A CLINICAL RESEARCH LC-MS/MS METHOD FOR THE ANALYSIS OF ANTIDEPRESSANTS IN PLASMA
Posters | 2023 | WatersInstrumentation
Effective monitoring of antidepressants in plasma is critical for pharmacokinetic research, therapeutic drug monitoring, and understanding drug interactions. A robust method that supports multiple analytes with high sensitivity accelerates clinical studies and improves treatment optimization.
This study describes the development and validation of a liquid chromatography–tandem mass spectrometry (LC-MS/MS) assay capable of quantifying ten commonly prescribed antidepressants in human plasma. The goal was to achieve rapid analysis, minimal sample volume, and reliable performance across a wide concentration range.
Sample preparation relies on protein precipitation:
Chromatographic separation and detection:
Method validation demonstrated:
The method’s advantages include:
Potential developments may include:
This LC-MS/MS approach offers a reliable, efficient solution for simultaneous antidepressant quantification in plasma, supporting clinical research and therapeutic monitoring with high precision and throughput.
LC/MS, LC/MS/MS, LC/QQQ
IndustriesClinical Research
ManufacturerWaters
Summary
Significance of the Topic
Effective monitoring of antidepressants in plasma is critical for pharmacokinetic research, therapeutic drug monitoring, and understanding drug interactions. A robust method that supports multiple analytes with high sensitivity accelerates clinical studies and improves treatment optimization.
Objectives and Study Overview
This study describes the development and validation of a liquid chromatography–tandem mass spectrometry (LC-MS/MS) assay capable of quantifying ten commonly prescribed antidepressants in human plasma. The goal was to achieve rapid analysis, minimal sample volume, and reliable performance across a wide concentration range.
Methodology and Instrumentation
Sample preparation relies on protein precipitation:
- Fifty microliters of plasma mixed with 150 µL internal standard in acetonitrile.
- Vortex agitation followed by centrifugation and dilution of the supernatant.
Chromatographic separation and detection:
- UPLC system with an XSelect Premier HSS T3 column (2.1×100 mm, 2.5 µm).
- Gradient elution using water, acetonitrile, and ammonium acetate.
- Xevo TQD mass spectrometer in positive electrospray ionization with multiple reaction monitoring.
- Five-minute run time per injection.
Main Results and Discussion
Method validation demonstrated:
- Linearity or quadratic calibration over concentration ranges (e.g., 7.7–1300 ng/mL for several analytes).
- Low-level sensitivity with precision ≤20% CV and bias ≤15% at the lower limit, except minor deviation for fluvoxamine.
- Precision better than 10% CV across low, mid, and high pools.
- Negligible matrix effects (normalized matrix factors 0.90–1.07) with internal standard compensation.
- No carryover or significant interference from common endogenous substances.
Benefits and Practical Applications
The method’s advantages include:
- Minimal sample volume requirement (50 µL).
- Fast and simple sample preparation.
- Short analysis time suitable for high-throughput studies.
- Simultaneous quantification of a comprehensive panel of antidepressants.
Future Trends and Applications
Potential developments may include:
- Integration with automated workflows for greater throughput.
- Expansion to additional analytes or metabolites.
- Application to other biological matrices, such as cerebrospinal fluid or dried blood spots.
- Adoption of high-resolution mass spectrometry for broader screening.
Conclusion
This LC-MS/MS approach offers a reliable, efficient solution for simultaneous antidepressant quantification in plasma, supporting clinical research and therapeutic monitoring with high precision and throughput.
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