夏天无中普鲁托品高效液相含量测定提取方法的研究

采用RP -HPLC测定了夏天无中普鲁托品的含量 ,比较了超声时间、提取溶剂、加热对夏天无中普鲁托品含量测定的影响 ,结果表明 :加热后超声法对普鲁托品的提取比普通超声提取法高 30 %以上     

一产香银杏内生真菌挥发油化学成分的GC-MS研究

利用气相色谱 质谱联用法 (GC MS) ,DB 5 30m× 0 .2 5mm× 0 .2 5 μm色谱柱 ,对产香银杏内生菌(Fusariumsp .)挥发油进行GC MS分析 ,分离出 2 4种组分 ,采用峰面积归一化 ,据GC MS联用所得质谱信息 ,鉴定出 1 5种成分 ,共占其色谱流出组分的 5 1 .0 7%。     

乌榄叶挥发油化学成分分析

采用气相色谱-质谱联用(GC-MS)方法首次对乌榄叶挥发油成分进行了测试分析,并应用色谱峰面积归一化法计算各成分的相对含量。分离出19个峰,确认了19种化合物,所鉴定的组分占挥发油总量的100%,主要成分是石竹烯(33.47)、α-蒎烯(18.03%)、d-柠檬烯(16.82%)、α-侧柏烯(11.74%)和α-水芹烯(6.51%)。     

臭茉莉叶挥发油化学成分的研究

利用GC-MS联用技术研究了臭茉莉叶挥发油的化学成分,应用色谱峰面积归一化法计算各成分的相对百分含量.分离出49个峰,鉴定了其中的34种成分,所鉴定的组分占挥发油总量的95.17 %.     

黄连-黄芩药对化学成分的UPLC-PDA-MS分析

本文建立了黄连-黄芩药对化学成分的UPLC-PDA-MS分析方法。实验采用ACQUITY UPLC BEH C18柱,流动相为0.05%甲酸水和甲醇梯度洗脱;检测波长280 nm;MS一级全扫描模式。综合分析标准品及不同样品的色谱峰保留时间、紫外光谱及MS一级全扫描质谱图,归属了黄连-黄芩提取液中的12个主要色谱峰,鉴别出8种成分,推断出2种成分,同时对鉴别出的8种成分进行了定量,被测成分在线性范围内均具有良好的线性关系(r≥0.9991),精密度、重复性的RSD均小于5.0%,加样回收率基本在95%～105%内。本方法快捷、准确,重复性好,能同时测定8个主要化学成分,可较全面地控制黄连-黄芩药对化学成分的含量。     

峰胶乙醇提取物化学成分的GC／MS研究

利用气相色谱-质谱联用法(GC-MS),HP-5MS 30 m×0.25 mm×0.25μm5%苯甲基聚硅氧烷弹性石英毛细管柱,对峰胶乙醇提取物化学成分进行了分析,分离出127种组分,采用峰面积归一化定量,鉴定出45种成分,共占其色谱流出组分总量的82.8%,其中萜类、黄酮类化合物约占31%.     

不同产地土荆芥挥发油GC指纹图谱研究

采用水蒸气蒸馏法提取了12个产地土荆芥的挥发油,通过GC法分析其成分.运用中药色谱指纹图谱相似度建立共有模式,以相关度评价图谱的相似性,以共有峰与对照峰的比值对各产地土荆芥药材挥发油进行聚类分析.结果表明:12个产地的土荆芥药材的挥发油气相色谱指纹图谱有17个共有峰,其中气相色谱指纹图谱的相似度在0.85以上的有11个,12个产地的土荆芥药材的挥发油可通过系统聚类归为两类,不同产地土荆芥药材的挥发油相似度较高.该方法简便,所得挥发油中各成分分离度高,建立的指纹图谱重现性好,可作为土荆芥药材挥发油的质量控制方法之一.     

毛脉酸模不同生长发育期HPLC色谱指纹图谱研究

采用HPLC-DAD方法,梯度洗脱,对10批不同生长发育期毛脉酸模根样品进行主成分分析。色谱条件为:Planetsil C18分析柱(5μm, 200 mm×4.6 mm),预柱Phenomenex ODS-C18(4×3.0 mm ID),柱温40℃,流动相A为甲醇;流动相B为水(磷酸调pH值为2.0),流动相A从30%甲醇到100%甲醇,时间为0~50 min,检测波长254 nm。10批毛脉酸模样品得到的色谱指纹图谱有27个共有峰,其特征峰指纹图谱可分为Ⅰ, Ⅱ, Ⅲ三组:第Ⅰ组包括0~17 min(1~14号峰),第Ⅱ组包括17~35 min(15~24号峰),第Ⅲ组包括35~50 min(25~27号峰)。HPLC-DAD方法分析毛脉酸模主成分,方法准确可靠,其本身具有多成分同时定性的优势;27个共有峰的出峰先后顺序及相对含量极具特征性、专属性,重复性好,形成了毛脉酸模特有的HPLC色谱指纹图谱,可作为毛脉酸模内在质量评价、鉴定及其最佳采收期确定提供科学依据。     

茯苓皮与白茯苓中三萜类成分的HPLC 指纹图谱与化学模式识别研究

建立茯苓皮与白茯苓中三萜类成分的HPLC指纹图谱，并对其进行化学模式识别研究，为菌物药茯苓的质量控制及标准制定提供依据。采用HPLC法，Agilent 5 TC-C₁₈ (2)色谱柱(250 mm×4.6 mm, 5μm),以乙腈-0.3%磷酸水溶液为流动相梯度洗脱，流速1.0 mL/min,柱温25℃,变波长方式检测，采集波长为242、203 nm,进样量10μL。建立了茯苓皮与白茯苓中三萜类成分指纹图谱，应用聚类分析(CA)、主成分分析(PCA)手段结合相似度评价对实验数据进行识别，以分析不同茯苓样品的相似性和差异性，找出可反映茯苓皮与白茯苓三萜成分特征的关键色谱峰。茯苓皮与白茯苓三萜成分指纹图谱的共有模式下确认了6个共有峰，分别为2号峰(茯苓新酸B)、3号峰(去氢土莫酸)、4号峰(茯苓新酸A)、9号峰(去氢茯苓酸)、10号峰(茯苓酸)、12号峰(松苓新酸);不同来源的茯苓样品相同药用部位间相似度均在0.90以上；依据CA和PCA分析结果将茯苓样品药用部位分为两大类。PCA分析结果显示包括代表去氢土莫酸、去氢茯苓酸、茯苓酸成分在内的7个共有色谱峰(3、5和6、...     

小叶臭黄皮叶挥发油化学成分的研究

采用水蒸气蒸馏法提取小叶臭黄皮叶挥发油,运用毛细管气相色谱-质谱联用法对挥发油成分进行了分析,共分离出84个峰,鉴定了其中的66种成分,所鉴定成分占挥发油总量的94.52%.其主要化学成分为α-芹子烯(15.76%)、石竹烯(15.05%)、β-芹子烯(9.54%)、α-蒎烯(6.43%)和α-石竹烯(5.39%)等.     

Complete anaerobic mineralization of pentachlorophenol (PCP) under continuous flow conditions by sequential combination of PCP‐dechlorinating and phenol‐degrading consortia

Complete mineralization of 50 µM of pentachlorophenol (PCP) was achieved anaerobically under continuous flow conditions using two columns connected in series with a hydraulic retention time of 14.2 days, showing the highest reported mineralization rate yet of 3.5 µM day^?1. The first column, when injected with a reductive PCP dechlorinating consortium, dechlorinated PCP to mainly phenol and traces of 3‐chlorophenol (3‐CP) using lactate supplied continuously as an electron donor. The second column, with an anaerobic phenol degrading consortium, decomposed phenol and 3‐CP under iron‐reducing conditions with substantial fermentative degradation of organic compounds. When 20 mM of lactate was introduced into the first column, the phenol degradation activity of the second column was lost in a short period of time, because the amorphous Fe(III) oxide (FeOOH) that had been packed in the column before use was depleted by lactate metabolites, such as acetate and propionate, flowing into the second column from the first column. The complete mineralization of PCP was maintained for a long period by reducing the lactate concentration to 4 mM, effectively extending the longevity of second‐column activity with no depletion of FeOOH for more than 200 pore volumes (corresponding to 3,000 days). The carbon balance showed that 50 µM PCP and 4 mM lactate in the influent had transformed to CO₂ (81%) and CH₄ (3%) and had contributed to biomass growth (8%). A comparison of the microbial consortia introduced into the columns and those flowing out from the columns suggested that the introduced population did not flow out during the experiments, although the microbial composition of the phenol column was considered to be affected by the inflow of microbes from the PCP dechlorination column. These results suggest that a sequential combination of reductive dechlorinating and anaerobic oxidizing consortia is useful for anaerobic remediation of chlorinated aromatic compounds in a microbial permeable reactive barrier. Biotechnol. Bioeng. 2010;107: 775–785. © 2010 Wiley Periodicals, Inc.     

Continuous fixed-bed column study and adsorption modeling: Removal of cadmium (II) and lead (II) ions in aqueous solution by dead calcareous skeletons

The sorption of Cd(II) and Pb(II) ions was conducted in a continuous fixed-bed column by using dead calcareous skeletons (CS). The column performances were evaluated by varying the adsorbent bed height, influent flow rate and metals initial concentration. The breakthrough curve for the bed height indicated that a longer bed column prolonged the life span of the column with a maximum capacity of 26.447 and 38.460 mg/g for the Cd(II) and Pb(II) column, respectively. The increased flow rate and initial concentration caused the column exhaustion time to occur earlier. The experimental column data were also expressed in column adsorption models, namely, the Thomas, Yoon–Nelson and Adam–Bohart models. The Thomas model fitted well with the Cd(II) data with the correlated curve (r² > 0.9). The Yoon–Nelson model was selected to predict the 50% breakthrough time achieved by the column system and provided the estimated breakthrough time for the columns that were not exhausted during the operation. The Adam–Bohart model was applicable for the initial part of adsorption with the saturation concentration data at the equilibrium. The saturation index of aragonite and calcite depicted that dissolution of calcium occurred in the aqueous solution. The experimental and theoretical data were correlated with a significant relationship trend (p < 0.01), which showed that the trend of experimental data fit well with the modeling trend. The trends of both the experimental and theoretical data were strongly and significantly correlated due to involving the column parameters and the components of CS.     

Improvement in HPLC separation of acetic acid and levulinic acid in the profiling of biomass hydrolysate

5-Hydroxymethylfurfural (HMF) and furfural could be separated by the Aminex HPX-87H column chromatography, however, the separation and quantification of acetic acid and levulinic acid in biomass hydrolysate have been difficult with this method. In present study, the HPLC separation of acetic acid and levulinic acid on Aminex HPX-87H column has been investigated by varying column temperature, flow rate, and sulfuric acid content in the mobile phase.The column temperature was found critical in resolving acetic acid and levulinic acid. The resolution for two acids increased dramatically from 0.42 to 1.86 when the column temperature was lowered from 60 to 30 °C. So did the capacity factors for levulinic acid that was increased from 1.20 to 1.44 as the column temperature dropped. The optimum column temperature for the separation was found at 45 °C. Variation in flow rate and sulfuric acid concentration improved not as much as the column temperature did.     

Narrowbore high-performance liquid chromatography for the simultaneous determination of sildenafil and its metabolite UK-103,320 in human plasma using column switching

A fully automated narrowbore high-performance liquid chromatography method with column switching was developed for the simultaneous determination of sildenafil and its active metabolite UK-103,320 in human plasma samples without pre-purification. Diluted plasma sample (100 μl) was directly introduced onto a Capcell Pak MF Ph-1 column (20×4 mm I.D.) where primary separation occurred to remove proteins and concentrate target substances using 15% acetonitrile in 20 mM phosphate solution (pH 7). The drug molecules eluted from the MF Ph-1 column were focused in an intermediate column (35×2 mm I.D.) by a valve switching step. The substances enriched in the intermediate column were eluted and separated on a phenyl-hexyl column (100×2 mm I.D.) using 36% acetonitrile in 10 mM phosphate solution (pH 4.5) when the valve status was switched back. The method showed excellent sensitivity (detection limit of 10 ng/ml), good precision (RSD≤2.3%) and accuracy (bias: ±2.0%) and speed (total analysis time 17 min). The response was linear (r²≥0.999) over the concentration range 10–1000 ng/ml.     

Removal of Phthalate Esters in Soil Column Inoculated with Microorganisms

The removal of phthalate esters, such as di-2-ethyl hexyl phthalate (DEHP) was efficiently effected by inoculating and retaining viable cells of Nocardia erythropolis, a bacterium known capable of rapidly degrading phthalate esters, in soil column. When an influent containing 3000 ppm of DEHP was passed through a column inoculated with Nocardia erythropolis, the eluent from the column was gas-chromatographically free of DEHP after 1 day. Residual DEHP on the support after 32 days in the column inoculated with Nocardia erythropolis was only 0.14% against the total amount of DEHP fed, whereas it was 5.2% in the uninoculated column. Microorganisms capable of utilizing DEHP were isolated from the inoculated and un- inoculated columns after 32 days operation and identified. The DEHP utilizing microorganisms in the inoculated column were found to belong to Nocardia erythropolis, Nocardia restricta and Pseudomonas putida (Biotype B), and those in the uninoculated column to Nocardia erythropolis, Pseudomonas putida (Biotype A and B) and Pseudomonas acidovorans. In particular, strain 1-1 of Nocardia erythropolis isolated from the inoculated column was morphologically and biochemically identical with the inoculated Nocardia erythropolis S-l. Ratio of all Nocardia erythropolis to total cells recovered increased from 10.8% immediately after inoculation to 27.2% after 32 days in inoculated column.     

Development and characterization of a chitosan-supported immunoaffinity chromatography column for the selective extraction of methandrostenolone from food and feed samples

The development of a chitosan-supported immunoaffinity chromatography (IAC) column and its application to the selective extraction of methandrostenolone (MA) from food and feed samples were described in this paper. Using hybridoma technique, a monoclonal antibody (mAb) against MA was produced. The IAC column was prepared by coupling the produced antibody with crosslinked chitosan. Scanning electron microscopy and IR spectroscopy was used to characterize the chitosan crosslinking and antibody coupling. 2% and 90% methanol were respectively selected as loading and eluting solution by optimization. The maximum capacity of the column for MA was 1790 ng/mL gel. The extraction recoveries of the column for MA at three different spiked concentrations ranged from 83.7 to 98.5%. After 2 cycles of usage, the column capacity and extraction recovery still remained 84.6% and 80.5%. To further verify the effect of matrix on the IAC cleanup, MA-fortified food and feed samples were extracted using the prepared IAC column, and MA recovery rates were found to be 86.2% and 70.4%, respectively.     

Continuous ethanol production using induced yeast aggregates

Summary The induction of yeast cell aggregates in a column reactor was initiated by packing yeast cell paste of Saccharomyces uvarum into the column, and then YMP broth was fed into the column from the bottom at a linear flow rate of 2.5 cm/h. Thereafter, yeast cells aggregated in the column within 48 h without a supply of oxygen. When this yeast aggregate column reactor was used for continuous ethanol production, a final ethanol concentration of 10.8% (w/v) was obtained from 23% (w/v) of glucose in a YMP broth with a dilution rate of 0.05 h^-1, and 4.9% (w/v) was obtained from 10% (w/v) of glucose with a dilution rate of 0.6 h^-1. The theoretical yield was above 97% in both cases. The ethanol production rates were 13 g¹ h^-1 l^-1 and 90 g¹ h^-1 l^-1 for producing 10.8% (w/v) and 4.9% (w/v) of ethanol respectively. This column reactor was maintained at a steady state for more than one month.     

聚焦色谱法测定肌型肌酸激酶亚型

报道了测定CK-MM亚型的聚焦色谱法,此法简单,快速,结果可靠,线性范围宽,最低检测限（8U／L）较正常参考值低,比国外报道的类似方法高6倍以上,分离度亦有改进.测定了20例健康人血清亚型分布,与文献报道结果相近.该法自动化程度高,已在急性心梗的诊断中实际应用.     

Resolution and determination of enantiomeric purity of the enantiomers of felodipine using chiral-AGP® as stationary phase

A direct chiral chromatographic reversed phase method for the determination of the enantiomers of felodipine is described. The influence of charged and uncharged modifiers as well as the effect of the mobile phase pH on the enantiomeric resolution is discussed. A high mobile phase pH and the addition of 2-propanol as organic modifier gave the highest separation factor (α = 1.3). The high mobile phase pH (pH = 7.6) is outside the recommended pH limit of silica based columns but was necessary to achieve baseline resolution of (R)- and (S)-felodipine. Improvement of column efficiency by increasing column temperature was utilized for optimization of the enantiomeric resolution (Rs = 1.7). The enantiomers of felodipine and three related compounds were separated within 15 min. The enantiomeric purity of (R)- and (S)-felodipine in injections and (R)-felodipine in bulk substance was higher than 99.5% and no racemization was observed after storage at accelerated conditions. A poor Chiral-AGP® column used for a long period was restored using a simple wash step together with repacking the top of the chromatographic column. © 1995 Wiley-Liss, Inc.     

Calculation of the molecular masses of two newly synthesized thermostable enzymes isolated from thermophilic microorganisms

Two thermostable enzymes synthesized by thermophilic microorganisms were isolated and purified. A thermostable ß-galactosidase was produced in a continuous fermentation process by Bacillus stearothermophilus TP 32 as an intracellular enzyme. After applying different concentration procedures the raw extract enzyme was prepurified on a Sephadex G-200 size exclusion column. The isolated ß-galactosidase fraction was then separated with HPLC on a TSK G 3000 SW size exclusion column to determine the molecular mass based on calibration curves of standard proteins. The other enzyme, a thermostable protease, was synthesized by Bacillus stearothermophilus TP 26 as an extracellular enzyme. After its concentration, the enzyme was purified on a classical size exclusion column (Sephacryl S-200) and on a HPLC size exclusion column (BIO-SIL TSK-250). The micropreparatively isolated fraction was separated again on this HPLC column to determine its molecular mass. The optimum temperature of both enzymes was approximately 75°C.