大体积样品堆积-毛细管电泳-紫外检测分析鼠肝中不同亚型金属硫蛋白

制备了均匀稳定的聚丙烯酰胺涂层毛细管,有效抑制了毛细管内壁对金属硫蛋白(MT)的吸附,大大提高了MT的分离度和分离重现性。基于此,建立了大体积样品堆积-毛细管电泳-紫外检测法(LVSS-CE-UV)分析鼠肝中MT的新方法。在最优化的条件下,该方法对两种MT亚型(MT-1/2)的富集倍数分别为13、11倍,检出限分别为0.80、1.01μg·m L~(-1)。将所建立的LVSS-CE-UV方法用于经Cd~(2+)、Zn~(2+)诱导的Sprague Dawley大鼠肝脏中MT-1/2的定量分析,结果表明经Cd~(2+)、Zn~(2+)诱导的鼠肝内均检测出MT-1/2。其中,经Zn~(2+)诱导的鼠肝内MT-1与MT-2的含量分别为31.9、24.3μg·g~(-1);Cd~(2+)诱导组的MT-1与MT-2分别为15.9、31.2μg·g~(-1)。     

Continuous‐Bed Columns Containing Sol‐Gel Bonded Packing Materials for Capillary Electrochromatography

Sol‐gel bonded packing materials in continuous‐bed columns have been prepared for capillary electrochromatography (CEC). Three packing materials were investigated: small‐pore Spherisorb ODS1 (3 μm, 80 Å) with octadecyl as stationary phase, small‐pore mixed‐mode Spherisorb ODS/SCX (3 μm, 80 Å) with octadecyl and propyl sulfonic acid as stationary phases, and large‐pore Nucleosil ODS (7 μm, 1 400 Å) with octadecyl as stationary phase. The characteristics of these columns were compared in terms of electroosmotic flow, efficiency, inertness, and retention factors. In contrast to columns containing sol‐gel bonded ODS, columns containing sol‐gel bonded mixed‐mode ODS/SCX generated nearly pH independent electroosmotic flow (EOF) over pH 2–9. Columns containing sol‐gel bonded large‐pore ODS produced nearly three times lower reduced plate height than those containing small‐pore ODS. Efficiencies of 220,000 plates per meter and 175,000 plates per meter were obtained from columns containing sol‐gel bonded 7 μm, 1 400 Å ODS and columns containing sol‐gel bonded 3 μm, 80 Å ODS, respectively, which are among the highest reported efficiencies for continuous‐bed columns. In CEC, over one million plates per meter and pH independent EOF are expected from continuous‐bed columns containing sol‐gel bonded 1.5 μm particles with large pores and mixed‐mode stationary phases.     

Determination of key flavonoid aglycones by means of nano‐LC for the analysis of dietary supplements and food matrices

A method for the analysis of flavonoids (myricetin, quercetin, naringenin, hesperitin, and kaempferol), with interesting bioactivity, has been developed and validated utilizing nano‐LC technique. In order to find optimal conditions, capillary columns (75 μm id × 10 cm) packed with different types of stationary phases, Kinetex® C18 core–shell (2.6 μm particle size), Hydride‐based RP‐C18 (sub‐2 μm particle size), and LiChrospher® 100 RP‐18 endcapped (5 μm particle size) were evaluated. The method was validated using Hydride‐based RP‐C18 stationary phase, with sub‐2 μm particle size. A good chromatographic performance, expressed in terms of repeatability (RSD, in the range 1.63–4.68% for peak area), column‐to‐column reproducibility (RSD not higher than 8.01% for peak area), good linearity and sensitivity was obtained. In particular limit of detection values between 0.07 and 0.31 μg/mL were achieved with on column focusing technique. The method was applied to the determination of studied flavonoids in dietary supplements as well as in food matrices. The amount of quercetin found in the first analyzed dietary supplement, was in agreement to the labeled content. In the other samples, where the content of flavonoids was not labeled, most of the studied flavonoids were determined in amounts somewhere comparable to those reported in literature.     

聚硅氧烷离子液体用于快速气相色谱固定相的研究

合成了聚硅氧烷键合离子液体[PSOMIM][NTf2],并将其用作快速气相色谱柱的固定相.初步探索了采用短柱及小内径毛细管柱(3 m×75 μm i.d.)时的分离性能及固定相膜厚对分离性能的影响.与常规柱(8m×0.25 mmi.d.)相比,在不损失分离度的前提下,分离速度可提高1～6倍;当膜厚为0.056 μm时,可以将分离速度提高2～4倍.实验结果表明,聚硅氧烷键合离子液体固定相可以有效弥补由于缩短柱长所导致的分离度减小的问题,在快速气相色谱固定相方面具有较好的应用前景.     

Systematic comparison of a new generation of columns packed with sub‐2 μm superficially porous particles

The aim of this study was to evaluate the possibilities/limitations of recent RP‐LC columns packed with 1.6 μm superficially porous particles (Waters Cortecs) and to compare its potential to other existing sub‐2 μm core–shell packings. The kinetic performance of Kinetex 1.3 μm, Kinetex 1.7 μm and Cortecs 1.6 μm stationary phases was assessed. It was found that the Kinetex 1.3 μm phase outperforms its counterparts for ultra‐fast separations. Conversely, the Cortecs 1.6 μm packing seemed to be the best stationary phase for assays with longer analysis time in isocratic and gradient modes, considering small molecules and peptides as test probes. This exceptional behaviour was attributed to its favourable permeability and somewhat higher mechanical stability (ΔP_max of 1200 bar). The loading capacity of these three columns was also investigated with basic and neutral drugs analysed under acidic conditions. It appears that the loading capacities of Cortecs 1.6 μm and Kinetex 1.7 μm were very close, while it was reduced by 2–7‐fold on the Kinetex 1.3 μm packing. However, this observation is dependent on the nature of the compound and certainly also on mobile phase conditions.     

梯度加压毛细管电色谱分离蛋白质

 以1.5 μm无孔硅胶颗粒(non-porous silica,NPS)为固定相,采用电压和压力联合驱动流动相,用反相梯度加压毛细管电色谱(p-CEC)在7.5 min内实现了核糖核酸酶A、细胞色素C、溶菌酶和肌红蛋白等4种蛋白质的快速、高效的分离。比较了梯度加压毛细管电色谱和微柱液相色谱(μ-HPLC)分离蛋白质的结果,同时考察了固定相、离子对试剂三氟醋酸(TFA)浓度和电压等条件对梯度加压毛细管电色谱分离蛋白质的影响。结果表明,梯度p-CEC可以通过调节电压精细调节带电溶质的保留,提高分离选择性,缩短分离时间,得到较高的柱效。该方法在蛋白质分离分析及蛋白质组学的研究中具有很大的应用潜力，为高效快速地分离蛋白质开辟了新的途径。     

Microfabricated Monolith Columns for Liquid Chromatography. Sculpting Supports for Liquid Chromatography

Monolith columns are generally fabricated by polymerization of monomers within a column. This paper reviews an alternative strategy in which the bed is microfabricated in an inorganic material by ablation. Channels of 1.5 μm width and 10 μm depth were sculpted in quartz by deep reaction ion etching. Using this approach chromatographic beds were constructed in which cubic support structures were created and arranged in rows to mimic particles in a conventional column. Beds ranging from hundreds of thousands to millions of “particles” with volumes of 15 nL to 15 μL were produced. Columns that had been derivatized with an octadecyl silane stationary phase were used to separate both low molecular weight analytes and peptides in the CEC mode. Plate height in the CEC mode was 1.2 μm at maximum efficiency.     

Comparison of a new high‐resolution monolithic column with core‐shell and fully porous columns for the analysis of retinol and α‐tocopherol in human serum and breast milk by ultra‐high‐performance liquid chromatography†

The reduction of analysis time, cost, and improvement of separation efficiency are the main requirements in the development of high‐throughput assay methods in bioanalysis. It can be achieved either by ultra‐high‐performance liquid chromatography (UHPLC) using stationary phases with small particles (<2 μm) at high back pressures or by using opposite direction—monolithic stationary phases with low back pressures. The application of new types of monolithic stationary phases for UHPLC is a novel idea combining these two different paths. The aim of this work was to test the recently introduced second‐generation of monolithic column Chromolith® HighResolution for UHPLC analysis of liposoluble vitamins in comparison with core‐shell and fully porous sub‐2 μm columns with different particle sizes, column lengths, and shapes. The separation efficiency, peak shape, resolution, time of analysis, consumption of mobile phase, and lifetime of columns were calculated and compared. The main purpose of the study was to find a new, not only economical option of separation of liposoluble vitamins for routine practice.     

Syntheses, Characterization and Anti-HIV Activity of Charge Transfer Heteropolycomplexes

IntroductionAcquired immunodeficiency syndrome(AIDS) is a fatal disease caused by human immun-odeficiency virus type 1 (HIV-l ). Although this kind of disease was fOund only about tenyears ago, it has attracted extensive attention because Of its epidemic speed and high deathrate. Now, scientists are, at an unprecedented speed, accumulating the relevant knowledge inexpectation of discovering the methods to prevent and cure the disease. Furthermore, manystudies have indicated that the patien…     

Voltammetric examinations of ferrocene on microelectrodes and microarrayelectrodes

Voltammetric investigations of ferrocene in organic media with planar, disk and band shaped microelectrodes (ME) and microarrayelectrodes (MAE) were carried out in stationary solutions and under flow-through conditions with flow-injection analysis (FIA). The electrodes were embedded in cylindrical electrode bodies made of epoxy resin. During the FIA experiments miniaturized flow-through cells with a three electrode configuration (wall-jet, thin-layer principle) were used. As detectors microelectrodes and microarrayelectrodes consisting of platinum wires (radius: 10 μm), gold wires (radius: 12.5 μm), carbon fibres (radius: 3.5 μm) and gold foils (foil thickness: 30 μm) were constructed using fine precision manufacturing methods by sealing the electrode materials in insulating resins.     

A novel stability-indicating HPLC method for the determination of enantiomeric purity of eluxadoline drug: Amylose tris(3,5-dichlorophenyl carbamate) stationary phase

A simple and sensitive stability-indicating chiral HPLC method has been developed and validated per International Conference on Harmonization guidelines for the determination of enantiomeric purity of eluxadoline (Exdl). The impact of different mobile phase compositions and chiral stationary phases on the separation of Exdl enantiomer along with process- and degradation-related impurities has been studied. Homogeneity of Exdl and stable results of Exdl enantiomer in all degraded samples reveal the fact that the proposed method was specific (stability indicating). Amylose tris(3,5-dichlorophenyl carbamate) stationary phase column Chiralpak IE-3 (150 × 4.6 mm, 3 μm) provided better resolution with polar organic solvents than cellulose derivative, crown ether, and zwitterion stationary phases and nonpolar solvents. The mobile phase consisted of acetonitrile, tetrahydrofuran, methanol, butylamine, and acetic acid in the ratio of 500:500:20:2:1.5 (v/v/v/v/v). Isocratic elution was performed at a flow rate of 1.0 mL/min, column temperature of 35°C, injection volume of 10 μL, and UV detection of 240 nm. The United States Pharmacopeia (USP) resolution of the Exdl enantiomer was found to be more than 4.0 within a 65-min run time. Exdl enantiomer detector response linearity over the concentration range of 0.859–4.524 μg/mL was found to be R² = 0.9985. The limit of detection, limit of quantification, and average percentage recovery values were established as 0.283 μg/mL, 0.859 μg/mL, and 96.0, respectively.     

Analysis of metallothioneins by means of capillary electrophoresis coupled to electrospray mass spectrometry with sheathless interfacing

Capillary electrophoresis (CE) coupled to electrospray mass spectrometry via sheathless interfacing has been applied to the analysis of mammalian metallothionein (MT) extracts. In a rabbit-liver extract, four (MT-2C, MT-2A, MT-2D and MT-2E) out of six known MT sub-isoforms were unambiguously identified under three CE-resolved peaks. A fourth peak was found to contain MT-1A and/or MT-2B, whose molecular masses differ by only 1 Da. Traces of non-N-acetylated MT-2D and MT-2E were observed in a fifth, minor peak. In a rat-liver extract, both MT-1 and MT-2 were resolved and identified. Non-N-acetylated MT-2 was also identified in a resolved, minor peak. Minimum detectable amounts of MTs have been estimated to be approximately 0.6 fmol per sub-isoform.     

聚(烯烃砜)作为抗蚀剂和记录材料的应用性能研究

本文报道了两种不同类型的聚(烯烃砜),即聚(环己烯砜)和聚(苯乙烯砜),并对它们进行了物理表征,给出了元素分析、红外光谱、核磁分析、凝胶渗透色谱及热重分析等的测试数据。用聚(环己烯砜)和聚(苯乙烯砜)作为抗蚀剂,其曝光特性:前者,灵敏度为5×10^-6库仑/厘米²,分辨率为0.75微米,反差约1.5;后者分别为6×10^-5库仑/厘米²,0.36微米及约2.5。尤为重要的是,聚(苯乙烯砜)具有优良的耐干法刻蚀的性能。聚(环己烯砜)作为强磁场聚焦电子照相记录材料,分辨率高于1.5微米。聚(苯乙烯砜)作为远紫外抗蚀剂,分辨率达0.5微米。     

Comparison of core-shell versus fully porous particle packings for chiral liquid chromatography productivity

A loading and productivity study was done using three racemates on vancomycin and teicoplanin-bonded chiral stationary phases of different particle formats. Two columns were packed with 2.7 μm superficially porous particles and two columns were packed with identically bonded 5 μm fully porous particles. The last two columns were packed with specially synthesized 4.5 μm vancomycin and teicoplanin superficially porous particles. The loading of different chiral compounds showed that the columns filled with 2.7-μm chiral stationary phases were inappropriate for preparative separations due to their very low permeability which precluded high flow rates. However, columns containing 4.5 μm superficially porous (core-shell) particles were as effective for small-scale preparative chiral separations as columns filled with classical 5 μm fully porous particles. Comparing the 4.5 μm superficially porous particles and 5 μm fully porous particles teicoplanin columns, the observed respective productivities of 270 and 265 mg/g chiral phase/h for 5-methyl-5-phenyl hydantoin enantiomers were obtained. Particular attention was given to the peculiar case of the mianserin enantiomeric separation on vancomycin columns that gave observed productivities of 200 and 205 mg/g chiral phase/h on the 4.5 μm superficially porous particles and 5 μm fully porous particles, respectively.     

Synthesis and anti-HIV activity of new homo acyclic nucleosides, 1-(pent-4-enyl)quinoxalin-2-ones and 2-(pent-4-enyloxy)quinoxalines

A series of acyclonucleosides 6,7-disubstituted 1-(pent-4-enyl)quinoxalin-2-one derivatives and the O-analogs were synthesized by a one-step condensation of the corresponding quinoxaline bases with 5-bromo-1-pentene.The acyclonucleosides prepared were assayed against HIV-1 and HIV-2 in MT-4 cells. 6,7-Dimethyl-2-(pent-4-enyloxy)quinoxaline showed inhibition of HIV-1 with EC₅₀ value of 0.22 ± 0.08 μg/ml and a therapeutic index of 13. This means that it was cytotoxic to MT-4 cells at CC₅₀ of 2.6 ± 0.1 μg/ml. __________ Translated from Khimiya Geterotsiklicheskikh Soedinenii, No. 8, pp. 1243–1250, August, 2007.     

High performance liquid chromatographic resolution of the optical isomers of D,L-tryptophane,D,L-5-hydroxytryptophan and D,L-dopa on cellulose columns

The application of HPLC for the purpose of separation of some amino acid racemates with aromatic substituents is described. Using simple untreated cellulose with an average particle size of 7 μm as stationary phase, complete resolution of D,L-tryptophane and D,L-5-hydroxytryptophane can be obtained. D,L-3,4-dihydroxyphenylalanine is resolved partially. The α-value and resolution for D,L-tryptophane was found to be 1.5.     

Separation of metallothionein isoforms of mouse liver cytosol by capillary zone electrophoresis

Metallothionein (MT) isoforms of mouse liver cytosol were separated by capillary zone electrophoresis (CZE) using a polyacrylamide-coated tube at neutral pH, samples prepared from non-treated, heat-treated, and ethanol-precipitated specimens were compared. The liver was homogenized in three kinds of media, 0.25 M sucrose containing 100 mM Tris-HCl buffer at pH 7.4 (BS), BS containing 1% ascorbic acid (BS-C), and BS containing 5 mM beta-mercaptoethanol (BS-M). Mouse liver was used 24 h after subcutaneous injection of 50 mg Zn kg(-1). In the non-treated specimen of the cytosol fraction, the MT-2 isoform was separated in all three media, while the MT-1 isoform was difficult to identify. In the ethanol-precipitated specimen, MT isoforms were separated well using either BS or BS-C. However, when BS-M was used, a small MT-2 peak was obtained the MT-1 peak could not be identified. MT-1 isoform in the heat-treated specimen was difficult to identify. In contrast, MT-2 isoform was separated well in all three kinds of media. In the non-treated specimen of the control liver cytosol, the MT-2 isoform was detected using all three media, the MT-1 peak was undetected. Based on these results, MT isoforms can be detected in the crude cytosol fraction of liver using CZE combined with a polyacrylamide-coated tube at neutral pH.     

Nano and rapid resolution liquid chromatography–electrospray ionization–time of flight mass spectrometry to identify and quantify phenolic compounds in olive oil

The applicability of nanoLC‐ESI‐TOF MS for the analysis of phenolic compounds in olive oil was studied and compared with a HPLC method. After the injection, the compounds were focused on a short capillary trapping column (100 μm id, effective length 20 mm, 5 μm particle size) and then nanoLC analysis was carried out in a fused silica capillary column (75 μm id, effective length 10 μm, 3 μm particle size) packed with C18 stationary phase. The mobile phase was a mixture of water + 0.5% acetic acid and ACN eluting at 300 nL/min in a gradient mode. Phenolic compounds from different families were identified and quantified. The quality parameters of the nanoLC method (linearity, LODs and LOQs, repeatability) were evaluated and compared with those obtained with HPLC. The new methodology presents better sensitivity (reaching LOD values below 1 ppb) with less consumption of mobile phases, but worse repeatability, especially inter‐day repeatability, resulting in more difficulties to get highly accurate quantification. The results described in this article open up the application fields of this technique to cover a larger variety of compounds and its advantages will make it especially useful for the analysis of samples containing low concentration of phenolic compounds, as for instance, in biological samples.     

Polydimethylsiloxane-functionalized monolithic silica column for reversed-phase capillary liquid chromatography

A polydimethylsiloxane (PDMS)-modified monolithic silica column was prepared for performing reversed-phase capillary liquid chromatography. The prepared PDMS column has a permeability of 6.4×10(-14) m(2) with a plate height <9.2 μm. Alkylbenzenes and polycyclic aromatic hydrocarbons (PAHs) were well separated with the PDMS stationary phase, which exhibited similar selectivity and separation mechanism to that of octadecyl stationary phase. The hydrophobic interactions between the analytes and the PDMS stationary phase mainly play the roles for the separation of alkylbenzenes and PAHs. The characteristics of the PDMS column for the separation of alkylbenzenes and PAHs demonstrated that it would be a promising alternative to the octadecyl column.     

Separation of complex sugar mixtures on a hydrolytically stable bidentate urea‐type stationary phase for hydrophilic interaction near ultra high performance liquid chromatography

A stationary phase bearing both bridged bis‐ureido and free amino groups (USP‐HILIC‐NH₂–2.5SP) for high‐speed hydrophilic interaction liquid chromatography separations was prepared using a one‐pot two‐step procedure starting from 2.5 μm totally porous silica particles. Highly polar compounds, such as polyols, hydroxybenzoic acids, and sugars, were successfully analyzed in shorter times and with higher peak efficiency, when compared to results obtained with a bidentate urea‐type column packed with 5 μm particles. Increased sugarophilicity and better peak shape were attested for the USP‐HILIC‐NH₂–2.5SP column (100 × 3.2 mm id) when compared with two commercially available UHPLC columns, namely an acquity BEH amide packed with totally porous 1.7 μm microparticles and a HILIC Kinetex column packed with core–shell 2.6 μm particles. Finally, the new column was employed in the separation of complex mixture of sugars (mono‐, di‐, and oligosaccharides) and in the analysis of beer samples. The resulting chromatograms showed good selectivity and overall resolution, while the catalyzing effect of the free amino moieties resulted in excellent peak shapes and in the absence of split peaks due to sugar anomerization phenomena.