Electric probe measurements of high-voltage sheath collapse in cathodic arc plasmas due to surface charging of insulators

High-voltage sheath dynamics near a negatively biased substrate in cathodic arc plasmas are investigated using a biased electrical probe. Since the sheath is devoid of electrons, the sheath boundary can be inferred from the position where a positively biased probe draws no electron current. The extent of the sheath is primarily dependent on the plasma density, the ion velocity and the applied voltage. Using insulating substrates, the sheath boundary eventually retracts due to a dynamic reduction in the applied voltage. This reduction is caused by positive charge accumulation on the insulator surface. The collapse time of the sheath is dependent on the plasma density and the substrate characteristics. We believe this to be the first direct observation of the reduction in the width of the high-voltage sheath when implanting an electrical insulator using plasma-based ion implantation (PBII). This information is important when determining the optimal parameters for plasma-based ion implantation of insulators. Our measurements are compared with theoretical predictions based on the Child-Langmuir equations for high-voltage sheaths. By choosing appropriate values for the secondary electron coefficient the theory could be made to fit the experimental data. A discussion of the validity of the choice of secondary electron coefficients is presented.     

Transition Metal Ion-binding Properties of a 14-Membered N2O2S2- Macrobicyclic Ligand

The selective liquid–liquid extraction of various transition metal cations from the aqueous phase to the organic phase was carried out using a 14-membered N₂O₂S₂-macrobicycle. Metal picrates such as Pb²⁺, Co²⁺, Zn²⁺, Ni²⁺,Cu²⁺ and Cd²⁺ were used in this extraction studies. It was found that the ligand showed moderate selectivity towards Pb²⁺ only among the other metals. The extraction constant (log K _ex) was determined to be 13.8 for Pb²⁺ complex.     

Studien über den Hofmannschen Abbau quartärer Ammoniumverbindungen

Ohne Zusammenfassung     

Protein immobilization capacity and covalent binding coverage of pulsed plasma polymer surfaces

Three carbon surfaces were deposited using pulsed plasma enhanced chemical vapour deposition method: a low and a high nitrogen-containing plasma polymer surfaces and a diamond-like carbon surface. The surfaces were analysed using both X-ray photoelectron spectroscopy (XPS) technique and the enzyme-linked immunosorbent assay (ELISA) method combining with sodium dodecyl sulphate (SDS) cleaning to investigate the capacity and covalent binding of the immobilized proteins. A good correlation was found on quantification of remaining protein after SDS cleaning using the ELISA method and the XPS technique. All surfaces had similar initial capacity of protein attachment but with large different resistance to SDS cleaning. The analysis showed that the high nitrogen-containing plasma polymer was the best biocompatible material due to its highest resistance to SDS cleaning, i.e. with the highest quantity (∼80%) of proteins bound covalently.     

Capillary electrophoresis of liposomes functionalized for protein binding

CE enabled assessing the attachment of hexa-histidine-tagged proteins to functionalized phospholipid liposomes. The liposomes were made of 1-palmitoyl-2-oleoyl-sn-glycero-3-phosphocholine, phosphatidyl-ethanolamine, cholesterol and distearoyl-glycero-3-phosphoethanolamine-N-methoxy(polyethylene glycol) in a molar ratio of 29:26:40:5. The unilamellar vesicles, which had an average diameter of 170 nm, were labelled by inclusion of FITC-dextran for fluorescence detection. CE was carried out in poly(vinyl alcohol) (PVA)-coated capillaries at 25 degrees C with a BGE consisting of Tris-HCl (50 mM, pH 8.0). For conjugation of the liposomes with the proteins (soluble synthetic receptor fragments with molecular mass of 60 and 70 kDa, respectively), Ni(2+) was implanted into the vesicle surface by an anchor lipid containing a nitrilotriacetate acid (NTA) group as complexation agent for the metal ions. The difference in surface charge enabled the separation of the different species of interest by CE: plain vesicles, vesicles functionalised with Ni-NTA, vesicle-protein complexes and the species formed upon removal of the Ni-ions by complexation with EDTA. Loss of the Ni-ions resulted in the release of the proteins and the reappearance of the plain Ni-free NTA-liposome species in the electropherograms.     

Nuclear spin-lattice and nuclear spin-spin relaxation time measurements in EuB6 at low temperatures using the spin-echo technique

Experimental results on the nuclear spin-lattice and nuclear spin-spin relaxation times in the ferromagnetic EuB₆ at temperatures below 4·2 K are presented using the external magnetic field,H _ext, in the range of 0 ⩽H _ext ⩽ 10 kG. Nuclear spin-spin relaxation time computed on the basis of the Suhl-Nakamura process turns out to be 3·2μs, which compares well with the experimental value 11·1μs obtained with the 10 kG magnetic field at 1·7 K. It is found that in the ferromagnetic EuB₆,T ₁ is approximately 5 × 10³ times larger thanT ₂ at 1·7 K with the 10 kG magnetic field. Thus the effect ofT ₁ onT ₂ can be neglected. From the experimental value ofT ₂, the value of the homogeneous line broadening is found to be 14 kHz. The corresponding value obtained from the cw method is 175 kHz. This evidently shows the presence of the inhomogeneous line broadening in the cw NMR.     

Comparison of protein surface attachment on untreated and plasma immersion ion implantation treated polystyrene: protein islands and carpet

Surface attachment of the enzyme horseradish peroxidase (HRP) was studied on untreated and ion beam implanted polystyrene (PS) films. The PS films of 100 nm thickness on a silicon wafer were treated using the plasma immersion ion implantation (PIII) technique, with argon ions of energy 20 keV and fluences of up to 2 x 10(16) ions/cm2. Differential transmittance Fourier transform infrared (FTIR) spectra confirmed the presence of proteins on the PS surfaces by detection of the amide A, I, and II protein vibrations. Spectroscopic ellipsometry over the UV-vis spectral region provided the optical constants and thickness of the protein layer, while tapping mode atomic force microscopy (AFM) was used to image the protein distribution on the surface. The combination of AFM, ellipsometry, and FTIR analysis showed that, on the untreated PS surface, HRP formed islands 8 nm in height and 30 nm in lateral size, covering approximately 27% of the PS surface. After PIII modification of the PS surface, the protein covered 100% of the surface area.