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Published:
Journal of Analytical Toxicology,
ISSN 0146-4760,
Volume 24,
Number 7, October,
pp. 543-549
Here is where the title stuff goes
Liquid
Chromatography–Electrospray Ionization Mass Spectrometry for the Detection
of Lysergide and a Major Metabolite, 2-Oxo-3-Hydroxy-LSD, in Urine and Blood
Jason H.
Sklerov, Joseph Magluilo, Jr., Karoline K. Shannon, and Michael L. Smith
Office of the Armed Forces Medical Examiner, Division of Forensic Toxicology,
Armed Forces Institute of Pathology, 1413 Research Boulevard, Building 102,
Rockville, Maryland 20850-3125
A method is
presented for the quantitative measurement of lysergide (LSD) and its metabolite
2-oxo-3-hydroxy-LSD (O-H-LSD) in urine and blood. O-H-LSD has been reported
to have urinary concentrations many times higher than LSD. Measuring its presence
in urine would significantly extend the detection time for confirming LSD abuse.
A single-step liquid–liquid extraction was performed on 5-mL urine samples
prior to separation by gradient liquid chromatography (LC). Electrospray ionization
was used to produce the positively charged ions of O-H-LSD, 2-oxo-3-hydroxy-LAMPA
(O-H-LAMPA, internal standard), LSD, and iso-LSD. Varying the orifice voltage
in the intermediate-pressure region of the source generated the fragmentation
necessary to produce qualifying ions. Selected ion monitoring allowed detection
limits of 400 pg/mL and 100 pg/mL for O-H-LSD and LSD, respectively. The method
was linear for O-H-LSD from 400 to 8000 pg/mL and for LSD from 100 to 6000 pg/mL.
LSD-positive samples (n = 9) analyzed by the liquid chromatography–mass
spectrometry method were found to contain mean concentrations of 6378 pg/mL
O-H-LSD (332–21371 pg/mL) and 844 pg/mL LSD (177–2456 pg/mL). O-H-LSD
urinary concentrations were between 0.9 and 19.8 times higher than LSD (mean
= 10.2). Whole-blood samples were also analyzed following additional sample
cleanup. LSD was measured in the blood samples, but no O-H-LSD was detected.
Enzymatic hydrolysis was carried out on LSD-positive samples (n = 6) to evaluate
the existence of conjugated O-H-LSD. b-Glucuronidase from Helix pomatia was
incubated with urine samples at 37°C, pH 5.2 for 24 h. At an enzymatic activity
of approximately 4000 units per milliliter of urine, no significant (p = 0.05)
difference was seen between hydrolyzed and nonhydrolyzed samples suggesting
an absence of O-H-LSD-glucuronic acid conjugation.
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