副溶血性弧菌细胞猝灭及代谢物组提取方法的优化

以气相色谱-质谱联用(GC-MS)为分析方法,比较了液氮和75%甲醇(-80℃)两种溶液对副溶血性弧菌细胞的猝灭效果,以及氯仿、75%冰甲醇、水、甲醇-氯仿-水(10∶3∶1,V/V)、甲醇-氯仿-水(3∶1∶1,V/V)、甲醇-氯仿(1∶1,V/V)6种提取剂对副溶血性弧菌代谢物组的提取效果。结果表明,用75%甲醇(-80℃)猝灭副溶血性弧菌时,出现了代谢物泄漏现象,而液氮猝灭则不存在这个现象;检索发现,采用75%冰甲醇提取获得了47种代谢物,峰面积标准偏差为8.02%,其它5种提取剂获得代谢物种类少于40种,且重现性差。比较色谱峰数量、面积和重现性后发现,液氮猝灭、75%冰甲醇提取适于副溶血性弧菌代谢物组提取。     

岩香菊精油的气相色谱-气相色谱-质谱联用分析

在植物挥发油等复杂有机混合物的气相色谱-质谱联用(GC-MS)分析中,常遇到分离不良的色谱峰,所取得的质谱不易识别和解析。多维色谱法则是解决复杂有机混合物分离的有力工具。对质谱工作而言,把多维色谱的卓越分离能力与质谱仪的定性鉴定能力结合起来,构成一个气相色谱-气相色谱-质谱联用(GC-GC-MS)系统,就能大大改进常规GC-MS系统的功能,但有关报道很少,尚未得到     

气相色谱-质谱联用在农药残留检测方面的应用进展

气相色谱-质谱联用(GC-MS)既具有气相色谱高分离效能,又具有质谱准确鉴定化合物结构的特点,可达到同时准确快速测定食品中微量的多种农药残留及衍生物,因此已被很多国家研究者开发和应用.GC/MS/MS,二维气相色谱、惰性离子源等是气相色谱-质谱联用新的进展.     

现代质谱及其联用技术在抗癌药物研究中的应用

综述了质谱及其联用技术(如气相色谱-质谱,液相色谱-质谱,毛细管电泳-质谱等)在抗癌药物的分离鉴定、药物代谢产物的研究及药物作用机理方面的应用,总结了其发展潜力。     

新型靛红腙类合成大麻素质谱裂解规律研究

研究了新型靛红腙类合成大麻素在电子轰击(EI)和电喷雾(ESI)电离模式下的质谱裂解规律,并建立了可疑物中该类合成大麻素的鉴定方法。采用气相色谱-质谱联用(GC-MS)和液相色谱-高分辨质谱联用(LC-Q-Orbitrap/MS)技术,对5种新型靛红腙类合成大麻素(MDA-19 (BZO-HEXOXIZID),5C-MDA-19 (Pentyl MDA-19,BZO-POXIZID),CHM-MDA-19 (BZO-CHMOXIZID),4en-pentyl MDA-19(BZO-4en-POXIZID),5F-MDA-19 (5F-BZO-POXIZID))的主要碎片离子和碎裂过程进行分析,并对获得的质谱图进行解析,推测该类合成大麻素的EI-MS及ESI-MSⁿ碎裂规律。EI-MS可获得比ESI-MSⁿ更多的碎片离子用于该类合成大麻素的结构推断。碎片离子6,7和8对应的质荷比(m/z)118 (C₈H₈N⁺),132(C₈H₆NO<...     

高效液相色谱-串联质谱法测定磷酸西格列汀中基因毒性杂质乙二胺的含量

通过对甲苯磺酰氯对乙二胺进行衍生化,采用高效液相色谱-串联质谱法(HPLC-MS/MS)测定磷酸西格列汀中基因毒性杂质乙二胺的含量。以Waters CORTECS^? C₁₈色谱柱为固定相,以不同体积比的5 mmol·L^-1乙酸铵-乙酸缓冲溶液(pH 5.6)和乙腈的混合溶液为流动相进行梯度洗脱。串联质谱分析中采用电喷雾离子源正离子(ESI⁺)模式,选择反应监测(SRM)模式。乙二胺的线性范围为0.50～33.5μg·L^-1,检出限(3.3s/k)为0.55μg·L^-1,以空白样品为基体进行加标回收试验,所得回收率为102%～103%。对平行配制的6份加标供试品溶液进行重复性和重现性试验,所得测定值的相对标准偏差均小于3.0%。     

裂解同时烷基化气相色谱/质谱鉴定醇酸树脂

 用裂解同时烷基化气相色谱-质谱联用技术（SPM-GC-MS）对不同类型的醇酸树脂进行分析研究,将衍生化试剂四甲基氢氧化胺与样品同时裂解,经高效毛细管气相色谱分离,质谱鉴定,可区分醇酸树脂中的多元醇、多元酸、植物油类型,由此对改性醇酸树脂作结构鉴定。与直接裂解-气相色谱-质谱联用技术比较,具有样品前处理快速、简单,用量少,灵敏度高,定性准确,谱图直观等特点。     

醋酸铀酰负离子气相分解反应的密度泛函理论研究

采用密度泛函理论(DFT), 选择杂化密度泛函TPSSh和TZVP基组, 对一个UO₂(CO₃)₃^4-负离子的结构进行优化, 理论计算所得结果(键长等参数)与实验数据一致. 应用TPSSh/TZVP(ECP)方法对醋酸铀酰负离子UO₂(CH₃COO)₃^-的气相分解反应进行了理论计算, 成功地解释了含+5价铀的气相自由基负离子的稳定性, 并对2个负离子(CH₃COO)UO₂CH₃^-和CH₃UO₂OH^-分别与水的复分解反应进行了理论计算, 所得数据与质谱的实验结果较好地吻合.     

热解析-气相色谱或气相色谱-质谱法分析大气可吸入颗粒物中的半挥发性有机化合物

研制了一种热解析装置,并与气相色谱或气相色谱-质谱联用,定性定量分析了大气可吸入颗粒物中的半挥发性有机物。装置为直热式加热,升温速率快;直接安装在色谱进样器上方,无需冷阱聚焦。将热解析装置与气相色谱联用,优化了样品承载体材质、热解析条件和进样模式,并用于16种多环芳烃和9种正构烷烃的检测。结果表明,热解析-气相色谱方法对多环芳烃和正构烷烃的检出限分别为0.014~0.093 ng和0.016~0.026 ng,线性相关系数大于0.9975;用于3个城市PM10中的痕量多环芳烃和正构烷烃的定量测定,回收率分别在95%~135%(多环芳烃)和95%~115%(正构烷烃)之间。将热解析装置与气相色谱-质谱联用,比较了3个城市7种粒径分布的PMx(x=10,5,2,1,0.5,0.25,0.1)中的多环芳烃和正构烷烃,结果表明,不同粒径颗粒物均含有正构烷烃和PAHs,但含量相差很大。     

金属离子对蛇毒蛋白生物活性及结构效应的影响

从旅顺产白眉蝮蛇(Gloydius blomhoffii brevicaudus, GBB) 蛇毒中纯化得到了3种电泳和质谱纯蛋白活性组分, 其酶解肽段采用高效液相色谱-电喷雾串联质谱(HPLC-nESI-MS/MS)进行序列测定, 与其它同源性蛇毒蛋白氨基酸序列比对发现, 3种蛋白为新的蛇毒磷脂酶A₂、类凝血酶和金属蛋白酶, 分别将其命名为GBB-bPLA₂, GBB-TLE和GBB-MP. 电感耦合等离子体发射光谱法(ICP-AES) 测得每个GBB-bPLA₂和GBB-MP中含有一个Ca²⁺; 每个GBB-TLE中含有2个Zn²⁺. Ca²⁺可分别使GBB-bPLA₂和GBB-MP的荧光发射波长向短波方向移动2.0和1.6 nm, 使二者的荧光发射强度提高14.0%和11.0%; Ca²⁺的存在可显著提高二者的热稳定性, 使GBB-bPLA₂和GBB-MP的热变性温度分别提高1.5和2.0 ℃. Zn²⁺使GBB-TLE的荧光发射强度增高4.3%, 但对GBB-TLE的酯酶水解活性、荧光发射波长和热变性温度无显著影响. 金属离子的存在能够不同程度地影响蛇毒蛋白结构热稳定性, 但对蛇毒蛋白生物活性的作用则不同.     

Pyrolysis mass spectrometry for distinguishing potential hoax materials from bioterror agents

Pyrolysis mass spectrometry (PyMS) was investigated as a rapid tool to distinguish potential bioterror hoax materials from samples containing pathogenic bacteria. A pyrolysis time-of-flight (TOF) mass spectrometer equipped with an alternative ionization technique, metastable atom bombardment (MAB), was used to produce sample spectra. These spectra were analyzed by principal component and discriminant analysis for pattern recognition. Materials investigated were two strains of Vibrio parahaemolyticus, one of which produced the tdh toxin, two Salmonella enterica serotypes, a biological mosquito control product containing spores of Bacillus thuringiensis, and several white to off-white powders (which could be used as hoax materials), such as flour, corn starch, methyl cellulose, and xanthan gum. PyMS distinguished bacterial samples from hoax materials. Furthermore, pattern analysis differentiated Vibrios from Salmonellae, Salmonella enterica Anatum from S. enterica Heidelberg, and the two V. parahaemolyticus strains from each other. The B. thuringiensis mixture was distinguished from other bacteria and powders, suggesting that PyMS with pattern recognition may differentiate samples containing pathogens, including Bacillus spp., from nonbiological agents and that it can be a rapid method for detection of bacteria. MS data acquisition took only 7 min for each sample.     

Evaluation of different polymerase chain reaction methods for the identification of Vibrio parahaemolyticus strains isolated by cultural methods

Control of contamination by Vibrio parahaemolyticus in fishery products is often hampered by the lack of standardized methods and by the uncertainty associated with biochemical identification of the isolates. In this study, 5 polymerase chain reaction (PCR) methods for the identification of V. parahaemolyticus to the species level were evaluated by using 25 Vibrio reference strains and 163 isolates from fishery products, environmental sources, and clinical samples. Sequence targets of the methods were toxR, gyrB, and tlh genes (tested with 2 protocols), and the fragment pR72H. Isolate identification was confirmed by sequencing of the 16S rRNA gene and by PCR protocols for the identification of other Vibrio species. The PCR assay targeting the toxR gene achieved the highest performance (100% inclusivity and exclusivity). The 2 PCR protocols based on tlh gene detection, although showing the same inclusivity (100%), differed in the exclusivity (50 and 91%, respectively). Finally, the results provided by the PCR assays targeting the gyrB gene and pR72H fragment were less reliable and, in some cases, difficult to assess. According to the results of this study, the characteristics of accuracy expressed by the toxR identification method make it a suitable candidate as a reference method for the molecular identification of V. parahaemolyticus strains.     

Urinary Metabonomics Study of Heart Failure Patients with HILIC and RPLC Separation Coupled to TOF–MS

In this study, urinary metabolic profiles of patients with heart failure (HF) and healthy individuals were analyzed by LC-TOF–MS. Both reversed-phase chromatography and hydrophilic interaction chromatography were used to separate the endogenous metabolites in urine. Partial least-squares to latent structure-discriminant analysis was used for discriminating HF patients from healthy persons and the selection of potential biomarkers. The results suggested that the combination of LC–MS and multivariate statistical analysis could be used for HF diagnosis. The MS/MS experiments were carried out to identify the potential biomarkers which are important for the contribution to the discrimination. As a result, 12 potential biomarkers for HF were identified and the related metabolic pathways were studied.     

气相色谱-质谱法对当归及其炮制品挥发油的指纹图谱和潜在标志物研究

建立了一种基于气相色谱-质谱技术(GC-MS)的化学指纹图谱,以发现当归及其不同炮制品潜在标志物的方法.利用GC-MS获得当归及其不同炮制品挥发油化学指纹图谱,对产生的75样本×259变量数据进行归一化、修正80％规则和数据缩放等方法预处理,通过正交校正偏最小二乘法(OPLS)模式识别方法对样品进行模式识别,根据模型的变量重要性因子(VIP)和非参数检验结果筛选出12个潜在标志物.经相关分析和结构鉴定,其中11个化合物分别被鉴定为丁内酯、萜烯醇、6-丁基-1,4环庚二烯、2-壬酮、6-十一烷酮、2-甲氧基苯酚、δ-榄香烯、4,5,6,7-四甲基苯酞、Z-丁烯基酞内酯、亚油酸甲酯、1,7-异丙基-4-甲基-1,4,5,6,7,7a-六氢-2H-茚-2-酮.     

酚类环境雌激素的色谱分析方法

综述了近年来酚类环境雌激素的色谱分析研究进展,包括气相色谱和气质联用,高效液相色谱和各种检测器联用技术。比较了使用气相色谱和液相色谱两种方法的优缺点,并对环境雌激素样品预处理作了介绍。     

Metabonomics investigation of human urine after ingestion of green tea with gas chromatography/mass spectrometry, liquid chromatography/mass spectrometry and (1)H NMR spectroscopy

A method using gas chromatography/mass spectrometry (GC/MS), liquid chromatography/mass spectrometry (LC/MS) and (1)H NMR with pattern recognition tools such as principle components analysis (PCA) was used to study the human urinary metabolic profiles after the intake of green tea. From the normalized peak areas obtained from GC/MS and LC/MS and peak heights from (1)H NMR, statistical analyses were used in the identification of potential biomarkers. Metabolic profiling by GC/MS provided a different set of quantitative signatures of metabolites that can be used to characterize the molecular changes in human urine samples. A comparison of normalized metabonomics data for selected metabolites in human urine samples in the presence of potential overlapping peaks after tea ingestion from LC/MS and (1)H NMR showed the reliability of the current approach and method of normalization. The close agreements of LC/MS with (1)H NMR data showed that the effects of ion suppression in LC/MS for early eluting metabolites were not significant. Concurrently, the specificity of detecting the stated metabolites by (1)H NMR and LC/MS was demonstrated. Our data showed that a number of metabolites involved in glucose metabolism, citric acid cycle and amino acid metabolism were affected immediately after the intake of green tea. The proposed approach provided a more comprehensive picture of the metabolic changes after intake of green tea in human urine. The multiple analytical approach together with pattern recognition tools is a useful platform to study metabolic profiles after ingestion of botanicals and medicinal plants.     

Characteristics of the H(+)-translocating adenosine triphosphatase of Vibrio parahaemolyticus

We have characterized H(+)-translocating adenosine triphosphatase (ATPase) in membrane vesicles of Vibrio parahaemolyticus. The ATPase required high concentrations (about 0.5 M) of Na2SO4 (or other salts) for its maximum activity. Magnesium ion stimulated the ATPase activity, but Ca2+ did not. The activity of ATPase was inhibited by tetrachlorosalicylanilide, an H+ conductor, but not by another H+ conductor, carbonylcyanide-m-chlorophenylhydrazone. The activity was strongly inhibited by dicyclohexylcarbodiimide or Zn2+, and partially inhibited by azide, but not at all by vanadate.     

Fully automated trace level determination of parent and alkylated PAHs in environmental waters by online SPE-LC-APPI-MS/MS

Polycyclic aromatic hydrocarbons (PAHs) are ubiquitous compounds that enter the environment from natural and anthropogenic sources, often used as markers to determine the extent, fate, and potential effects on natural resources after a crude oil accidental release. Gas chromatography-mass spectrometry (GC-MS) after liquid–liquid extraction (LLE+GC-MS) has been extensively used to isolate and quantify both parent and alkylated PAHs. However, it requires labor-intensive extraction and cleanup steps and generates large amounts of toxic solvent waste. Therefore, there is a clear need for greener, faster techniques with enough reproducibility and sensitivity to quantify many PAHs in large numbers of water samples in a short period of time. This study combines online solid-phase extraction followed by liquid chromatography (LC) separation with dopant-assisted atmospheric pressure photoionization (APPI) and tandem MS detection, to provide a one-step protocol that detects PAHs at low nanograms per liter with almost no sample preparation and with a significantly lower consumption of toxic halogenated solvents. Water samples were amended with methanol, fortified with isotopically labeled PAHs, and loaded onto an online SPE column, using a large-volume sample loop with an auxiliary LC pump for sample preconcentration and salt removal. The loaded SPE column was connected to an UPLC pump and analytes were backflushed to a Thermo Hypersil Green PAH analytical column where a 20-min gradient separation was performed at a variable flow rate. Detection was performed by a triple-quadrupole MS equipped with a gas-phase dopant delivery system, using 1.50 mL of chlorobenzene dopant per run. In contrast, LLE+GC-MS typically use 150 mL of organic solvents per sample, and methylene chloride is preferred because of its low boiling point. However, this solvent has a higher environmental persistence than chlorobenzene and is considered a carcinogen. The automated system is capable of performing injection, online SPE, inorganic species removal, LC separation, and MS/MS detection in 28 min. Selective reaction monitoring was used to detect 28 parent PAHs and 15 families of alkylated PAHs. The methodology is comparable to traditional GC-MS and was tested with surface seawater, rainwater runoff, and a wastewater treatment plant effluent. Positive detections above reporting limits are described. The virtual absence of sample preparation could be particularly advantageous for real-time monitoring of discharge events that introduce PAHs into environmental compartments, such as accidental releases of petroleum derivates and other human-related events. This work covers optimization of APPI detection and SPE extraction efficiency, a comparison with LLE+GC-MS in terms of sensitivity and chromatographic resolution, and examples of environmental applications.     

Concentration of sodium ion as the determining factor for the association of dansyl amino acids with the teicoplanin molecule in reversed-phase liquid chromatography

The mechanism of the binding of D,L dansyl amino acids to teicoplanin was investigated. Na+ was used as an indicator of the interactions between the solutes and teicoplanin. The number (n) of sodium ions, Na+, excluded from the solute-teicoplanin interface when analyte transfer occurred was determined. A thermodynamic study and enthalpy-entropy compensation were performed to further explore the interaction mechanism. From these results, it was shown that teicoplanin was balanced between 2 conformational states characterized by distinct enantioselective properties. This approach indicates that liquid chromatography (LC) is a useful tool to extract physicochemical and molecular information from retention data. Thus, LC can be used as a complementary technique with the conventional techniques of molecular interaction analysis.     

ULTRAVIOLET SENSITIVITY OF VIBRIO PARAH AEMOLYTICUS, A CAUSATIVE BACTERIUM OF FOOD POISONING

Abstract. A pathogenic strain of Vibrio parahaemolyticus , strain WP1, is about 5 times more sensitive to killing by ultraviolet light than is the non-pathogenic strain WP28, but WP1 cells have an efficient liquid-holding recovery. The cellular DNA of both strains is fragmented shortly after ultraviolet irradiation, but the fragmented DNA is converted in a short time to the initial large molecular size in WP28 cells. In WP1 cells, however, the DNA molecules were degraded rapidly without any apparent rejoining in a growth condition. Post-irradiation liquid-holding made the DNA of WP1 cells stable, as supported by the recovery of DNA synthetic activity in these cells.