Improved Screening for 250 Pesticides in Matrix using a LC-Triple Quadrupole Mass Spectrometer
Applications | 2016 | Thermo Fisher ScientificInstrumentation
Food safety and environmental regulations demand comprehensive monitoring of pesticide residues at trace levels in diverse matrices. Fast and reliable multi-residue screening is essential to protect public health and ensure compliance with regulatory limits.
This study aims to demonstrate the impact of an active collision cell drag field in Q2 on signal intensity at very short dwell times. By applying a drag field, the method seeks to achieve data acquisition rates up to 500 SRM per second to simultaneously screen 250 pesticides in an onion matrix.
The workflow involved liquid chromatography separation followed by selected reaction monitoring on a triple quadrupole mass spectrometer. Key parameters:
The analysis was conducted on a Thermo Scientific TSQ Quantiva triple quadrupole mass spectrometer equipped with an Ion Max NG source and a Thermo Scientific Dionex UltiMate 3000 XRS LC system.
Implementation of the Q2 drag field maintained signal intensity and reproducibility even at 1 millisecond dwell time, yielding less than 3.2 percent RSD for azoxystrobin. The active collision cell enabled data acquisition of more than 500 SRMs per second without signal loss. Screening of 250 pesticides in an onion matrix at 1 to 100 ppb demonstrated robust performance, with exemplary precision (R^2 > 0.997) for fenamiphos and flonicamid calibration curves. The Ion Max NG source further reduced background interference and improved sensitivity in complex matrices.
Further enhancements may include integration with ultra high performance liquid chromatography, expansion to other challenging matrices, coupling with high resolution mass spectrometry for non-targeted analysis, and implementation in automated, high-throughput laboratory workflows.
The use of a drag field in the Q2 collision cell of a triple quadrupole mass spectrometer enables 1 millisecond dwell times at 500 SRM per second, facilitating rapid and comprehensive screening of 250 pesticides in complex matrices with high sensitivity, precision, and robustness.
LC/MS, LC/MS/MS, LC/QQQ
IndustriesEnvironmental, Food & Agriculture
ManufacturerThermo Fisher Scientific
Summary
Significance of the Topic
Food safety and environmental regulations demand comprehensive monitoring of pesticide residues at trace levels in diverse matrices. Fast and reliable multi-residue screening is essential to protect public health and ensure compliance with regulatory limits.
Objectives and Study Overview
This study aims to demonstrate the impact of an active collision cell drag field in Q2 on signal intensity at very short dwell times. By applying a drag field, the method seeks to achieve data acquisition rates up to 500 SRM per second to simultaneously screen 250 pesticides in an onion matrix.
Methodology
The workflow involved liquid chromatography separation followed by selected reaction monitoring on a triple quadrupole mass spectrometer. Key parameters:
- Chromatography: Dionex UltiMate 3000 XRS LC system with Hypersil Gold aQ column (100 x 2.1 mm, 1.9 μm)
- Gradient elution from 2 to 100 percent methanol with 0.1 percent formic acid and 5 mM ammonium formate
- Flow rate 300 μL per minute
- MS mode: SRM with heated electrospray ionization at 425 °C vaporizer and 350 °C capillary temperatures
- Sheath gas 45 and auxiliary gas 10 (arbitrary units), 3000 V positive ion mode
- Collision gas pressure 1.5 mTorr
- Dwell times evaluated at 100, 20, 5, 2 and 1 millisecond with a 1 millisecond interscan delay
Instrumentation Used
The analysis was conducted on a Thermo Scientific TSQ Quantiva triple quadrupole mass spectrometer equipped with an Ion Max NG source and a Thermo Scientific Dionex UltiMate 3000 XRS LC system.
Main Results and Discussion
Implementation of the Q2 drag field maintained signal intensity and reproducibility even at 1 millisecond dwell time, yielding less than 3.2 percent RSD for azoxystrobin. The active collision cell enabled data acquisition of more than 500 SRMs per second without signal loss. Screening of 250 pesticides in an onion matrix at 1 to 100 ppb demonstrated robust performance, with exemplary precision (R^2 > 0.997) for fenamiphos and flonicamid calibration curves. The Ion Max NG source further reduced background interference and improved sensitivity in complex matrices.
Benefits and Practical Applications
- Shortens HPLC run times and enables adoption of UHPLC workflows
- Simultaneous monitoring of hundreds of analytes without individual time windows
- Simplifies method development and reduces risk of retention time shifts
- Delivers high-throughput, reliable multi-residue screening in food safety and environmental analysis
Future Trends and Potential Applications
Further enhancements may include integration with ultra high performance liquid chromatography, expansion to other challenging matrices, coupling with high resolution mass spectrometry for non-targeted analysis, and implementation in automated, high-throughput laboratory workflows.
Conclusion
The use of a drag field in the Q2 collision cell of a triple quadrupole mass spectrometer enables 1 millisecond dwell times at 500 SRM per second, facilitating rapid and comprehensive screening of 250 pesticides in complex matrices with high sensitivity, precision, and robustness.
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