In situ determination of nerve agents in various matrices by portable capillary electropherograph with contactless conductivity detection

Rapid, efficient and robust methods for sampling and extracting genuine nerve agents sarin, soman and VX were developed for analyzing these compounds on various solid matrices, such as concrete, tile, soil and vegetation. A portable capillary electrophoretic (CE) system with contactless conductometric detection was used for the in situ analysis of the extracted samples. A 7.5 mM MES/HIS-based separation electrolyte accomplished the analysis of target analytes in less than 5 min. The overall duration of the process including instrument start-up, sample extraction and analysis was less than 10 min, which is the fastest screening of nerve agents achieved with liquid phase separation methods to date. The procedure can easily be performed by a person in a protective suit and is therefore suitable for real-life applications. The CE results were validated by an independent GC-MS method and a satisfactory correlation was obtained. The use of a proper sampling strategy with two internal standards and "smart" data-processing software can overcome the low reproducibility of CE. This has a significant impact on the potential acceptance of portable CE instrumentation for the detection and analysis of genuine chemical warfare agents (CWA).     

On-chip potential gradient detection with a portable capillary electrophoresis system

A portable chip-CE system with potential gradient detection (PGD) was developed and applied to the determinations of alkali metals and alkaloids. The separation efficiency appeared to be satisfactory and nonaqueous capillary electrophoresis (NACE) proved to be applicable to PGD or conductivity detection. The power supplies, separation and detection were built on a device of 3 kg in weight. A branch channel near the end of the separation channel was designed to perform PGD and make the application of relatively high field strength possible. The study is the first report on the application of PGD on the microchip platform. The design of the chip-CE system shows several advantages, such as simplicity, miniaturization and wide applicability.     

Effective length calibration method for processing the fluorescence signal detected by charge‐coupled device in capillary electrophoresis

A novel method named effective length calibration method has been developed to process the fluorescence signal detected by charge‐coupled device during capillary electrophoresis. The new method treated each pixel as an individual point detector, and effectively binned a large number of pixels into a final electropherogram without losing the narrow detection window defined by a single pixel. Capillary electrophoresis separations of DNA were carried out and detected by charge‐coupled device and conventional detector (photomultiplier tube). Detection properties including signal‐to‐noise ratio, peak width, detection frequency, and tilt of detector were investigated. It was found that the new method achieved much higher signal‐to‐noise ratio and smaller peak width than the conventional detector did. A Detection width of 0.5 μm was easily achieved.     

Bacterial surface layer proteins as a novel capillary coating material for capillary electrophoretic separations

A novel concept for stable coating in capillary electrophoresis, based on recrystallization of surface layer proteins on hydrophobized fused silica capillaries, was demonstrated. Surface layer protein A (SlpA) from Lactobacillus acidophilus bacteria was extracted, purified and used for coating pre-silanized glass substrates presenting different surface wettabilities (either hydrophobic or hydrophilic). Contact angle determination on SlpA-coated hydrophobic silica slides showed that the surfaces turned to hydrophilic after coating (53 ± 5°), due to a protein monolayer formation by protein-surface hydrophobic interactions. Visualization by atomic force microscopy demonstrated the presence of a SlpA layer on methylated silica slides displaying a surface roughness of 0.44 ± 0.02 nm. Additionally, a protein layer was visualized by fluorescence microscopy in methylated silica capillaries coated with SlpA and fluorescein isothiocyanate-labeled. The SlpA-coating showed an outstanding stability, even after treatment with 20 mM NaOH (pH 12.3). The electroosmotic flow in coated capillaries showed a partial suppression at pH 7.50 (3.8 ± 0.5 10⁻⁹ m² V⁻¹ s⁻¹) when compared with unmodified fused silica (5.9 ± 0.1 10⁻⁸ m² V⁻¹ s⁻¹). To demonstrate the potential of this novel coating, the SlpA-coated capillaries were applied for the first time for electrophoretic separation, and proved to be very suitable for the isotachophoretic separation of lipoproteins in human serum. The separations showed a high degree of repeatability (absolute migration times with 1.1–1.8% coefficient-of-variation (CV) within a day) and 2–3% CV inter-capillary reproducibility. The capillaries were stable for more than 100 runs at pH 9.40, and showed to be an exceptional alternative for challenging electrophoretic separations at long-term use.     

Thiol-s-triazine as a Stabilizer for Thermal Discoloration

The formation of longer polyene chains (thermal discoloration) has been found to be avoidable by using thiol-s-triazines, such as 2-anilino-4,6-dithiol-s-triazine (AF), which hardly reacts with the original chlorine atoms but tends to replace the activated chlorine (allylic chloride) that plays an important role in triggering zipperlike dehydrochlorination. The optimum stabiliizing system is: PVC, 100; DOP, 50; AF, 0.18; Zn stearate, 0.5; Ba stearate, 1.5 parts.     

Bonded dimethylacrylamide as a permanent coating for capillary electrophoresis

A method for coating capillaries for capillary electrophoresis with chemically bonded polydimethylacrylamide has been developed, and the properties of the capillaries have been evaluated. The coated capillaries provided high separation efficiency, 12 x 10(5) theoretical plates/m was obtained for cytochrome c. The electroosmotic flow at pH 8.0 was 10 x 10(-10) to 6 x 10(-10) m2 V(-1) s(-1). The coated capillaries were quite stable at high pH. At least 150 runs could be done at pH 10 without appreciable performance deterioration. The excellent performance of the coated capillaries was illustrated by separation of basic proteins, acidic proteins, 9-fluorenylmethyl chloroformate-derivatized neurotransmitter amino acids, peptide reference mixtures and peptides digested from a bacteria protein.     

Iterative averaging of spectra as a powerful way of suppressing spurious resonances in signal processing

The fast Padé transform (FPT) was applied to magnetic resonance spectroscopic (MRS) time signals encoded in vivo on a 1.5 T scanner from the parietal-temporal brain region of a pediatric patient who had suffered cerebral asphyxia. An iterative averaging procedure was implemented to the 9th iteration, whereby spurious structures on the total shape spectra were effectively suppressed. The parametric and non-parametric \(\hbox {FPT}^{(\pm )}\) were verified to reconstruct equivalent total shape spectra. Via the parametric FPT, the spectral region of interest was chosen to bypass the giant water resonance, automatically generating spectral envelopes without the need for windowing. The dense component spectra were reliably reconstructed by the \(\hbox {FPT}^{(+)}\), in the “usual” mode (mixture of absorption and dispersion components) and “ersatz” mode (reconstructed phases set to zero). Via the latter, interference effects were well-visualized for closely-overlapping and hidden resonances. The most stringent test was performed for the complex frequencies and associated complex amplitudes reconstructed by the \(\hbox {FPT}^{(+)}\). Exceedingly small variances were obtained for all four Padé-reconstructed parameters per genuine resonance, once convergence was achieved at the 7th to 9th iterated averages. This now fully-validated methodology can generate denoised spectra and accurate spectral parameters for in vivo MRS data encoded within neurodiagnostics. Such a multi-faceted Padé-based strategy for processing the dense spectra of the brain could vitally improve pediatric neurodiagnostics. A wider range of clinical applications becomes within reach, including areas of cancer diagnostics where the added value of in vivo MRS is urgently needed. The broad theoretical underpinnings of incorporating quantum mechanics into signal processing provide the basis for these innovative advances.     

Normalized ytterbium induced 13C-NMR shifts as a simple aid for structural and 13C signal assignments in multifunctional and natural compounds

The LIS-RS analysis described in the preceding communication was applied to phenols, ethers,. esters, chromanes, and nitrogen derivatives. For most functionalities the Cβ-RS values are in the range of 40-50%; the smaller Cγ and Cδ values vary consistently as a function of the stereochemistry. Only the induced shifts in acetoxy compounds show no significant conformational dependence. The binding strength at different complexation sites in one molecule differs often enough for a simple analysis, as in monofunctional systems. In other cases the RS variations even in multi binding site compounds such as quinine still allow ¹³C-NMR signal reassignments.     

Selection of aptamers for signal transduction proteins by capillary electrophoresis

High‐affinity aptamers for important signal transduction proteins, i.e. Cdc42‐GTP, p21‐activated kinase1 (PAK1) and MRCK (myotonic dystrophy kinase‐related Cdc42‐binding kinase) α were successfully selected in the low micro‐ to nanomolar range using non‐systematic evolution of ligands by exponential enrichment (SELEX) with at least three orders of magnitude enhancement from their respective bulk affinity of naïve DNA library. In the non‐SELEX procedure, CE was used as a highly efficient affinity method to select aptamers for the desired molecular target through a process that involved repetitive steps of partitioning, known as non‐equilibrium CE of equilibrium mixtures with no PCR amplification between successive steps. Various non‐SELEX conditions including the type, concentration and pH of the run buffer were optimized. Other considerations such as salt composition of selection buffer, protein concentration and sample injection size were also studied for high stringency during selection. After identifying the best enriched aptamer pool, randomly selected clones from the aptamer pool were sequenced to obtain the individual DNA sequences. The dissociation constants (K_d) of these sequences were in the low micromolar to nanomolar range, indicating high affinity to the respective proteins. The best binders were also subjected to sequence alignment to generate a phylogenetic tree. No significant consensus region based on approximately 50 sequences for each protein was observed, suggesting the high efficiency of non‐SELEX for the selection of numerous unique sequences with high selectivity.     

Peroxodisulfate as a chemical initiator for methacrylate-ester monolithic columns for capillary electrochromatography

Organic monolithic stationary phases for CEC were synthesized in situ in fused-silica capillaries. Polymerization mixtures were composed of butyl methacrylate, ethylene dimethacrylate, and [2-(methacryloyloxy)ethyl]trimethyl ammonium chloride in the presence of a porogenic solvent, using ammonium peroxodisulfate as chemical initiator, and N,N,N',N'-tetramethylethylenediamine to activate the reaction. The influence of the amount of initiator, temperature, and composition of porogenic solvent on the physical and chromatographic properties of monolithic stationary phases has been investigated. A minimum plate height of 14.5 microm was obtained at 18 wt% of 1,4-butanediol in the polymerization mixture. The produced monolithic stationary phases exhibited a good repeatability and batch-to-batch and mixture-to-mixture reproducibility, with RSD values below 5.6% in the electrochromatographic parameters studied. A comparison with columns prepared by thermal initiation with alpha,alpha'-azobisisobutyronitrile (AIBN) was also performed. The most efficient column initiated with peroxodisulfate showed better efficiencies and selectivities than that prepared with AIBN at the same composition mixture.     

Thermal processing of algal biomass for biofuel production

Concerns over the environment and energy security have led to considerable research efforts into the development of renewable alternatives to fossil-based fuels and chemical from biomass. Algae has been identified as the biomass with great potential for utilization in this regard, due to several advantages algae has over terrestrial plants, such as a higher growth rate and photosynthetic efficiency, better CO₂ sequestration, and the ability to grow in non-arable land with low quality water. Conversion technologies, particularly thermochemical conversion, are actively being researched and developed to produce renewable chemicals and fuels. A major advance in this regard is thermal conversion of whole algal biomass, especially wet processing that can significantly reduce the cost of production. This short review looks at major developments in thermal processing of algal biomass with primary focus on the past two years.     

The analytical laboratory computer as a management aid

Intelligent use of the data available in the store of the analytical laboratory computer can provide much of the information necessary for the optimization of laboratory resources. The research manager can use such information to monitor the activity of various projects and the cost effectiveness of the analytical service.     

Rapid analysis of native neomycin components on a portable capillary electrophoresis system with potential gradient detection

A simple method based on capillary electrophoresis with potential gradient detection was developed to separate and detect neomycin components within 4 min without a derivatization step. Satisfactory separation and good repeatability were obtained using a separation buffer composed of 1 mM ammonium citrate (pH 3.5). The linearity of the method ranged from 10 to 1000 ppm with a limit of detection for neomycin B of about 7 ppm. After a simple dilution and filtering pretreatment step, neomycin components in three real samples were successfully analyzed without any major interference. Due to its simplicity and reliability, this method could provide an excellent alternative to the assays currently listed in U.S. and European Pharmacopoeia. The experiments were performed on a portable capillary electrophoresis system and, hence, the method can be readily applied to field analysis and point-of-care testing. Figure Photo of portable CE-P2-PGD system     

An analysis of coating-efficiency as a measure for capillary column performance

Summary An expression is proposed for the value of the Coating-Efficiency C. E. starting from the Golay-equation, extended to situations of appreciable pressure drop by Giddings. A comparison is made between the coating-efficiency following this theory and the simplified expression for coating-efficiency as generally used in the literature, that neglects the effects of resistance to mass transfer in the liquid phase and the pressure drop. It is shown that the complete equation from the coating-efficiency explains the observations made in practice. Application of the theory described will lead to a better check on film formation in capillary columns.     

Carbon nanotube-enhanced separation of DNA fragments by a portable capillary electrophoresis system with contactless conductivity detection

It was demonstrated that separation of DNA fragments by a CE-contactless conductivity detection system (CE-CCD) could be enhanced with multiple-wall carbon nanotubes (MWCNs) as buffer additive. For HaeIII digest of PhiX174 DNA, optimized MWCN concentration was obtained when the MWCN was above its threshold concentration, at which MWCN could form a network in the buffer as pseudostationary phase to provide additional interaction sites. In the case of larger DNA, MWCN near or below its threshold concentration was enough to provide great improvement of the resolution, which was shown by the separation of the 2-Log DNA ladder. Furthermore, the buffer containing MWCN could provide a more stable baseline in the CE-CCD system, owing to less fluctuation of its conductivity. Compared with CE-UV, CE-CCD with MWCN could provide lower LODs as well as better resolution.     

Affinity capillary electrophoresis with a DNA-nanoparticle conjugate as a new tool for genotyping

We have developed a novel method for genotyping based on free solution affinity capillary electrophoresis. We prepared DNA-nanoparticle conjugates by mixing biotin-modified DNA and NeutrAvidin-modified polystyrene nanoparticles; this mixture was then injected into a capillary. Subsequently, we injected the fluorescent-labeled sample DNAs into the capillary, applied the voltage, increased its temperature after 7 min, and detected the fluorescence at its anodic end. This novel method was applied for genotyping human c-K-ras, and the three genotypes were definitely distinguishable with high reproducibility. This method can be easily automated, and it is useful for high-throughput gene mutation analysis.     

Formamide as solvent for capillary zone electrophoresis

A comprehensive investigation of a number of aspects when using formamide as background electrolyte solvent in capillary zone electrophoresis was presented. It included (i) the change of the ion mobility with ionic strength, (ii) the influence of the ionic strength on diffusion coefficients, and (iii) on the separation efficiency expressed by the maximum reachable plate numbers (when only longitudinal diffusion contributed to zone broadening), (iv) the effect of the solvent on pKa values (taken from the literature) of neutral and cation acids, (v) the establishment of the a pH scale in formamide by dissolving acids with known pKa values and their salts at defined proportion (thus circumventing the problem of calibrating the pH meter), (vi) the agreement between the experimentally derived and the theoretical dependence of the effective mobility on pH, (vii) the uptake of water of this hygroscopic solvent from the humidity of the environment and its consequence to the ion mobilities, pKa values, and the chemical stability of the solvent (e.g., hydrolysis), and finally (viii) the use of conductivity and indirect UV absorption to enable detection of analytes below the optical cutoff of formamide.