UPLC-MS/MS Method for the Routine Analysis of Tobacco Specific Nitrosamines (TSNAs) in Tobacco Products Using RADAR Technology
Applications | 2016 | WatersInstrumentation
Tobacco specific nitrosamines TSNAs are recognized carcinogens present in tobacco and tobacco smoke. Monitoring their levels in diverse tobacco products is essential to comply with regulatory standards and to assess health risks associated with consumption. The complexity of tobacco matrices and high levels of nicotine and alkaloids create challenges for selective detection and accurate quantification of TSNAs.
The primary goal of the study was to establish a robust and high throughput UPLC MS MS method for routine determination of four priority TSNAs in various tobacco products such as snus moist snuff dry snuff and chewing tobacco. The research leveraged the RADAR acquisition mode on a tandem quadrupole mass spectrometer to simultaneously collect MRM and full scan data facilitating method optimization and matrix interference assessment.
A solid sample preparation involving cleanup steps and dilution was employed to reduce matrix effects. Chromatographic separation used a water mobile phase with 10 mM ammonium acetate and two organic modifiers in methanol a neutral buffer and 0.1 percent acetic acid. RADAR mode enabled real time evaluation of full scan MS to detect coeluting interferences while MRM transitions provided quantitative data.
Comparison of two organic phase modifiers showed that using 0.1 percent acetic acid improved separation between nicotine and the TSNA NNN peak eliminating coelution observed with the neutral buffer. Quantitative recovery testing at 50 ng per gram for NNN NNK NAT and 12.5 ng per gram for NAB demonstrated that acidified mobile phase delivered recovery rates within 106 to 112 percent and relative standard deviations below 3 percent across all tobacco matrices. The RADAR full scan data allowed identification of potential interferences leading to a more rugged analytical procedure.
The integration of full scan and targeted MRM workflows paves the way for broader screening capabilities enabling untargeted compound discovery alongside routine measurements. Coupling RADAR mode with advanced data processing and machine learning could further enhance matrix deconvolution and automating method optimization for diverse sample types.
The presented UPLC MS MS method using RADAR acquisition delivers a fast accurate and robust solution for TSNA analysis in tobacco products. The dual data acquisition approach accelerates method refinement and improves confidence in quantitative results by actively monitoring matrix interferences. This strategy supports regulatory testing and research applications requiring reliable carcinogen measurements.
LC/MS, LC/MS/MS, LC/QQQ
IndustriesFood & Agriculture
ManufacturerWaters
Summary
Significance of the Topic
Tobacco specific nitrosamines TSNAs are recognized carcinogens present in tobacco and tobacco smoke. Monitoring their levels in diverse tobacco products is essential to comply with regulatory standards and to assess health risks associated with consumption. The complexity of tobacco matrices and high levels of nicotine and alkaloids create challenges for selective detection and accurate quantification of TSNAs.
Objectives and Study Overview
The primary goal of the study was to establish a robust and high throughput UPLC MS MS method for routine determination of four priority TSNAs in various tobacco products such as snus moist snuff dry snuff and chewing tobacco. The research leveraged the RADAR acquisition mode on a tandem quadrupole mass spectrometer to simultaneously collect MRM and full scan data facilitating method optimization and matrix interference assessment.
Methodology and Instrumentation
A solid sample preparation involving cleanup steps and dilution was employed to reduce matrix effects. Chromatographic separation used a water mobile phase with 10 mM ammonium acetate and two organic modifiers in methanol a neutral buffer and 0.1 percent acetic acid. RADAR mode enabled real time evaluation of full scan MS to detect coeluting interferences while MRM transitions provided quantitative data.
Instrumentation Used
- Xevo TQD triple quadrupole mass spectrometer equipped with RADAR acquisition
- UPLC system with reversed phase column and controlled gradient delivery
Main Results and Discussion
Comparison of two organic phase modifiers showed that using 0.1 percent acetic acid improved separation between nicotine and the TSNA NNN peak eliminating coelution observed with the neutral buffer. Quantitative recovery testing at 50 ng per gram for NNN NNK NAT and 12.5 ng per gram for NAB demonstrated that acidified mobile phase delivered recovery rates within 106 to 112 percent and relative standard deviations below 3 percent across all tobacco matrices. The RADAR full scan data allowed identification of potential interferences leading to a more rugged analytical procedure.
Benefits and Practical Applications
- Rapid method development through simultaneous qualitative and quantitative data acquisition
- Enhanced matrix effect control by real time monitoring of interferences
- Improved accuracy and precision in TSNA quantification across complex tobacco matrices
- High throughput analysis suitable for routine quality control and regulatory compliance
Future Trends and Opportunities
The integration of full scan and targeted MRM workflows paves the way for broader screening capabilities enabling untargeted compound discovery alongside routine measurements. Coupling RADAR mode with advanced data processing and machine learning could further enhance matrix deconvolution and automating method optimization for diverse sample types.
Conclusion
The presented UPLC MS MS method using RADAR acquisition delivers a fast accurate and robust solution for TSNA analysis in tobacco products. The dual data acquisition approach accelerates method refinement and improves confidence in quantitative results by actively monitoring matrix interferences. This strategy supports regulatory testing and research applications requiring reliable carcinogen measurements.
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