Determination of Microcystins and Nodularin in Drinking Water by UHPLC/MS/MS using a Luna® Omega 1.6 μm Polar C18 (EPA Method 544)
Applications | 2016 | PhenomenexInstrumentation
The growing occurrence of harmful cyanobacterial blooms in water sources poses serious health risks due to the production of potent hepatotoxins such as microcystins and nodularin. Monitoring these toxins at trace levels in drinking and irrigation water is critical to protect public health and ensure compliance with regulatory standards.
This application explores a robust UHPLC/MS/MS method based on EPA Method 544 for the simultaneous determination of nodularin and six microcystin congeners (MC-YR, MC-LR, MC-RR, MC-LA, MC-LY, MC-LW, MC-LF) in drinking water. The study aims to demonstrate high-resolution separations and sensitive quantitation across a wide polarity range using a single chromatographic run.
The separation employed a Luna Omega 1.6 µm Polar C18 column (100 × 2.1 mm) to achieve balanced polar and nonpolar interactions. The mobile phase consisted of water (A), methanol (B), and 1 mM ammonium fluoride (C) with a gradient from 80% A/10% B/10% C to 20% A/70% B/10% C over 13 minutes at 0.2 mL/min and 40 °C. Detection was performed on a Thermo Scientific Accela UHPLC coupled to a TSQ Quantum Ultra MS/MS in positive ESI and SRM mode, targeting the [M+H]+ precursors (except MC-YR and MC-RR detected as [M+2H]2+).
The optimized method achieved baseline separation of all analytes within 14 minutes. Retention times ranged from 8.47 to 13.13 minutes, and the SRM transitions provided high selectivity and signal-to-noise ratios, confirming the method’s sensitivity and reproducibility. The inclusion of MC-LW, although not listed in EPA Method 544, underscores the column’s broad applicability for additional congeners.
Advancements may include larger analyte libraries encompassing emerging microcystin variants, integration with high-throughput and automated workflows, improved ambient ionization techniques, and development of columns with tailored selectivity to further enhance sensitivity and reduce analysis time. Coupling with real-time monitoring systems may revolutionize early warning capabilities.
The presented UHPLC/MS/MS approach delivers a fast, sensitive, and comprehensive tool for monitoring microcystins and nodularin in drinking water, combining the balanced retention properties of Polar C18 phases with the selectivity of tandem mass spectrometry. This method supports regulatory compliance and public health protection.
Consumables, LC columns, LC/MS, LC/MS/MS, LC/QQQ
IndustriesEnvironmental
ManufacturerPhenomenex
Summary
Significance of the Topic
The growing occurrence of harmful cyanobacterial blooms in water sources poses serious health risks due to the production of potent hepatotoxins such as microcystins and nodularin. Monitoring these toxins at trace levels in drinking and irrigation water is critical to protect public health and ensure compliance with regulatory standards.
Objectives and Study Overview
This application explores a robust UHPLC/MS/MS method based on EPA Method 544 for the simultaneous determination of nodularin and six microcystin congeners (MC-YR, MC-LR, MC-RR, MC-LA, MC-LY, MC-LW, MC-LF) in drinking water. The study aims to demonstrate high-resolution separations and sensitive quantitation across a wide polarity range using a single chromatographic run.
Methodology and Instrumentation
The separation employed a Luna Omega 1.6 µm Polar C18 column (100 × 2.1 mm) to achieve balanced polar and nonpolar interactions. The mobile phase consisted of water (A), methanol (B), and 1 mM ammonium fluoride (C) with a gradient from 80% A/10% B/10% C to 20% A/70% B/10% C over 13 minutes at 0.2 mL/min and 40 °C. Detection was performed on a Thermo Scientific Accela UHPLC coupled to a TSQ Quantum Ultra MS/MS in positive ESI and SRM mode, targeting the [M+H]+ precursors (except MC-YR and MC-RR detected as [M+2H]2+).
Main Results and Discussion
The optimized method achieved baseline separation of all analytes within 14 minutes. Retention times ranged from 8.47 to 13.13 minutes, and the SRM transitions provided high selectivity and signal-to-noise ratios, confirming the method’s sensitivity and reproducibility. The inclusion of MC-LW, although not listed in EPA Method 544, underscores the column’s broad applicability for additional congeners.
Benefits and Practical Applications
- High efficiency and resolution for complex cyclic peptides
- Robust sensitivity for trace-level detection in drinking water matrices
- Compatibility with regulatory protocols (EPA Method 544)
- Potential for expanded panels including non-target congeners
Future Trends and Applications
Advancements may include larger analyte libraries encompassing emerging microcystin variants, integration with high-throughput and automated workflows, improved ambient ionization techniques, and development of columns with tailored selectivity to further enhance sensitivity and reduce analysis time. Coupling with real-time monitoring systems may revolutionize early warning capabilities.
Conclusion
The presented UHPLC/MS/MS approach delivers a fast, sensitive, and comprehensive tool for monitoring microcystins and nodularin in drinking water, combining the balanced retention properties of Polar C18 phases with the selectivity of tandem mass spectrometry. This method supports regulatory compliance and public health protection.
References
- Aqeel Z., Lomas S., Schiessel D. Determination of Microcystins and Nodularin in Drinking Water by UHPLC/MS/MS using a Luna® Omega 1.6 µm Polar C18 (EPA Method 544). Phenomenex Application Note TN41750416_W; 2016.
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