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Acarbose impurity analysis: method migration from UV detection to universal charged aerosol detection

Applications | 2023 | Thermo Fisher ScientificInstrumentation
HPLC
Industries
Pharma & Biopharma
Manufacturer
Thermo Fisher Scientific

Summary

Significance of the Topic


Acarbose is a widely used α-glucosidase inhibitor for type 2 diabetes that lacks strong chromophores, making impurity profiling by UV detection challenging. Comprehensive control of related substances is essential to ensure drug safety and comply with pharmacopoeial limits. Charged aerosol detection (CAD) offers a universal, MS-compatible alternative capable of detecting non-UV-active impurities and simplifying quantification without response factor corrections.

Objectives and Study Overview


The primary goal was to migrate the European Pharmacopoeia (Ph. Eur.) UV method for acarbose impurity analysis to a Thermo Scientific Vanquish UHPLC system coupled with CAD. Two chromatographic approaches were evaluated:
  • An amide-HILIC separation on Accucore 150 Amide HILIC column
  • A graphite separation on Hypercarb column

This comparison assessed method robustness, sensitivity, and compliance with Ph. Eur. monograph requirements for eight specified impurities (A–H).

Methodology and Instrumentation


All experiments used a Vanquish Flex UHPLC system with Charged Aerosol Detector H and nitrogen generator. Three methods were compared:
  • Ph. Eur. reference: Hypersil APS-2 column, phosphate buffer, UV detection at 210 nm
  • Amide-HILIC CAD: 100×2.1 mm, 2.6 µm column, 50 mM ammonium acetate (pH 5.8) with acetonitrile gradient, 45 °C
  • Hypercarb CAD: 150×4.6 mm, 3 µm column, 0.1% TFA in water and acetonitrile, 90 °C

Sample preparation followed Ph. Eur. monograph: test solution at 20 mg/mL and reference solutions spiked with certified impurity mix. Data were processed in Chromeleon CDS.

Main Results and Discussion


The Ph. Eur. UV method showed limited stability of APS-2 columns and required response factors for quantification. Switching to volatile buffer on APS-2 generated high CAD background and poor sensitivity. The amide-HILIC CAD method achieved baseline separation of impurities with a 0.20% LOQ, eliminating correction factors. The Hypercarb CAD method provided sharper peaks, lower LOQ (0.10%), and tolerated acidic conditions at high temperature to suppress epimerization. CAD also revealed additional low-level saccharide fragments (maltose, maltotriose) not detected by UV.

Benefits and Practical Applications


  • Universal detection of non-UV-active impurities without response factors
  • Improved column stability under MS-compatible volatile mobile phases
  • Enhanced sensitivity and selectivity for polar sugar derivatives
  • Potential to reveal unexpected impurities in production batches


Future Trends and Potential Applications


Further integration of CAD with mass spectrometry could provide confirmation of impurity identities. Exploration of alternative stationary phases and gradient strategies may lower LOQ and shorten runtimes. The CAD approach may be extended to other carbohydrate-based APIs and non-chromophoric drug substances in pharmaceutical quality control.

Conclusion


The migration from UV to CAD detection on a Vanquish UHPLC system successfully met Ph. Eur. requirements for acarbose impurity profiling. Both amide-HILIC and Hypercarb methods delivered stable separations, enhanced sensitivity, and universal quantification, offering robust solutions for routine quality control of non-UV-active analytes.

Reference


  1. European Pharmacopoeia 11.0, Monograph 2089.
  2. Leistner A, Holzgrabe U. J Pharm Biomed Anal. 2022;221:115063.
  3. Menz M et al. Thermo Fisher Sci Tech Note 72806; 2021.
  4. Porsch B, Kratka J. J Chromatogr A. 1991;543:1–7.
  5. Fu X et al. J Chromatogr A. 2020;1620:460981.

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