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Two-Dimensional Liquid Chromatography Isolation and Quantitation of IgG and Exosomes from Cell Culture Media

Presentations | 2026 | Clemson University | MDCWInstrumentation
2D-LC
Industries
Pharma & Biopharma
Manufacturer

Summary

Significance of the Topic


Advances in biologics production and extracellular vesicle research demand robust analytical workflows capable of extracting multiple high-value products from complex cell culture media. Two-dimensional liquid chromatography (2D-LC) offers a promising solution by coupling affinity capture of monoclonal antibodies with downstream hydrophobic interaction chromatography to isolate both IgG and exosomes in a single integrated process.

Study Objectives and Overview


This work aimed to develop and validate a 2D-LC method that:
  • Recovers therapeutic IgG from CHO cell culture supernatants via Protein A affinity on capillary-channeled polymer fibers (C-CP).
  • Recovers and purifies exosomes from the Protein A effluent using a second dimension hydrophobic interaction chromatography (HIC).
  • Demonstrates quantitative performance, high purity, and feasibility for process analytical technology (PAT) integration.

Methodology and Instrumentation


The process employed two sequential separation dimensions:
  • Dimension 1 (1D): Protein A affinity chromatography on polypropylene C-CP fiber columns, eluted by pH gradient to capture IgG selectively.
  • Dimension 2 (2D): Hydrophobic interaction chromatography on polyester C-CP fibers with an inverse salt/organic modifier gradient to retain and elute exosomes.

Instrumentation included:
  • Two HPLC pumps delivering mobile phases for each dimension.
  • A modular 2D switch for timed transfer of 1D effluent to 2D loop.
  • UV detectors for IgG quantitation in 1D and exosome quantitation in 2D.
  • Custom C-CP fiber columns (PP for Protein A, PET for HIC) mounted in capillaries.

Results and Discussion


IgG Performance:
  • Recovery linear over 1–8 µg injections (R² = 0.99).
  • Yield exceeded 95% with RSD <5%.
  • Purity confirmed by SDS-PAGE, comparable to commercial columns.

Exosome Performance:
  • Average particle diameter 83 ± 23 nm by nano-flow cytometry.
  • Immunolabeling showed ~66% tetraspanin‐positive vesicles (CD9, CD63, CD81).
  • Membrane staining indicated ~93% vesicle integrity.
  • Recovery of ~1.8×1011 particles/mL with <7% RSD.
  • Host cell protein content reduced by >99% (3 mg/mL to 3 µg/mL).
  • Purity >5×1010 particles/µg protein, meeting NIH guidelines.

Benefits and Practical Applications


This approach enables concurrent capture of therapeutic antibodies and high-purity exosomes from the same bioreactor harvest, delivering:
  • Resource recovery by valorizing the Protein A effluent.
  • Enhanced PAT capabilities for real-time monitoring of cell culture health and productivity.
  • Cost savings using inexpensive C-CP fiber columns (<$5 each) with in-house chemistry modification.

Future Trends and Potential Applications


Potential extensions include:
  • Analytical scale C-CP columns for high-throughput screening.
  • Isotopic labeling (e.g., Yb) of exosomes for ICP-MS quantitation.
  • Functional assays of HIC-isolated exosomes in cellular uptake studies.
  • Anion exchange chromatography using polymer fiber modifications.
  • Adaptations for liposome and adeno-associated virus (AAV) separations.

Conclusion


The developed 2D-LC workflow successfully integrates Protein A affinity and HIC on capillary-channeled polymer fiber columns to isolate and quantify both therapeutic IgG and exosomes from CHO supernatant. The method achieves high yield, purity, and reproducibility using cost-effective materials, offering a scalable platform for downstream processing and advanced bioprocess analytics.

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