Effect of aeration and unsaturated fatty acids on expression of the Saccharomyces cerevisiae alcohol acetyltransferase gene

The reduction of acetate ester synthesis by aeration and the addition of unsaturated fatty acids to the medium has been reported to be the result of the reduction in alcohol acetyltransferase (AATase) activity induced by inhibition of this enzyme. However, regulation of the AATase gene ATF1 has not been reported. In this study, ATF1 gene expression was studied by Northern analysis, and the results showed that the ATF1 gene was repressed both by aeration and by unsaturated fatty acids. The results also showed that the reduction of AATase activity is closely related to the degree of repression of ATF1 mRNA, which suggested that the gene repression is the primary means of reducing AATase activity in vivo. Using the Escherichia coli lacZ gene as a reporter gene, it was shown that a 150-bp fragment of the 5' flanking sequence played a major role in the repression by aeration and unsaturated fatty acid addition.     

Gangliosides of dogfish (Squalus acanthias) brain

The major research objectives in organ transplantation are to palliate the lack of organs, to decrease the adverse effects of chronic immunosuppression and to improve medium-term and long-term graft survival. Xenotransplantation and induction of a permanent and specific tolerance to an allograft therefore represent two main lines of research which could partly resolve the problems of organ transplantation. The objective of this article is to evaluate the possible role of gene therapy in the development of xenotransplantation and induction of allograft tolerance. They review the various gene vectors currently available as well as the routes of administration of these vectors specific to transplantation. The place of gene therapy is then evaluated in the context of allo- and xenotransplantation. In allotransplantation, transfection of certain genes of interest into the transplant organ before implantation or into the recipient's immune system is considered. Transfection into the transplant organ of genes coding for immunomodulating cytokines (TGF-beta, IL-4, IL-10, etc.), molecules which block the second signal (CTLA4-Ig) or molecules responsible for apoptosis (Fas/FasL) is discussed. The value of gene therapy in the recipient's immune system consists of transfection onto the recipient's bone marrow cells of genes coding for major histocompatibility system molecules (HLA-DR, DQ, etc.). In xenotransplantation, gene therapy will certainly play a major role in the development of transgenic pigs expressing, on the surface endothelium of their organs, certain human molecules which regulate the activity of complement (CD55, CD59, etc.) or which modify the expression of glycosylated xenoantigens (alpha-galactosyl) recognized by performed antibodies.     

Negative strand of hepatitis C virus RNA in the liver of patients with chronic hepatitis C after interferon treatment

In patients receiving interferon therapy for chronic hepatitis C, serum hepatitis C virus (HCV) RNA often reverts from an undetectable to a detectable form after completion of treatment. Detection of the negative strand of HCV-RNA in liver tissue is regarded as an index of viral proliferation. Therefore, we investigated changes in the hepatic negative-strand HCV-RNA following interferon therapy to determine whether this parameter could predict the long-term response to treatment. The subjects of this study were 27 patients with chronic active hepatitis C. Serum positive-strand and hepatic tissue negative-strand HCV-RNA were detected using polymerase chain reaction. At the completion of interferon treatment, serum HCV-RNA was not detected in 21 patients. One year following treatment it remained undetectable in 14 of these patients but it had reverted to a detectable form in seven. The 14 patients in whom hepatic negative-strand RNA was not detected between 2 weeks and 12 months after treatment, had not relapsed after another year. In the 13 remaining patients, negative-strand RNA was found in liver tissue and serum RNA either reverted to a detectable form or remained detectable throughout. From these findings, we conclude that the detection of negative-strand HCV-RNA in liver tissue 2 weeks after the completion of interferon therapy is useful for predicting the long-term effect of therapy.     

Calcification of cervical ligamentum flavum--analysis of calcium compounds and histopathological findings

We operated 3 patients with cervical myelopathy due to calcification of ligamentum flavum (CLF). Specimens collected surgically were subjected to X-ray diffraction (XRD), Fourier transform infrared spectroscopy (FTIR) and Raman spectroscopy (Raman) analysis and also histopathological examination. The calcium compounds deposited were calcium pyrophosphate dihydrate (CPPD) in Case 1, apatite in Case 2, and a double-layer structure with an outer CPPD layer and an inner carbonate apatite layer in Case 3. Histopathologically, CPPD deposition in Case 1 could be distinguished from apatite deposition in Case 2 and 3 by hematoxylin-eosin stain. Chondrocytes were observed in all 3 cases, suggesting the chondrocytes may have played a role in calcification in these three cases. To date, 62 cases of CLF (including the present cases) have been reported, and analysis of calcium compound has been performed for 29 of them. Of these 29, 15 were analyzed as calcium phosphate compounds, 9 as CPPD and 4 cases as mixed crystals like Case 3. However the analysis method and result about CPPD are no problem, the analysis result of calcium phosphate compounds depends on the using methods. Calcium phosphate or undetectable compounds was identified by XRD as hydroxyapatite (HAp), and by FTIR as calcium phosphate or undetectable compound. Analysis of calcium phosphate compounds should be condacted and identified by XRD, FTIR, and Raman. We propose two possible mechanisms for the formation of the double-layer structure in Case 3: one is formation of apatite first followed by deposition of CPPD outside, and the other is formation of CPPD first followed by conversion of CPPD in the central region to apatite. What the process of formation of the double-layer was in this cases remains unclear.     

Effects of the creep deformation on the fractal dimension of the grain boundaries in an austenite steel

The change in the fractal dimension of the grain boundaries during creep was investigated using an austenitic SUS304 steel at 973 K. The fractal dimension of the grain-boundary surface profile (the fractal dimension of the grain boundaries, D, 1 < D < 2) in the plane parallel to the tensile direction (in the parallel direction) and in the transverse direction, was examined on specimens deformed up to rupture (about 0.30 creep strain). Grain boundaries became serrated and the fractal dimension of the grain boundaries increased with increasing creep strain, because the density of slip lines which formed ledges and steps on grain boundaries increased as the creep strain increased. The increase in the fractal dimension due to creep deformation was slightly larger under the higher stress (118 MPa) than under the lower stress (98 MPa), while the increase of the fractal dimension with strain was a little larger in the specimens tensile-strained at room temperature (293 K) than in the crept specimens. These results were explained by the grain-boundary sliding and the diffusional recovery near grain boundaries, which lowered the increase of the fractal dimension with the creep strain. The fractal dimension of the grain boundaries in the parallel direction was slightly larger than that in the transverse direction in both creep at 973 K and tensile deformation at room temperature, especially at the large strains. This could be correlated with the shape change of the grains by creep or plastic deformation. Grain-boundary cracks were principally initiated at grain-boundary triple junctions in creep, but ledges, steps and carbide precipitates on serrated grain boundaries were not preferential nucleation sites for the cracks.     

Application of AC plasma display panels to radiation detectors

Radiation detector proposals that use plasma display panels are rare. In this work, we confirmed a radiation detector that uses plasma display panels that are focused on the breakdown voltage shift in the ramp waveform. We adapted the cell structures, gas contents, and waveforms of plasma display panels (AC‐PDPs) for radiation detectors. Hard X‐rays and gamma rays induce electron emission into the discharge gas, resulting in generating electrons, electron multiplication, and charge accumulation on dielectrics. The radiation dose rate of hard X‐rays and gamma rays (Cs137) is measured as a breakdown voltage shift between anodes and cathodes. For gamma rays, the detection sensitivity in this experiment is not as high as in the case of hard X‐rays, but the detector can locate gamma rays. These results suggest that adapted AC‐PDPs can detect both hard X‐rays and gamma rays and can be used in a large two‐dimensional radiation detector.     

Monohexosylceramides of larval and adult forms of the tapeworm,spirometra erinacei

The occurrence of glycosphingolipids with unique carbohydrate structures in different species of cestode, Platyhelminth, which had been shown, previously, prompted us to study the molecular species of the monohexosylceramides (cerebrosides) in the pseudophyllidean cestode,Spirometra erinacei. The purpose of the study was to obtain a basis for future investigations of the physiological role of glycolipids in parasitism. Cerebrosides were isolated froms. erinacei at two growth stages, i.e., from the larval form (plerocercoid) and from the adult tapeworms (intestinal form). The cerebrosides were separated into four subfractions by silica gel column chromatography, and their constituents were analyzed by gasliquid chromatography, gas chromatography/mass spectrometry, and high-performance liquid chromatography/mass spectrometry. The hexoses of the cerebrosides consisted primarily of galactose in both growth stages, while only a small amount of glucose was detected. The ceramides were composed of sphinganine (d18∶0) and phytosphingosine (t18∶0) as sphingoid bases, and of nonhydroxy fatty acids ranging from C₁₆ to C₃₀ and hydroxy stearic acid (18h∶0). The cerebrosides of adult tapeworms contained more 18h∶0 than those of plerocercoids. The combination of hexoses and ceramides in the cerebroside molecules was slightly different in the two growth stages: the glucocerebrosides of plerocercoids contained only d18∶0-nonhydroxy fatty acids in their ceramide moieties, whereas those of adult tapeworms contained varying ceramide moieties. Our data indicate that the molecular species of glycolipids present were essentially homeostatic throughout growth in spite of the entirely different environmental conditions, although there were slight differences in the hexose distribution in the two growth stages.     

Gasification of coal impregnated with catalyst during pulverization: effect of catalyst type and reactant gas on the gasification of Shin-Yubari coal

Shin-Yubari coal was impregnated with several catalysts of different chemical types during pulverization. The resultant system was more homogeneous and reactive than systems prepared by impregnation of coarse coal. The relative activities of the catalysts were determined as a function of gasification temperature, catalyst loading and gasifying agent. The activity sequence in steam was K ? Ba ? Ni ? Fe ? coal ash. Each catalyst had a unique reaction profile. For example, using steam the specific rate or the rate per remaining fixed-carbon weight decreased with time for the iron-catalysed reaction, whereas it increased for the potassium-catalysed reaction. A similar order of activity was observed in carbon dioxide, but a different sequence was noted for the hydrogenation reaction. Transition metal catalysts were the most active. The hydrogenation reaction profiles were different from the oxidation profiles.     

A convenient preparative method of 3-hydroxy acids,and the reaction of 3-hydroxy acids with acidic materials

3-Hydroxy acids were synthesised in good yield from ketones and carboxylic acids using lithium naphthalenide in the presence of diethylamine. From cyclohexanone and propionic acid, 2-(1′-hydroxycyclohexan-1′-yl) propionic acid ( I ) was obtained in 98.3% yield. 3-Hydroxy acids were treated with various acidic materials to give 3,4-unsaturated carboxylic acids and γ-butyrolactones. From the reaction of ( I ) with p-toluenesulphonic acid or potassium bisulphate, 2-(cyclohexen-1′-yl) propionic acid ( II ) (a 3,4-unsaturated acid) was obtained (yield 98%), and with 97% sulphuric acid 2-(1′-hydroxycyclohexan-1′-yl) propionic acid lactone ( III ) was formed (93% yield). Several new γ-butyrolactones were obtained in good yield by this method.     

Enzymatic synthesis of N-acyl-l-amino acids in a glycerol-water system using acylase I from pig kidney

N-Medium- and long-chain acyl-l-amino acids were enzymatically synthesized from the corresponding l-amino acids and fatty acids using a reverse hydrolysis. Enzymes that are suitable for the synthetic reaction of N-acyl-l-amino acids were screened on the basis of hydrolytic activity toward N-lauroyl-l-glutamic acid as an indicator. Acylase I from pig kidney (EC 3.5.1.14) showed the highest N-acyl-l-amino acid hydrolytic activity among 57 commercially available enzymes tested. Acylase I effectively catalyzed the synthesis of N-lauroyl-l-amino acids except for N-lauroyl-l-proline and N-lauroyl-l-tyrosine in a glycerol-water system. Under the optimized reaction conditions, N-lauroyl-l-arginine and N-lauroyl-l-glutamic acid were obtained in conversions of 82 and 44%, respectively. The equilibrium constants calculated from the conversion obtained were 5.6, 15.4, 18.0, and 39.4 for the syntheses of N-lauroyl-l-glutamic acid, N_α-lauroyl-l-lysine, N-lauroyl-l-glutamine, and N-lauroyl-l-methionine, respectively. N-Acyl-l-arginines with myristic acid and palmitic acid as the fatty acid were also synthesized using acylase I.