of intact proteins directly from non-embedded and OCT-embedded mouse and human (control and type 2 diabetes) pancreas so that small endocrine compartments (islets of Langerhans) may be analyzed in control and pathological tissues. Sample preparation methods, in terms of increased sensitivity while limiting lateral diffusion of analytes, have been investigated. By combining protein localization, high mass accuracy, and the clearly resolved isotope patterns we were able to assign protein identities with additional confidence, including proteins of similar average mass and with interspersed isotopomers. These capabilities allowed us to ascertain the presence of many protein adducts that, with a low resolving power instrument, could be misinterpreted as distinct protein ions. (C) 2017 Published by Elsevier B.V.
机译:完整蛋白质的基质辅助激光解吸/电离质谱成像(MALDI-MSI)主要使用基于飞行时间(TOF)的质谱仪进行,以线性模式操作。线性MALDI-TOF系统提供有限的质量分辨率和质量准确度,使得将标识与MSI数据集中的峰值分配。在这项工作中,我们报告了基于15T傅里叶变换离子回旋共振(FTICR)质谱法的超高质量分辨率MALDI-MSI,用于分析非嵌入和OCT嵌入式鼠标和人(对照和2型糖尿病)的完整蛋白质)胰腺可以在对照和病理组织中分析小内分泌隔室(朗格汉斯胰岛)。已经研究了样品制备方法,其在限制分析物的横向扩散的同时增加的灵敏度。通过组合蛋白质定位,高质量准确度和清晰分辨的同位素模式,我们能够以额外的置信度分配蛋白质身份,包括类似平均质量的蛋白质和散射同位素。这些能力使我们能够确定许多蛋白质加合物的存在,即通过低分辨率功率仪器误解为不同的蛋白质离子。 (c)2017年由Elsevier B.V发布。

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