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Author(s): Susanto D, English AM, Sharma R, Kwong E
J Mass Spectrom. 2011 May;46(5):508-16 Authors: Susanto D, English AM, Sharma R, Kwong E
Article GUID: 21520348
Author(s): Yang E; Gamberi C; Chaurand P;
Matrix-assisted laser/desorption ionization imaging mass spectrometry (MALDI IMS) is an analytical technique for understanding the spatial distribution of biomolecules across a sample surface. Originally employed for mammalian tissues, this technology has b...
Article GUID: 31038251
Title: | Mapping the fly Malpighian tubule lipidome by imaging mass spectrometry |
Authors: | Yang E, Gamberi C, Chaurand P, |
Link: | https://pubmed.ncbi.nlm.nih.gov/31038251/ |
DOI: | 10.1002/jms.4366 |
Category: | J Mass Spectrom |
PMID: | 31038251 |
Dept Affiliation: | BIOLOGY
1 Department of Chemistry, University of Montreal, Pavillon Roger-Gaudry, 2900, boul. Édouard-Montpetit, Montreal, QC, Canada, H3C 3J7. 2 Biology Department, Concordia University, Montreal, QC, Canada, H4B 1R6. |
Description: |
Matrix-assisted laser/desorption ionization imaging mass spectrometry (MALDI IMS) is an analytical technique for understanding the spatial distribution of biomolecules across a sample surface. Originally employed for mammalian tissues, this technology has been adapted to study specimens as diverse as microbes and cell cultures, food such as strawberries, and invertebrates including the vinegar fly Drosophila melanogaster. As an ideal model organism, Drosophila has brought greater understanding about conserved biological processes, organism development, and diseased states and even informed management practices of agriculturally and environmentally important species. Drosophila displays anatomically separated renal (Malpighian) tubules that are the physiological equivalent to the vertebrate nephron. Insect Malpighian tubules are also responsible for pesticide detoxification. In this article, we first describe an effective workflow and sample preparation method to study the phospholipid distribution of the Malpighian tubules that initially involves the manual microdissection of the tubules in saline buffer followed by a series of washes to remove excess salt and enhances the phospholipid signals prior to matrix deposition and IMS at 25-µm spatial resolution. We also established a complementary methodology for lipid IMS analysis of whole-body fly sections using a dual-polarity data acquisition approach at the same spatial resolution after matrix deposition by sublimation. Both procedures yield rich signal profiles from the major phospholipid classes. The reproducibility and high-quality results offered by these methodologies enable cohort studies of Drosophila through MALDI IMS. |