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AdvanceBio Peptide Mapping - An HPLC Column Technology for Faster Protein Biocharacterizations

Presentations | 2014 | Agilent TechnologiesInstrumentation
Consumables, LC columns
Industries
Manufacturer
Agilent Technologies

Summary

Significance of the Topic


Peptide mapping is a cornerstone method in the analytical characterization of biotherapeutics. By enzymatically or chemically cleaving proteins into peptides, subtle changes such as point mutations, mis-translations, and post-translational modifications become detectable. Accurate peptide maps are critical for confirming primary structures, mapping disulfide bonds, monitoring degradation pathways (e.g., deamidation, oxidation), and ensuring lot-to-lot consistency in manufacturing complex proteins like monoclonal antibodies.

Objectives and Study Overview


This work introduces the AdvanceBio Peptide Mapping column, a superficially porous 2.7 µm C18 phase, designed to accelerate peptide mapping without sacrificing resolution. The study aimed to:
  • Reduce run times compared with traditional HPLC and UHPLC methods.
  • Maintain or improve separation performance in UV and LC/MS analyses.
  • Demonstrate robustness, reproducibility, and compatibility with high back pressures.
  • Benchmark against competitive superficially porous and UHPLC columns.

Methodology


Enzymatic digests of model proteins (BSA, IgG1) and complex mixtures (E. coli lysate) were separated on AdvanceBio Peptide Mapping columns of varying lengths (50 mm to 250 mm) at HPLC-compatible pressures (below 500 bar). Gradients from 3–10% to 40–70% acetonitrile in water (0.1% TFA) were optimized for run times ranging from 115 minutes down to 14 minutes.

Used Instrumentation


  • Agilent Infinity 1290 LC system (HPLC/MS coupling)
  • Agilent 1260 Bio-Inert HPLC system
  • 6530 Q-TOF mass spectrometer
  • Agilent AdvanceBio Peptide Mapping columns, 2.1×100–250 mm, 2.7 µm superficially porous C18

Main Results and Discussion


Rapid methods on 2.1×100 mm columns (0.6 mL/min) delivered 99.6–99.8% IgG sequence coverage in 14–40 min with conserved PTM detection (deamidation forms). Compared to competitive superficially porous columns, AdvanceBio delivered higher peak counts and narrower peaks at similar back pressures. Under HPLC-pressure conditions, it matched UHPLC speed and performance using sub-2 µm phases but at lower system pressures (~433 bar vs. 700 bar). Robustness tests (200 injections at pH 2.2, 55 °C) showed minimal retention shifts and consistent peak shapes. Column lifetime testing (>5000 injections) resulted in <40% plate loss.

Benefits and Practical Applications


  • Up to 8× faster analysis times while preserving resolution.
  • Improved throughput in quality control and biocharacterization workflows.
  • Compatibility with LC/MS for PTM profiling and peptide sequencing.
  • Versatile use in peptide impurity profiling (e.g., melittin), small protein separations, and complex cell-lysate analyses.

Future Trends and Opportunities


Advancements may include integration with high-resolution MS for deeper proteoform analysis, automation in peptide mapping protocols, microfluidic-based peptide separations, and expansion to multi-omics workflows. Improved column chemistries may further enhance stability at extreme pH or temperature conditions.

Conclusion


The AdvanceBio Peptide Mapping column technology provides a compelling solution for high-efficiency, high-throughput peptide profiling under HPLC conditions. It ensures reliable detection of critical structural attributes and PTMs while offering robustness and reproducibility across diverse applications.

Reference


  • Agilent Peptide Mapping How-To Guide, pub# 5991-2348EN
  • Agilent Biocolumns Selection Guide
  • Martosella et al., Glycoprotein EPO mapping, pub# 5991-2085EN & 5991-1813EN
  • Martosella et al., IgG1 mapping, pub# 5991-3585EN

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