海洛因与甲基苯丙胺毒品滥用者毛发特征分析的比较

根据海洛因和甲基苯丙胺滥用者毛发中毒品及其代谢物的分布特点,通过实验比较了两类毒品滥用者毛发的分析特点。海洛因吸食者毛发采用甲醇超声释放待测物,而后直接调整pH值进行液相萃取,萃取物挥干后进行衍生化并进行GC/MS检测;甲基苯丙胺吸食者毛发在碱性条件下消解,然后采用小体积萃取,直接在提取液中衍生化,并进行GC/MS检测。通过空白毛发标准添加6-单乙酰吗啡、吗啡和可待因进行分析,3种鸦片类毒品最小检测限均小于3μg/g,RSD(n=5)为2.5%~9.6%;通过空白毛发标准添加苯丙胺、甲基苯丙胺、3,4-(亚甲二氧基)苯丙胺和3,4-(亚甲二氧基)-甲基苯丙胺进行分析,4种苯丙胺类毒品的最小检测限为0.05μg/g,RSD(n=5)为5%~14%。     

海洛因与甲基苯丙胺毒品滥用者毛发特征分析的比较

根据海洛因和甲基苯丙胺滥用者毛发中毒品及其代谢物的分布特点,通过实验比较了两类毒品滥用者毛发的分析特点。 海洛因吸食者毛发采用甲醇超声释放待测物,而后直接调整pH值进行液相萃取,萃取物挥干后进行衍生化并进行GC/MS检测;甲基苯丙胺吸食者毛发在碱性条件下消解,然后采用小体积萃取,直接在提取液中衍生化,并进行GC/MS检测。 通过空白毛发标准添加6-单乙酰吗啡、吗啡和可待因进行分析,3种鸦片类毒品最小检测限均小于 3 μg/g,RSD(n=5)为2.5%~9.6%;通过空白毛发标准添加苯丙胺、甲基苯丙胺、3,4-(亚甲二氧基)苯丙胺和3,4-(亚甲二氧基)-甲基苯丙胺进行分析,4种苯丙胺类毒品的最小检测限为0.05 μg/g,RSD(n=5)为5%~14%。     

超声液相萃取-GC/MS-SIM法定量检测唾液中苯丙胺类毒品

建立了一种人体唾液中苯丙胺(AM)、甲基苯丙胺(MAM)、 3, 4-亚甲二氧基苯丙胺(MDA)、 3, 4-亚甲二氧基甲基苯丙胺(MDMA)毒品的超声波液液萃取-气相色谱/质谱-选择离子检测方法. 对萃取溶剂、萃取时间等参数进行了考查, 确定了乙酸乙酯为萃取溶剂, 在超声波下液液萃取2 min. 用该溶剂对添加毒品的唾液进行提取, 采用气相色谱/质谱-选择离子检测法(GC/MS-SIM)检测, 获得了良好线性, 相对标准偏差在15%内, 准确性均在80%～115%之间, 最小检测限可达0.05 μg/mL. 该方法未对毒品进行衍生化处理, 可用于缴获毒品及嫌疑吸毒者人体生物检材中苯丙胺类毒品的分析.     

毛发中海洛因代谢物的释放与分析方法研究

通过对海洛因吸食者毛发和空白添加标准品毛发的碱消解、酸消解、甲醇超声提取、甲醇-5 mol/L HCl超声提取、甲醇-三氟乙酸超声提取5种毛发中毒品及其代谢物的释放方法考察,确立了甲醇超声提取-液液萃取-气相色谱/质谱-选择离子检测的方法.本方法可最大程度地抑制海洛因的中间代谢物6-单乙酰吗啡的水解,其水解率仅为2.63%,极大地提高了海洛因滥用的毛发证据作用.利用本方法对添加6-单乙酰吗啡的毛发进行萃取和检测,6-单乙酰吗啡的回收率为52.6%,相对标准偏差RSD为4.6% ;对添加不同浓度的吗啡、可待因、6-单乙酰吗啡3种毒品的毛发进行萃取和检测,其线性良好(r＞0.99),相对标准偏差均小于15%.此外,考察了甲醇消解的影响因素,吸毒者毛发中的毒品释放效果随毛发的细碎程度和超声时间延长而提高.     

胶体金免疫层析法测定酸奶中组胺含量及教学应用

建立了一种快速检测酸奶中组胺含量的胶体金免疫层析测定方法。将直径40nm的胶体金颗粒与组胺特异性单克隆抗体偶联制备金标抗体,研究了胶体金溶液pH、抗体用量、层析时间及抗原用量等对方法灵敏度的影响。结果显示,最佳反应条件为标记pH8.8、3.6μL抗体标记0.5 mL胶体金,层析时间7 min,抗原用量1 mg/mL,此时胶体金免疫层析方法对组胺的检测限为1.11μg/g。酸奶样品组胺含量的添加回收实验结果与仪器法吻合。将该方法用于本科实践课程"食品与发酵工业分析"的现场教学,效果良好。     

胶体金免疫层析法快速检测牛奶、奶粉、饲料中的三聚氰胺

建立了快速检测牛奶、奶粉、饲料样品中三聚氰胺的胶体金免疫层析分析法。将三聚氰胺进行分子修饰得到两种衍生物,分别与牛血清白蛋白(BSA)和卵清白蛋白(OVA)相连制得免疫原和包被抗原。运用杂交瘤抗体制备技术得到抗三聚氰胺的单克隆抗体(mAb)。利用柠檬酸三钠还原法制得平均粒径18 nm的胶体金,将胶体金与抗三聚氰胺单克隆抗体相连,所形成的金标抗体(Au-mAb)包被在胶体金垫上,包被抗原和羊抗鼠二抗分别包被在硝酸纤维素膜(NC)上作为检测线(T线)和质控线(C线)。将胶金垫、NC膜、样品垫和吸水纸组装成免疫层析快速检测试剂条。将标准溶液(或待测液)滴加到样品垫上,10 min后可在NC膜C线和T线位置上用肉眼观察到胶体金的颜色(红色),通过比对颜色的深浅判断样品中三聚氰胺的含量。结果表明,三聚氰胺的检出限为10μg/L;选用了其它10种物质对免疫层析试剂条进行了特异性实验,免疫层析试剂条与2-氯-4,6-二氨基-1,3,5-三嗪和环丙氨嗪的交叉反应率约为1%,与其它8种物质没有交叉反应;加标样品用免疫层析试剂条和酶联免疫吸附分析法(ELISA)同时检查,结果一致。本方法适用于牛奶、奶粉、饲料样品中三聚氰胺的现场快速检测。     

唾液中苯丙胺类毒品的液相小体积萃取GC/MS-SIM检测

建立了一种便捷的唾液中4种毒品(苯丙胺(AM)、甲基苯丙胺(MAM)、3,4-(亚甲二氧基)苯丙胺(MDA)、3,4(亚甲二氧基)-甲基苯丙胺(MDMA))的液相小体积超声提取-气相色谱/质谱-选择离子检测分析方法并考察了小体积萃取溶剂和体积对萃取效果的影响.该方法用100μL环己烷对唾液中的毒品进行提取,直接抽取提取液用气相色谱/质谱-选择离子(GC/MS-SIM)检测,获得良好线性,相对标准偏差在15%内,准确性均在80%～120%之间,最小检测限可达0.1μg/mL.该方法灵敏、简便、快速,可用于缴获毒品及嫌疑吸毒者人体生物检材中苯丙胺类毒品的分析.     

动态液相微萃取-微波衍生化-气相色谱/选择离子检测-质谱法测定毛发中的苯丙胺类毒品

建立了一种便捷的毛发中4种苯丙胺毒品的检测方法。采用动态液相微萃取法用氯仿提取毛发消解液中的苯丙胺类毒品,然后在微波加热的条件下用N-甲基-双三氟乙酰胺(MBTFA)进行衍生化处理,将反应液直接用气相色谱/选择离子检测-质谱法（GC/SIM-MS）检测。以2-甲基苯乙胺为内标,在空白毛发中添加标准品做标准曲线得到4种苯丙胺类毒品的线性相关系数均不小于0.996。衍生化后4种毒品在毛发中的最小检测限(S/N=3)均为50 pg/mg。4种苯丙胺类毒品在毛发中的添加浓度为5 ng/mg时,5次测定的相对标准偏差（RSD）分别为苯丙胺6.0%,甲基苯丙胺13.9%,3,4-(亚甲二氧基)苯丙胺10.2%,3,4(亚甲二氧基)-甲基苯丙胺9.2%。应用所建立的方法对苯丙胺类毒品吸食者的毛发进行检测,检出了这4种毒品,毛发样品的最小用量为4.6 mg (约20 cm 长)。该方法灵敏、简便、快速,可用于毛发中低含量苯丙胺类毒品的分析。     

毒品检测芯片1次可快速查出10类毒品

日前,公安部科技信息化局主持了对吉林省公安厅物证鉴定中心承担的“十一五”国家科技支撑计划项目“组合型常见毒品现场快速检测技术研究”的课题验收。专家一致认为,课题组在表面等离子体共振技术基础上研制开发了基于两瓣电流式光电位置测定技术的现场毒品检测系统,现场一次性高通量检测多种毒品成分的生物芯片系统,窄缝进样高灵敏微流控电泳芯片样机,为毒品检测提供了新的现场快速筛查手段,部分关键技术达到国际先进水平。近年来,新的同类毒品即设计型毒品不断出现,对毒品检测鉴定提出了更高要求。国内对毒品及代谢物的快速分析,主要是利用进口的免疫试剂盒,但该方法干扰因素多,经常出现假阳性。而使用常规仪器分析检测技术每次只能对一个样品或一种毒品成分进行检测鉴定,在遇到严打专项斗争和发生突发事件,大量样本需要测定和多种毒品成分需要定性筛查时,便显出通量小、速度慢的缺陷。根据课题成果开发的具有自主知识产权的常见毒品电化学传感器,可代替进口免疫试剂盒,为不具备大型分析仪器的基础化验室办案现场提供了简易的快速筛选分析方法。其生物芯片可一次性高通量快速检测吗啡、苯丙胺、甲基苯丙胺、氯胺酮、大麻、丁丙喏啡、可卡因、美沙酮等10类毒品成分,基本涵盖了国内...     

海洛因滥用者唾液中毒品代谢物的SPE-GC/MS-SIM分析

本文首先考查了不同类型不同厂家的固相萃取柱的萃取效果,采用提取效果较好的50 mg/mL的Clean-screen CSDAUL01混合型强阳离子固相萃取柱,对唾液中的吗啡、可待因、6-单乙酰吗啡等3种鸦片类毒品进行提取后,将提取液吹干;再经MBTFA衍生化后,进行GC/MS-SIM检测。以乙基吗啡为内标,3种毒品的线性相关系数均大于0.99,线性范围为10～1000 ng/mL,相对回收率分别为85%～110%、94%～107%和75%～92%;相对标准偏差小于10%。3种毒品的检测限分别为2 ng/mL、1 ng/mL和2 ng/mL。该方法灵敏度高、重现性好、操作简便,可用于鸦片类毒品滥用者及中毒者唾液中的毒品及其代谢物的检测。     

热解吸-电喷雾离子源-三重四极杆质谱法快速筛查火锅底料和肉汤中非法添加罂粟壳

通过简单的金属探针直接接触火锅底料和肉汤表面采集待测物,经热解吸离子源进一步热解吸和电喷雾离子化,最终进入三重四极杆质谱检测器在多反应监测模式下进行定性分析,实现了火锅底料和肉汤中罂粟壳的现场实时快速检测。结果表明,设置热解吸温度为260℃,以0.1%甲酸水溶液（含10 mmol/L甲酸铵-乙腈（1:1,v/v）作为注射溶剂、注射泵流速为200 μL/h时,仪器响应值最优,灵敏度最高;5种生物碱中罂粟碱、那可丁、蒂巴因在火锅底料和肉汤中的检出限均为2 μg/kg,可待因、吗啡在火锅底料中的检出限为10 μg/kg,在肉汤中的检出限为5 μg/kg。该法与罂粟壳胶体金卡片快检试剂盒相比,灵敏度具有明显优势。应用该法对50批次市售火锅底料、肉汤等样品进行检测,发现1批次鸡汤含有那可丁、罂粟碱、蒂巴因和吗啡4种生物碱,与高效液相色谱-三重四极杆质谱法的检测结果一致。由此说明该方法具有无需样品制备和色谱分离的特点,是一种快速、绿色、环保的分析方法,能够满足对食品中罂粟壳的快速定性分析。     

Detection of hazelnuts and almonds using commercial ELISA test kits

Three commercial sandwich enzyme-linked immunosorbent assay (ELISA) test kits for the detection of hazelnuts and almonds were evaluated. Limits of detection and dynamic ranges were determined for hazelnuts and almonds spiked into cooked oatmeal, dipping chocolate, and muffins (baked). The limit of detection values varied from 1 to 38 μg/g, depending on the food matrix and ELISA test kit. Percent recoveries based on the standards supplied with the test kits varied from 10% to 170%. It is impossible to ascertain whether the percent recoveries reflect the performance of the ELISAs or differences between the protein content of the nuts used to spike the samples and the test kit standards. Unfortunately, reference materials do not exist that can be used to compare the results from different test kits and standardize the test kit standards. Also, insufficient knowledge regarding the epitope specificity of the antibodies used in the ELISAs further hinders interpretation of the results generated by the different test kits.     

孔雀石绿的磁性免疫层析快速检测方法研究

开发了一种适用于现场快速检测孔雀石绿(MG)的免疫层析试纸条,在超顺磁性纳米微球上偶联MG单克隆抗体作为检测探针,分别将孔雀石绿完全抗原(MG-B SA)和羊抗鼠IgG喷涂于NC膜的T线和C线.结果 发现,T线最佳喷涂量为0.25 mg/mL,抗体最佳偶联量为20 μg,构建的试纸条可在25 min内实现养殖用水及鱼肉...     

Interlaboratory evaluation of two enzyme-linked immunosorbent assay kits for the determination of crustacean protein in processed foods

The labeling of foods containing material derived from crustaceans such as shrimp and crab is to become mandatory in Japan because of increases in the number of allergy patients. To ensure proper labeling, 2 novel sandwich enzyme-linked immunosorbent assay (ELISA) kits for the determination of crustacean protein in processed foods, the N kit (Nissui Pharmaceutical Co., Ltd, Ibaraki, Japan) and the M kit (Maruha Nichiro Holdings, Inc., Ibaraki, Japan), have been developed. Five types of model processed foods containing 10 and/or 11.9 microg/g crustacean soluble protein were prepared for interlaboratory evaluation of the performance of these kits. The N kit displayed a relatively high level of reproducibility relative standard deviation (interlaboratory precision; 4.0-8.4% RSDR) and sufficient recovery (65-86%) for all the model processed foods. The M kit displayed sufficient reproducibility (17.6-20.5% RSDR) and a reasonably high level of recovery (82-103%). The repeatability relative standard deviation (RSDr) values regarding the detection of crustacean proteins in the 5 model foods were mostly < 5.1% RSDr for the N kit and 9.9% RSDr for the M kit. In conclusion, the results of this interlaboratory evaluation suggest that both these ELISA kits would be very useful for detecting crustacean protein in processed foods.     

Diagnosis of Helicobacter pylori infection with the (13)C-urea breath test by means of GC-MS analysis

The diagnosis of Helicobacter pylori (H. pylori) infection by GC-MS detection of the (13)CO(2) enrichment in (13)C-urea breath test ((13)C-UBT) samples is reported. This study aimed to optimize the (13)C-UBT with regards to the diagnostic cut-off value, sampling time, and frequency. The H. pylori status of 103 dyspeptic patients was obtained by histological examination, the rapid urease test as well as with the GC-MS (13)C-UBT. Analytical and diagnostic accuracies were determined by comparison of the GC-MS (13)C-UBT results with that of the analytical and diagnostic gold standards, namely GC-isotope ratio MS (IRMS) and histology. The (13)CO(2) enrichment values obtained with GC-MS analysis, correlated favorably (r(2) = 0.993) with those obtained by GC-IRMS analysis. When compared to histology, the GC-MS (13)C-UBT had a diagnostic sensitivity of 92% and a specificity of 93%. The positive predictive value (PPV), negative predictive value (NPV), and accuracy were 95, 89, and 92%, respectively. It was concluded that SIM GC-MS is capable of analyzing nonradioactive (13)C-UBT samples, with a precision and accuracy sufficient to distinguish between H. pylori positive and negative patients.     

Immunochemical analytical methods for the determination of peanut proteins in foods

Peanut proteins can cause allergenic reactions that can result in respiratory and circulatory effects in the body sometimes leading to shock and death. The determination of peanut proteins in foods by analytical methods can reduce the risk of serious reactions in the highly sensitized individual by allowing for the detection of these proteins in a food at various stages of the manufacturing process. The method performance of 4 commercially available enzyme-linked immunosorbent assay (ELISA) kits was evaluated for the detection of peanut proteins in milk chocolate, ice cream, cookies, and breakfast cereals: ELISA-TEK Peanut Protein Assay, now known as "Bio-Kit" for peanut proteins, from ELISA Technologies Inc.; Veratox for Peanut Allergens from Neogen Corp.; RIDASCREEN Peanut Kit from R-Biopharm GmbH; and ProLisa from Canadian Food Technology Ltd. The 4 test kits were evaluated for accuracy (recovery) and precision using known concentrations of peanut or peanut proteins in the 4 food matrixes. Two different techniques, incurred and spiked, were used to prepare samples with 4 known concentrations of peanut protein. Defatted peanut flour was added in the incurred samples, and water-soluble peanut proteins were added in the spiked samples. The incurred levels were 0.0, 10, 20, and 100 microg whole peanut per g food; the spiked levels were 0.0, 5, 10, and 20 microg peanut protein per g food. Performance varied by test kit, protein concentration, and food matrix. The Veratox kit had the best accuracy or lowest percent difference between measured and incurred levels of 15.7% when averaged across all incurred levels and food matrixes. Recoveries associated with the Veratox kit varied from 93 to 115% for all food matrixes except cookies. Recoveries for all kits were about 50% for cookies. The analytical precision, as measured by the variance, increased with an increase in protein concentration. However, the coefficient of variation (CV) was stable across the 4 incurred protein levels and was 7.0% when averaged across the 4 food matrixes and analytical kits. The R-Biopharm test kit had the best precision or a CV of 4.2% when averaged across all incurred levels and food matrixes. Because measured protein values varied by test kit and food matrix, a method was developed to normalize or transform measured protein concentrations to an adjusted protein value that was equal to the known protein concentration. The normalization method adjusts measured protein values to equal the true protein value regardless of the type test kit or type food matrix.     

Application of a liquid chromatography tandem mass spectrometry method for the simultaneous detection of seven allergenic foods in flour and bread and comparison of the method with commercially available ELISA test kits

To protect the allergic consumer, analytical methods need to be capable of detecting allergens in finished products that typically contain multiple allergens. An LC/MS/MS method for simultaneous detection of seven allergens was developed and compared with commercially available ELISA kits. The detection capabilities of this novel method were demonstrated by analyzing incurred material containing milk, egg, soy, peanut, hazelnut, walnut, and almond. Bread was chosen as a model matrix. To assess the influence of baking on the method's performance, analysis was done before and after baking. The same samples were analyzed with ELISA test kits from ELISA Systems, Morinaga, Neogen, and r-Biopharm. Peanut, hazelnut, walnut, and almond could be detected with both ELISA and LC/MS/MS regardless of whether the product was baked or not. LC/MS/MS clearly showed superior detection of milk in processed matrixes compared to ELISA, which exhibited significantly lower sensitivities when analyzing the baked products. Similar results were obtained when analyzing egg; however, one kit was capable of detecting egg in the processed samples as well.     

Two new standard reference materials for the determination of drugs of abuse in human hair

Two new standard reference materials (SRM) for drugs of abuse in human hair have been developed. SRM 2379 consists of hair spiked with cocaine, benzoylecgonine, cocaethylene, phencyclidine, amphetamine, and methamphetamine. SRM 2380 consists of hair spiked with codeine, morphine, monoacetylmorphine, and tetrahydrocannabinol (THC). The SRMs were prepared by soaking the hair in a solution of the target analytes in water-dimethylsulfoxide. The concentration of each analyte was determined using two methods, one based upon gas chromatography/mass spectrometry (GC/MS) and one based upon liquid chromatography/mass spectrometry (LC/MS). Both methods used 0.1 M HCl for extraction of all the analytes from the hair, except for THC, which was extracted with 1 M NaOH. For isolation of the analytes from the extracts, the GC/MS-based methods used different clean-up procedures from those used for the LC/MS-based methods. The results from the two methods were in good agreement with mean differences for the analytes ranging from 4% to 16%. These materials will enable laboratories performing analyses of hair for drugs of abuse to test the accuracy of their methods.     

Certification of drugs of abuse in a human serum standard reference material: SRM 1959

A new standard reference material (SRM) for drugs of abuse in human serum (SRM 1959) has been developed. This SRM is intended to be used as a control material for laboratories performing analysis of drugs of abuse in blood to evaluate the accuracy of their methods. SRM 1959 is a frozen human serum material fortified with seven compounds for which analyses are performed to determine evidence of illegal drug use: benzoylecgonine (BZE), methadone (METH), methamphetamine (MAMP), morphine (MOR), nordiazepam (NOR), phencyclidine (PCP), and 11-nor-Δ⁹-tetrahydrocannabinol-9-carboxylic acid (THC-9-COOH). Two independent methods involving isotope dilution (ID)-gas chromatography/mass spectrometry (GC/MS) and ID-liquid chromatography/mass spectrometry (LC/MS) were used for the value assignment. For THC-9-COOH, an additional measurement using LC/tandem mass spectrometry (LC/MS/MS) was also included. All methods used isotopically labeled compounds as internal standards and solid-phase extractions to isolate the analytes from the serum. The GC/MS methods used different clean-up procedures from those used for the LC/MS-based methods. Repeatability with within-set coefficients of variation (CVs) ranged from 0.5% to 4.3% for the GC/MS methods and from 0.2% to 1.2% for the LC/MS-based methods. Intermediate precision with between-set CVs for all the methods ranged from 0.1% to 1.1%. Agreement between the GC/MS and LC/MS methods ranged from 0.8% to 8.8%. The results from the methods were combined to obtain the certified concentrations and their expanded uncertainties.