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Quantitative Analysis of Oxytocin in Rat Plasma Using LC/MS/MS

Applications | 2020 | ShimadzuInstrumentation
LC/MS, LC/MS/MS, LC/QQQ
Industries
Clinical Research
Manufacturer
Shimadzu

Summary

Significance of the Topic


Oxytocin is a nonapeptide hormone vital for uterine contraction during labor and increasingly studied for its role in social bonding and behavior. Accurate quantification in biological fluids is essential for pharmacokinetic profiling, neuroscience research, and validating therapeutic interventions.

Objectives and Study Overview


This study demonstrates a validated LC–MS/MS method using a Shimadzu LCMS-8050 triple quadrupole system to measure oxytocin levels in rat plasma. The work covers sample preparation, analytical conditions, calibration performance, and recovery evaluation.

Methodology and Instrumentation


Sample and Pretreatment:
  • Rat blood (SLC Wistar) collected with heparin anticoagulant and centrifuged to obtain plasma.
  • Protein precipitation by adding ten volumes of acetonitrile to plasma, followed by centrifugation.
  • Supernatant concentrated under reduced pressure and reconstituted in 30% methanol.

Chromatographic Conditions:
  • Column: Shim-pack GISS-HP (2.1 × 50 mm, 3 μm).
  • Mobile phase A: water; B: methanol; gradient: 30% B to 50% B over 5 min then return to 30% B.
  • Column temperature: 40 °C; flow rate: 0.3 mL/min; injection volume: 2 μL.

Mass Spectrometry Conditions:
  • Ionization: ESI in negative mode.
  • Detection mode: MRM transition 1005.4 → 939.4 m/z (CE +56 V).
  • Nebulizing gas: 2.0 L/min; drying gas: 15.0 L/min; heating gas: 5.0 L/min.
  • DL temperature: 150 °C; interface: 350 °C; block heater: 500 °C.

Instrumentation Used


  • UHPLC: Shimadzu Nexera X2 system.
  • Mass spectrometer: Shimadzu LCMS-8050 triple quadrupole.
  • Analytical column: Shim-pack GISS-HP (2.1 × 50 mm, 3 μm).

Main Results and Discussion


Calibration performance was linear over 0.1–500 ng/mL with r² ≥ 0.9996 and RSD ≤ 8.3% at the lowest level. The blank rat plasma contained approximately 0.23 ng/mL endogenous oxytocin. Spike-and-recovery at 2 ng/mL yielded a 91% recovery, demonstrating method accuracy. Typical MRM chromatograms displayed clear separation and peak shape at 10 ng/mL and 2 ng/mL levels.

Benefits and Practical Applications


This method offers high sensitivity and reproducibility for oxytocin quantification in preclinical studies. It supports pharmacokinetic analysis, behavioral research on social bonding, and quality control of peptide formulations in drug development settings.

Future Trends and Opportunities


Advancements may include automation of sample preparation, microflow LC–MS for reduced solvent consumption, and multiplexed assays combining oxytocin with related neuropeptides. Integration with high-resolution MS could expand specificity and enable metabolite profiling.

Conclusion


A robust LC–MS/MS protocol for oxytocin in rat plasma was established, featuring straightforward sample prep, excellent linearity, and reliable recovery. This approach facilitates quantitative studies in pharmacology and neuroscience.

References


No external literature references were cited in the source document.

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