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Published:
Journal of Analytical Toxicology,
ISSN 0146-4760,
Volume 25, Number 5, July/August, pp. 316-322
Investigation Into Some Aspects of EMIT d.a.u., TLC, and
GCMS Urinalysis of Bromazepam
B.M.
El-Haj, A.M. Al-Amri, M.H. Hassan, and R.K. Bin-Khadem
Sharjah Police Forensic Science Laboratory, Emirate of Sharjah, United
Arab Emirates
Among the different
1,4-benzodiazepine urinary metabolites, those of bromazepam possess distinctive
chemical features that may be used in their selective isolation and detection.
The detection of bromazepam metabolites in urine was carried out using EMIT
d.a.u., thin-layer chromatography (TLC), and gas chromatographymass spectrometry
(GCMS). The positive EMIT d.a.u. benzodiazepine assay for bromazepam was
found to be due to the 3-hydroxybromazepam (3HOB) metabolite. The detection
by TLC and GCMS was carried out after enzyme or acid hydrolysis of the
glucuronide conjugates. Both the 2-amino-3-hydroxy- 5-bromobenzoylpyridine (AHBBP)
metabolite and the acid hydrolysis product of 3-HOB, 2-amino-5-bromobenzoylpyridine
(ABBP), were selectively detected by TLC. The bromazepam metabolites in urine
could be both isolated and detected selectively by GCMS in the presence
of the metabolites of other 1,4-benzodiazepines that were sometimes used in
combination with bromazepam. Both 3-HOB and AHBBP were detected by GCMS
only after trimethylsilyl (TMS) derivatization and not as the free compounds
or the acetyl derivatives. Only ABBP was detected in three forms: ABBP, the
TMS derivative, and the acetyl derivative. Evidence has been obtained from the
enzyme hydrolysis and the TLC studies for the formation of the glucuronide conjugate
of AHBBP at the 3-OH group rather than at the 2-NH2 group. All the results have
been validated using reference 3-HOB and AHBBP.
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