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INCREASE IMAGE CLARITY AND SPECIFICITY USING DUAL MSI SOURCES AND MULTI-REFLECTING TIME-OF-FLIGHT ANALYZING METABOLITES IN MOUSE TESTIS

Posters | 2022 | Waters | ASMSInstrumentation
MALDI, MS Imaging, LC/TOF, LC/HRMS, LC/MS, LC/MS/MS
Industries
Metabolomics
Manufacturer
Waters

Summary

Importance of the Topic


The distribution and composition of lipids within the mammalian testis are critical for understanding spermatogenesis, male fertility and associated metabolic disorders. Advanced mass spectrometry imaging (MSI) methods provide spatially resolved molecular information, overcoming challenges posed by the complex and heterogeneous testicular tissue architecture.

Objectives and Study Overview


This study aims to enhance image clarity and molecular specificity in mouse testis lipid analysis by combining two ambient and vacuum ionization MSI sources (DESI and MALDI) on a high-resolution Multi-Reflecting Time-of-Flight (MRT) platform. Comparative analysis of lipid profiles across different cell types—Sertoli cells, germ cells and Leydig cells—was performed to reveal compartment-specific lipid remodeling.

Methodology


Mouse testis sections were cryosectioned and mounted on glass slides. MALDI experiments used α-Cyano-4-hydroxycinnamic acid matrix applied with a nebulizing sprayer. DESI imaging required no matrix, relying on charged droplets for desorption and ionization. Data were acquired on two instruments:
  • SELECT SERIES™ MRT mass spectrometer (quadrupole Multi-Reflecting TOF) at ~200,000 FWHM resolution
  • SYNAPT™ G2-Si Q-oaTOF with DESI XS source at ~25,000 FWHM resolution

Instrumentation Used


Key hardware and software components included:
  • MALDI: HTX M5 nebulizer, 355 nm Nd:YAG laser
  • DESI: DESI XS source with Leu-enkephalin internal standard
  • Data processing: Waters MassLynx™, HDI™ for image generation
  • Statistical analysis: MetaboAnalyst for PCA and heat maps
  • Lipid identification: LIPID MAPS® database

Main Results and Discussion


High-resolution MSI enabled clear separation of lipid classes and isotope fine structure with sub-500 ppb mass accuracy. Principal component analysis on eight regions of interest distinguished lipid profiles in Sertoli, germ and Leydig compartments. Key findings:
  • Distinct glycerophospholipids and triglycerides localized to specific cell types
  • Seminolipids (e.g. C16:0‐alkyl‐C16:0 acyl) predominated in seminiferous tubules
  • MRT resolution resolved peaks <20 mDa apart, revealing isotope fine structure unresolvable on lower-resolution Q-oaTOF
  • DESI vs. MALDI comparison showed complementary lipid coverage and similar spectral features

Benefits and Practical Applications


This dual-source approach on a single high-resolution platform increases confidence in lipid identification, enhances spatial specificity and enables detailed mapping of metabolic pathways in reproductive biology. It can be applied to drug distribution studies, biomarker discovery and pathology imaging.

Future Trends and Opportunities


Advances in MSI spatial resolution and ionization technologies will further refine cell-level metabolomic mapping. Integration with ion mobility and multiplexed imaging modalities promises deeper insights into tissue heterogeneity, disease mechanisms and therapeutic targeting.

Conclusion


The combined DESI and MALDI MSI on a Multi-Reflecting TOF instrument successfully distinguished lipid distributions across testicular compartments with ultra-high mass resolution and sub-500 ppb accuracy. This methodology enhances molecular specificity and paves the way for comprehensive spatial lipidomics in biomedical research.

References


1. Rodemer C et al. Human Molecular Genetics. 2003;12(15):1881–1885.
2. Vos JP et al. Biochim Biophys Acta. 1993;1211:1250–149.
3. Siangcham T et al. PLoS ONE. 2015;10(3):e0120412.
4. Ishizuka I et al. J Biochem. 1973;73(1):77–87.
5. Goto-Inoue N et al. Glycobiology. 2009;19(9):950–957.

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