共查询到19条相似文献,搜索用时 140 毫秒
1.
用二维(弱阳,疏水)色谱柱首次完成了在线单柱二维液相色谱法快速纯化牛胰腺中的细胞色素C.在将牛胰腺粗提液进样到该二维色谱柱后,在弱阳离子交换模式下,以梯度洗脱方式进行一维色谱分离,并将分离得到的细胞色素C样品液收集到色谱仪的附加样品储液管内.然后将储液管中样品液全部排出,并二次进样到同一根二维色谱柱中,与此同时也完成了对该样品液的缓冲溶液交换,按疏水色谱(HIC)分离模式进行分离.最终对细胞色素C完成了第二维的HIC纯化.上述全部操作均为在线,在一具有正压的封闭体系中进行并可在52分钟内完成.细胞色素C的最终产品纯度高达94.7%(RSD=1.91%),质量回收率为80.5%(RSD=2.20%).预计此在线单柱二维液相色谱法也可能用于牛胰腺中其他功能蛋白的快速纯化,并可能将其放大到制备和生产规模. 相似文献
2.
建立了在线净化/固相萃取(SPE)-高效液相色谱(HPLC)快速、准确测定饮用水和环境水体中的两种痕量除草剂百草枯和敌草快的方法。样品用大体积自动进样器注入在线净化小柱并流经固相萃取小柱,通过双梯度高效液相色谱系统中的上样泵实现净化和富集后,通过阀切换将固相萃取小柱切换至分析流路中;用分析泵将待测物从富集柱冲洗至分析柱进行测定。上样泵流速和分析泵流速分别为0.7和0.6 mL/min,采用等度洗脱方式完成两种除草剂的分离和检测。检测波长分别为260 nm (百草枯)和311 nm (敌草快),进样体积为2.5 mL,整个分析时间为16 min。该方法在1.0~20 μg/L范围内线性关系良好,两种除草剂的线性相关系数均大于0.9980,检出限分别为0.10和0.12 μg/L(S/N=3)。该方法前处理简单,快速,可用于饮用水和环境水体中痕量除草剂的测定。 相似文献
3.
4.
《分析化学》2014,(12):1873
高效液相色谱的应用范围十分广泛,约有80%的有机物均可使用高效液相色谱进行分析。近年来其发展颇为迅猛,功能不断完善。2006年获得匹兹堡金奖产品的赛默飞UltiMate 3000 DGLC双三元液相色谱,便是杰出的代表。其采用独特的双泵设计,每个泵作为一个单独的体系,有各自独立的比例阀和流动相体系,同时单独控制三种不同的流动相,在Chromeleon变色龙软件的支持下,结合独特的阀切换技术,通过灵活的流路连接设计,一套系统即可以轻松实现在线固相萃取、中心切割及全二维液相色谱分离、流动相在线除盐、柱后衍生和反梯度补偿、并联/串联色谱等高级应用。本刊中有多篇文章利用UltiMate 3000 DGLC双三元液相色谱的在线固相萃取( online SPE)技术和二维及全二维液相色谱分离技术,解决了他们遇到的复杂难题。 相似文献
5.
在线固相萃取/高效液相色谱法测定环境水样中的4种痕量邻苯二甲酸酯 总被引:5,自引:0,他引:5
建立了一种在线固相萃取/高效液相色谱测定水样中4种痕量邻苯二甲酸酯(邻苯二甲酸甲酯、邻苯二甲酸乙酯、邻苯二甲酸丁酯和邻苯二甲酸(2-乙基)己酯)的新方法.样品由外加泵注入一根固相萃取小柱上进行富集,再将富集柱切换至高效液相色谱系统中,将富集在固相萃取小柱的邻苯二甲酸酯洗脱至分析柱进行分析.在线固相萃取柱为IonPac(... 相似文献
6.
7.
8.
建立了在线固相萃取/高效液相色谱-四极杆/静电场轨道阱高分辨质谱测定饲料中黄曲霉毒素B1(AFB1)、黄曲霉毒素B2(AFB2)、黄曲霉毒素G1(AFG1)及黄曲霉毒素G2(AFG2)的方法。采用IMMUNOPREPONLINE AFLATOXIN(Part Code:P900)柱为在线固相萃取柱,Diamonsil Plus C18(150 mm×4.6 mm,5μm)柱为分析柱。样品中加入一定量的Na Cl和乙腈-水(80∶20,体积比)溶解,超声提取后,用于后续进样。样品溶液注入在线固相萃取小柱中,通过阀切换技术和HPD共聚焦洗脱模式将保留在SPE柱上的靶标物转移到分析柱中继续进行分离分析,采用外标法定量,采用正离子全扫描模式进行分析。在优化的色谱-质谱条件下,该方法对4种黄曲霉毒素的线性范围为0.5~50.0μg/L,检出限可达0.2μg/kg,定量下限可达0.5μg/kg。在0.5、1.0、5.0μg/kg 3个加标水平下,饲料中4种黄曲霉毒素的回收率为94.6%~114.3%,相对标准偏差不大于8.3%。该方法分析时间短、自动化程度高、检测通量大、检测成本低,可作为饲料中AFB1、AFB2、AFG1、AFG2的快速检测方法。 相似文献
9.
建立了牛奶中环丙沙星、达氟沙星、恩诺沙星、沙拉沙星和二氟沙星残留量的快速测定方法。牛奶样品经0.2%三氯乙酸-乙腈(90∶10)沉淀蛋白后,直接进样分析,采用涡流色谱柱作为在线固相萃取柱,通过双梯度液相色谱的左泵结合大体积进样方式对目标分析物进行富集和净化,利用在线100μL定量环中的强洗脱溶剂快速转移目标分析物,并以右泵作为在线稀释泵和分析泵,通过柱头浓集作用改善分离效果。通过荧光检测,方法检出限为0.01~0.13μg/L,远低于欧盟规定限量,且在一定浓度范围内,方法的线性较好,加标回收率为75.9%~95.7%。该方法简便、快速、灵敏度较高,适用于牛奶样品中环丙沙星等5种兽药残留的快速检测。 相似文献
10.
在线固相萃取-超高效液相色谱-串联质谱法测定乳制品中双酚A等4种内分泌干扰物 总被引:2,自引:0,他引:2
建立了乳制品中三氯生、三氯卡班、双酚A和壬基酚4种内分泌干扰物的在线固相萃取超高压液相色谱-串联质谱(On-line SPE LC-MS/MS)检测方法。液态乳制品或奶粉样品中加入乙酸缓冲液,目标物经β-葡糖醛酸苷肽酶/芳基磺酸酯酶酶解后,用乙腈提取,冷冻离心10 min后,取上清液,用水稀释,在线固相萃取串联质谱法测定。样品溶液经Xbridge C8柱富集,BEH C18色谱柱分离,甲醇和水梯度洗脱,三重四极杆质谱电喷雾负离子模式下采集数据,同位素内标法定量。4种目标化合物的线性范围为0.005~5.0μg/L,相关系数R2>0.99;方法的定量限为0.03~1.0μg/kg,3个添加水平的平均加标回收率为80.2%~106.7%, RSD<15%。本方法快速、简单、灵敏度高,适用于乳制品中4种内分泌干扰物的同时检测。应用本方法对原料乳和北京市售液奶样品进行了分析,结果表明,壬基酚的检出率最高。 相似文献
11.
Telzenac® (Eltenac; 0.5 mg kg?1) was administered intravenously to two thoroughbred horses. After initial alkaline saponification followed by enzymolysis of the urinary phase II conjugates, the combined unconjugated compounds and aglycones were isolated by mixed mode solid phase extraction (SPE). The acidic isolate was either methylated or silylated (trimethylsilyl ether, TMS) and analysed by positive ion electron ionisation gas chromatography-mass spectrometry (GC-EI+-MS). Eltenac and two isobaric metabolites, hydroxyeltenac (aromatic oxidation) and eltenac sulfoxide were tentatively identified. Base peaks in the EI+ spectra of underivatised, methylated and TMS derivatised eltenac are formed by an initial loss of H2O, CH3OH or (CH3)3-Si-OH respectively, followed by successive losses of a chlorine atom and a carbonyl group. Similar fragmentation patterns were observed for the methyl and TMS derivatives of the two metabolites. Triamcinolone acetonide was used as the internal marker for the semi-quantification of eltenac. Selected samples were base-hydrolysed and extracted on-line on a C2 SPE column using a Prospekt sample handler. The retained analytes were eluted directly on to an analytical LC column and analysed by high performance liquid chromatography positive ion atmospheric pressure chemical ionisation MS in the selective ion recording mode. Most of the drug was excreted in less than 24 h. However it could still be detected in urine by full-scan GC-EI+-MS for over 96 h. 相似文献
12.
Alnouti Y Srinivasan K Waddell D Bi H Kavetskaia O Gusev AI 《Journal of chromatography. A》2005,1080(2):99-106
A technique using a fully automated on-line solid phase extraction (SPE) system (Symbiosis, Spark Holland) combined with liquid chromatography (LC)-mass spectrometry (MS/MS) has been investigated for fast bioanalytical method development, method validation and sample analysis using both conventional C18 and monolithic columns. Online SPE LC-MS/MS methods were developed in the automated mode for the quantification of model compounds (propranolol and diclofenac) directly in rat plasma. Accuracy and precision using online SPE LC-MS/MS with conventional C18 and monolithic columns were in the range of 88-111% and 0.5-14%, respectively. Total analysis cycle time of 4 min per sample was demonstrated using the C18 column. Monolithic column allowed for 2 min total cycle time without compromising the quality and validation criteria of the method. Direct plasma sample injection without on-line SPE resulted in poor accuracy and precision in the range of 41-108% and 3-81%. Furthermore, the increase in back pressure resulted in column damage after the injection of only 60 samples. 相似文献
13.
Zang X Luo R Song N Chen TK Bozigian H 《Rapid communications in mass spectrometry : RCM》2005,19(22):3259-3268
An on-line solid-phase extraction liquid chromatography/tandem mass spectrometry (SPE LC/MS/MS) assay using a newly developed SPE column and a monolithic column was developed and validated for direct analysis of plasma samples containing multiple analytes. This assay was developed in an effort to increase bioanalysis throughput and reduce the complexity of on-line SPE LC/MS/MS systems. A simple column-switching configuration that requires only one six-port valve and one HPLC pumping system was employed for on-line plasma sample preparation and subsequent gradient chromatographic separation. The resulting analytical method couples the desired sensitivity with ease of use. The method was found to perform satisfactorily for direct plasma analysis with respect to assay linearity, specificity, sensitivity, precision, accuracy, carryover, and short-term stability of an eight-analyte mixture in plasma. A gradient LC condition was applied to separate the eight analytes that cannot be distinctly differentiated by MS/MS. With a run time for every injection of 2.8 min, a minimum of 300 direct plasma injections were made on one on-line SPE column without noticeable changes in system performance. Due to the ruggedness and simplicity of this system, generic methods can be easily developed and applied to analyze a wide variety of compounds in a high-throughput manner without laborious off-line sample preparation. 相似文献
14.
建立了同时测定全血、尿液和肝组织等生物样品中18种氨基甲酸酯类农药的在线固相萃取/液相色谱-线性离子阱质谱(On-line SPE/LC-LIT/MS)分析方法。样品经乙腈处理,稀释和离心后直接进样。经Waters OasisHLB在线SPE柱富集纯化,以BETASIL C18柱为分析柱,甲醇-水(均含0.1%甲酸)为流动相进行梯度洗脱;使用电喷雾电离(ESI)正离子模式测定,扫描方式为选择反应监测(SRM)和连续反应监测(CRM)。18种农药在考察的质量浓度范围内线性关系良好(权重因子1/X),相关系数为0.994 3~0.999 4;在全血和尿液中的检出限为0.1~5 ng/m L,在肝组织中的检出限为0.1~5 ng/g;3个加标水平的回收率为90.2%~114.5%,相对标准偏差(n=4)为0.5%~7.5%。该方法简单准确,灵敏度高,能够满足生物样品中18种氨基甲酸酯类农药的快速分析要求。 相似文献
15.
建立一种在线固相萃取-离子色谱测定4种芳环磺酸盐中硫酸根离子含量的新方法。将自装填的多孔石墨化碳固相萃取柱应用于离子色谱系统,对样品进行在线前处理。样品经过多孔石墨化碳固相萃取柱基体消除后进入收集环,通过阀切换方式使待测硫酸根离子转入阴离子分析柱和检测系统。固相萃取流路用1.5 mmol/L碳酸钠以0.8 mL/min的流速对基体在线富集,进样量为20μL,分析柱为SH-AC-3(250 mm×4.0 mm)+SH-AG-3(50 mm×4.0 mm)色谱柱,柱温为35℃,在6 mmol/L碳酸钠-4 mmol/L碳酸氢钠条件下等度洗脱,流速为0.8 mL/min。结果表明:硫酸根离子在0.50~20.00 mg/L范围内呈良好的线性关系,线性相关系数为0.998 3,保留时间、峰高和峰面积的相对标准偏差均在0.28%~2.86%之间,方法检出限为0.010 6 mg/L,回收率为91.01%~109.3%,具有良好的线性关系和重复性。整个在线分析过程在25 min之内完成。该方法进样量少、快速、高效。 相似文献
16.
Chen L Ding L Jin H Song D Zhang H Li J Zhang K Wang Y Zhang H 《Analytica chimica acta》2007,589(2):239-246
A rapid technique based on dynamic microwave-assisted extraction coupled with on-line solid-phase extraction of high-performance liquid chromatography (DMAE-SPE-HPLC) has been developed. A TM010 microwave resonance cavity built in the laboratory was applied to concentrate the microwave energy. The sample placed in the zone of microwave irradiation was extracted with 95% acetonitrile (ACN) aqueous solution which was driven by a peristaltic pump at a flow rate of 1.0 mL min−1. The extraction can be completed in a recirculating system in 10 min. When a number of extraction cycles were completed, the extract (1 mL) was diluted on-line with water. Then the extract was loaded into an SPE column where the analytes were retained while the unretained matrix components were washed away. Subsequently, the analytes were automatically transferred from the SPE column to the analytical column and determined by UV detector at 238 nm. The technique was used for determination of organochlorine pesticides (OCPs) in grains, including wheat, rice, corn and bean. The limits of detection of OCPs are in the range of 19-37 ng g−1. The recoveries obtained by analyzing the four spiked grain samples are in the range of 86-105%, whereas the relative standard deviation (R.S.D.) values are <8.7% ranging from 1.2 to 8.7%. Our method was demonstrated to be fast, accurate, and precise. In addition, only small quantities of solvent and sample were required. 相似文献
17.
The present study describes the first fully automated method based on on-line solid-phase extraction (SPE) coupled to hydrophilic interaction chromatography-electrospray-mass spectrometry (HILIC-(ESI)MS) to determine a group of polar drugs that includes illicit drugs (such as cocaine, morphine, codeine and metabolites) and pharmaceuticals in environmental water samples. The SPE was performed using a highly retentive polymeric sorbent. The HILIC separation was optimised and the initial high organic content of the chromatographic mobile phase, was also suitable for the proper on-line elution of the analytes retained in the SPE column and for enhancing the ESI ionisation efficiency. This method allows the loading of samples of up to 250ml of ultrapure water or 10ml of environmental water samples spiked at low ngl(-1) levels of the analytes. The method yields near 100% recoveries for all the analytes. The method was also validated with environmental water samples with linear ranges from 5 to 1000ngl(-1) and limits of detection ≤2ngl(-1) for most of the compounds. 相似文献
18.
Kuhlenbeck DL Eichold TH Hoke SH Baker TR Mensen R Wehmeyer KR 《European journal of mass spectrometry (Chichester, England)》2005,11(2):199-208
An on-line liquid chromatography/tandem mass spectrometry (LC-MS/MS) procedure, using the Prospekt- 2 system, was developed and used for the determination of the levels of the active ingredients of cough/cold medications in human plasma matrix. The experimental configuration allows direct plasma injection by performing on- line solid phase extraction (SPE) on small cartridge columns prior to elution of the analyte(s) onto the analytical column and subsequent MS/MS detection. The quantitative analysis of three analytes with differing polarities, dextromethorphan (DEX), dextrorphan (DET) and guaifenesin (GG) in human plasma presented a significant challenge. Using stable-isotope-labeled internal standards for each analyte, the Prospekt-2 on-line methodology was evaluated for sensitivity, suppression, accuracy, precision, linearity, analyst time, analysis time, cost, carryover and ease of use. The lower limit of quantitation for the on-line SPE procedure for DEX, DET and GG was 0.05, 0.05 and 5.0 ng mL(-1), respectively, using a 0.1 mL sample volume. The linear range for DEX and DET was 0.05-50 ng mL(-1) and was 5-5,000 ng mL(-1) for GG. Accuracy and precision data for five different levels of QC samples were collected over three separate days. Accuracy ranged from 90% to 112% for all three analytes, while the precision, as measured by the %RSD, ranged from 1.5% to 16.0% 相似文献
19.
An analytical method was developed for the determination in urine of 2 metabolites of diazinon: 6-methyl-2-(1-methylethyl)-4(1H)-pyrimidinone (G-27550) and 2-(1-hydroxy-1-methylethyl)-6-methyl-4(1H)-pyrimidinone (GS-31144). Two of the urine sample preparation procedures presented rely on gas chromatography/mass selective detection (GC/MSD) in the selected ion monitoring mode for determination of G-27550. For fast sample preparation and a limit of quantitation (LOQ) of 1.0 ppb, urine samples were purified by using ENV+ solid-phase extraction (SPE) columns. For analyte confirmation at an LOQ of 0.50 ppb, classical liquid/liquid partitioning was used before further purification in a silica SPE column. An SPE sample preparation procedure and liquid chromatography/electrospray ionization/mass spectrometry/mass spectrometry (LC/ESI/MS/MS) were used for both G-27550 and GS-31144. The limit of detection was 0.01 ng for G-27550 with GC/MSD, and 0.016 ng when LC/ESI/MS/MS was used for both G-27550 and GS-31144. The LOQ was 0.50 ppb for G-27550 when GC/MSD and the partitioning/SPE sample preparation procedure were used, and 1.0 ppb for the SPE only sample preparation procedure. The LOQ was 1.0 ppb for both analytes when LC/ESI/MS/MS was used. 相似文献