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High-Sensitivity Analysis of a Steroid Panel Samples using Micro-Flow LC-MS/MS for Clinical Research

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LC/MS, LC/MS/MS, LC/QQQ
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Clinical Research
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Shimadzu

Summary

Importance of the Topic


The accurate measurement of steroid hormones in human serum is critical for clinical research, diagnostics, and environmental health studies. Low circulating levels in specific populations, such as pediatric or post-menopausal subjects, pose analytical challenges. Enhancing sensitivity and minimizing sample volume requirements supports broader applications in endocrinology, toxicology, and personalized medicine.

Study Objectives and Overview


This work aimed to develop and validate a high-sensitivity assay for simultaneous quantification of seventeen steroid compounds in serum. By integrating a micro-flow liquid chromatography–tandem mass spectrometry (micro-LC-MS/MS) platform with trap-and-elute configuration, the method sought to achieve lower limits of quantitation (LOQs) than conventional approaches, facilitating reliable detection at sub-picogram levels.

Methodology and Instrumentation


Sample Preparation:
  • Serum (300 µL) spiked with isotope-labeled internal standards.
  • Supported liquid-liquid extraction (SLE) using ethyl acetate/hexane.
  • Drying and reconstitution in methanol prior to analysis.

Instrumental Setup:
  • Shimadzu Nexera Mikros microflow LC with trap-and-elute modules.
  • Trapping column: CERI C8 (5 µm, 5×0.3 mm); analytical column: Shimadzu PLONAS Biphenyl (2.7 µm, 100×0.2 mm).
  • Triple-quadrupole MS (LCMS-8060) with micro-ESI source.
  • Mobile phases: water/methanol or acetonitrile/isopropanol gradients for trapping; water + 0.15 mM NH4F and methanol + 0.15 mM NH4F for analytical flow at 4 µL/min.

Main Results and Discussion


Calibration and Linearity:
  • Linear response across target ranges with 1/x² weighting and accurate internal standard correction.
  • Correlation coefficients consistently above 0.995.
Lower Limits of Quantitation:
  • LOQs ranged from 0.1 to 10 pg/mL, corresponding to as low as 6 fg on column for certain steroids.
  • Precision (%RSD < 15%) and accuracy (80–120%) met acceptance criteria at LOQ levels.
Chromatographic Performance:
  • Effective separation of isobaric steroids prevented cross-interference.
  • Rapid gradient enabled analysis cycle under 20 minutes.

Benefits and Practical Applications


The developed assay offers:
  • High sensitivity for low-abundance steroids in limited-volume clinical samples.
  • Robust quantitation suitable for biomarker discovery, hormonal profiling, and environmental exposure assessments.
  • Scalability for high-throughput laboratory workflows.

Future Trends and Opportunities


Advancements may include further miniaturization of flow systems, integration with automated sample preparation, and expansion of target panels to cover novel steroid metabolites. Coupling to high-resolution MS could enhance specificity, while multiplexing strategies may increase throughput for large-scale cohort studies.

Conclusion


A micro-flow LC-MS/MS method was successfully established for simultaneous quantification of seventeen serum steroids with exceptional sensitivity and reproducibility. This platform addresses key challenges in clinical and research settings by providing reliable detection at ultra-low concentrations.

Reference


N. Shirai et al., "High-Sensitivity Analysis of a Steroid Panel Samples using Micro-Flow LC-MS/MS for Clinical Research," Shimadzu Corp. Application Note WP219.

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