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Carbohydrate analysis with HPAE-PAD

Guides | 2013 | Thermo Fisher ScientificInstrumentation
Ion chromatography, IC-MS
Industries
Food & Agriculture, Energy & Chemicals , Pharma & Biopharma, Clinical Research
Manufacturer
Thermo Fisher Scientific

Summary

Importance of the Topic


Carbohydrates are fundamental biomolecules involved in cellular signalling, immune response, and metabolic processes. Their high polarity, lack of UV–visible chromophores, and structural similarity present significant analytical challenges. High-Performance Anion-Exchange Chromatography with Pulsed Amperometric Detection (HPAE-PAD) addresses these difficulties by enabling direct, sensitive, and high-resolution analysis of underivatized sugars.

Objectives and Overview


This review outlines the principles and capabilities of HPAE-PAD for carbohydrate determination. It examines methodological features, instrumentation components, and practical applications across food and beverage analysis, biopharmaceutical glycoprotein profiling, biofuel feedstock monitoring, and pharmaceutical quality control.

Methodology and Instrumentation


HPAE-PAD separates carbohydrates at high pH on strong anion-exchange phases by exploiting their weak acid behavior. Detection uses pulsed amperometry on a gold electrode to oxidize analytes, offering sub-picomole sensitivity without derivatization. Key instrumentation includes:
  • Thermo Scientific Dionex ICS-5000+ and ICS-4000 systems featuring all-PEEK flowpaths and Reagent-Free™ IC for on-demand alkali generation
  • CarboPac PA20 and PA200 columns packed with pellicular MicroBead™ latex resin for superior resolution and rapid re-equilibration
  • Standard, microbore, and capillary formats reducing sample and eluent usage up to 100-fold
  • Electrochemical detector cells with disposable or conventional gold working electrodes and optional palladium hydrogen reference electrode

Main Results and Discussion


HPAE-PAD methods consistently achieve high resolution and sensitivity across a range of carbohydrate classes:
  • Monosaccharides and disaccharides separated in single isocratic runs with baseline resolution
  • Sialic acids and N-linked oligosaccharides profiled in glycoprotein digests, revealing structural details
  • Alcohols, sugar acids, phosphates, and nucleotides quantified in complex matrices
  • 3-D amperometry enabling post-run integration window adjustment to resolve co-eluting species
  • Coupling with mass spectrometry via electrolytic suppression for reliable identification in biofluids and fermentation broths

Benefits and Practical Applications


HPAE-PAD delivers significant advantages for routine and research laboratories:
  • Low detection limits (sub-picomole to femtomole) without chemical derivatization
  • Reduced analysis cost and waste through RFIC™ eluent generation and capillary formats
  • Automation options for sample cleanup and real-time process monitoring in biopharmaceutical and biofuel production
  • Compliance with pharmacopeial methods for antibiotic and impurity testing in pharmaceuticals
  • Enhanced throughput in food quality control, including infant formula, honey, coffee, and biofuel sugars

Future Trends and Potential Applications


Emerging directions include deeper integration with high-resolution mass spectrometry for structural elucidation, advanced waveform designs for improved selectivity, expanded automation for in-line monitoring, and portable HPAE-PAD platforms for field and point-of-care testing.

Conclusion


HPAE-PAD stands as a versatile, robust technique for comprehensive carbohydrate analysis. Its combination of high resolution, low detection limits, and flexible instrumentation meets the evolving needs of analytical chemistry in research, industry, and quality control.

Reference


No literature references were provided in the source document.

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