Direct Analysis of Metallic Elements in Cell Culture Medium by Atomic Absorption Spectrophotometry (AAS)
Applications | 2020 | ShimadzuInstrumentation
Monitoring trace metal concentrations in CHO cell culture is essential to ensure consistent antibody yield and quality. Metallic cofactors such as zinc influence enzyme activity and glycan composition on IgG antibodies, affecting therapeutic properties. Rapid and reliable metal analysis supports process control in biopharmaceutical manufacturing.
This study evaluates atomic absorption spectrophotometry (AAS) as a cost-effective, straightforward alternative to ICP-MS and complex chelate methods for quantifying Cu, Mn, Co, Fe, and Zn in three commercial CHO media. It aims to demonstrate operational simplicity, sensitivity, and accuracy across two atomization modes: graphite furnace (electric thermal) and flame.
Samples from three CHO media (A, B, C) were diluted (factors ranging from 2× to 2000×) and acidified to 0.5 % HNO3. Calibration curves were generated using 1000 mg/L standards diluted to appropriate ranges. Analyses employed a Shimadzu AA-7000 spectrophotometer with automatic switching between graphite furnace and flame atomization and an autosampler. Spectroscopic parameters (wavelengths 213.9–324.8 nm, slit widths 0.2–0.7 nm) and temperature programs were optimized for each element to achieve LOQs down to low ppb levels.
Calibration curves for both modes showed correlation coefficients (r) above 0.999. Limit of quantitation, defined as 10σbL, was established via 10 replicates of blank medium. Electric thermal mode delivered ppt–ppb sensitivity with sample volumes of 5–50 µL, while flame mode covered ppb–ppm with 1–2 mL volumes. Measured concentrations varied among vendors, reflecting formulation differences. Spike recovery tests yielded 90–118 % across elements, indicating reliable quantitation with minimal matrix effects. Fe and Zn data from both modes were comparable, confirming method consistency.
The study confirms atomic absorption spectrophotometry as a robust, accessible technique for quantifying trace metals in CHO cell culture media. Its simplicity, flexibility between atomization modes, and strong analytical performance make AAS a valuable tool for quality control in biopharmaceutical production.
Shimadzu AA-7000 atomic absorption spectrophotometer with graphite furnace and flame atomizer, autosampler.
AAS
IndustriesPharma & Biopharma
ManufacturerShimadzu
Summary
Significance of the Topic
Monitoring trace metal concentrations in CHO cell culture is essential to ensure consistent antibody yield and quality. Metallic cofactors such as zinc influence enzyme activity and glycan composition on IgG antibodies, affecting therapeutic properties. Rapid and reliable metal analysis supports process control in biopharmaceutical manufacturing.
Objectives and Study Overview
This study evaluates atomic absorption spectrophotometry (AAS) as a cost-effective, straightforward alternative to ICP-MS and complex chelate methods for quantifying Cu, Mn, Co, Fe, and Zn in three commercial CHO media. It aims to demonstrate operational simplicity, sensitivity, and accuracy across two atomization modes: graphite furnace (electric thermal) and flame.
Methodology and Instrumentation
Samples from three CHO media (A, B, C) were diluted (factors ranging from 2× to 2000×) and acidified to 0.5 % HNO3. Calibration curves were generated using 1000 mg/L standards diluted to appropriate ranges. Analyses employed a Shimadzu AA-7000 spectrophotometer with automatic switching between graphite furnace and flame atomization and an autosampler. Spectroscopic parameters (wavelengths 213.9–324.8 nm, slit widths 0.2–0.7 nm) and temperature programs were optimized for each element to achieve LOQs down to low ppb levels.
Key Results and Discussion
Calibration curves for both modes showed correlation coefficients (r) above 0.999. Limit of quantitation, defined as 10σbL, was established via 10 replicates of blank medium. Electric thermal mode delivered ppt–ppb sensitivity with sample volumes of 5–50 µL, while flame mode covered ppb–ppm with 1–2 mL volumes. Measured concentrations varied among vendors, reflecting formulation differences. Spike recovery tests yielded 90–118 % across elements, indicating reliable quantitation with minimal matrix effects. Fe and Zn data from both modes were comparable, confirming method consistency.
Benefits and Practical Applications
- Simple sample preparation: dilution and minimal acid addition.
- Dual-mode analysis extends dynamic range from ppt to ppm.
- Cost-effective alternative to ICP-MS with lower running expenses.
- Rapid throughput: results in minutes per element per sample.
- High precision (RSD ≤3 %) and accuracy (recovery ~100 %).
Future Trends and Potential Applications
- Integration with LC/MS/MS-based profiling for comprehensive medium analysis.
- Automation of sample dilution and standard addition to mitigate matrix effects.
- Advances in high-throughput AAS to monitor additional trace metals.
- Application in real-time bioprocess monitoring and control strategies.
- Development of combined assays for simultaneous trace metal and metabolite quantification.
Conclusion
The study confirms atomic absorption spectrophotometry as a robust, accessible technique for quantifying trace metals in CHO cell culture media. Its simplicity, flexibility between atomization modes, and strong analytical performance make AAS a valuable tool for quality control in biopharmaceutical production.
Used Instrumentation
Shimadzu AA-7000 atomic absorption spectrophotometer with graphite furnace and flame atomizer, autosampler.
References
- Marreiro DD et al. Zinc and oxidative stress: current mechanisms. Antioxidants. 2017.
- Prabhu R et al. Zinc supplementation decreases galactosylation of recombinant IgG in CHO cells. Appl Microbiol Biotechnol. 2018.
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