Detection of reducing sugars in urine specimens by paper-chromatography

Summary The separation by paper chromatography and identification of reducing sugars in urine is described.

---

Zusammenfassung Die papierchromatographische Trennung und Identifizierung reduzierender Zucker im Harn wird beschrieben.

---

Résumé On décrit la séparation par Chromatographie sur papier et l'identification des sucres réducteurs dans l'urine.

     

Detection of nitric oxide in single cells

Nitric oxide (NO) is endogenously generated by nitric oxide synthase (NOS) enzymes and is involved in a surprisingly wide range of biological functions. As efforts are made to elucidate the regulatory mechanisms of NOS expression and function, there is increasing interest in following NOS activity directly by monitoring NO production. Additionally, spatial and temporal measurements of NO are important for understanding its function and metabolism. In this work, developments in technology enabling NO detection in biological systems are reviewed. Measuring NO at single cell levels is important as NOS is heterogeneously distributed; however, such measurements are difficult as physiological NO levels are in the low nanomolar to low micromolar range. Here, three categories of analytical techniques enabling NO detection at single cell levels are highlighted: fluorescence microscopy, capillary electrophoresis with laser induced fluorescence detection, and electrochemistry. For each, the basic principles, performance, applications, figures of merits and limitations are presented in terms of single cell NO detection.     

Detection of negative ions in glow discharge mass spectrometry for analysis of solid specimens

A new method is presented for elemental and molecular analysis of halogen-containing samples by glow discharge time-of-flight mass spectrometry, consisting of detection of negative ions from a pulsed RF glow discharge in argon. Analyte signals are mainly extracted from the afterglow regime of the discharge, where the cross section for electron attachment increases. The formation of negative ions from sputtering of metals and metal oxides is compared with that for positive ions. It is shown that the negative ion signals of F^? and TaO₂F^? are enhanced relative to positive ion signals and can be used to study the distribution of a tantalum fluoride layer within the anodized tantala layer. Further, comparison is made with data obtained using glow-discharge optical emission spectroscopy, where elemental fluorine can only be detected using a neon plasma. The ionization mechanisms responsible for the formation of negative ions in glow discharge time-of-flight mass spectrometry are briefly discussed.     

Detection of single oxygen molecules with fluorescence-labeled hemocyanins

This study introduces a method to detect individual oxygen molecules by fluorescence microscopy of single hemocyanins. These respiratory proteins from a tarantula bind oxygen with high affinity. A spectrometric signature of the oxygenated protein is transferred to an attached fluorescence label, which can be detected at the single-molecule level. This technique opens new perspectives for the development of small and sensitive oxygen sensors as well as for the investigation of cooperative oxygen binding in respiratory proteins.     

Detection by ESR of oxygen molecules formed as defects in single crystals

ESR spectra of alkali perhalate and halate crystals recorded at low temperature after UV- or X-irradiation contain “families” of ESR signals attributable to O₂ molecules trapped in definite orientations with respect to the host lattice. Preliminary spin hamiltonians are reported for O₂ molecules formed during photolysis of KBrO₄ crystals.     

A method for trace element determination of single Daphnia specimens using total reflection X-ray fluorescence spectrometry

Two new preparation techniques for total-reflection X-ray fluorescence (TXRF) element determination of single freshwater crustacean specimens (dry weight: 3–40 μg ind⁻¹) have been developed and tested using Daphnia pulex from a deep, oligotrophic freshwater lake located in southern Chile. Dry method: Specimens were washed with 0.2 μm filtered lake water and frozen in liquid nitrogen. The freeze-dried Daphnia specimens were weighed using an ultra-fine microbalance and placed on quartz glass carriers for TXRF analysis. Wet method: Specimens were washed with 0.2 μm filtered lake water and placed on quartz glass carriers for TXRF analysis and dried in air. The dry weight was determined using the previously established body length–dry weight relationship. Method validation for both the dry and the wet preparation method in combination with TXRF spectrometry for the element determination in small single freshwater crustaceans showed that both methods can be used for routine investigations. There were no significant differences between the dry and the wet methods concerning the elements Ca, K, Fe, Zn, Br, P, Cu, but the determination of Mn, S and Sr revealed significant differences between the two methods. It seems that the dry method yields more precise results, but the wet method is easier to handle in the field when samples cannot be fixed with liquid nitrogen.     

Integration of a contactless conductivity detector into a commercial capillary cassette. Detection of inorganic cations and catecholamines

A contactless conductivity detector integrated into the capillary cassette of Agilent ^3DCE equipment is described. The detector is user-friendly, compact and easily modified. The UV detector of the ^3DCE equipment is available parallel with the contactless conductivity detector increasing the detection power. Two electrolyte solutions, 2-(N-morpholino)ethanesulfonic acid–histidine solution (20 mM, pH 6.0) and ammonium acetate (10 mM, pH 4.0), were used as the separation media for inorganic cations and organic catecholamines, respectively. The detection limit for all metal cations except barium was under 0.5 mg/l, and that for four catecholamines was ca. 10 mg/l. This last value was the same order of magnitude as achieved with parallel UV detection.     

Spectrophotometric and titrimetric determination of catecholamines

Ammonium metavanadate is used to determine adrenaline, noradrenaline, isopropylnoradrenaline and methyldopa by titrimetric and photometric procedures. Oxidation of these catecholamines produces aminochrome derivatives which can be measured spectrophotometrically at 485 nm. Beer's law is obeyed over the ranges 0.09-0.90 mg for adrenaline, 0.07-0.65 mg for noradrenaline, 0.07-0.75 mg for isopropylnoradrenaline and 0.10-0.95 mg for methyldopa.     

Radon measurements in groundwater

A device was developed for the collection, containment, and bubbling of radon from groundwater samples to facilitate concentration measurements in the field without the need for fragile glassware. Wellwater supplies were collected in high-potential areas of New York State in a comparison of the device with traditional methods (liquid scintillation and laboratory-based Lucas-cell counters). Waterborne radon levels to 4100 Bq L^–1 reveal the potential contribution to indoor air from everyday water use in a home, as levels of 1500 Bq L^–1 contribute about 150 Bq m^–3 (the EPA-recommended limit) to indoor-air radon levels. With a Geographic Information System (GIS), spatial coordinates from each site are used to correlate concentrations with bedrock geology.     

Detection of a single DNA base-pair mismatch using an anthracene-tagged fluorescent probe

A novel anthracene-tagged oligonucleotide can discriminate between a fully-matched DNA target sequence and one with a single mismatching base-pair through a remarkable difference in fluorescence emission intensity upon duplex formation.     

Detection of DNA fragmentation in a single apoptotic cardiomyocyte by electrophoresis on a microfluidic device

The detection of doxorubicin-induced apoptosis in individual cardiomyocytes was performed on a microfluidic device. Microstructures integrated on a CD-like plastic disk were adapted for the selection of individual cells their lysis in an alkaline environment and the separation of released apoptotic DNA fragments. The fragments with typical 180 base pairs ladder pattern were electrophoretically resolved in a 2% solution of linear polyacrylamide with 0.1 M NaOH on a migration distance of 6 mm. The laser-induced fluorescence of fragments labeled by ethidium bromide was monitored by a photomultiplier tube mounted on a confocal microscope. The causal relation between the enhanced doxorubicin concentration and the extent of DNA fragmentation in a single cell was confirmed. The results show that the extent of DNA fragmentation is proportional to the time of a cell treatment. Onset of necrosis was evident in cardiomyocytes treated by doxorubicin for more than 24 h. The adverse effect of doxorubicin, an important cytostatics used for the treatment of many solid tumors, leads to the destruction of cardiomyocytes and, consequently, may result in the heart failure of treated individuals. Therefore, the monitoring of the extent of apoptotic DNA damage of cardiac myocytes represents critical step toward understanding of the development of chronic doxorubicin-induced cardiomyopathy.     

Detection of 27 molecules in a single injection volume by Hadamard transform capillary electrophoresis.

A concentration detection limit of 100 fM was achieved for the fluorescein ion by improving the experimental setup used for Hadamard transform capillary electrophoresis. Two argon-ion lasers, a gating laser for sample injection and a probe laser for the excitation of analyte molecules, were employed for the efficient photodegradation of analyte molecules in laser-induced fluorescence detection using an optically gated sample-injection method. In addition, a dichroic mirror, located in the pathway of the probe laser was used to exclude the other lines of the argon-ion laser. Using a Hadamard matrix on the order of 2046, the concentration limit of detection for fluorescein ion was determined to be 100 fM at S/N = 3, in which the average number of molecules in a single injection volume was calculated to be 27. The influences of the output power in both the gating and probe lasers on the sensitivity are also discussed.     

Plasma free and conjugated catecholamines in clinical disorders

Conclusion The data suggest that sulfation of CA may not simply be ascribed to platelets, to the liver, to vascular beds, or to organs along the vena cava including the adrenal glands. The unchanged degree of conjugation in patients with increased spillover of NE and E point to a balance between free and sulfated CA. A normal ratio of free to conjugated NE and E observed in patients receiving high dosage DA infusion further indicates that there is an adequate sulfate supply and no apparent substrate inhibition of the conjugation process. Hypothyroidism may affect the balance of free to conjugated CA in a yet unknown way.

---

Freie und konjugierte Catecholamine bei unterschiedlichen Erkrankungen

     

Detection of single nucleotide polymorphism using tension-dependent stochastic behavior of a single-molecule template

Single nucleotide polymorphism (SNP) is the most common genetic variation among individuals. The association of SNP with individual's response to pathogens, phenotypic variations, and gene functions emphasizes the importance of sensitive and reliable SNP detection for biomedical diagnosis and therapy. To increase sensitivity, most approaches employ amplification steps, such as PCR, to generate detectable signals that are usually ensemble-averaged. Introduction of amplification steps increases the complexity of a system, whereas ensemble averaging of signals often suffers from background interference. Here, we have exploited the stochastic behavior of a single-molecule probe to recognize SNP sequence in a microfluidic platform using a laser-tweezers instrument. The detection relies on on-off mechanical signals that provide little background interference and high specificity between wild type and SNP sequences. The microfluidic setting allows multiplex sensing and in situ recycling of the SNP probe. As a proof-of-concept, we have detected as low as 100 pM of an SNP target associated with coronary heart diseases within half an hour without any amplification steps. The mechanical signal permits the detection of single mutations involving either G/C or A/T pairs. We anticipate this system has the capacity to function as a highly sensitive generic biosensor after incorporation of a specific recognition element, such as an aptamer for example.     

Detection of single ion channel activity on a chip using tethered bilayer membranes

Membrane-bound ion channels are promising biological receptors since they allow for the stochastic detection of analytes at high sensitivity. For stochastic sensing, it is necessary to measure the ion currents associated with single ion channel opening and closing events. However, this calls for stability, high reproducibility, and long lifetimes. A critical issue to overcome is the low stability of the ion channel environment, that is, the bilayer membrane. A promising technique to surmount this is to connect the lower part of the membrane to a surface forming a tethered bilayer membrane. By reconstituting the synthetic ion channel, gramicidin A, into a tethered bilayer as part of a microchip design, we have been able to record the activity of single ion channels. The observed activity was compared with that obtained by a conventional electrophysiology method, tip dipping, to confirm its authenticity. These findings allow for the construction of stable biosensors based on ion channels and provide a novel technique for the characterization of ion channel activity.