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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
11

Evaluation and comparison of various sample preparation techniques for the analysis and quantitation of THC, synthetic cannabinoids, and metabolites by LC-MS/MS in human whole blood and urine

Boyle, Sarah 09 October 2019 (has links)
A cannabinoid refers to any natural or synthetic compound that interacts with the CB1 and CB2 receptors. There are currently three different groups of cannabinoids: endogenous cannabinoids, phytocannabinoids and synthetic cannabinoids. The most common phytocannabinoid is delta-9-tetrahydrocannabinol (THC), which is the active component in the Cannabis sativa or marihuana plant1–3. Two examples of synthetic cannabinoids that are present in case reports from 2012 to 2018 are AB-FUBINACA and AB-PINACA4–7. THC and synthetic cannabinoids are commonly encountered drugs in forensic toxicology cases, therefore, being able to extract these compounds and their metabolites is imperative for toxicological interpretation. There are a variety of commercially available sample preparation techniques for these analytes. Companies such as UCT, Biotage, Millipore-Sigma, Tecan, and Thermo Fisher Scientific manufacture these products. The focus of this research was to evaluate these techniques for their cleanliness, efficiency and cost effectiveness. Sample preparation techniques are designed to remove the different components of the matrix and other prescription or illicit substances present in the sample that could interfere with the assay, increase the analyte recovery, extraction efficiency, decrease variability, and clean-up the sample to allow for less instrument downtime and longer column life8. This study focused on comparing a liquid-liquid extraction (LLE), solid phase extraction (SPE), and supported liquid extraction (SLE). The primary purpose of this study was to develop and validate the three above mentioned sample preparation techniques for the analysis of THC, 11-hydroxy-THC, 11-nor-9-carboxy-THC (THCCOOH), AB-FUBINACA, AB-FUBINACA metabolite 3, and AB-PINACA in blood and urine. Parameters assessed followed Academy Standards Board (ASB) Standard 036, Standard Practices for Method Validation in Forensic Toxicology, including recovery, suppression, and matrix effects. For urine and blood analysis, the calibration range was determined to be 1 ng/mL to 50 ng/mL for all three techniques. Urine recovery was highest for the LLE method, with all compounds having a recovery greater than 50%. The SLE method had the lowest LOQ results for urine, with 0.5 ng/mL for 11-hydroxy-THC and THCCOOH, 0.75 ng/mL for THC, AB-FUBINCA and AB-FUBINACA metabolite 3, and 1 ng/mL for AB-PINACA. Ion suppression was reduced using the SLE method for urine along with having the shortest sample preparation time of 1 hr for up to 48 samples. For blood analysis, the LLE method had the greatest recovery of all analytes. The LLE method also had reduced suppression and matrix effects compared to the SPE method. Sample preparation was shorter for the SPE method, consuming 2 hrs for an average sample batch, compared to 4 hrs for the LLE method, which included a 2 hr freezing step. In conclusion, for urine analysis, all three sample preparation techniques were acceptable for the analysis of THC, synthetic cannabinoids, and their metabolites, with the SLE method being the preferred method. For blood analysis a LLE and SPE method were developed and are adequate for the analysis of THC, synthetic cannabinoids, and their metabolites, with the LLE method being the preferred method.
12

Comparison of sample preparation techniques on twenty-three drugs in human whole blood and urine

McGowan, Courtney K. 10 October 2019 (has links)
In forensic toxicology, analysis of drugs and metabolites in biological fluids is performed to determine cause of death, suspected drug use, drug facilitated sexual assaults, or whether someone was driving under the influence. Analyte identification and concentration determination can be determined in a variety of matrices (e.g., blood, urine, or oral fluid) and can be complex. It is therefore necessary to have optimal sample preparation and instrumental conditions that work for all matrices of interests. Determining the best approach can be challenging due to the amount of time and resources to perform expansive evaluations of sample preparation, stationary/mobile phases, liquid chromatography (LC) conditions and mass spectrometry (MS) operating parameters. In this study three different sample preparation methods were validated for blood and urine. The three sample preparation methods were solid-phase extraction (SPE), supported liquid extraction (SLE), and liquid-liquid extraction (LLE). Six different drug groups were used as the analytes being tested by the methods. These drug groups were amphetamines, local anesthetics, opioids, hallucinogens, antidepressants, and novel psychoactive substances (NPS). A total of twenty-three drugs were used: amphetamine, methamphetamine, (3,4-methylenedioxyamphetamine (MDA), 3,4-methylenedioxy-N-ethylamphetamine (MDEA), and 3,4-methylenedioxymethamphetamine (MDMA), benzoylecgonine (BZE), cocaine, lidocaine, codeine, methadone, morphine, 6-monoacetylmorphine (6-MAM), fentanyl, oxycodone, lysergic acid diethylamide (LSD), phencyclidine (PCP), amitriptyline, citalopram, fluoxetine, trazodone, ethylone, α-pyrrolidinopentiophenone (α-PVP), and 25I-NBOMe. The methods were validated according to guidelines set forth by the Scientific Working Group for Forensic Toxicology (SWGTOX) Standard Practices for Method Validation in Forensic Toxicology and the American Academy of Forensic Science (AAFS) Standards Board (ASB) draft of Standard Practices for Method Validation in Forensic Toxicology. Parameters of calibration model, bias, precision, limit of detection (LOD), limit of quantitation (LOQ), dilution integrity, ion suppression/enhancement, interference studies, and stability were evaluated. Recovery was also assessed to determine the efficiency of the extraction. Calibration models met the 0.98 R2 minimum requirement. For all sample preparations the compounds evaluated in each were found to be stable for at least 72 hours. Interferences were found to be similar across all three sample preparation methods. Parameters of bias, precision, and dilution integrity were largely comparable between all three methods. Overall for LOD, SLE resulted in lower values for blood and urine ranging for 0.1 to 5 ng/mL. Overall for LOQ, SLE resulted in lower values for blood and LLE resulted in lower values for urine in the range of 0.5-10 ng/mL. SLE resulted in the highest recovery for all twenty-three analytes, due to LLE failing to extract consistently or completely for benzoylecgonine, morphine, and 6-monoacetylmorphine. Overall, SLE resulted in the lowest percent values for ion suppression and enhancement for both blood and urine. Overall, blood resulted in high ion suppression (exceeding -20%) for SPE and LLE. Final determination overall was that SLE was the best sample preparation method for all twenty-three analytes. This was determined based on the evaluation of recovery, ion suppression/enhancement, and LOD, as well as sample preparation time. Sample preparation time for SLE was approximately 1 hour, while SPE took 2.5 hours and LLE 2 hours.
13

FRACTIONATION OF LIGNIN DERIVED COMPOUNDS FROM THERMOCHEMICALLY PROCESSED LIGNIN TOWARDS ANTIMICROBIAL PROPERTIES

Dodge, Luke A. 01 January 2018 (has links)
The overuse of antibiotics in agriculture is an emerging concern, due to their potential detrimental impact to the environment. This study focuses on exploring antimicrobial properties of lignin derived compounds. Lignin is of interest as a feedstock to replacing some petroleum-based chemicals and products because it is the most abundant source of renewable aromatic compounds on the planet. Two lignin rich streams, residues from the enzymatic hydrolysis of dilute acid and alkaline pretreated corn stover, were decomposed via pyrolysis and hydrogenolysis, respectively. The resulting liquid oils were subjected to sequential extractions using a series of solvents with different polarities. Chemical compositions of the extracted fractions were characterized through HPLC and GC/MS. These extracted compounds were screened against Saccharomyces cerevisiae (S. cerevisiae), Escherichia coli, and Lactobacillus amylovorus for antimicrobial properties. Six lignin model monomers: guaiacol, vanillin, vanillic acid, syringaldehyde, 2,6-dimethoxyphenol, and syringic acid were compared to the oils and extracted fractions for antimicrobial properties. Development of lignin-derived chemicals with antimicrobial properties could provide a novel use for this underutilized natural resource.
14

Detection and quantitation of nine fentanyl analogs in urine and oral fluid using QSight Triple Quad LC-MS/MS

Ke, Yiling 09 July 2020 (has links)
The opioid epidemic has become a serious public health problem in the United States. The increasing abuse of synthetic opioids has raised concerns in the society. Fentanyl is a synthetic opioid analgesic which has resulted in an increasing number of drug overdoses since 2013. In addition, fentanyl analogs, originally manufactured for use as analgesics or animal tranquilizers, have emerged in the United States drug market. Fentanyl and its analogs, similar to other opioids, work as full µ-agonists, binding with µ-receptors in the brain. Fentanyl and its analogs elicit more potent effects compared to the traditional opioids being abused such as morphine or heroin. With the emergence of fentanyl analogs in the drug market, identifying and differentiating those analogs becomes a challenge due to their structural similarities to fentanyl. The purpose of this research was to develop a method of identifying and quantifying nine fentanyl analogs in urine and oral fluid using the QSight® Triple Quad LC-MS/MS, coupled with a Halo® C18, 2.7µm column. The method was validated based on AAFS Standards Board (ASB) Standard 036, Standard Practices for Method Validation in Forensic Toxicology. The analytes in this research included fentanyl, norfentanyl, acetyl fentanyl, carfentanil, cyclopropyl fentanyl, methoxyacetyl fentanyl, valeryl fentanyl, furanyl fentanyl and 4-anilino-N-phenethylpiperdine (4ANPP). All samples, calibrators, and quality controls (QC) were prepared by spiking certified reference standards into donated human urine or human oral fluid. Supported liquid extraction (SLE) was performed as the sample preparation method using ISOLUTE® SLE+ 1mL columns followed by evaporation. All samples were reconstituted with 200 µL methanol. The mobile phases used in this method were 5mM ammonium formate in Millipore water with 0.1% formic acid and methanol with 0.1% formic acid. A 10-minute LC method achieved complete resolution of the analytes, with specific retention times ranging from 3.5 to 5.7 minutes. For urine and oral fluid analysis, the calibration range for all analytes was established from 1 to 70 ng/mL. The resulting r2 values were greater than 0.988 for all analytes. Bias and precision were evaluated at 3, 25 and 60 ng/mL, and bias and percent coefficient of variation (%CV) for within and between run precision had acceptable values within ±20%. The limit of detection (LOD) was 0.1 ng/mL for most fentanyl analogs, with a LOD of 0.01 ng/mL for valeryl fentanyl and furanyl fentanyl. Carryover was not detected for any analytes in either matrix. Recovery of all compounds following SLE for both urine and oral fluid was above 50%. For urine, the ion enhancement and suppression of all analytes was within 25%. For oral fluid, the ion enhancement and suppression of most analytes was within 25% except valeryl fentanyl, which experienced suppression of 35%. The matrices analyzed had no interference effect on the detection or quantitation of analytes in this method. The interference effects of different commonly encountered drugs were studied and showed minimal impacts on the results generated from this method. All analytes were stable for up to 72 hours at room temperature, except cyclopropyl fentanyl. In conclusion, using the QSight® Triple Quad LC-MS/MS following SLE effectively identified and quantified fentanyl analogs present in both urine and oral fluid. This method has shown its potential to be applied to casework samples for fentanyl analogs detection.
15

Design and Development of 2-Functionalized Calix[4]arenes and Their Investigation in the Separation of Lanthanides

Menon, Sreejit Rajiv, Menon January 2016 (has links)
No description available.
16

Continuous extraction and destruction of chloro-organics in wastewater using ozone-loaded Volasil (TM) 245 solvent

Tizaoui, Chedly, Slater, M.J., Ward, D.B. January 2005 (has links)
No / Extracting waterborne contaminants to ozone-loaded Volasil¿245 (a siloxane solvent in which ozone is ten times more soluble than water) has been studied as a means of enhancing reaction kinetics and thus, providing more rapid wastewater decontamination. Investigation was carried out with respect to 2-chlorophenol and dichloromethane. Using a pilot scale continuous flow liquid¿liquid/ozone water treatment system, 2-chlorophenol was extracted to the ozone-loaded solvent phase and considerable extents of destruction were achieved. However, the approach was demonstrated to yield slightly less destruction than direct gas contact for the same utilization of ozone and enhanced reaction kinetics were not shown to occur. This was suggested to be due to increased interfacial mass transfer resistance and/or the promotion of less destructive reaction pathways. Modification of the existing pilot system, by conversion from co- to counter-current solvent-loading, enabled greater dissolved ozone concentrations to be achieved within the solvent. Increasing the counter-current exchange column height to not, vert, similar2.5 m was suggested for achieving a near optimum level of performance. The liquid¿liquid/ozone approach was demonstrated to be an effective means of indirectly exposing wastewater contaminants to concentrated ozone. As such the technology may be applicable as an alternative to direct gas contact in instances where the avoidance of contaminant sparging is desired (i.e. where contaminants are highly volatile, pungent and/or toxic) or foaming occurs
17

Quantification of Progesterone and 17-β Estradiol in Mouse Serum by Liquid Chromatography-Tandem Mass Spectrometry

Kennard, Benjamin, Cobble, Allison, Gravitte, Amy, Galloway, Kaleigh, Kintner, Jen, Hall, Jennifer, Brown, Stacy C 05 May 2020 (has links)
Quantification of progesterone and 17-β estradiol in mouse serum by liquid chromatography-tandem mass spectrometry Authors: Benjamin Kennard, Allison Cobble, Amy Gravitte, Keleigh Galloway, Jen Kintner, Jennifer Hall, Stacy Brown Introduction: In the United States, Chlamydia trachomatis is a commonly appearing sexually transmitted infection1. It affects the U.S. healthcare system to a tune of about $500 million dollars annually2. In women, it generally appears asymptomatic and can lead to severe secondary complications such as pelvic inflammatory diseases or infertility1. Female sex hormones, estrogen and progesterone, are being identified to have a role in chlamydial infection. Specifically, this study aims to create quantification methods to detect levels of estrogen and progesterone in mice, infected with Chlamydia muridarum, plasma samples. Methods: Progesterone samples were prepared using solid-liquid extraction (SLE+) cartridges with ethyl acetate as the elution solvent. Estradiol samples were prepared using liquid-liquid extraction (LLE) with methyl tert-butyl ether and subsequent derivatization with DMIS. Following sample preparation, hormones were quantified in samples using LC-MS/MS with a gradient elution of 1 mM ammonium fluoride in water and acetonitrile. The separation was achieved using a UCT C18 column (100 x 21.mm, 1.8 μm particle size) maintained at 50oC. The mass spectrometer was set up to isolate molecular ions for progesterone (m/z 315.0910) and derivatized estradiol (m/z 431.1835). Quantification was facilitated by the use of deuterium-labeled internal standards and their corresponding molecular ions in the mass spectrometer (d9-progesterone; m/z 324.1230 and d5-estradiol; m/z 436.2922). Results: Several aspects of the assay presented have been optimized for maximum analyte recovery and analytical sensitivity, including column choice, mobile phase, derivatizing agents for estradiol, and extraction protocols for progesterone. The LC-MS/MS method was investigated for precision and accuracy over three separate days. The dynamic range of the progesterone assay was 5 – 100 ng/mL, with a limit of detection of 1 ng/mL. Likewise, the estradiol assay was linear in the range of 5 – 100 ng/mL, with a limit of detection of 0.5 ng/mL. The average precision, represented by % RSD was 0.74 – 8.5% and 6.3 – 13.4% for progesterone and estradiol, respectively. The accuracy of the method, represented by % error was 1.6 – 14.4% and 4.0 – 10.5% for progesterone and estradiol, respectively. Successful validation was defined as < 15% RSD and error (< 20% at the limit of quantification), per current FDA Guidelines. Conclusions: The developed LC-MS/MS method is specific for progesterone and estradiol, and the extraction is suitable for preparation of mouse serum samples. This assay could be successfully applied to hormone quantification in mouse samples to support the investigation of the link between chlamydia infection and hormone levels in female animals. References 1. Chlamydia - 2017 Sexually Transmitted Diseases Surveillance. https://www.cdc.gov/std/stats17/chlamydia.htm. Accessed October 23, 2018. 2. Owusu-Edusei K, Chesson HW, Gift TL, et al. The Estimated Direct Medical Cost of Selected Sexually Transmitted Infections in the United States, 2008. Sex Transm Dis. 2013;40(3):197-201. doi:10.1097/OLQ.0b013e318285c6d2
18

Utilização de hidrometalurgia e biohidrometalurgia para reciclagem de placas de circuito impresso. / Hydrometallurgy and biohydrometallurgy applied to printed circuit board recycling.

Silvas, Flávia Paulucci Cianga 15 October 2014 (has links)
A geração global de resíduo eletrônico (REEE) cresce a uma taxa de cerca de 40 milhões de toneladas por ano. Este constante incremento na geração dos REEEs somado às recentes legislações tem impulsionado pesquisas focadas no desenvolvimento de processos para recuperação de materiais e sustentabilidade da indústria eletroeletrônica. Dentro destes resíduos encontram-se as placas de circuito impresso (PCIs) que estão presentes na maioria dos EEEs, têm composição heterogênea que varia conforme a fonte, país de proveniência e época, e tecnologia de fabricação. Assim, este trabalho teve por objetivo a realização de rota hidrometalúrgica (extração sólido/líquido) e biohidrometalúrgica para reciclagem de placas de circuito impresso provenientes de impressoras visando a recuperação de cobre. Para tanto fez-se inicialmente a caracterização da PCI e o desenvolvimento de uma rota combinada de processamento físico seguida por processo hidrometalúrgico ou biohidrometalúrgico. O processamento físico e de caracterização foi composto por etapas de cominuição, separação magnética, classificação granulométrica, visualização em lupa binocular, microscópio eletrônico de varredura acoplado com detector de energia dispersiva de raios X (MEV/EDS), digestão ácida, perda ao fogo e análise química por AAS e ICP. Já, o processamento hidrometalúrgico foi composto por duas etapas de extração sólido/líquido: a primeira em meio sulfúrico e a segunda em meio sulfúrico oxidante. Para os ensaios de biolixiviação utilizou-se uma cepa bacteriana composta por 3 espécies microbianas: Acidithiobacillus ferrooxidans, Acidithiobacillus thiooxidans e Leptospirillum ferrooxidans. Verificou-se que a placa possui 4 camadas de Cu intercaladas por fibra de vidro, é lead free e seus componentes representam 53,3 % do seu peso. A porcentagem em massa correspondente ao material não magnético é de 74,6 % e do magnético 25,4 %. Os materiais moído e não magnético apresentaram tendência em se acumular nas frações mais grossas. Já na fração magnética, o acúmulo do material ocorreu na fração mais fina (0,053 mm). A separação dos metais através de classificação granulométrica não foi possível. A PCI estudada é composta por: 44% de metais, 28,5 % de polímeros e 27,5 % de cerâmicas. Sendo: Ag-0,31 %; Al3,73 %; Au0,004 %; Cu 32,5 %; Fe1,42 %; Ni0,34 %; Sn0,96 % e Zn0,64 %. A extração de Cu no processamento hidrometalúrgico foi de 100 % e o fator de recuperação 98,46 %, o que corresponde a uma recuperação de 32 kg de Cu em 100 kg de PCI. Já no processamento biohidrometalúrgico, a extração de Cu alcança 100 % quando utilizados 2 % de densidade de polpa e 100 % de inóculo. O fator de recuperação é de 100 % e a recuperação de Cu em 100 kg de PCI é de 32,5 kg. O processamento hidrometalúrgico apresenta como vantagens quando comparado ao biohidrometalúrgico: menor tempo de extração (8 h versus 4 dias); seletividade de Cu; maior densidade de polpa (10 % versus 2 %). Já a biolixiviação utiliza menor temperatura de trabalho (36 ºC versus 75 ºC) e dispensa a etapa de separação magnética. / The increase in the generation of waste electrical and electronic equipment (WEEE), 40 tons per year, allied with the enactment of new laws encouraged researches focused on the developing of processes to reclaim materials and on the sustainability of the electrical and electronics industry. Whithin the WEEEs, printed circuit boards (PCB) composition is heterogeneous and varies according to several factors, including: kind of EEE, when and where it was produced and fabrication technology. The goal of this work is to perfom a hydrometallurgical route (solid/liquid extraction) and a biohydrometallurgical route to recycle PCB from discarded printers aiming the recovery of copper. To do so, the first step is to characterize the PCB and the development of a combined fisical processing followed by hydrometallurgical and biohydrometallurgical routes. The fisical and the characterization processes, in that order, consisted on griding, magnetic separation, granulometric screening, visual assessement by binocular magnifier, scanning electron microscopy with energy dispersive X-ray spectroscopy (SEM/EDS), acid digestion, loss on fire, and chemical analyzes by AAS and ACP-OES. The hydrometallurgical stage consisted on two steps: solid/liquid extraction by sulfuric acid leaching and solid/liquid extraction by sulfuric acid leaching with an oxidizing agent. The bioleaching tests used a mixed bacterial strain: Acidithiobacillus ferrooxidans, Acidithiobacillus thiooxidans and Leptospirillum ferrooxidans. The results showed that PCB consisted on 4 layers of copper and fiber glass, not possesing lead (leadfree) on its composition and its components constitute 53.3 % weight percentage. The non-magnetic fraction (NMA) weight percentage represents 74.6 %, the magnetc fraction (MA) represents 25.4 %. The grinded material and the non-magnetic fraction presented an inclination to build up on thickest fractions. On the magnetic fraction this behavior occurred on the thinnest fraction (0.053 mm). The metal separation using granulometric screening was not possible and the visual assessement by binocular magnifier was conclusive for this research. The composition of the studied PCB is: 44 % metal, 28.5 % polymer and 27.5 % ceramics. Beeing: Ag-0.31 %, Al-3.73 %, Au-0.004 %, Cu-32.5 %, Fe-1.42 %, Ni-0.34 %, Sn-0.96 %, Zn-0.64 % and other metals-4.10 %. Copper extraction in the hydrometallurgical process achieved 100 % and the recuperation factor 98.46 %, which means a recovery of 32 kg of copper in 100 kg of PCB. However in biohydrometallurgical process, the copper extraction reached 100 % on the forth day using a 2 % pulp density and 100 % inoculum. The recuperation factor achieved 100 % and, therefore, copper recovery in 100 kg of PCB is equivalent to 32.5 kg. The hydrometallurgical processing has many advantages compared to the biohydrometallurgical processing: a smaller extraction time (8 h versus 4 days); Cu selectivity; higher pulp density (10 % versus 2 %). However, bioleaching uses an inferior working temperature (36 ºC versus 75 ºC) and dont require magnetic separation.
19

Triagem de métodos de purificação de óleos com acidez elevada para produção de biodiesel / Screening of purification methods of high acid oils for biodiesel production

Grabauskas, Daniel 18 October 2013 (has links)
O presente estudo teve como objetivo selecionar procedimentos de purificação de óleos vegetais, com enfoque na desacidificação, comparando a eficiência de métodos de refino alternativos (adsorção e extração liquido-liquido) com o convencional (alcalino). Para tanto, foram utilizados óleos com baixo impacto na cadeia alimentícia, como óleo de andíroba e óleo de macaúba, visando contribuir para a ampliação de matérias-primas lipídicas na produção de biodiesel. A triagem do método de purificação mais adequado foi baseada na redução de ácidos graxos livres, na quantidade recuperada de matéria-prima após o refino e na qualidade do biodiesel gerado. Adotando óleos com diferentes teores de ácidos graxos livres, óleo de andíroba (17,7%) e óleo de macaúba (7,9%) a desacidificação por adsorção, empregando diferentes adsorventes foi excluída com base nos baixos valores de desacidificação (<34,1%) e de recuperação em massa de óleo (22,2-43,1%). A acidez mais elevada do óleo de andíroba se mostrou como um fator limitante adicional, portanto, o uso deste óleo foi eliminado para as etapas posteriores de triagem. Em contrapartida, o refino por extração liquido-liquido (ELL) usando etanol como solvente forneceu valores mais elevados de recuperação mássica (>75,9%) e de redução de ácidos graxos livres (>48,8%). Buscou-se por meio da utilização de um método estatístico determinar as condições adequadas de refino por ELL usando etanol hidratado. Esta etapa foi realizada por meio de uma matriz de planejamento fatorial composto de face centrada 22, avaliando simultaneamente a influência da porcentagem mássica de agua no solvente alcoólico (2, 4 e 6%) e da razão mássica solvente/óleo (1:1, 1,5:1, 2:1). De acordo com a análise estatística foi possível estabelecer que a adição de 5,3% de agua no etanol e razão mássica etanol/óleo de 1,79:1 maximizaram a remoção de ácidos graxos livres (64,4%) sem ocasionar elevadas perdas de óleo refinado (93,9%). Adotando as condições otimizadas de ELL, o óleo de macaúba foi refinado em único e duplo estagio. Constatou-se que o teor de ácidos graxos livres em relação ao óleo bruto (7,9%) foi reduzido expressivamente em ambos os casos para valores de 2,9% (refino em único estagio) e de 1,0% (refino em duplo estagio), com a vantagem de não promover oxidação do material lipídico. Entretanto, a recuperação mássica de óleo refinado obtida na ELL em duplo estagio foi menor, da ordem de 78,5%. Para validar a metodologia de purificação, foram realizadas reações de etanólise das amostras de óleo refinado por ELL em único e duplo estagio, óleo bruto e óleo refinado por via alcalina utilizando como catalisador oxido nióbio impregnado com sódio. Enquanto a acidez do óleo bruto inibiu o catalisador, os produtos originados pelas amostras de óleo refinadas por ELL em único e duplo estagio contiveram teores em ésteres etílicos (97,4% e 97,8%, respectivamente) que atenderam as especificações recomendadas pela Agencia Nacional de Petróleo, Gás Natural e Biocombustível para uso como combustível. Esses valores foram similares a conversão alcançada na reação conduzida com o óleo refinado por via alcalina (99,0%), que teve desvantagens como recuperação mássica de 80,1% e aumento do índice de peroxido, indicando que a extração liquido-liquido tem potencial para desenvolvimento e aplicação em processos de refino de óleos vegetais para posterior utilização na síntese de biodiesel. / This study aimed at comparing the purification of non-edible vegetable oils by two different types of refining (adsorption and liquid-liquid extraction) with conventional alkali refining, contributing to the expansion of lipid feedstocks for biodiesel production. The use of non-edible vegetable oils is related to the final cost of biodiesel by increasing product competitiveness. The screening of the purification methods for vegetable oils (andiroba oil and macaw palm oil) was based on the reduction of free fatty acids content, oil mass recovery after the refining and the quality of biodiesel. Adopting oils with different levels of free fatty acids, andiroba oil (17.7%) and macaw palm oil (7.9%), the deacidification by adsorption, employing different adsorbents was excluded on the basis of the low deacidification values (<34.1%) and the oil mass recovered (22.2-43.1%). The higher acidity of andiroba oil was found to be an addition drawback and therefore, this oil was disqualified for further testing. On the other hand, the purification by liquid-liquid extraction (LLE) of macaw palm oil using ethanol as solvent gave higher values for oil mass recovery (>75.9%) and reduction of free fatty acids (>48.8). To determine the suitable conditions for oil refining by LLE using hydrated ethanol as solvent a statistical method was proposed. For this a 22 central composite face-centered experimental design was adopted to simultaneously evaluate the influence of the water percentage in the alcoholic solvent (2, 4, and 6%), and mass ratio of solvent-to-oil (1:1, 1.5:1 and 2:1). According to the statistical analysis it was possible to establish that the addition of 5.3% of water in the ethanol and mass ratio of ethanol to oil of 1.79:1 maximizes the removal of free fatty acids (64.4%) resulting in high refined oil recovered (93.9%). Adopting the optimized LLE conditions, the macaw palm oil was refined in single and double-stage. It was noted that the level of free fatty acids in relation to crude oil (7.9%) was significantly reduced in both cases for values of 2.9% (refining in single stage) and 1.0% (refining in double-stage), with the advantage of not promoting lipid oxidation. However, the percentage of the recovered refined oil obtained in LLE double-stage was slightly lower, in the order of 78.5%. To validate the purification methodology, ethanolysis reactions catalyzed by niobium oxide impregnated with sodium were performed using samples refined by LLE (single and double-stage), oil refined by alkali neutralization and crude oil. The obtained dataset demonstrated that the catalyst was inhibited by the high acidity level of the crude oil, while refined oil by LLE (single-stage and double-stage) gave levels of ethyl esters contents of 97.4% and 97.8%, respectively that meet the criteria established by the Brazilian National Agency of Petroleum, Natural Gas and Biofuels to be used as a fuel. These values were similar to that attained in the reaction using refined oil by alkaline protocol (99.0%), which had disadvantages such as oil mass recovered of 80.1% and oil oxidation (increased peroxide value), indicating that the liquid-liquid extraction has the potential for development and application in vegetable oils refining processes for further using as feedstocks in the biodiesel synthesis.
20

Detection and quantitation of 17 synthetic cannabinoids in human whole blood using LC-MS/MS following supported liquid extraction

Lee, Daniel 25 October 2018 (has links)
Synthetic cannabinoids have become a growing concern in society. The extensive list of synthetic cannabinoids and the abuse rate has drawn the attention by government agencies throughout the world. These synthetic cannabinoids can adopt a number of different structures, while still acting on endogenous cannabinoid (CB1 and CB2) receptors. In addition, due to structural modifications of these synthetic cannabinoids, many of these compounds can bind to CB1 and CB2 receptors with greater affinity causing severe adverse and life-threatening effects. Because of their structural dissimilarity to the phytocannabinoid Δ9-THC, combating the rapid growth and emergence of synthetic cannabinoids with conventional THC-based methods has become an ongoing struggle. The purpose of this research was to develop and validate a robust and reliable method to accurately identify and quantify 17 synthetic cannabinoids in human whole blood using liquid chromatography-tandem mass spectrometry (LC-MS/MS). The method was validated in accordance to SWGTOX guidelines for quantitative analysis using the following analytes: 4-cyano-CUMYL-BUTINACA, 5F-3,5-ABPFUPPYCA, 5F-ADB-PINACA, 5F- PY-PINACA, ADB-PINACA, APP-PICA, CUMYL-THPINACA, EMB-FUNICACA, JWH-250, MDMB-FUBICA, MEP-CHMICA, MO-CHMINACA, NM2201, PB-22, RCS-8, UR144, and XLR11. With this developed method, total analysis time was 8 minutes with samples eluting from 3.8 to 5.8 minutes. Calibration curves for each analyte had acceptable R2 values > 0.99 using a weighting factor of 1/x. A linear dynamic range of 0.5 – 25 ng/mL was used for all analytes, except for APP-PICA and NM2201 which were quantifiable at 0.1 ng/mL and PB-22 which used a quadratic model. Extraction of analytes using supported liquid extraction (SLE) cartridge improved sample-prep time by more than half, compared to traditional solid phase extraction (SPE) methods. Percent recovery of analytes using SLE was determined to be from 54.92 to 83.36%. Bias and Precision was assessed at 1, 3, 7, and 20 ng/mL for all analytes. All samples had acceptable calculated percent bias and percent coefficient of variation (%CV) within ±20%. No carryover was observed with this method. Matrix effect, using 10 different sources, did not have any interfering effects on detection and quantification of analytes. Ionization suppression and enhancement was observed at various levels, from -4.47 to 76.67%, but had little effect on other validation parameters. Analysis of other commonly encountered drugs (clonazepam, diazepam, (+) methadone, morphine, fentanyl, cocaine, amphetamine, 3,4-methylenedioxymethamphetamine (MDMA), 25I-NBOMe, and phencyclidine (PCP)) does not show any source of interference. The overall development and validation of this method demonstrates a sensitive and reliable way to positively identify 17 different synthetic cannabinoids in human whole blood in rapid time. / 2020-01-31

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