High Speed Analysis of α-Acids and β-Acids in Hops
Applications | 2021 | ShimadzuInstrumentation
The rapid and reliable determination of α-acids, β-acids and iso-α-acids in hops is critical for beer quality control, flavor consistency and emerging health applications. Traditional HPLC analyses require ca. 30 minutes per run. A five-minute high-speed method enhances sample throughput, reduces solvent costs and supports timely decision-making in breweries and analytical laboratories.
The study aimed to develop and validate a high-speed HPLC method for simultaneous quantitation of α-acids, β-acids and iso-α-acids in hop pellets. Key goals included:
The described five-minute HPLC method using a Shim-pack Velox C18 core-shell column on a Nexera XR system provides accurate, reproducible and high-throughput analysis of α-acids, β-acids and iso-α-acids in hops. It offers significant improvements over conventional protocols and is readily adaptable for routine brewery quality control and research purposes.
HPLC
IndustriesFood & Agriculture
ManufacturerShimadzu
Summary
Significance of the topic
The rapid and reliable determination of α-acids, β-acids and iso-α-acids in hops is critical for beer quality control, flavor consistency and emerging health applications. Traditional HPLC analyses require ca. 30 minutes per run. A five-minute high-speed method enhances sample throughput, reduces solvent costs and supports timely decision-making in breweries and analytical laboratories.
Objectives and overview
The study aimed to develop and validate a high-speed HPLC method for simultaneous quantitation of α-acids, β-acids and iso-α-acids in hop pellets. Key goals included:
- Reducing analysis time to approximately five minutes per injection.
- Maintaining low system backpressure despite using methanol.
- Achieving accurate quantitation and high recovery rates for different hop varieties.
Methodology and instrumentation
- Instrument: Shimadzu Nexera XR UHPLC system.
- Column: Shim-pack Velox C18 core-shell (50 × 3.0 mm I.D., 1.8 µm).
- Mobile phases: A – 10 mmol/L sodium phosphate buffer (pH 2.6) with 0.2 mmol/L EDTA; B – methanol.
- Gradient: B conc. 80% at 0 min to 90% at 3 min, return to 80% by 5 min.
- Flow rate: 0.7 mL/min, column temperature 40 °C, injection volume 2 µL.
- Detection: UV at 314 nm (α- and β-acids); UV at 270 nm added for iso-α-acids.
- Sample preparation: 10 g hop pellets ground, extracted with methanol/diethyl ether in acidified conditions, phase separation, filtration through 0.22 µm.
- Standards: International Calibration Extract 4 dissolved in methanol; grouped into α- and β-acid homologues.
Main results and discussion
- Chromatographic separation achieved within five minutes with clear grouping of α-acids and β-acids peaks and baseline resolution.
- Maximum system backpressure ≈ 26 MPa, demonstrating the column’s ability to handle methanol without excessive pressure.
- Quantitation of two hop pellet samples (Hop A and Hop B) showed α-acid concentrations of 5.1% and 9.5%, β-acid concentrations of 14.3% and 24.0%, with recovery rates of 98–102% for α-acids and 90–97% for β-acids. Relative standard deviations were ≤ 2.4%.
- Simultaneous iso-α-acid analysis by spiking Hop A extract with 200 mg/L yielded a 99.7% recovery, validating the extended detection method at 270 nm and gradient adjustment to 60–100% B.
Benefits and practical applications
- High throughput through five-minute runs supports large-scale screening in brewing QA/QC.
- Core-shell column enables low backpressure and sustained column life even with high organic solvent content.
- Simultaneous multi-component analysis streamlines workflow and reduces instrument downtime.
- Robust quantitation and recovery make the method suitable for routine quality control of hops and hop extracts.
Future trends and potential applications
- Integration with mass spectrometry for enhanced specificity and trace-level detection of hop-derived compounds.
- Adoption of green solvents or aqueous-rich mobile phases to reduce environmental footprint.
- Development of on-line sample preparation or automated extraction modules to further accelerate analysis.
- Application to novel hop varieties and bioactive components for functional food and nutraceutical research.
Conclusion
The described five-minute HPLC method using a Shim-pack Velox C18 core-shell column on a Nexera XR system provides accurate, reproducible and high-throughput analysis of α-acids, β-acids and iso-α-acids in hops. It offers significant improvements over conventional protocols and is readily adaptable for routine brewery quality control and research purposes.
References
- American Society of Brewing Chemists. ASBC Methods of Analysis, Hops-14.
- European Brewery Convention. EBC Analytica, Method 7.7.
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