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Double Barrel ESI Source and Novel Tandem NanoLC-MS Setup Enables 24/7 Proteome Profiling with Close to 100% MS Utilization

Posters | 2020 | Thermo Fisher ScientificInstrumentation
LC/HRMS, LC/MS, LC/MS/MS, LC/Orbitrap
Industries
Proteomics
Manufacturer
Thermo Fisher Scientific

Summary

Significance of the Topic

Nano-flow UHPLC coupled with high-resolution accurate-mass mass spectrometry is the benchmark for deep proteome profiling but often underutilizes MS acquisition time due to sample loading, column washing, and equilibration steps. The presented tandem nanoLC-MS platform overcomes these limitations by enabling parallel processing on two analytical columns, driving near-complete instrument utilization and high throughput.

Objectives and Study Overview

The primary aim was to engineer an automated dual-column nanoLC-MS/MS system achieving close to 100% MS utilization for 24/7 proteome profiling, while preserving chromatographic performance and reproducibility for complex protein digests.

Methodology and Used Instrumentation

A 200 ng HeLa tryptic digest was analyzed using two self-packed 75 µm I.D. × 40 cm C18 columns (1.9 µm) in a Thermo Scientific UltiMate 3000 RSLCnano tandem setup housed in a Sonation Double Barrel Column Oven. Dual-spray electrospray ionization interfaced both columns directly with a Q Exactive HF-X Orbitrap MS. Sample loading, washing, and equilibration on one column ran concurrently with peptide separation on the other, controlled by NCS-3500RS and NCP-3200RS pumps and a WPS-3000TPL RS autosampler. Key conditions:
  • Solvent A: 0.1% formic acid in water (with 5% DMSO)
  • Solvent B: 0.1% formic acid in 80% acetonitrile (with 5% DMSO)
  • Flow rate: 250 nL/min, column temperature: 60 °C
  • Gradient lengths: 45, 90, 120 min; injection volume: 10–20 µL
  • MS acquisition: data-dependent mode, m/z 375–1500
  • Data analysis: Thermo Scientific Proteome Discoverer 2.4 with 1% FDR using spectral library and Sequest HT

Main Results and Discussion

  • MS utilization exceeded 95% across all tested gradients, enabling continuous 24/7 operation.
  • The 90 min direct-injection method delivered over 73,000 unique peptides and more than 6,700 protein groups per run, equivalent to identification rates above 800 peptides per minute.
  • Reproducibility was exceptional: >90% protein group overlap and >80% peptide overlap between runs, peptide retention time variation under 1 min (96% consistency), and protein abundance variability below 25% (74% consistency).

Benefits and Practical Applications

This tandem nanoLC-MS configuration dramatically enhances throughput and duty cycle, making it ideal for large-scale discovery proteomics, clinical biomarker studies, and routine QA/QC. The high reproducibility supports robust quantification and deep proteome coverage in both shotgun and targeted workflows.

Future Trends and Possibilities

Anticipated advancements include integration of multiplexed labeling (e.g., TMT), AI-driven method optimization, seamless coupling with automated sample preparation, and real-time data processing pipelines. The modular approach could also accommodate additional fragmentation techniques and targeted acquisition modes for specialized applications.

Conclusion

The novel tandem nanoLC-MS platform achieves near-complete utilization of MS acquisition time and exceptional reproducibility, establishing a new standard for high-throughput, deep proteome profiling. Its 24/7 operational capability and flexibility offer a powerful alternative to conventional single-column systems in both discovery and targeted proteomics.

Reference

  1. RSLCnano pre-concentration nano LC kit. UltiMate 3000 RSLCnano Standard Applications Guide, Thermo Fisher Scientific.
  2. Pynn C., Boychenko A., Decrop R., Baynham M., Jehle P., Ruehl M. Tandem nanoLC-MS: maximum MS utilization for deep-dive proteomic analysis. Thermo Fisher Scientific TN 72899.
  3. R Core Team (2019). R: A language and environment for statistical computing. R Foundation for Statistical Computing, Vienna, Austria.

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