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Determination of Amino Acid Composition of Cell Culture Media and Protein Hydrosylate Standard

Applications | 2017 | Agilent TechnologiesInstrumentation
Consumables, HPLC, LC columns
Industries
Pharma & Biopharma
Manufacturer
Agilent Technologies

Summary

Importance of the topic


Accurate determination of amino acid composition is critical for cell culture optimization, quality control of biopharmaceuticals and monitoring of protein hydrolysate standards. Amino acids serve both as building blocks of proteins and key metabolites that influence cell growth and productivity. A reliable, high-throughput analytical method supports process development, regulatory compliance and ensures consistent product quality.

Objectives and Overview


This study introduces an automated HPLC method based on the Agilent AdvanceBio Amino Acid Analysis solution incorporating online OPA and FMOC derivatization. The goals were to reduce sample preparation time, improve precision over manual derivatization, demonstrate system suitability, establish limits of detection and quantification, and apply the method to cell culture media and protein hydrolysate standards.

Methodology and Instrumentation


An Agilent 1290 Infinity LC system with binary pump, autosampler and thermostatted column compartment was used. Online precolumn derivatization employed sequential mixing of borate buffer, sample, OPA and FMOC reagents via an injector program. Detection was by DAD at 338 nm for OPA derivatives and 262 nm for FMOC derivatives with a timed wavelength switch. Separation was achieved on an AdvanceBio AAA C18 column (4.6 × 100 mm, 2.7 µm) with a gradient of phosphate-borate buffer and acetonitrile/methanol/water. Mobile phase A contained 10 mM Na2HPO4 and 10 mM Na2B4O7 at pH 8.2; mobile phase B was 45:45:10 acetonitrile:methanol:water. Flow rate was 1.5 mL/min, run time 18 minutes including re-equilibration.

Main Results and Discussion


The method resolved 23 amino acids with high efficiency. Retention time RSD values were below 1.2% at 100 pmol levels and area RSD values below 5%, demonstrating excellent precision. Linearity was established over 0.9 to 1,000 pmol (R2 > 0.99). Limit of detection was approximately 0.9 pmol and limit of quantification approximately 3.8 pmol. System suitability according to Ph Eur requirements showed resolution between leucine and isoleucine well above the 1.5 threshold (observed >4.5). Application to MEM, NEAA and RPMI media, plus a protein hydrolysate standard, yielded compositional profiles matching theoretical values and confirmed method accuracy and selectivity.

Benefits and Practical Applications


  • Automated online derivatization reduces operator variability and contamination risk.
  • Rapid, sensitive and reproducible analysis suitable for routine QC.
  • Minimal sample preparation—direct vial transfer to autosampler.
  • High resolution of isobaric amino acids ensures regulatory compliance.
  • Supports fed-batch media optimization and metabolic profiling.

Future Trends and Potential Applications


  • Integration with mass spectrometry for enhanced specificity and structural information.
  • Miniaturization and high-throughput robotics for process analytical technology.
  • Real-time monitoring of amino acid levels in bioreactors to enable adaptive feeding strategies.
  • Expansion to peptide mapping and modified amino acid analysis.
  • Application in nutritional analysis, clinical diagnostics and environmental testing.

Conclusion


The Agilent AdvanceBio AAA solution with online OPA/FMOC derivatization on a 1290 Infinity LC system delivers a fast, precise and sensitive platform for amino acid analysis. Its robustness, regulatory suitability and compatibility with routine lab workflows make it an ideal choice for cell culture media profiling and protein hydrolysate standard testing.

References


  • European Pharmacopoeia 9.0 (2.2.56) Amino Acid Analysis

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