Determination of neurotransmitters in PC 12 cells by microchip electrophoresis with fluorescence detection

A sensitive fluorescence detection system with an Hg-lamp as the excitation source and a photon counter as the detector for microchip CE (MCE) has been developed. O-Phthaldialdehyde (OPA, lambda(ex) = 340 nm) was employed to label the catecholamine neurotransmitters such as dopamine (DA), norepinephrine (NE), and amino acid neurotransmitters including alanine (Ala), taurine (Tau), glycine (Gly), glutamic acid (Glu), and aspartic acid (Asp). The separation of seven derivatized neurotransmitters was successfully performed in MCE and the detection limits (S/N = 3) for DA, NE, Ala, Tau, Gly, Glu, and Asp were 0.85, 0.49, 0.23, 0.15, 0.13, 0.18, and 0.29 fmol, respectively. The system was then successfully applied for separation and determination of neurotransmitters in rat pheochromocytoma (PC 12) cells, and the average amounts of analyte per cell from a cell population were 2.5 fmol for DA, 3.3 fmol for Ala, 8.2 fmol for Tau, 4.0 fmol for Gly, and 1.9 fmol for Glu, respectively. By single-cell injection mode, electrophoresis separation and quantitative measurement of Glu in individual PC 12 cells was obtained. The average value of Glu per cell from single PC 12 cells analysis was found to be 3.5 +/- 3.1 fmol.     

Separating nanoparticles by surface charge group using pH-controlled passivated gel electrophoresis

Because ionically stabilized colloids in aqueous dispersions have net surface charges that depend on pH, it is potentially possible to separate mixtures of nanospheres having identical radii, yet different types of stabilizing surface charge groups, efficiently using passivated gel electrophoresis (gel-EP). To demonstrate this, we separate a binary dispersion of polystyrene nanospheres that have nearly identical radii and surface group densities, yet different types of anionic stabilizing surface charge groups: sulfate and carboxylate. We achieve an efficient separation by adjusting the pH of the running buffer to lie between the pK_a values of these charge groups, resulting in significantly different protonation and, consequently, different electrophoretic propagation velocities of the nanospheres. The measured steady-state propagation velocities of both types of anionic nanoparticles as a function of pH can be fit well by an equilibrium model of pH-dependent protonation of anionic surface charge groups. Thus, pH-controlled passivated gel-EP opens a route for separating similarly sized charged colloidal objects that are stabilized by a variety of different surface charge groups.     

The surface properties of tetradecyltrimethylammonium bromide observed by capillary electrophoresis

The electroosmotic flow (EOF) is measured as a function of tetradecyltrimethylammonium bromide (TTAB) concentration and is shown to have distinct zones that are pH dependent. The data is correlated with previously proposed surface structures ranging from unimolecular adsorption to hemimicelles and micelles of TTAB adsorbed on the hydrated fused silica. A plot of the TTAB concentration at zero EOF versus pH shows that the zero point of charge (zpc) is pH dependent and that a linear extrapolation of the data intercepts close to the pH value for the zpc of a fused-silica surface. This shows that different surface properties at different pH values at any given TTAB concentration are generally dealt with. Therefore, these pH-dependent structures of the fused-silica surface have to be taken into account while studying these phenomena.     

Simultaneous determination of polyamines and catecholamines in PC-12 tumor cell extracts by capillary electrophoresis with laser-induced fluorescence detection

A method to detect polyamines and catecholamines in PC-12 tumor cell extracts by capillary electrophoresis with laser-induced fluorescence detection (CE-LIF) is described for the first time. Both derivatization conditions and buffer concentrations and pH were optimized. Under optimized conditions the polyamines (putresine, spermine, spermidine) and catecholamines (dopamine, norepinephrine, epinephrine, serotonin) were derivatized with fluorescein isothiocyanate and separated at 25 kV in a fused-silica capillary (50 microm ID x 40 cm) with 0.1 M borate, pH 9.0, in less than 18 min. The influence of running buffer conditions, such as buffer pH and concentrations, were also investigated. Linearity of the analytes ranged from 0.05 to 1.0 micromol/L, and the detection limit (S/N = 3 ) ranged from 0.03 to 2.50 nmol/L. The concentrations of polyamines and catecholamines in PC-12 tumor cell extracts were determined with this method.     

Determination of catecholamines in pheochromocytoma cell (PC-12) culture medium by microdialysis-microbore liquid chromatography

An in vitro microdialysis system was constructed for the measurement of catecholamines in pheochromocytoma cell culture medium. The novel microdialysis device is composed of a petri dish, a dialysis membrane and two transmission tubes. The dialysis membrane is located in the space of a petri dish such that it is immersed in the culture medium. Catecholamines contained in the culture medium diffused into a designed dialysis membrane with sufficient recovery (about 60%). Dialysates were collected by a sampling loop and introduced by an on-line injector to a microbore liquid chromatographic system for analysis of catecholamines. This assay yielded a detection limit of 0.2–0.5 pg/injection with acceptable intra- and inter-assay reproducibilities in 5 μl of dialysates. To evaluate the on-line microdialysis system, PC-12 cells were cultured in a petri dish within an incubator. The baseline concentration of dopamine in PC-12 cell culture medium was about 0.29 ng/ml which was elevated to 2.43 ng/ml after treatment with 0.5 mM potassium cyanide. In conclusion, the present microassay provides for the sensitive, direct measurement of catecholamines in culture medium while minimizing pretreatment procedures for sample preparation.     

Bioactive compounds from Selaginella involven Spring that protect PC-12 cells

Two new compounds named as 3b 12 16-trihydroxy-6 8 11 13-abietatrien（1） （8R 80S）-4 40 8-trihydroxyl-3 30-dimethoxyl-90-lignanolide（2） and a new natural product 4 40-dihydroxyl-3 30 5 50-dimethoxyldiphenyl diketone（3） were isolated from the whole herbs of Selaginella involven Spring.The structures were elucidated by spectroscopic analyses including UV,IR,1D,2D NMR and MS methods.Additionally,these three compounds exhibited potent protective effect against the injury of PC-12 cells induced by hypoxia/reoxygenation.     

Determination of the surface charge of lignocellulosic fiber by a derived spectroscopic technique

This paper proposed a derived spectroscopic technique for determining the surface charge of lignocellulosic fiber. In this method, chitosan quaternary ammonium iodide with higher molecule weight was selected to minimize its interaction with the negative charge inside of fiber pores. It was based on spectroscopically measuring the UV absorbance of I^? (the counter ion) in the filtrates from a set of solutions that containing the fixed amount of fibers and the different amount of cationic polymer (from under- to over-saturation). By plotting the derived absorbance at 245 nm versus the volume of chitosan addition, a transition point is determined, from which the fiber surface charge can be calculated. The results showed that the present method has a good measurement precision (RSD?<?3.24%) and accuracy (relative differences?<?3.11%, when compared with the conductivity titration method). It is suitable to be used for determining the surface charge of lignocellulosic fibers.

     

Determination of tobacco alkaloids in single plant cells by capillary electrophoresis

A new capillary electrophoresis system with direct UV detection for the analysis of the tobacco alkaloids nicotine, nornicotine and anabasine in plant microsamples was developed. An electrolyte containing a high concentration of citric acid to provide good buffer capacity at pH 3.6 was found to be most suitable in terms of sensitivity and separation efficiency. At this low pH the tobacco alkaloids are present in cationic form, showing high mobility and increased UV absorption. This system was used for the analysis of nicotine in single epidermal leaf cells of tobacco plants. Only vacuolar concentrations of nicotine were determined, as the vacuole occupies >95% of the entire volume in epidermal cells. The procedure of sample acquisition and preparation for nicotine analysis of vacuolar samples in the pl range is shown. The results indicate a gradient of nicotine from the leaf base to the tip with higher concentrations present in the cells at the tip. Compared to simultaneously measured bulk leaf samples containing all types of cells, tissues and compartments, the concentrations in epidermal cells are much higher. As nicotine is the major defence substance against insects in tobacco and the epidermis is the most exposed leaf tissue this result is physiologically plausible.     

Determination of individual microsphere properties by capillary electrophoresis with laser-induced fluorescence detection

Capillary electrophoresis with postcolumn laser-induced fluorescence detection was used to individually detect 6.0, 1.0, 0.5, and 0.2 num diameter polystyrene microspheres and individually measure their electrophoretic mobility. The analysis of a nanoliter-size volume from a microsphere suspension results in an electropherogram characterized by several narrow spikes in a well-defined migration time window. Each spike is associated with one microsphere because, when one single microsphere is introduced into the capillary by micromanipulation, the electropherogram has only one spike in the same migration time window. The distributions of individual measurements resulting from an electropherogram were used to evaluate the reproducibility from run to run, observe the effect of sodium dodecyl sulfate (SDS) added to the running buffer, and to investigate the origin of electrophoretic dispersion. As expected from the interactions between microspheres and SDS, the addition of this surfactant to the running buffer narrowed the range and shifted the average electrophoretic mobility to more negative values. After evaluating common sources of broadening in capillary electrophoresis, electrophoretic dispersion was attributed to microsphere heterogeneity. Unlike electropherograms displaying Gaussian-like profiles, the two-dimensional representations of the individual measurements provide a new alternative to evaluate and study electrophoretic-related properties of microspheres.     

Determination of acidic herbicides in surface water by solid-phase extraction followed by capillary zone electrophoresis

A rapid solid-phase extraction-capillary zone electrophoresis (CZE) method for determining 2,4-dichlorophenoxyacetic acid, 4-(2,4-dichlorophenoxy) butyric acid, and 2,4,5-trichlorophenoxyacetic acid in real water samples is described. Factors affecting the recoveries and detection of the targets are investigated. With samples being acidified to pH 2 and salted by sodium sulfate to 2% (w/w), an average recovery of greater than 85% is obtained using ethyl acetate as the eluent on an octadecylsilane-bonded silica cartridge. A running buffer of 5 mM sodium tetraborate in a water-acetonitrile mixture (70:30, v/v) adjusted to pH 9 is employed in the CZE analysis, and the targets can be analyzed within 7 min with good reproducibility and acceptable sensitivity. The method is suitable for detecting herbicide residues of sub-parts-per-billion levels in surface water. A local pond water is analyzed, and the concentrations of 2,4-dichlorophenoxyacetic acid and 4-(2,4-dichlorophenoxy) butyric acid are detected to be 0.27 +/- 0.03 ppb and 0.61 +/- 0.08 ppb, respectively.     

330 - Determination of surface charge of bilayer lipid membranes

The determination of the membrane surface charge is based on the measurement of the surface potential difference at both sides of the bilayer lipid membrane (BLM) connected with the asymmetrical concentration of the electrolyte in both solutions. In the short-circuit regime the intramembrane potential jump is caused by the difference in the two surface potentials. In order to find the intramembrane potential jump the BLM capacitance dependence on voltage was used. In some range of electrolyte concentrations a dependence of the potential jump on the surface charge was found. The charge density was calculated by applying the Gouy-Chapman theory of the diffuse double layer. Surface charges were determined for BLM of common bovine brain lipids, phosphatidylethanolamine, dioleyllecithin and azolectine.     

Determination of surfactants by capillary electrophoresis

Capillary electrophoresis has been increasingly used during the past few years for the separation and determination of surfactants. These substances are applied in many household and industrial products such as laundry detergents, cosmetics and pharmaceuticals, often as homologous and isomeric mixtures. Product development and control as well as toxicological and environmental analyses require selective and sensitive analytical methods. This review presents capillary electrophoretic techniques to determine important representatives of cationic, anionic, and neutral surfactants. The application of different buffer additives such as organic solvents, cyclodextrins or micelles to enhance the resolution of complex mixtures is discussed. Besides direct and indirect UV and fluorescence detection, examples for conductivity and mass spectrometric detection are also given. Derivatization procedures to improve the detectability and implement charge in neutral analytes are described. The successful use of capillary electrophoresis for surfactant determinations has proven that it can serve as a routine technique in many real-world applications. Robust, validated methods for the quantitation of single compounds, such as alkylbenzene sulfonates, sodium dodecyl sulfate and benzalkonium salts, are now available. Characteristic peak patterns (fingerprint analysis) can be used for the identification of surfactants in multicomponent formulations (e.g. ethoxylates and phosphonates).     

Determination of polyhexamethyleneguanidine by capillary electrophoresis

The electrophoretic behavior of polyhexamethyleneguanidine hydrochloride (PHMG HC), hexamethylenediamine (HMDA), and guanidine hydrochloride (GHC) was studied. It was shown that PHMG HC and the initial toxic components of its synthesis, GMDA and GHC, can be separated. A procedure was developed for determining PHMG HC oligomers, GMDA, and GHC in aqueous solutions in concentrations from 0.007 to 0.05 mg/mL by capillary electrophoresis. The procedure was applied to the analysis of model mixtures of these compounds.     

The effect of surface wettability on induction and growth of neurites from the PC-12 cell on a polymer surface

Surface properties of polymeric devices that are used to regenerate nervous damage are a point to be considered for axon regeneration in nerve system. In our previous studies, we prepared a wettability gradient on polyethylene (PE) surfaces using a corona discharge treatment from a knife-type electrode whose power increases gradually along the sample length. The PE surfaces were oxidized gradually with increasing power. The effect of surface wettability on the different types of cells has an important role for cell adhesion and proliferation. The purpose of this study is to investigate neurite formation on polymer surfaces with different wettability. Induction and growth of neurites from the rat pheochromocytoma (PC-12) cells attached on the polymer surfaces with different hydrophilicity were investigated using the wettability gradient PE surfaces prepared by a corona discharge treatment. Neurites were investigated for number and length of neurites in terms of surface wettability. It was observed that neurite formation of PC-12 cells was increased more onto the positions with moderate hydrophilicity of the wettability gradient surface than onto the more hydrophobic or hydrophilic positions. From those results, it could be assumed that initial adhesion of PC-12 cells was caused by more calf serum (CS) protein than nerve growth factor (NGF), whereas the neurite formation of PC-12 cells was caused by more NGF than CS protein. It follows from what has been said thus far that PC-12 cells are a differentiated neuronal phenotype with a long neurite at around the position 2.5 cm (water contact angle of about 55 deg). In conclusion, surface wettability plays an important role for neurite formation on the polymer surfaces for axon regeneration.     

Electrophoresis of cells and the biological relevance of surface charge

Recent developments in electrophoresis of cells are reviewed. Problems and progress in automation and miniaturization of analytical electrophoresis instruments as well as in the interpretation of experimentally determined electrophoretic mobility (EPM) data are summarized: In recent times, the EPM determination techniques not only became more reliable and faster, but also more knowledge could be gained about the cell surface electrical properties, the structure of the glycocalyx as well as its influence on the cell peripheral regions and microenvironment by applying cell electrophoresis. In addition, ways are shown to solve discrepancies between physical requirements of a preparative cell electrophoresis procedure and the quantities of ions, which have to be dissolved in cell suspension media. As the modern machines allow the purification of untagged cells suspended in more cell friendly and physiological media, they are likely to be valuable tools in several useful practical applications in clinical transplantation, gene therapy and treatment of disease states.     

Determination of trace metals by capillary electrophoresis

A new analytical procedure is developed using a strong complexing agent, 1,10-phenanthroline (Phen), for direct UV detection of Zn, Mn, Cu, Co, Cd, and Fe at microg/L concentrations in environmental water samples. The metal chelates formed showed different electrophoretic mobilities and solved the comigration problem for capillary electrophoresis (CE) separation of free metal ions. To obtain stable metal-Phen chelates during the capillary zone electrophoresis (CZE) run, both pre-column and on-column complexation are required and threefold excess of Phen over metal ions should be added to the sample. The optimized background electrolyte (BGE) consists of 30 mM hydroxylamine hydrochloride and 0.1% methanol at pH 3.6. Under hydrodynamic sampling, CE run at + 20 kV in 65 cm x 0.05 mm ID fused-silica column with detection at 265 nm, baseline separation, satisfactory working ranges (10 microg/L to 5.5 mg/L), sensitive detection limits (1-3 microg/L), good repeatability for migration times (relative standard deviation, RSD 0.36-0.81%, n = 5), peak area (RSD 3.2-4.2%, n = 5) and peak height (RSD 3.2-4.5%, n = 5) were obtained for the metal cations investigated. The reliability of the method was established by parallel determination using the inductively coupled plasma-atomic emission spectrometry (ICP-AES) method giving results within statistical variation. The procedure developed is shown to provide a quick, sensitive, precise, and economic method for simultaneous determination of metal cations that can form stable chelates with Phen.     

Determination of cationic surfactants by capillary electrophoresis

A method is described for the separation of quaternary alkylbenzylammonium compounds as well as alkyl pyridinium salts by capillary electrophoresis using direct UV detection. The influence of the organic buffer modifier on the electrophoretic behaviour of the analytes is discussed. In addition to fused silica capillaries, also C8, C18 and neutral surface coatings are used. Separation is also performed in completely non-aqueous media. The results of method development are applied to the determination of cationic surfactants in cosmetics and pharmaceuticals. A comparison with HPLC with respect to efficiency, reproducibility and detection limits is presented. Received: 1 July 1996 / Revised: 6 November 1996 / Accepted: 10 November 1996     

Determination of enzymatic activity and properties of secretory phospholipase A2 by capillary electrophoresis.

A capillary electrophoretic (CE) system coupled with a diode array UV detector was used for the assay of secretory phospholipase A2 (sPLA2) activity. This method is based on monitoring both the breakdown of substrates and the formation of products simultaneously using micellar electrokinetic chromatographic techniques. Under our developed separation conditions, we analyzed the substrates and products quantitatively, and investigated enzyme activity as a function of reaction time and presence of enzyme activator or inhibitor. Matrix-assisted laser desorption/ionization time-of-flight mass spectrometry was also utilized to confirm the phosphatidylcholine, a substrate of sPLA2. In order to test the feasibility of the developed method for measurement of enzymatic activity, we compared it to the conventional radioactive assay method for sPLA2. On the basis of our results, the conventional method can be complemented, or even replaced, by this new CE method which possesses the advantages of short analysis time, use of non-radiolabeled and inexpensive substrates, simple measurement of enzymatic activity, and exact quantitation of substrate and product.     

毛细管区带电泳法测定粉针剂中头孢拉定的含量

用毛细管区带电泳法测定头孢拉定的含量 ,未涂层毛细管柱 (75 μm×48.5cm ,有效长度 40cm) ,电压 2 8kV ,检测波长 2 3 0nm ,温度 2 0℃ ,进样 5×1 0 3Pa× 3s。运行缓冲液为 2 5mmol/L硼砂缓冲液。方法的线性范围 3 1 .2 2μg/mL～ 749.2 8μg/mL ,检测限为 1 .1 7μg/mL。