MALDI imaging mass spectrometry of N-linked glycans on formalin-fixed paraffin-embedded murine kidney

被引:67
作者
Gustafsson, Ove J. R. [1 ,6 ]
Briggs, Matthew T. [1 ,6 ]
Condina, Mark R. [2 ]
Winderbaum, Lyron J. [1 ]
Pelzing, Matthias [2 ]
McColl, Shaun R. [4 ,5 ]
Everest-Dass, Arun V. [3 ]
Packer, Nicolle H. [3 ]
Hoffmann, Peter [1 ,5 ,6 ]
机构
[1] Univ Adelaide, Adelaide Prote Ctr, Sch Mol & Biomed Sci, Adelaide, SA 5005, Australia
[2] Bruker Pty Ltd, Preston, Vic 3072, Australia
[3] Macquarie Univ, Biomol Frontiers Res Ctr, Fac Sci, Sydney, NSW 2109, Australia
[4] Univ Adelaide, Chemokine Biol Lab, Sch Mol & Biomed Sci, Adelaide, SA 5005, Australia
[5] Univ Adelaide, Ctr Mol Pathol, Adelaide, SA 5005, Australia
[6] Univ Adelaide, Inst Photon & Adv Sensing IPAS, Adelaide, SA 5005, Australia
基金
澳大利亚研究理事会;
关键词
MALDI imaging; MALDI; Mass spectrometry; Glycans; N-linked; LASER-DESORPTION IONIZATION; OVARIAN-CANCER; NEGATIVE-IONS; TISSUE; PROTEINS; IDENTIFICATION; FRAGMENTATION; PEPTIDES; ACCURACY; SECTIONS;
D O I
10.1007/s00216-014-8293-7
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Recent developments in spatial proteomics have paved the way for retrospective in situ mass spectrometry (MS) analyses of formalin-fixed paraffin-embedded clinical tissue samples. This type of analysis is commonly referred to as matrix-assisted laser desorption/ionization (MALDI) imaging. Recently, formalin-fixed paraffin-embedded MALDI imaging analyses were augmented to allow in situ analyses of tissue-specific N-glycosylation profiles. In the present study, we outline an improved automated sample preparation method for N-glycan MALDI imaging, which uses in situ PNGase F-mediated release and measurement of N-linked glycans from sections of formalin-fixed murine kidney. The sum of the presented data indicated that N-glycans can be cleaved from proteins within formalin-fixed tissue and characterized using three strategies: (i) extraction and composition analysis through on-target MALDI MS and liquid chromatography coupled to electrospray ionization ion trap MS; (ii) MALDI profiling, where N-glycans are released and measured from large droplet arrays in situ; and (iii) MALDI imaging, which maps the tissue specificity of N-glycans at a higher resolution. Thus, we present a complete, straightforward method that combines MALDI imaging and characterization of tissue-specific N-glycans and complements existing strategies.
引用
收藏
页码:2127 / 2139
页数:13
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