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Analysis of Charge Variant of Monoclonal Antibody

Applications | 2022 | ShimadzuInstrumentation
Consumables, HPLC, LC columns
Industries
Pharma & Biopharma
Manufacturer
Shimadzu

Summary

Significance of the Topic


Charge heterogeneity in monoclonal antibodies can affect therapeutic efficacy, immunogenicity and regulatory approval. Accurate separation and quantification of these variants are essential for ensuring product quality and consistency in biopharmaceutical development and manufacturing.

Study Objectives and Overview


This application note demonstrates the use of a strong cation exchange method on a Shim-pack Bio IEX SP-NP column coupled with a Nexera XS inert HPLC system to resolve charge variants of a cetuximab biosimilar. The aim was to achieve baseline separation of ten distinct variants within a 30-minute analysis.

Methodology


  • Sample: Cetuximab biosimilar at 2.5 mg/mL
  • Mobile Phase A: 20 mM MES/HEPES buffer, pH 5.0
  • Mobile Phase B: 20 mM MES/HEPES buffer, pH 10.6
  • Gradient Program: 0 → 100 % B over 15–20 min, return to 0 % B by 30 min
  • Flow Rate: 0.3 mL/min
  • Column Temperature: 25 °C
  • Injection Volume: 5 µL, six injections for reproducibility assessment
  • Detection: UV absorbance at 280 nm

Used Instrumentation


  • HPLC System: Shimadzu Nexera XS inert
  • Column: Shim-pack Bio IEX SP-NP, 100 × 4.6 mm I.D., 3 µm
  • Sample Vial: TORAST-H glass vial

Key Results and Discussion


The method achieved baseline separation of ten charge variants, with retention times spanning 24.69 to 29.92 min. Relative standard deviations for retention times were below 0.05 % (n=6), indicating excellent run-to-run precision. The clear resolution of acidic and basic species supports detailed profiling of mAb charge heterogeneity.

Benefits and Practical Applications


  • High resolution enables comprehensive characterization of antibody charge profiles
  • Robust and reproducible performance is suitable for routine quality control
  • Applicable to biosimilarity assessments, lot comparability and stability studies

Future Trends and Potential Applications


  • Online coupling with mass spectrometry for molecular-level variant identification
  • Automation and high-throughput workflows for large-scale screening
  • Advanced data analytics and machine learning for pattern recognition in charge distributions

Conclusion


This strong cation exchange method on the Shim-pack Bio IEX SP-NP column provides a reliable, high-resolution tool for analyzing monoclonal antibody charge variants, addressing critical needs in biopharmaceutical development and regulatory compliance.

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

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