Beam optics studies for the planned hybrid electrostatic-magnetic guided slow positron beam in Hong Kong

Design simulations are presented of a variable energy (0–40 keV) slow-positron beam that incorporates the convenience of magnetic guidance with the desirability of some electrostatic focusing produced by a lens structure operating in a low but increasing magnetic field region. Filtering of unmoderated positrons and gamma rays is to be accomplished using two conventionalE×B filters. In a novel way it is proposed that the final beam energy be adjusted using a simple linear de-acceleration stage and that the optimal electrostatic element potentials for efficient extraction, focusing and filtering of positrons be floated relative to the de-acceleration potential. The resulting intense and easily controllable sub-millimetre diameter beam should be suitable for both lateral and depth profiling of defects in semiconductor materials.Paper presented at the 132nd WE-Heraeus-Seminar on Positron Studies of Semiconductor Defects, Halle, Germany, 29 August to 2 September 1994     

Capillary electrophoresis for determination of free and albumin-bound bilirubin and the investigation of drug interaction with bilirubin-bound albumin

Capillary electrophoresis (CE) is a promising technique for assessment of free bilirubin and its interaction with albumin, as it requires only a small sample volume and provides a rapid and efficient separation of free bilirubin from its albumin-bound complex in a one-phase system. In order to maintain the equilibrium without dissociation of bilirubin from the albumin/bilirubin complex as in real clinical conditions, the coupling of CE with frontal analysis (FA) was investigated. A very large sample plug was introduced hydrodynamically into the capillary (36 cm length, 50 microm inner diameter) at 15 psi x s to develop the frontal conditions during CE separation. The working conditions for CE/FA separation of bilirubin and albumin were optimized as follows: +20 kV; running buffer, 10 mmol/L phosphate and 1 mmol/L ethylenediaminetetraacetic acid (EDTA), pH 7.4. The working range for bilirubin was found to vary from 5 to 206 micromol/L; precision with relative standard deviation (RSD) <2.0% for n = 3 and detection limit (signal to noise, S/N = 2) was 2 micromol/L. The residual binding capacity of a simulated cord blood serum for bilirubin was 26 mg/100 mL at pH 7.4. Bilirubin was shown to be displaced from albumin when aspirin was added. The free bilirubin concentration was found to increase to clinical significant concentrations from 11.9 to 21.1% when increasing aspirin was added in the range of 5-50 mg/100 mL, respectively. Thus, the investigation of aspirin displacement of bilirubin from albumin is clinically important and the CE/ FA method is a suitable procedure for this purpose.     

Genotyping the -6A/G functional polymorphism in the core promoter region of angiotensinogen gene by microchip electrophoresis

Angiotensinogen (AGT) gene has been regarded as one of the candidate genes for essential hypertension. In our study, the role of AGT gene as a putatively predisposing gene for hypertension was evaluated by genotyping a A (-6) G polymorphism in the core promoter region in 123 patients with essential hypertension and 103 healthy controls. A microchip electrophoresis method coupled with polymorphism chain reaction (PCR)-restriction fragment length polymorphism (RFLP) assay was used for genotyping the A (-6) G single-nucleotide polymorphism. The separation and detection of the digested PCR amplicons were completed just in 280 s or less. The genotype frequency fulfilled the criteria of the Hardy-Weinbery equilibrium (X2 = 3.067, P > 0.05). The results showed a higher frequency of the -6 A allele (0.70) in the normotensive subjects, which is higher than those reported in Germany (0.47) and Czech (0.40) populations, but similar to that found in Japanese populations (0.73). The frequencies of genotype AA, AG, and GG were 0.46, 0.49, and 0.05 in hypertensive subjects, and 0.44, 0.53, and 0.03 in control subjects. There is no significant difference in the distributions of the genotype and allele between the two groups (X2 = 0.88, P > 0.05; X2 = 0.024, P > 0.05). These findings differ from some of the results obtained in other ethnic groups, indicating the potential importance of ethnic origin in the assessment of genetic risk identifiers for a complex disease.     

Luminescence Behavior of Polynuclear Alkynylcopper(I) Phosphines

A series of soluble trinuclear and tetranuclear copper(I) complexes containing ₃-^l acetylides , and have been synthesized and shown to exhibit rich photoluminescent behavior at room temperature. The electrochemistry of the trinuclear Cu(I) acetylide complexes and the excited-state redox properties of have been investigated. The X-ray crystal structures of and have been determined.     

On mathematical models of stress-strain relationship for living soft tissues

How detailed must a mathematical expression of the mechanical properties of a tissue be? The answer depends on the use intended for the constitutive equation. With the objective of application to physiology and medicine, a simplified approach is recommended. We point out that all biological tissues are composites and have complex behavior. In general, there is no "natural" state. Preconditioning is necessary to obtain repeatable experimental results. The viscoelastic properties of several tissues are examined and a unique feature is pointed out in that the stress-strain relationship in cyclic loading and unloading is not very sensitive to strain rate, and that the hysteresis loop is virtually constant for a wide range of frequencies. This is interpreted as being due to a continuously distributed spectrum of relaxation times which spread over a very wide range. This unique feature justifies the assumption of "pseudoelasticity," and the use of a pseudo strain-energy function to derive the stress-strain relationship in specific loading processes. Basic materials and tissues of higher structures may need other considerations. For example, in the lung the contribution of the surface tension between the air-liquid interface on the interalveolar septa is a major factor. The derivation of the stress-strain relationship for the lung tissue is presented.     

Experimental and theoretical investigations of the loss of amino acid side chains in electron capture dissociation of model peptides

Loss of side chains from different amino acid residues in a model peptide framework of RGGGXGGGR under electron capture dissociation conditions were systematically investigated, where X represents one of the twenty common amino acid residues. The alpha-carbon radical cations initially formed by N-Calpha cleavage of peptide ions were shown to undergo secondary dissociation through losses of even-electron and/or odd-electron side-chain moieties. Among the twenty common amino acid residues studied, thirteen of them were found to lose their characteristic side chains in terms of odd-electron neutral fragments, and nine of them were found to lose even-electron neutral side chains. Several generalized dissociation pathways were proposed and were evaluated theoretically with truncated leucine-containing models using ab initio calculations at B3-PMP2/6-311++G(3df,2p)//B3LYP/6-31++G(d,p) level. Elimination of odd-electron side chain was associated with the initial abstraction of the hydrogen from the alpha-carbon bearing the side chain by the N-terminal alpha-carbon radical. Subsequent formation of alpha-beta carbon-carbon double bond leads to the elimination of the odd-electron side chain. The energy barrier for this reaction pathway was 89 kJmol-1. This reaction pathway was 111 kJmol-1 more favorable than the previously proposed pathway involving the formation of cyclic lactam. Elimination of even-electron side chain was associated with the initial abstraction of the gamma-hydrogen from the side chain by the N-terminal alpha-carbon radical. Subsequent formation of beta-gamma carbon-carbon double bond leads to the elimination of the even-electron side chain and the migration of the radical center to the alpha-carbon. The energy barrier for this fragmentation reaction was found to be 50 kJmol-1.     

Preparation and Characterization of a Novel Palladium Complex: cis‐Dichloride(1,2‐bis(diphenylphosphino)vinyl‐P,P′,C)palladium(II)‐(bis(diphenylphosphino)methane‐P,P′)cobaltacarbonyl

A novel palladium complex 4, cis‐dichloride(1,2‐bis(diphenylphosphino)vinyl‐P,P′,C)palladium(II)‐(bis(diphenylphosphino)methane‐P,P′)cobaltacarbonyl, was obtained and characterized from the treatment of [(μ‐Ph₂PCH₂PPh₂)Co₂(CO)₄][(Ph₂PC≡CPPh₂)‐PdCl₂] 3 with hydrochloric acid. The framework of 4 can be regarded as a grouping of two metal‐containing fragments: ‐Co(CO)₂(dppm) and PdCl2(μ‐P,P‐Ph₂PCH=C(‐)PPh₂).     

The binding characteristics and intracellular localization of temoporfin (mTHPC) in myeloid leukemia cells: phototoxicity and mitochondrial damage

The state of aggregation of the photosensitizer meso-tetrahydroxyphenylchlorin (mTHPC) in both cell free and intracellular environment was elucidated by comparing its absorption and excitation spectra. In methanol, mTHPC existed as monomers and strongly fluoresced. In aqueous solutions such as phosphate-buffered saline (PBS), mTHPC formed nonfluorescent aggregates. Some portion of mTHPC monomerized in the presence of 10% fetal calf serum PBS. In murine myeloid leukemia M1 and WEHI-3B (JCS) cells, cytoplasmic mTHPC were monomeric. By using organelle-specific fluorescent probes, it was found that mTHPC localized preferentially at the mitochondria and the perinuclear region. Photodynamic treatment of mTHPC-sensitized leukemia cells caused rapid appearance of the apoptogenic protein cytochrome c in the cytosol. Results from flow cytometric analysis showed that the release of cytochrome c was especially pronounced in JCS cells, and well correlated with the extent of apoptotic cell death as reported earlier. Electron microscopy revealed the loss of integrity of the mitochondrial membrane and the appearance of chromatin condensation as early as 1 h after light irradiation. We conclude that rapid release of cytochrome c from photodamaged mitochondria is responsible for the mTHPC-induced apoptosis in the myeloid leukemia JCS and M1 cells.