External Contamination of Hair with Cocaine: Evaluation of External Cocaine Contamination and Development of Performance-Testing Materials

Stout, Peter; Ropero‐Miller, Jeri D.; Baylor, Michael; Mitchell, John M.

doi:10.1093/jat/30.8.490

Cited by 78 publications

(57 citation statements)

References 24 publications

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“…All of the hair types observed in this study were also used in a model drug contamination study in which hair samples were externally contaminated with cocaine, subjected to model hygienic treatment and then subjected to laboratory decontamination procedures including an aqueous buffer decontamination and a methanolic decontamination [17]. Hair samples subjected to aqueous phosphate buffer decontamination had lower concentrations of cocaine remaining than those hair samples subjected to methanolic decontamination protocols.…”

Section: Resultsmentioning

confidence: 99%

Morphological changes in human head hair subjected to various drug testing decontamination strategies

Stout

Ropero-Miller

Baylor

et al. 2007

Forensic Science International

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Section: Resultsmentioning

confidence: 99%

Morphological changes in human head hair subjected to various drug testing decontamination strategies

Stout

Ropero-Miller

Baylor

et al. 2007

Forensic Science International

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“…The participating laboratories employed different wash procedures, some extensive, but they failed to decontaminate the hair. 64 Standardized decontamination wash procedures that will effectively remove any trace of external contamination without actively removing the drugs incorporated into the hair are not currently available and, as such, the possible role of external contamination must be considered when interpreting hair testing findings.…”

Section: Washingmentioning

confidence: 99%

“…The majority of published hair testing methods are for drugs of abuse, including opiates, 42,60,69 cocaine, 64,87,98 amphetamines 66,67,75,84 and cannabinoids, 58,85,86,99 employing GC-MS or LC-MS-MS. Although new methods have been reported using specialist analytical instrumentation including quadruple time-of-flight and matrix-assisted laser desorption/ionization time of flight, 97,100 standard instrumentation and method parameters (temperature programme, ions selected for monitoring, collision energies, etc.)…”

Section: Confirmation Techniquesmentioning

confidence: 99%

Hair testing is taking root

Cooper

2011

Ann Clin Biochem

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An increasing number of toxicology laboratories are choosing to expand the services they offer to include hair testing in response to customer demands. Hair provides the toxicologist with many advantages over conventional matrices in that it is easy to collect, is a robust and stable matrix that does not require refrigeration, and most importantly, provides a historical profile of an individual's exposure to drugs or analytes of interest. The establishment of hair as a complementary technique in forensic toxicology is a direct result of the success of the matrix in medicolegal cases and the wide range of applications. However, before introducing hair testing, laboratories must consider what additional requirements they will need that extend beyond simply adapting methodologies already validated for blood or urine. Hair presents many challenges with respect to the lack of available quality control materials, extensive sample handling protocols and low drug concentrations requiring greater instrument sensitivity. Unfortunately, a common pitfall involves over-interpretation of the findings and must be avoided.

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“…Approaches for preventing evidentiary false-positives due to external contamination of the hair specimens have been described since 1992 [2]. These criteria do not endorse a general acceptance [3,4]. Excluding laboratory mistakes, a false positive post mortem hair result can be observed in case of contamination from environmental pollution (external contamination) or after drug incorporation into the hair from the individual body fluids, such as sweat or putrefactive fluid (post mortem artefact).…”

Section: Introductionmentioning

confidence: 99%

“…As it can be observed from the scientific literature [2][3][4][5][6][7][8], several approaches have been proposed to get round the contamination scenario. All are dealing with living subjects and none have been developed for post mortem specimens, collected under very bad conditions.…”

Section: Introductionmentioning

confidence: 99%

External post mortem artefact: a key issue in hair result interpretation

Kintz¹,

Villain²,

Cirimele³

2008

Ann Toxicol Anal

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-Purpose: Excluding laboratory mistakes, a false positive hair result can be observed in case of contamination from environmental pollution (external contamination) or after drug incorporation into the hair from the individual body fluids, such as sweat or putrefactive fluid (post mortem artefact). From our 18 years experience of hair testing, it appears that artefact(s) cannot be excluded in some post mortem cases, despite a decontamination procedure. As a consequence, interpretation of the results is a challenge that deserves particular attention. Our strategy will be reviewed in this paper. Methods: Three authentic cases are presented to document our hypothesis. Results: Case 1: a 24-year old man was found dead in a friend's house. He was not known as a drug addict. The analysis of femoral blood was interpreted as ecstasy poisoning (MDMA = 770 ng/mL, MDA = 56 ng/mL). Segmental hair analysis (GC/MS) was as follows: MDMA = 0.94, 0.87 and 0.90 ng/mg in the 0-3, 3-6 and 6-9 cm, respectively. No MDA was detected. Case 2: at the time of death, cyamemazine, which was never prescribed to the subject, was detected in femoral blood at 3660 ng/mL. The body was exhumed 18 months after burial. Segmental hair cyamemazine analysis (LC/MS-MS) was as follows: 3.1 ng/mg (0-2 cm), 2.9 ng/mg (2-4 cm) and 3.1 ng/mg (4-6 cm). Case 3: the skeleton of a young girl was found in a water well 20 years after her disappearance. 7-amino-flunitrazepam was detected in her cerebral material at 0.67 ng/g. Some hair fibers, attached to the skull were collected. Segmental hair 7-aminoflunitrazepam analysis (LC/MS-MS) was as follows: 15 pg/mg (0-2 cm) and 19 pg/mg (2-4 cm). In all cases, a decontamination procedure with 2 washes of 5 mL of dichloromethane for 5 min was achieved and the last dichloromethane bath was negative for each target drug. From the histories, there was no suspicion of chronic drug use. In all cases, the concentrations detected were homogenous, irrespective of the tested segment. This can be considered as good indicative of potential external contamination. In contrast to smoke, it seems that contamination due to aqueous matrices (sweat, putrefactive fluid, blood) is much more difficult to remove. To explain potential incorporation of 7-aminoflunitrazepam via putrefactive material, the authors incubated negative hair strands in blood spiked at 100 ng/mL and stored at +4 • C, room temperature and +40 • C for 7, 14 and 28 days. After routine decontamination, 7-aminoflunitrazepam tested positive in hair, irrespective of the incubation temperature, as early as after 7 days (233-401 pg/mg). In all periods, maximum concentrations were observed after incubation at room temperature. The highest concentration (742 pg/mg) was observed after 28 days incubation at room temperature. Conclusion: It is concluded that a standard decontamination procedure is not able to completely remove external contamination in case of post mortem specimens. Homogenous segmental analyses can be probably indicative of external contamination and th...

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External Contamination of Hair with Cocaine: Evaluation of External Cocaine Contamination and Development of Performance-Testing Materials

Cited by 78 publications

References 24 publications

Morphological changes in human head hair subjected to various drug testing decontamination strategies

Morphological changes in human head hair subjected to various drug testing decontamination strategies

Hair testing is taking root

External post mortem artefact: a key issue in hair result interpretation

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