Der Nachweis des Cadmiums durch selektive Papierchromatographie

Zusammenfassung Durch die Anwendung eines H₂S-haltigen Laufmittels werden die Ionen Cu²⁺, Pb²⁺, Bi³⁺ und Hg²⁺ am Startpunkt des Chromatogramms als Sulfide fixiert, während Cd²⁺ nach kurzer Laufzeit in scharf begrenzter Zone als Sulfid im Chromatogramm nachgewiesen wird. Als Arbeitsgefäße dienen Reagensgläser. Die Spezifitäten liegen für 5 g Cd bei Cd²⁺Cu²⁺=12000, Cd²⁺Pb²⁺=12000, Cd²⁺Bi³⁺=12000, Cd²⁺Hg²⁺=1100.Herrn Prof. Dr. O. Glemser, Direktor des Anorganisch-chemischen Insituts der Universität Göttingen, danken wir für Unterstützung der Arbeit.     

Breakthrough of polymers in interactive liquid chromatography

Two separate peaks are observed for narrow polymer standards in both isocratic and gradient HPLC. One peak appears around the solvent front (the "solvent-plug peak" or "breakthrough peak"), whereas the second peak is retained significantly--or even highly. Although the effect has been observed many times before, it has never been rigorously explained. In this paper we provide a detailed explanation for the breakthrough peak. The two completely separate peaks are demonstrated not to represent to different fractions of the sample (e.g., the low- and high-molecular-mass parts of the distribution). Both peaks are representative of the entire polymeric sample for narrow polymer standard. Because the amount of the polymer in the breakthrough peak may vary, the quantitative analysis of the polymers by LC is jeopardized. The effects of the sample solvent, the (initial) mobile phase composition, the injection volume, the injected sample concentration, the column temperature, and the analyte structure and molecular mass on the breakthrough peak were investigated in LC experiments involving standards of polystyrene and poly(methyl methacrylate). Three necessary and sufficient conditionsare suggested for the breakthrough phenomenon to be observed. Recommendations to avoid the breakthrough phenomenon are given, culminating in a structured method for selecting the best possible sample solvents.     

The Azo(Azoxy) Functionality as a π2 Component in Photo [2+2] cycloadditions ‘syn’- and ‘anti’-3,4-diazatricyclo[4.2.2.22,5]dodeca-3,7-diene,syntheses, photolyses,X-ray-structure analysis,and PE spectra

The propensity of the N?N bond to undergo photo [2 + 2] cycloadditions has been further explored. In the specifically designed 1,5-azo/enes 1–3 , no [2 + 2] cycloaddition has been observed upon either direct or sensitized excitation with light of various wave lengths at temperatures down to 77 K, in line with expectations based on X-ray ( 1 : d = 2.71 Å, ω = 129°) and PE measurements ( 1 : I₁ = 8.0₀, I₂ = 9.0₅ eV; 2 ; I₁ = 8.0₀, I₂ = 9.2₅eV). The steric/stereoelectronic demands for the participation of the N?N bond in pericyclic reactions are clearly more stringent than those for the C?C bond.     

Molekül- und Kristallstruktur des 1,4-Bis[tris(tetrahydrofuran)lithium]-octaphenyltetrasilans

Molecular and Crystal Structure of 1,4-Bis[tris(tetrahydrofuran)lithium]-octaphenyltetrasilane 1,4-Dilithium-octaphenyltetrasilane prepared from octaphenyl-cyclo-tetrasilane and lithium in tetrahydrofuran (THF) [4], can be isolated from tetrahydrofuran/n-pentane as an adduct with six molecules of tetrahydrofuran per formula unit. The orange-red compound crystallizes in the triclinic space group P1 {a = 1159.6(3); b = 1268.4(2); c = 1367.8(3) pm; α = 92,23(2)° β = 113.79(2)° γ = 111.62(2)° at ?5 ± 3°C; Z = 1}. An x-ray structure determination (R_w = 0.046) shows the existence of a centrosymmetric molecule with an extended planar Li? Si₄? Li unit; either lithium atom is bound to silicon and to the oxygen atoms of three molecules of tetrahydrofuran. Characteristic bond lengths and angles are: Li? Si 271; Si? Si 241 and 243; Si? C 190 to 192 pm; Li? Si? Si 126°; Si? Si? Si 127°. ²⁹Si and ⁷Li n.m.r. measurements at low temperatures indicate the presence of three different adducts.     

Na5AlF2(PO4)2: Darstellung,Kristallstruktur und Ionenleitfähigkeit

Na₅AlF₂(PO₄)₂: Synthesis, Crystal Structure and Ionic Conductivity Two different procedures (precipitation from aqueous solution and solid state reaction) for the synthesis of hitherto unknown Na₅AlF₂(PO₄)₂ were optimized. The crystal structure was determined using diffractometer data (P3 , a = b = 10.483(1), c = 6.607(1) Å, MoKα, 1080 independent reflections, R_w = 0.025). PO₄-tetrahedra and AlO₄F₂-“octahedra” are connected via common vertices forming a twodimensionally extended heteropolyanion. Sodium is located in interconnected spacings of the [AlF₂(PO₄)₂]-part of the structure. Ionic conductivity as expected because of these structural features was affirmed experimentally.     

A structure refinement of the high pressure modification BaI2-II

A high pressure phase BaI₂-II, which can be quenched and retained as a metastable form at ambient conditions, is reported. The structure has been determined by X-ray investigations using single crystals. BaI₂-II crystallizes in an anti-Fe₂P-type arrangement, space group $\text{P}\text{6}\text{2m, a = 9.142(6)}$Å, c = 5.173(3)Å, which is slightly denser than the PbCl₂-type structure found at normal pressure. Structural features of the two phases are discussed in comparison.     

Functional organization of the outer membrane of escherichia coli: phage and colicin receptors as components of iron uptake systems.

The functional interaction of outer membrane proteins of E. coli can be studied using phage and colicin receptors which are essential components of penetration systems. The uptake of ferric iron in the form of the ferrichrome complex requires the ton A and ton B functions in the outer membrane of E. coli. The ton A gene product is the receptor protein for phage T5 and is required together with the ton B function by the phages T1 and ?80 to infect cells and by colicin M and the antibiotic albomycin, a structural analogue of ferrichrome, to kill cells. The ton B function is necessary for the uptake of ferric iron complexed by citrate. Iron complexed by enterochelin is only transported in the presence of the ton B and feu functions. Cells which have lost the feu function are resistant to the colicins B, I or V while ton B mutants are resistant to all 3 colicins. The interaction of the ton A, ton B, and feu functions apparently permits quite different "substrates" to overcome the permeability barrier of the outer membrane. It was shown for ferrichrome dependent iron uptake that the complexing agent was not altered and could be used repeatedly. Only very low amounts of 3H-labeled ferrichrome were found in the cell. It is possible that the iron is mobilized in the membrane and that desferri-ferrichrome is released into the medium without having entered the cytoplasm. Growth on ferrichrome as the sole iron source was used to select revertants of T5 resistant ton A mutants. All revertants exhibited wild-type properties with the exception of partial revertants. In these 4 strains, as in the ton A mutants, the ton A protein was not detectable by SDS polyacrylamide gel electrophoreses of outer membranes. Albomycin resistant mutants were selected and shown to fall into 5 categories: 1) ton A; 2) ton B mutants; 3) mutants with no iron transport defects and normal ton A/ton B functions, which might be target site mutants; 4) mutants which were deficient in ferrichrome-mediated iron uptake but had normal ton A/ton B functions. We tentatively consider that the defect might be located in the active transport system of the cytoplasmic membrane; 5) a variety of mutants with the following general properties: most of them were resistant to colicin M, transported iron poorly, and, like ton B mutants, contained additional proteins in the outer membrane. The outer membrane protein patterns of wild-type and ton B mutant strains were compared by slab gel electrophoresis in an attempt to identify a ton B protein. It was observed that under most growth conditions, ton B mutants overproduced 3 proteins of molecular weights 74,000-83,000. In extracted, iron-deficient medium, both the wild-type and ton B mutant strains had similar large amounts of these proteins in their outer membranes. The appearance of these proteins was suppressed by excess iron in both wild-type and mutant. From this evidence it is apparent that the proteins appear as a response to low intracellular iron rather than being controlled by the ton B gene...     

Immunoaffinity screening with capillary electrochromatography

Highly efficient capillary electrochromatographic separations of cardiac glycosides and other steroids are presented. Employing butyl-derivatized silica particles as stationary phase resulted in a nearly three times faster electroosmotic flow (EOF) compared to capillary electrochromatography (CEC) with octadecyl silica particles. On-column focusing with a preconcentration factor of 180 was performed and separation efficiencies of up to 240,000 plates per meter were obtained. Using label-free standard UV absorbance, detection limits of 10-80 nM were reached for all steroids tested. For screening of cardiac glycosides, e.g., digoxin and digitoxin in mixtures of steroids, CEC was combined with immunoaffinity extraction using immobilized polyclonal anti-digoxigenin antibodies and F(ab) fragments. Simply adding small amounts of antibody carrying particles to the samples and comparing chromatograms before and after antibody addition allowed screening for high affinity antigens in mixtures with moderate numbers of compounds. Under conditions of competing antigens, affinity fingerprints of immobilized anti-digoxigenin and anti-digitoxin antibodies were obtained, reflecting the cross-reactivity of eleven steroids. The method provides high selectivity due to the combination of bioaffinity interaction with highly efficient CEC separation and UV detection at several wavelengths in parallel. This selectivity was exploited for the detection of four cardiac glycosides in submicromolar concentrations in an untreated urine sample.     

Reinvestigation of the Conformation of Cyclosporin A in Chloroform

New investigations of cyclosporin A in CDCl₃ have been performed to obtain additional and more accurate distance restraints than utilized in our previous studies of cyclosporin A. Build-up rates at 600 MHz using 6 different mixing times at low temperatures (252.5 K) were determined and transformed into distances using the two-spin approximation. With the new distance restraints in the MD simulations using the GROMOS package, we can unambiguously conclude the presence of a βII′-turn. The new structure resembles the X-ray structure more than the structure previously determined, especially regarding the orientation of the MeBmt side chain. In the new structure and in the solid state, the side chain is folded over the backbone (although there are substantial differences in the χ₁ torsion), in contrast to the old structure, where the side chain is extended away from the backbone.     

Ionophoretische Trennung von ReCl62?, ReBr62? und ReO4?

Zusammenfassung Es wurde die ionophoretische Trennung von ReCl₆ ^2–, ReBr₆ ^2– und ReO₄ ^– unter Verwendung verschiedener Papiersorten untersucht. Am geeignetsten erwies sich das Papier 2045 b Gl von Schl. & Sch.

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Summary The ionophoretic separation of ReCl₆ ^2–, ReBr₆ ^2–, and ReO₄ ^– has been examined using different kinds of paper. Best results have been obtained with the paper 2045 b Gl from Schleicher & Schüll.

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Herrn Prof. G. Brauer danke ich für Förderung. Für die Überlassung von Rheniumverbindungen bin ich der Fa. W. C. Heraeus, Hanau, verpflichtet. Die Neutronenaktivierung wurde freundlicherweise von den Herren Dr. Marth und Dr. Köhler von der Reaktorstation in Garching bei München vorgenommen. Das Bundesministerium für Atomkernenergie und Wasserwirtschaft unterstützte die Untersuchung durch eine Sachbeihilfe.