In vitro production of GHB in blood and serum samples under various storage conditions

Zörntlein, S. W.; Kopp, A.; Becker, Julie; Kaufmann, T. J.; Röhrich, J.; Urban, R.

doi:10.1016/j.forsciint.2011.07.030

SAFETYLIT WEEKLY UPDATE

We compile citations and summaries of about 400 new articles every week.

RSS Feed

HELP: Tutorials | FAQ

CONTACT US: Contact info

Search Results

Journal Article

In vitro production of GHB in blood and serum samples under various storage conditions
Citation	Zörntlein SW, Kopp A, Becker J, Kaufmann TJ, Röhrich J, Urban R. Forensic Sci. Int. 2012; 214(1-3): 113-117.
Affiliation	Institute of Legal Medicine, Johannes Gutenberg-University of Mainz, Am Pulverturm 3, D-55131 Mainz, Germany.
Copyright	(Copyright © 2012, Elsevier Publishing)
DOI	10.1016/j.forsciint.2011.07.030
PMID	21880442
Abstract	The in vitro production of GHB was observed in freshly collected, untreated whole blood samples using glass BD-Vacutainers and polypropylene S-monovettes. GHB concentrations were determined daily over a period of one week and after 3, 6 and 9 weeks again. Furthermore, the GHB concentration in 40 untreated random whole blood samples stored at 4°C for a longer period of time (10 samples 12 month, 10 samples 24 month and 20 samples 36 month) was also determined. For comparison, the in vitro production of GHB in freshly collected and prepared serum samples was observed. GHB serum concentrations were determined three times over a period of one week and once again after six weeks. Sample preparation was performed by means of methanolic extraction following the precipitation of whole blood and serum samples. A methanolic standard calibration was done in a low range of 0.005-0.1μg/mL (LOD: 0.004, LLOQ: 0.013). For quantification a spiked blood bank serum with a determined GHB concentration of 0.09μg/mL was used. Corrected calibrations in the range of 0.09-5.09μg/mL were used (LOD: 0.08μg/mL, LLOQ: 0.30μg/mL), recovery: 91.3% (high level: 4.09μg/mL) 50.5% (low level: 0.19μg/mL). RESULTS: Relevant elevation of GHB was observed in all whole blood samples stored in liquid form (4°C or room temperature). In two of the 40 whole blood samples stored over a longer period of time at 4°C, GHB concentrations in the range of 13μg/mL were even determined. These findings constitute grounds for caution. Even a GHB cut-off level of 5μg/mL cannot be considered as "absolutely positive" proof of a case of exogenous administration, at least in untreated liquid blood samples in long time storage. However, no significant elevations of GHB were otherwise observed in any of the serum samples independently of storage temperature nor in the whole blood samples that were frozen for storage. CONCLUSIONS: The results suggest that the cut-off for exogenous GHB of 5μg/mL could be lowered significantly, with the consequence of winning valuable time for the potential victim, but only if serum is collected for GHB determination or if the whole blood sample is frozen immediately after collection and the procedure well documented. Language: en