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Increasing Recovery and Chromatographic Performance of “Acidic” Peptides Using Waters ACQUITY PREMIER Solution

Applications | 2021 | WatersInstrumentation
Consumables, HPLC, LC columns
Industries
Proteomics
Manufacturer
Waters

Summary

Significance of the Topic


In liquid chromatography of peptides, undesirable interactions between acidic peptides and metal surfaces lead to poor peak shapes, reduced recovery, and inconsistent assay performance. These challenges impact biopharmaceutical development and routine analysis, where reliable quantitation and identification of peptide fragments are critical for drug characterization and quality control.

Study Objectives and Overview


This application note evaluated the Waters ACQUITY PREMIER Solution, which incorporates MaxPeak High Performance Surface (HPS) technology, to determine its effectiveness in reducing metal-induced adsorption of an acidic peptide (VDNALQSGNSQESVTEQDSK, pI 3.9). Three LC configurations were compared: a conventional stainless-steel system, the same system with a PREMIER column, and a fully integrated PREMIER Solution (system and column). The goal was to assess improvements in detector response, peak shape, recovery, and fragment identification for a typical reversed-phase peptide mapping assay.

Methodology and Instrumentation


A tryptic digest of NIST mAb reference material containing the T14 peptide was analyzed under RPLC-MS conditions with a linear gradient (0.68% B/min; A: water/0.1% FA; B: acetonitrile/0.1% FA). Three configurations were tested:
  • Conventional UPLC H-Class Bio Binary PLUS System with stainless-steel column
  • Same system with an ACQUITY PREMIER Column (MaxPeak HPS surface)
  • ACQUITY PREMIER System with MaxPeak HPS column

Data were acquired on a SYNAPT XS high-resolution mass spectrometer using MSE data independent acquisition. Peptide identification and processing employed the UNIFI Scientific Information System.

Main Results and Discussion


Use of MaxPeak HPS surfaces dramatically reduced peak tailing and increased signal response:
  • Conventional setup: maximum ion count ~5.2×10⁴
  • PREMIER column on conventional system: ~1.2×10⁶ (23-fold increase)
  • Fully integrated PREMIER Solution: ~1.8×10⁶ (34-fold increase)

Peak area measurements demonstrated up to 4-fold improved recovery with the integrated PREMIER Solution. In MSE experiments, fragment ion detection increased from 11 b/y ions on the conventional system to 36 b/y ions with MaxPeak HPS technology, enhancing confidence in peptide assignment.

Benefits and Practical Applications


  • Improved peak symmetry and reduced tailing for acidic peptides
  • Enhanced sample recovery, boosting signal intensity and quantitation accuracy
  • Greater reproducibility and lower assay variability
  • Improved fragment coverage in MS-based peptide mapping, supporting robust data interpretation

These improvements translate into faster method development, higher laboratory throughput, and reliable analysis of metal-sensitive biomolecules.

Future Trends and Opportunities


Advances in surface chemistry for LC hardware will continue to address non-specific adsorption, extending benefits to a wider range of analytes, including modified peptides and small biomolecules. Integration with high-throughput and automated workflows will further reduce analysis time in biopharmaceutical research and QC. Continued optimization of barrier coatings and novel materials may enable even higher recoveries and expanded applicability in metabolomics and proteomics.

Conclusion


The Waters ACQUITY PREMIER Solution with MaxPeak HPS technology effectively mitigates adsorption of acidic peptides on metal surfaces. By improving recovery, peak shape, and fragment ion detection, it enhances data quality and robustness of LC-MS assays, supporting more efficient biopharmaceutical analysis and development.

References


No external literature references were cited in this application note.

Content was automatically generated from an orignal PDF document using AI and may contain inaccuracies.

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