Performance of a simple UV LED light source in the capillary electrophoresis of inorganic anions with indirect detection using a chromate background electrolyte

Light emitting diodes (LEDs) are known to be excellent light sources for detectors in liquid chromatography and capillary electromigration separation techniques, but to date only LEDs emitting in the visible range have been used. In this work, a UV LED was investigated as a simple alternative light source to standard mercury or deuterium lamps for use in indirect photometric detection of inorganic anions using capillary electrophoresis with a chromate background electrolyte (BGE). The UV LED used had an emission maximum at 379.5 nm, a wavelength at which chromate absorbs strongly and exhibits a 47% higher molar absorptivity than at 254 nm when using a standard mercury light source. The noise, sensitivity and linearity of the LED detector were evaluated and all exhibited superior performance to the mercury light source (up to 70% decrease in noise, up to 26.2% increase in sensitivity, and over 100% increase in linear range). Using the LED detector with a simple chromate-diethanolamine background electrolyte, limits of detection for the common inorganic anions, Cl-, NO3-, SO4(2-), F- and PO4(3-) ranged from 3 to 14 microg L(-1), using electrostatic injection at -5 kV for 5 s.     

Chemiluminescence as a PDT light source for microbial control

The photodynamic therapy (PDT) is a combination of using a photosensitizer agent, light and oxygen that can cause oxidative cellular damage. This technique is applied in several cases, including for microbial control. The most extensively studied light sources for this purpose are lasers and LED-based systems. Few studies treat alternative light sources based PDT. Sources which present flexibility, portability and economic advantages are of great interest. In this study, we evaluated the in vitro feasibility for the use of chemiluminescence as a PDT light source to induce Staphylococcus aureus reduction. The Photogem? concentration varied from 0 to 75 μg/ml and the illumination time varied from 60 min to 240 min.The long exposure time was necessary due to the low irradiance achieved with chemiluminescence reaction at μW/cm2 level. The results demonstrated an effective microbial reduction of around 98% for the highest photosensitizer concentration and light dose. These data suggest the potential use of chemiluminescence as a light source for PDT microbial control, with advantages in terms of flexibility, when compared with conventional sources.     

发光二极管诱导荧光检测器的研制

探讨了以亮度发光二极管为诱导荧光检测激发光源的可行性，考察了直流驱动和脉冲驱动发光二极管(LED)对输出光强的影响以及LED塑料保护层厚度对输出光强的影响。发现脉冲驱动比直流驱动能提高光强3倍，无塑料保护层相对有保护层可提高光强2．5倍。采用毛细管电泳柱上检测方式对检测系统进行了评价，最小检出浓度为0．18μmol／L。结果表明该装置可以满足普通分析需求。     

Application of a xenon arc lamp as a light source for evaporative light scattering detection

The standard tungsten-halogen light source used in a commercial evaporative light scattering detector (ELSD) was replaced with a 180 W xenon arc lamp. The xenon arc lamp possesses a broader spectrum in the UV region than the halogen source. The influence of the UV transmittance of five selected solvents was studied with a size-exclusion chromatography column. This solvent parameter was not observed to influence the ELSD response between the two light source settings. With the solvents studied, better sensitivity was obtained with the xenon arc lamp than the halogen lamp. This high-energy source was applied to ceramide III analysis with an octadecyl-grafted silica column and methanol:tetrahydrofuran 97:3 as the mobile phase, and the sensitivity of the quantification of ceramide III increased 16-fold for injected amounts of 14∼140 ng. The molecular species in a sample of naturally occurring ceramides was analyzed using two C18 columns at 40 °C and gradient elution from 100% acetonitrile to 100% isopropanol in 30 min. The increased ELSD sensitivity achieved when using the xenon arc lamp allowed both the minor and major ceramide species to be observed, in contrast to the results achieved when the halogen lamp was used, where the increased photomultiplier voltage needed to observed the signals from the minor species caused the signals from the major ceramide species to occur above the detector response window.     

Analysis of micro-contact printed protein patterns by SPR imaging with a LED light source

We demonstrate the characterization of mu-contact printed protein patterns and analysis of protein-protein interactions by two-dimensional (2-D) surface plasmon resonance imaging (SPRi). Advancements in SPRi image quality from employing a light emitting diode (LED) as the light source are described. We show that a LED offers an ideal point source that can eliminate interference artifacts and speckles found when using a laser source. The attainable thickness resolution in fixed-angle imaging is comparable to that of a monochromatic source, providing a solid foundation for quantitative analysis with the system. The SPR imaging technique reported here affords sub-nanometer thickness sensitivity and micrometer lateral resolution, allowing for convenient studies of biomolecular interactions and surface morphologies of ultrathin films. Spatially well-defined protein patterns of bacterial toxins were obtained by microcontact printing using a polydimethylsiloxane (PDMS) stamp on a functionalized self-assembled monolayer on Au. The influence of protein concentration in the inking solution on transfer efficiency was investigated, and a nonlinear correlation was observed between the solution concentration and the amount of protein immobilized on the surface. Quantitative analysis of protein interaction was performed with toxin-specific antibody, showing a concentration-dependent relationship that verifies the retention of biological activity of the protein after printing. The study demonstrates the feasibility and effectiveness of using LEDs as light sources in SPR imaging, opening doors for developing compact SPR instruments for direct, sensitive, and label-free detection of biohazardous molecules.     

Analysis of riboflavin in beer by capillary electrophoresis/blue light emitting diode (LED)-induced fluorescence detection combined with a dynamic pH junction technique

A simple, inexpensive and reliable method for the routine analysis of riboflavin in beer by capillary electrophoresis-light emitting diode (CE-LED) induced fluorescence detection is described. A simple and straightforward sample preparation is involved and the method is based on an inexpensive blue LED as the light source combined with an on-line sample concentration technique. For this detection system, using a normal micellar electrokinetic chromatography (MEKC), stacking-MEKC and dynamic pH junction techniques, the detection limits were found to be 480, 20 and 1 ng mL⁻¹, respectively. In addition, the number of theoretical plates for riboflavin was determined to be 3.8×10⁴ by means of a dynamic pH junction and this was improved to 3.2×10⁶ when the dynamic pH junction-sweeping mode was applied. The concentrations of riboflavin in 12 samples of different types of commercial beer were found to be in the range of 130-280 ng mL⁻¹.     

Development of chemoselective photoreduction of nitro compounds under solar light and blue LED irradiation

Solar light and blue light irradiation of the commercially available heterogeneous nano photocatalyst TiO₂–P25 leads to reduction of nitro compounds to give the corresponding amines. The methodology provides a green and mild approach to this useful class of organic compounds. Aromatic nitro compounds containing a wide range of functional groups tolerated the conditions to give, chemoselectively the corresponding amines in excellent yields.     

A portable, inexpensive and microcontrolled spectrophotometer based on white LED as light source and CD media as diffraction grid

A portable, microcontrolled and low-cost spectrophotometer (MLCS) is proposed. The instrument combines the use of a compact disc (CD) media as diffraction grid and white light-emitting diode (LED) as radiation source. Moreover, it employs a phototransistor with spectral sensitivity in visible region as phototransductor, as well as a programmable interrupt controller (PIC) microcontroller as control unit. The proposed instrument was successfully applied to determination of food colorants (tartrazine, sunset yellow, brilliant blue and allura red) in five synthetics samples and Fe²⁺ in six samples of restorative oral solutions. For comparison purpose, two commercial spectrophotometers (HP and Micronal) were employed. The application of the t-paired test at the 95% confidence level revealed that there are not significant differences between the concentration values estimated by the three instruments. Furthermore, a good precision in the analyte concentrations was obtained by using MLCS. The overall relative standard deviation (R.S.D.) of each analyte was smaller than 1.0%. Therefore, the proposed instrument offers an economically viable alternative for spectrophotometric chemical analysis in small routine, research and/or teaching laboratories, because its components are inexpensive and of easy acquisition.     

Two-dimensional electrophoresis on a microfluidic chip for quantitative amino acid analysis

Analysis of complex biological samples requires the use of high-throughput analytical tools. In this work, a microfluidic two-dimensional electrophoresis system was developed with mercury-lamp-induced fluorescence detection. Mixtures of 20 standard amino acids were used to evaluate the separation performance of the system. After fluorescent labeling with fluorescein isothiocyanate, mixtures of amino acids were separated by micellar electrokinetic chromatography in the first dimension and by capillary zone electrophoresis in the second. A double electrokinetic valve system was employed for the sample injection and the switching between separation channels. Under the optimized conditions, 20 standard amino acids were effectively separated within 20 min with high resolution and repeatability. Quantitative analysis revealed linear dynamic ranges of over three orders of magnitudes with detection limits at micromolar range. To further evaluate the reliability of the system, quantitative analysis of a commercial nutrition supplement liquid was successfully demonstrated. Figure       

Spectrometer with microreaction chamber and tri-colour light emitting diode as a light source

This paper describes a tri-colour light emitting diode (LED)-photoresistor (PR)-based in situ spectrometer with geometry that differs from the previously presented and allows for small volumes of test solution (350 μl) and effective homogenisation of reagents. The emission maximums of the tri-colour LED (TC-LED) are at 470, 565 and 660 nm. The basic measuring characteristics of the prototype were evaluated. The prototype was tested for determination of calcium in natural waters with the o-cresolphtalein complexon and was proved to be useful for real life applications. The in situ spectrometer with microreaction chamber enables the rapid optimisation of experimental conditions, as was demonstrated on the example of oxidation of alcohols with potassium dichromate. The drop-based experimental approach to the ruggedness test is fast, economic and gives reliable results with the minimum waste production. The prototype, connected to the computer, functions as a kinetic microreactor suitable also for following rapid changes. In spite of the manual addition of the initialising reagent, the data are lost only during the first 3 s.     

Integration of a flow-type chemiluminescence detector on a glass electrophoresis chip

A glass electrophoresis microchip integrated a flow-type chemiluminescence (CL) detection cell has been developed and evaluated. The chip pattern is a double-T-type electrophoretic sample injection and separation combining with a Y-type chemiluminecent detector. The double-T geometry allows for high-efficiency sample injection and geometric definition of sample plug size. The branch of Y was used as CL reagent channel, and the CL reagent was delivered by a lab-made micropump. Bis[(2,4,6-trichlorophenyl)]oxalate-H₂O₂ CL system was employed to detect dansyl amino acids. On this microchip, dansyl-phenylalanine and -sarcosine were successfully separated by electrophoresis and detected within 250 s. The detection limits (S/N=3) of dansyl-phenylalanine and -sarcosine could reach to 2.8 and 3.2 μM, respectively, due to the vigorous dilution of sample with CL reagent and timely removal of the waste solution from reaction area.     

Electrokinetic sorting and collection of fractions for preparative capillary electrophoresis on a chip

A microfabricated device capable of selecting and collecting multiple components from a mixture separated by capillary electrophoresis (CE) is described. This collection is automated and can be easily controlled by a set of rules defined by an operator, enabling fast and consistent operation. The device consists of an electrokinetically steered fluidic network that can be divided into three sections: a CE part, a fractions distribution region and a set of storage channels. Sample fractions leave the CE channel and are detected in the interfacial region by fluorescence intensity measurements. If an upcoming peak is detected, separation is withheld and the potentials are reconfigured to force the fraction into one of the collection channels, where they become available for further processing or analysis. The sequence of separation and collection is repeated until all the bands of interest are captured. A mixture of three fluorescent dyes (Rhodamine 6G, Rhodamine B and Fluorescein) was used to demonstrate the principle. The components were repeatedly separated by means of CE and pooled in their respective storage channels. In comparison to previous developments, the system presented in this paper offers automatic collection of all fractions in a single run. Furthermore, it is possible to run the system in a repetitive mode for accumulative pooling if more fractionated sample is required.     

Mechanoluminescent light source for a fluorescent probe molecule

We have demonstrated an innovative ability of mechanoluminescent (ML) material as a light source for the first time. By appropriate smart size control and nondestructive mechanical stimulation, the ML particle can be considered a promising candidate of in situ light source for bio-imaging and photo-therapy even in a human body.     

Photocyanation of pyrene across an oil/water interface in a polymer microchannel chip

Photocyanation of pyrene (PyH) across an oil/water interface was explored by using two types of polymer microchannel chip. The chips (channel depth of 20 microm and width of 100 microm) were fabricated on the basis of photolithography and an imprinting method, with micromachined silicon templates being used for imprinting. As a typical example of the photoreaction, an aqueous NaCN solution and a propylene carbonate solution of PyH and 1,4-dicyanobenzene were brought separately into a Y-structured microchannel chip with the same flow velocity by pressure driven flow. Light irradiation onto the whole of the channel chip by a high-pressure Hg lamp resulted in formation of 1-cyanopyrene (PyCN), as confirmed by GC-MS analysis of the oil phase. The results demonstrated that the interfacial photochemical reaction of PyH proceeded successfully along the water/oil solution flow in the microchannel. Under optimum conditions by using a three-layer channel chip, absolute PyCN yields as high as 73% were attained with a reaction time of 210 s.     

Bismuth-containing layered double hydroxide as a novel efficient photocatalyst for degradation of methylene blue under visible light

Layered double hydroxide (LDH)-based photocatalysts have emerged as a very promising candidate to replace TiO₂, owing to their unique layered structure, tunable band gaps, low cost, ease of scale-up, and good photocatalytic activity. Bismuth-doped ZnCr-LDH was studied as photocatalyst in the photodegradation of methylene blue (MB). The structure and morphology of ZnCr-LDH and ZnCrBi-LDH were characterized using a different mode of delegated tools, e.g., FTIR, XRD, UV–Vis, FESEM–EDX, and TEM measurements. FESEM and TEM image of the synthesized LDHs showed that the synthesized LDH is smooth overlapping crystals, and they are approximately in hexagonal form. The material was found to be a good photocatalyst for degradation of methylene blue in visible light, and the results showed that the photocatalytic activity of ZnCrBi-LDH sample is higher than of ZnCr-LDH sample. According to the kinetic data, the reaction rate constant of ZnCrBi-LDH is approximately four times higher than the apparent reaction rate constant of ZnCr-LDH. The catalytic activity was retained even after four methylene blue degradation cycles, indicating that the LDH could be an important addition to the field of wastewater treatment.     

Application of plasma-polymerized films for isoelectric focusing of proteins in a capillary electrophoresis chip

The first use of plasma polymerization technique to modify the surface of a glass chip for capillary isoelectric focusing (cIEF) of different proteins is reported. The electrophoresis separation channel was machined in Tempax glass chips with length 70 mm, 300 microm width and 100 microm depth. Acetonitrile and hexamethyldisiloxane monomers were used for plasma polymerization. In each case 100 nm plasma polymer films were coated onto the chip surface to reduce protein wall adsorption and minimize the electroosmotic flow. Applied voltages of 1000 V, 2000 V and 3000 V were used to separate mixtures of cytochrome c (pI 9.6), hemoglobin (pI 7.0) and phycocyanin (pI 4.65). Reproducible isoelectric focusing of each pI marker protein was observed in different coated capillaries at increasing concentration 2.22-5 microg microL(-1). Modification of the glass capillary with hydrophobic HMDS plasma polymerized films enabled rapid cIEF within 3 min. The separation efficiency of cytochrome c and phycocyanin in both acrylamide and HMDS coated capillaries corresponded to a plate number of 19600 which compares favourably with capillary electrophoresis of neurotransmitters with amperometric detection.     

New benzo[b]furans as electroluminescent materials for emitting blue light

[structure: see text] New functionalized mono- and bis-benzo[b]furan derivatives were synthesized and developed as blue-light emitting materials. They possessed a CN, CHO, CH=CHPh, CH=CPh(2), or CH=CHCOOH group at the C4-position. Two benzo[b]furan nuclei in bis-benzo[b]furan derivatives were connected by a divinylbenzene bridge. With good volatility and thermal stability, bis-benzo[b]furan 7a was fabricated as a device. It emitted blue light with brightness 53430 cd/m(2) (at 15.5 V) and high maximum external quantum efficiency 3.75% (at 11 V).     

Thin-film polymer light emitting diodes as integrated excitation sources for microscale capillary electrophoresis

We report the use of a thin-film polymer light emitting diode as an integrated excitation source for microfabricated capillary electrophoresis. The polyfluorene-based diode has a peak emission wavelength of 488 nm, an active area of 40 microm x 1000 microm and a thickness of similar 2 mm. The simple layer-by-layer deposition procedures used to fabricate the polymer component allow facile integration with planar chip-based systems. To demonstrate the efficacy of the approach, the polyfluorene diode is used as an excitation source for the detection of fluorescent dyes separated on-chip by electrophoresis. Using a conventional confocal detection system the integrated pLED is successfully used to detect fluorescein and 5-carboxyfluorescein at concentrations as low as 10(-6) M with a mass detection limit of 50 femtomoles. The drive voltages required to generate sufficient emission from the polymer diode device are as low as 3.7 V.     

Facile solvothermal synthesis of highly active monoclinic scheelite BiVO4 for photocatalytic degradation of methylene blue under white LED light irradiation

In this study, BiVO₄ was successfully synthesized via the solvothermal process using a solvent mixture of ethylene glycol and water under different synthesis conditions of temperature and pH. Physicochemical properties such as crystal phase, morphology, and optical absorption of the as-synthesized BiVO₄ samples were characterized by X-ray diffraction (XRD), Raman spectra, field emission scanning electron microscopy (FE-SEM), and ultraviolet–visible diffraction reflection spectroscopy (UV–vis DRS). The XRD analysis showed that different synthesis conditions of temperature and pH significantly affected the growth of monoclinic BiVO₄ crystals oriented along (0 4 0) facets. Form SEM results, the synthesis conditions, including pH and temperature, have a great effect on the morphology of monoclinic structured BiVO₄. As the pH value increases in the range of 0–9 and temperature increases from 80 °C to 180 °C, the morphology of BiVO₄ changed from peanut-, rod-, and leaf-like shapes. The photocatalytic activities of as-synthesized BiVO₄ photocatalysts were evaluated by the photodegradation of methylene blue (MB) dye under irradiation of white LED light. We have found that by using appropriate synthesis conditions (the synthesis temperature of 140 °C and the synthesis pH of 7) the BiVO₄ exhibited high photocatalytic efficiency for MB degradation (about 82.30% after 180 min of irradiation). This result is due to the development of the BiVO₄ crystals oriented along (0 4 0) facets with an increase in the intensity ratio of I_(0 4 0)/I_(1 2 1). The growth of BiVO₄ crystals oriented along (0 4 0) facets may be beneficial to enhance the photocatalytic activity of monoclinic scheelite BiVO₄.     

Stoichiometry of the MexA-OprM binding, as investigated by blue native gel electrophoresis

Multidrug resistance has become a serious concern in the treatment of bacterial infections. A prominent role is ascribed to the active efflux of xenobiotics out of the bacteria by a tripartite protein machinery. The mechanism of drug extrusion is rather well understood, thanks to the X-ray structures obtained for the Escherichia coli TolC/AcrA/AcrB model system and the related Pseudomonas aeruginosa OprM/MexA/MexB. However, many questions remain unresolved, in particular the stoichiometry of the efflux pump assembly. On the basis of blue native polyacrylamide gel electrophoresis (BN-PAGE) (Wittig et al., Nat. Protoc. 2006, 1, 418-428), we analyzed the binding stoichiometry of both palmitylated and non-palmitylated MexA with the cognate partner OprM trimer at different ratios and detergent conditions. We found that β-octyl glucopyranoside (β-OG) detergent was not suitable for this technique. Then we proved that MexA has to be palmitylated in order to stabilized the complex formation with OprM. Finally, we provided evidence for a two by two (2, 4, 6, or upper) binding of palmitylated MexA per trimer of OprM.