Interaction of tetraphenyl-porphyrin derivatives with DPPC-liposomes: an EPR study

The effect of the symmetry and polarity of the porphyrin molecules on their membrane localization and interaction with membrane lipids were investigated by electron paramagnetic resonance (EPR). For this purpose, two glycoconjugated tetraphenyl porphyrin derivatives were selected, respectively, symmetrically and asymmetrically substituted. Small unilamellar liposomes composed of dipalmitoylphosphatidylcholine (DPPC) and spin labeled stearic acids were prepared. The spin probe was located at the 5th or 7th or 12th or 16th position of the hydrocarbon chain in order to monitor various regions of the lipid bilayer. EPR spectra of porphyrin-free and porphyrin-bound liposomes were recorded at various temperatures below and above the phase transition temperature of DPPC. The effect on membrane fluidity proved to be stronger with the asymmetrical porphyrin derivative than with the symmetrical one. The rigidity increased when the spin label was near lipid head groups. The difference observed between control and porphyrin-treated samples when measured below the main lipid transition temperature disappeared at higher temperature. When the spin label was near the end of the hydrophobic tails, the symmetrical porphyrin derivative caused increase in fluidity, while the asymmetrical one slightly decreased it. To explain this phenomenon we propose that the asymmetrical derivative exerts a stronger ordering effect caused by its fluorophenyl group located at the level of the lipid heads, which is attenuated to the hydrophobic tails. The perturbing effect of the symmetric derivative could not lead to similar extent of ordering at the head groups and looses the hydrocarbon chains deeper in the membrane.     

Ultrafast detection of microsatellite repeat polymorphism in endothelin 1 gene by electrophoresis in short capillaries

The methodology and instrumentation for fast denaturing electrophoresis in short capillaries was developed and exemplified by detection of short tandem repeat polymorphism in the endothelin 1 gene. The resolution of two nucleotides, which is required for the detection of a dinucleotide repeat polymorphism, was achieved in a capillary of an effective length of 2.5 cm at a temperature of 600C and an electric field strength of 600 V/cm in 42 s. Thus, the use of denaturing electrophoresis in short capillaries with laser-induced fluorescence detection resulted in a reduction of analysis time by a factor of 200 when compared to the conventional slab gel electrophoresis. The developed methodology and instrumentation is advantageous for an implementation in clinical diagnostics and genetic population screening where fast analytical instrumentation amenable to automation is of paramount importance.     

Conformational analysis 29: Preparation and1H and13C NMR,FTIR, MS,and crystallographic conformational and configurational study of 3-Oxo-1,3-oxathiane and its monomethyl derivatives

3-Oxo-1,3-oxathiane (1) and its monomethyl derivatives were prepared by oxidation of the corresponding 1,3-oxathianes. The structural analysis was carried out by¹H and¹³C NMR, FTIR, and mass spectrometry. At 298 K compound1 was a 1 1 (at 173 K a 3 1) mixture of the SO(ax) and SO(eq) chair forms. The major oxidation products of methyl 1,3-oxathianes attained exclusively the SO(ax), Me(eq) chair forms except that of the 5-methyl derivative, which consisted of 7% of the SO(eq), Me(ax) chair conformation in CDCl₃ solution. The minor products of oxidation existed in anancomeric SO(eq), Me(eq) chair conformations. The oxidation of 2-methyl- 1,3-oxathiane, however, led to 3,3-dioxo derivative (6) in addition to thetrans [SO(eq)] monoxide. The crystal structures of6 andtrans-3-oxo-5-methyl-1,3-oxathiane were solved by X-ray diffractometry.     

Voltammetric studies of a psychotropic drug with nitro groups. Determination of flunitrazepam in urine using HMDE

The adsorption behaviour of flunitrazepam at the hanging mercury drop electrode was studied by staircase voltammetry and by adsorptive stripping differential pulse voltammetry. Flunitrazepam is adsorbed in the whole potential range, from the most positive values up to the reduction potential. Flunitrazepam reduction product is also adsorbed. The time dependence of the voltammetric response proves that a diffusion-controlled adsorption takes place. Flunitrazepam can be determined (down to nanomolar levels) by using adsorptive preconcentration prior to the differential pulse voltammetric scan. An application of such a method to flunitrazepam determination in human urine is described. The detection limit was 30 ng per milliliter of urine with a 20-sec accumulation time; the mean relative standard deviation was lower than 3.2% and the mean recovery 97.8%.     

Cyclic sulfonium salts with S ... O interactions 2. Molecular structures with six-membered rings

1-[2-(N-methylcarbamoyl)phenyl]-3H-2,1-naphto-(1,8-d,e)-oxathiin-1-ium chloride (2), 1-[2-(N-methylcarbamoyl)-phenyl]-2-methyl-3-oxo-3H-1, 2-naphto-(1,8-d,e)-thiazin-1-ium chloride (3), 1-[8-(N-methylcarbamoyl)naphtyl]-2-methyl-3-oxo-3H-1, 2-naphto-(1,8-d,e)-thiazin-1-ium chloride (4) and 1-(8-carboxylatonaphtyl)-2-methyl-3-oxo-3H-1,2-naphto-(1,8-d,e)-thiazin-1-ium dipolar ion (5) cyclic sulfonium salts were prepared and their chemical properties investigated (spirosulfurane-formation, hydrolysis). The molecular structures obtained from x-ray diffraction can be described with a considerably distorted trigonal bipyramidal arrangement of the ligands about the sulfonium center, with O/N—S ... O=apical angles of 173.9, 164.9, 156.6, and 159.0°, as well as with S—O/N apical bond lengths of 1.648, 1.671, 1.664, and 1.682 Å. The structures exhibit relatively short S ... O close contacts with interatomic distances of 2.253, 2.448, 2.795, and 2.619 Å.     

Lipophilicity determination of some new crown ethers by reversed-phase thin-layer chromatography

Summary The lipophilicity of 28 modified crown ether derivatives was determined by reversed-phase thin-layer chromatography (RPTLC) using various organic phases and supports. The lipophilicity values determined in different RPTLC systems showed good correlations, however the quality of the organic phase (methanol, acetone, acetonitrile) and the support characteristics influenced to a small extent the determination.     

Strukturanalyse organischer Sulfide mit Hilfe der Gras-Chromatographie

Zusammenfassung Eine Methode der Identifizierung von Alkyl- und Arylgruppen organischer Sulfide wurde ausgearbeitet, die die Spaltung dieser Stoffe mit Raney-Nickel zur gaschromatographischen Bestimmung der dabei entstandenen Kohlenwasserstoffe ausnützt.

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Summary A method was developed for identifying alkyl- and aryl groups of organic sulfides. The method employs the cleavage of these materials with Raney nickel for the gas chromatographic determination of the resulting hydrocarbons.

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Résumé On a mis au point une méthode d'identification des groupes alkylés et arylés des sulfures organiques exploitant la dissociation de ceux-ci par le nickel Raney pour le dosage par chromatographic en phase gazeuse des carbures d'hydrogène qui se forment.

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Die Autoren danken den Kollegen Dr.M. Veea, Ing.J. Petránek und Ing.J. Gaspari für die Überlassung von Proben organischer Sulfide.     

Estudios sobre ácidos hidroxámicos

Résumé On propose un procédé de microdosage des groupements méthoxyles dans les pectines, qui repose sur la libération de ces groupements par saponification de l'hydroxylamine alcoolique dans un appareil, sur leur transformation en formiates de méthyle et sur leur distillation. Le formiate de méthyle forme ainsi l'acide formhydroxamique que l'on dose par colorimétrie à l'état de chélate avec le fer-III.On réalise l'hydrolyse de la pectine à 100° C en tube scellé. On fait réagir avec l'acide formique en excès, une partie aliquote de l'hydrolysat dans le micro-appareil de distillation déjà décrit. Le procédé convient pour 1 à 3 mg de pectine et la durée des opérations est de deux heures et demies. Sa spécificité est satisfaisante bien que le groupe éthoxyle puisse gêner. Son action est d'ailleurs peu vraisemblable, puisqu'il ne fait pas partie de la molécule de pectine. Les résultats du procédé sont en générale un peu plus bas que ceux des méthodes volumétriques servant à ce dosage. On a étudié la reproductibilité pour les esters méthyliques et l'on a mis en évidence une erreur par défaut de 2 à 4%. Les plus petites quantités de groupes méthoxyles que l'on puisse doser sont de 20g. Le procédé recommandé est une application particulière de méthodes applicables de façon générale au dosage des esters méthyliques dans les substances organiques. Ce sera l'objet d'une autre communication de cette série.

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Summary A micromethod is given for determining methoxyl groups in pectins. It is based of the liberation of these groups by saponification, conversion into methyl formate, and distillation of the latter into a receiver containing alcoholic hydroxylamine. The methyl formate reacts to give formhydroxamic acid, which is determined colorimetrically as iron(III) chelate.The hydrolysis of the pectin is conducted at 100° C in a sealed tube. An aliquot part of the hydrolysate is brought into reaction with excess formic acid in a microdistillation apparatus that was described previously. The procedure is suitable for 1 to 3 mg pectin and requires 21/2 hours for all partial operations. The specificity is satisfactory, even though ethoxyl may interfere. However, this latter is not likely to be encountered since ethoxyl has not been shown to be a constituent of the pectin molecule. The results given by the procedure are in general inferior to those of volumetric methods. The reproducibility was tested on methyl esters and showed a minus error of 2 to 4%. The smallest amount of methoxyl which can be determined in this way is 20g. The method proposed here is a special application of a method which can be applied in general to the determination of methyl esters in organic substances, which will be the subject of a later paper in this series.

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Zusammenfassung Es wird ein Mikroverfahren zur Bestimmung der Methoxylgruppen in Pektinen angegeben, das auf der Freisetzung dieser Gruppen durch Verseifung, deren Umwandlung in Methylformiat und dessen Destillation in eine Vorlage von alkoholischem Hydroxylamin beruht. Das Methylformiat bildet damit Formhydroxamsäure, die als Eisen(III)-chelat kolorimetrisch bestimmt wird.Die Hydrolyse des Pektins wird bei 100° C in einem verschlossenen Rohr ausgeführt. Einen aliquoten Teil des Hydrolysates läßt man in einem schon früher beschriebenen Mikrodestillationsapparat mit überschüssiger Ameisensäure reagieren. Das Verfahren eignet sich für 1 bis 3 mg Pektin und erfordert für alle Teiloperationen 2^1/2 Stunden. Seine Spezifität ist befriedigend, obwohl Äthoxyl stören kann. Dessen Einwirkung ist jedoch wenig wahrscheinlich, da es nicht als Bestandteil des Pektinmoleküls nachgewiesen ist. Die Ergebnisse des Verfahrens sind im allgemeinen niedriger als die Resultate volumetrischer Methoden. Die Reproduzierbarkeit wurde an Methylestern überprüftund zeigte einen Minusfehler von 2 bis 4%. Die Mindestmenge bestimmbares Methoxyl beträgt 20g. Das vorgeschlagene Verfahren ist eine spezielle Anwendung einer allgemein für die Bestimmung von Methylestern in organischen Substanzen anwendbaren Methode, die Gegenstand einer weiteren Mitteilung dieser Serie sein wird.

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Resumen Se indica una microtécnica de valoración de metoxilos en pectinas, basada en la liberación del radical metilo éster por saponificación; en su conversion en formiato de metilo y en su simultanea destilación y recepción en hidroxilamina alcalinizada. El formiato de metilo se transforma así en ácido formohidroxámico, cuya determinación fotocolorimétrica se realiza como quelato férrico.Estas operaciones requieren efectuar la hidrólisis de la pectina en tubo cerrado y a 100° C, y en tomar una alícuota del hidrolizado, que se pasa con un exceso de ácido fórmico al aparato de microdestilación, detallado en comunicaciones anteriores. El método permite operar con 1 a 3 mg de pectina y todas las operaciones insumen unas dos y media horas. La técnica presenta condiciones satisfactorias de especificidad, pudiendo interferir los radicales etoxilos, cosa poco probable, pues no son reconocidos como componente de la molécula de pectina. Los resultados obtenidos, comparados con los del método titrimétrico, son por lo general inferiores a éste y su reproducibilidad, verificada con ésteres metílicos, tiene errores por defecto de un 2 a 4%. La cantidad mínima de metoxilo valorado alcanza a 20g. La técnica que se indica, es una aplicacion particular de otra de carácter general, aplicable a la valoración de ésteres metílicos en sustancias orgánicas, que será motivo de otra futura comunicación de esta serie.

     

Determination of molybdenum, chromium and aluminium in human urine by electrothermal atomic absorption spectrometry using fast-programme methodology

Rapid and direct procedures for the determination of molybdenum, chromium and aluminium in human urine samples are developed. Fast-programme methodology is used to simplify the heating cycles. Hydrogen peroxide, nitric acid and Triton X-100 are added to the urine samples which are directly introduced into the furnace. For molybdenum, two successive injection steps are required due to the low level of this element in the samples analyzed. Calibration is carried out using aqueous standards for aluminium and the standard additions method for both molybdenum and chromium. The reliability of the procedures is checked by analyzing two certified reference materials.     

Determination of aristolochic acid by capillary zone electrophoresis

A simple and rapid capillary zone electrophoresis (CZE) method for the determination of aristolochic acid (AA) in dietary supplements and selected herbs is described. A clear separation of AA from other sample constituents was achieved within 5 minutes without any sample clean up. A mixture of 20 mM-morpholinethanesulphonic acid+10 mM-BisTrisPropane+0.2% hydroxyethylcelullose in 10% methanol serves as a background electrolyte. The linearity, accuracy, intra-assay and detection limit of the developed method are 200–6000 ng/mL, 95–103%, 3.5%, and 50 ng/ml, respectively. Ease of use, sufficient sensitivity and low running cost are the most important attributes of the CZE method. The proposed CZE method was compared with HPLC.