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Routine Comprehensive Tissue Imaging on the Xevo™ G3 QTof Mass Spectrometer Using a DESI™ XS Source

Applications | 2024 | WatersInstrumentation
LC/HRMS, LC/MS, LC/MS/MS, LC/TOF, MS Imaging
Industries
Clinical Research
Manufacturer
Waters

Summary

Significance of the Topic


This application note addresses the challenge of balancing acquisition speed and data quality in mass spectrometry imaging (MSI) of tissue sections. Rapid, high-resolution imaging of biological samples is critical for fields such as neurobiology, pharmacology, and clinical diagnostics. By exploring scan rates up to 20 scans per second on a Waters Xevo G3 QTof coupled to a DESI XS source, this study demonstrates how modern instrumentation can accelerate data collection without compromising sensitivity, spatial resolution, or mass accuracy.

Objectives and Study Overview


• Evaluate the performance of the Xevo G3 QTof MS with a DESI XS source across multiple scan speeds (2–20 scans per second).
• Assess the impact of increased acquisition speed on spectral intensity, feature detection, and spatial segmentation.
• Demonstrate reproducibility and robustness for routine MSI applications using murine brain sections.

Methodology


A single murine brain was cryosectioned at 18 µm thickness and mounted on glass slides. No chemical derivatization or matrix deposition was applied. Sequential sections were imaged under identical DESI conditions at four step rates corresponding to 2, 5, 10, and 20 scans per second. Total ion current (TIC) normalization was applied during data processing. Feature segmentation was performed using UMAP and HDBSCAN algorithms via Waters MicroApp Store, and region-of-interest (ROI) spectral profiles were extracted for comparative analysis.

Used Instrumentation


• Mass Spectrometer: Waters Xevo G3 QTof
• Ion Source: DESI XS with high-performance sprayer and heated transfer line
• Spray Solvent: 98% methanol/2% water at 2 µL/min
• Source Settings: cone voltage 30 V, source temperature 150 °C, transfer line 450 °C, N2 gas 15 psi, capillary voltage 0.6 V

Results and Discussion


Segmentation maps generated at different scan speeds showed visually comparable tissue structures. Correlation analyses of spectral profiles from four ROIs revealed high linearity (R²>0.94 across speeds) and minimal biological variation (R²>0.97 between adjacent sections). Unsupervised PCA clustering of TIC-normalized spectra grouped ROIs by tissue segment rather than scan rate. Key lipid markers (e.g., PS(40:6), PS(38:4), PE(p38:4)) maintained sub-2 ppm mass accuracy and ~30,000 FWHM resolution across all speeds. Overlay images of these lipids at 5, 10, and 20 scans per second were visually consistent, confirming spatial fidelity.

Benefits and Practical Applications


  • Increased throughput: up to a tenfold reduction in imaging time with minimal loss of data quality.
  • High sensitivity and dynamic range for lipidomic profiling in tissue sections.
  • Versatile platform supporting MS, MS/MS, and SONAR modes for discovery and targeted MSI workflows.

Future Trends and Opportunities


  • Integration of advanced clustering and machine-learning tools for real-time tissue classification.
  • Development of faster MS detectors and optimized ion optics to push scan rates beyond 20 sps.
  • Application of high-speed MSI in pharmaceutical drug distribution studies and rapid clinical diagnostics.

Conclusion


The Waters Xevo G3 QTof with DESI XS source delivers rapid, reproducible tissue imaging without sacrificing spatial resolution, mass accuracy, or sensitivity. Even at 20 scans per second, spectral profiles remain highly correlated to slower acquisitions. This robust platform is ideally suited for routine high-throughput MSI in research and quality control environments.

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