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Developments in Orbitrap mass spectrometry on a modified Tribrid mass spectrometer

Posters | 2019 | Thermo Fisher Scientific | ASMSInstrumentation
LC/HRMS, LC/MS, LC/MS/MS, LC/Orbitrap
Industries
Other
Manufacturer
Thermo Fisher Scientific

Summary

Importance of the topic


Advancements in mass spectrometry technology are critical for pushing the boundaries of proteomics and biomolecular analysis. By increasing sensitivity, resolving power, and acquisition speed, researchers can obtain richer datasets with better quantitation and coverage. Enhancing Orbitrap performance at elevated ion routing multipole pressures and high mass-to-charge ratios addresses key limitations in analyzing large biomolecules and multiplexed reporter ions.

Study objectives and overview


In this work, researchers aimed to extend the utility of a standard Orbitrap Fusion Lumos Tribrid instrument by:
  • Improving detection sensitivity for high m/z analytes through hardware modifications.
  • Enhancing resolution and speed for tandem mass tag (TMT) workflows using a new deconvolution algorithm.
  • Evaluating the impact of elevated IRM pressures on large molecule decay kinetics.

Methodology


The study involved both hardware and software alterations to the Tribrid system:
  • Modified gas inlet tubing to raise IRM pressure from typical 8 mtorr up to 20 mtorr, permitting better capture of heavy ions.
  • Adjusted C-trap central electrode injection voltage to optimize ion capture, termed CE-inject.
  • Integrated the phase-constrained spectrum deconvolution method (ΦSDM) into the instrument control software, forming the TurboTMT workflow for high-resolution TMT analysis.
  • Sample evaluation using Pierce FlexMix calibration solutions, bovine carbonic anhydrase, and TMT11plex yeast digest standard.

Instrumentation


The modified setup comprised:
  • Thermo Scientific Orbitrap Fusion Lumos Tribrid mass spectrometer with upgraded Enhanced Vacuum Technology.
  • Ion routing multipole (IRM) chamber with adjustable ultra-high-purity nitrogen gas pressure.
  • Ion Max NG electrospray source, QR5 segmented quadrupole filter, and high-capacity transfer tube.

Main results and discussion


Key findings from the modifications include:
  • IRM pressure increases did not compromise Orbitrap resolution and maintained stable signal decay up to 3 mtorr, enhancing sensitivity for ions at m/z 2122 and 2722.
  • Lowering the C-trap injection voltage improved capture efficiency for slow-moving high m/z species without significant losses at low m/z.
  • TurboTMT employing ΦSDM achieved sub-FT limited resolution (>200,000) on 128 ms transients, enabling baseline separation of TMT reporter isotopologues with short acquisition windows.
  • Application of TurboTMT increased peptide and protein identifications by up to 30% in TMT11plex experiments.

Practical benefits and applications


These enhancements provide:
  • Greater sensitivity for large biomolecule and high m/z analyses in proteomics and structural studies.
  • Faster high-resolution TMT quantitation, reducing cycle times for multiplexed experiments.
  • Broader dynamic range and improved quantitative accuracy in complex sample workflows.

Future trends and potential applications


Ongoing developments may include optimization of computational resources to extend ΦSDM window sizes, integration of super-resolution methods into routine workflows, and adaptation to even higher mass ranges. Such trends will support deeper proteome coverage, more robust large-molecule characterization, and expanded applications in clinical, structural, and biopharmaceutical analysis.

Conclusion


The combined hardware upgrades and software innovations on a Tribrid mass spectrometer significantly extend its analytical capabilities. Elevated IRM pressures improve detection of large ions, while TurboTMT and ΦSDM enable rapid, high-resolution quantitation of TMT reporter ions, enhancing the instrument’s versatility for advanced proteomic workflows.

References


  • Grinfeld et al. Analytical Chemistry 2016, 89(2), 1202–1211.
  • Scheffler et al. ASMS 2016, poster MP312.

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