IDentification of a microsomal retinoic acid synthase as a microsomal cytochrome P-450-linked monooxygenase system

• 1.1. To characterize an enzyme which metabolizes retinal in liver microsomes, several properties of the enzymatic reaction from retinal to retinoic acid were investigated using rabbit liver microsomes.
• 2.2. The maximum pH of the reaction in the liver microsomes was 7.6.
• 3.3. The K_m and V_max values for all-trans, 9-cis and 13-cis-retinals were determined.
• 4.4. The reaction proceeded in the presence of NADPH and molecular oxygen.
• 5.5. The incorporation of one atom of molecular oxygen into retinal was confirmed by using oxygen-18, showing that the reaction comprised monooxygenation, not dehydrogenation.
• 6.6. The monooxygenase activity was inhibited by carbon monoxide, phenylisocyanide and antiNADPH-cytochrome P-450 reductase IgG, but not by anti-cytochrome b₅ IgG.
• 7.7. The enzymatic activity inhibited by carbon monoxide was photoreversibly restored by light of a wavelength of around 450 nm.
• 8.8. The retinal-induced spectra of liver microsomes with three isomeric retinals were type I spectra.
• 9.9. The microsomal monooxygenase activity induced by phenobarbital or ethanol were more effective than that by 3-methylcholanthrene, clotrimazole or β-naphthoflavone.
• 10.10. These results showed that the monooxygenase reaction from retinal to retinoic acid in liver microsomes is catalyzed by a cytochrome P-450-linked monooxygenase system.

     

The breakdown of Tetrahymena ribosomes by lysosomal enzymes: Inhibition by cytosol

• 1.1. Extracts from Tetrahymena lysosomes contained acid RNase and proteinase. At pH 7.4 there was appreciable proteinase activity which was inhibited by a heat-stable protein present in cell sap.
• 2.2. Lysosomal enzymes rapidly converted 80S ribosomes to subunits at pH 7.4. Hydrolysis of ribosomal RNA was very slow at pH 7.4 but rapid at pH 5.0.
• 3.3. These reactions were inhibited by proteinase inhibitors and by cell sap, but the latter was relatively ineffective at pH 5.0.
• 4.4. It seems unlikely that ribosome breakdown in vivo is initiated by the release of lysosomal enzymes into the cytosol.

     

Effects of protein synthesis inhibitors on A- and L-site amino acid incorporation by bullfrog tadpole liver and tail fin cells

• 1.1. Cycloheximide and puromycin inhibited leucine transport and incorporation into isolated bullfrog tadpole tail and hepatic cells.
• 2.2. However, high concentrations of these 2 inhibitors did not affect alanine incorporation appreciably in either tissue.
• 3.3. NEM and DNP inhibited leucine and alanine incorporation in both cell types, but at different concentrations.
• 4.4. NEM stimulated leucine transport only in hepatocytes; alanine transport was inhibited by NEM in tail fin cells.
• 5.5. The results suggest different mechanisms of transport and protein synthesis for the 2 types of amino acids by tadpole liver and tail fin cells.

     

Impact of histamine treatment and feeding on the hydrolytic enzyme level of Tetrahymena in culture and in conditions of starvation

• 1.1. The unicellular Tetrahymena pyriformis contains and also produces hydrolytic enzymes, such as glucosidase, phosphatase and glucosaminidase.
• 2.2. Return of Tetrahymena to plain medium after treatment with bacteria alone, histamine alone or bacteria plus histamine was equally followed by persistence of the hydrolytic enzyme activity around the control value and an activity increase at about 60 min.
• 3.3. Incubation of Tetrahymena in salt (Losina-Losinsky) solution after the applied treatment accounted for reduction to practically zero of the glucosidase and glucosaminidase activities, whereas the phosphatase activity tended to increase rather than to decrease in both the bacterium-treated and histamine-treated cultures.
• 4.4. The enzyme activity patterns of the Tetrahymena cells pretreated (imprinted) with histamine did not differ from the control pattern either after re-exposure to histamine or after feeding with bacteria, but showed a uniformization of the activity pattern and a considerable decrease in enzyme activity on incubation (starvation) in salt (Losina-Losinsky) solution.

     

Biosynthesis of membrane and a membrane glycoprotein in Tetrahymena pyriformis

• 1.1. A membrane glycoprotein was isolated from Tetrahymena surface membrane with properties similar to mammalian erythrocyte glycoprotein.
• 2.2. This membrane glycoprotein had a specific acitivity less than whole membrane at various time intervals up to 40 hr.
• 3.3. In double labelling experiments, glucosamine contributed a greater degree of the labelling of this glycoprotein than did amino acids.
• 4.4. Greater incremental increases in the glucosamine radioactivity over amino acids at the longer time intervals suggests that the carbohydrate and protein moieties may have independent metabolic pathways.
• 5.5. When Tetrahymena was grown in proteose peptone-tryptone in the presence of labelled amino acid, the specific activity of the surface membrane was less than one-tenth of the specific activity obtained in defined growth media. Under these same conditions, there were only slight changes in the specific activities of glucosamine in the membrane.
• 6.6. Data is presented suggesting independent synthesis of the protein and oligosaccharide from different pools.

     

RNA synthesis in two species of anopheline mosquitoes

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• 1.1. A method is described for the extraction of adult mosquito nuclear RNA. The RNA is tightly bound to nuclear components. The nuclei were dispersed by the use of sodium chloride and urea of high ionic strength.
• 2.2. Deproteinization of the cytoplasmic minus mitochondria fraction resulted in the separation of a high molecular weight RNA. The RNA is derived from a polynucleotide precursor in the nucleus and transported to the cytoplasm.
• 3.3. The rate of RNA synthesis in Anopheles quadrimaculatus and A. albimanus was measured by the incorporation of radiolabelled adenine into RNA. The radioactive precursor was presumably converted to the adenine nucleotide by adenine phosphoribosyltransferase.
• 4.4. The conversion of adenine nucleotides to guanine nucleotides was essentially the same in the two species, however, differences were found in the specific activities of RNA purines.
• 5.5. Cellulose powder and DEAE profiles of nuclear and cytoplasmic RNAs from the two species were compared.

     

The activities of ribosome-degrading enzymes and of a proteinase inhibitor in Tetrahymena pyriformis during starvation

• 1.1. In starved Tetrahymena acid RNase decreased but acid proteinase and a heat-stable proteinase inhibitor both increased.
• 2.2. A greater proportion of proteinase than RNase was released from the lysosomes of growing cells by homogenization, but progressively less proteinase was released during starvation.
• 3.3. Inhibitors of protein synthesis enhanced the decrease in RNase and prevented the increase in proteinase and proteinase inhibitor. Chloroquine caused a large increase in both enzymes.
• 4.4. Proteinase and RNase may be located in different lysosomes which together participate in ribosome destruction, but this process is unlikely to be limited by the total amount of these lysosomal hydrolases.

     

Selective effect of melatonin on the proliferation of lymphoid cells

• 1.1. The present study was designed to investigate the effect of melatonin on the proliferation of normal lymphocytes and certain T-lymphomas and myelomas under in vitro conditions.
• 2.2. The results revealed that administration of 200 μM melatonin inhibited significantly the incorporation of [³H]thymidine into both normal mouse and human lymphocytes and T-lymphoblastoid cell lines.
• 3.3. On the contrary, melatonin provoked an increase of myeloma cell proliferation.
• 4.4. The influence of melatonin on hybridoma cell lines was negligible.
• 5.5. Collectively, these data demonstrated that the chief pineal indole affect selectively the processes of lymphoblastoid cell growth.

     

Purification of a proteinase and proteinase inhibitor from Tetrahymen a pyriformis

• 1.1. A cysteine proteinase and cysteine proteinase inhibitor have been purified from Tetrahymena.
• 2.2. The proteinase was purified by ammonium sulphate fractionation, gel filtration, ion exchange chromatography and affinity chromatography, and appeared homogeneous by gel filtration and electrophoresis (mol. wt approx 28,000). It hydrolysed BAPNA, degraded azocasein, and converted 80S ribosomes to subunits. Thiol reagents inhibited these activities.
• 3.3. The inhibitor was purified by heat treatment, ammonium sulphate fractionation and ion exchange chromatography, and appeared homogeneous by gel filtration and electrophoresis (mol. wt approx 12.500). The inhibitor was heat stable and it inhibited papain, as well as the Tetrahymena proteinase.

     

Absorption of glucose,glycine and palmitic acid by isolated midgut and hindgut from crickets

• 1.1. In vitro experiments indicated that midgut and hindgut anterior to the Malpighian tubules are important in absorption and processing of products of digestion in crickets.
• 2.2. Isolated hindguts from crickets (Gryllus assimilis, G. rubens and Scapteriscus acletus) absorbed and released into the incubation medium 20–30% of a load of [¹⁴C]glucose and 29–31% of a load of[¹⁴C]glycine.
• 3.3. Isolated midguts from the same crickets absorbed and released into the incubation medium 30–50% of the glucose and 43–52% of the glycine load.
• 4.4. Radiolabelled palmitate was absorbed into epithelial cells of isolated mid- and hindguts, but little was transported and released into the incubation medium.

     

The role of lipoproteins in the delivery of tumour-targeting photosensitizers

• 1.I. Serum lipoproteins play an important role in the in vivo transport of several porphyrinoid derivatives having a moderate or high degree of hydrophobicity.
• 2.2. There appears to exist a correlation between the extent of photosensitizer association with low-density lipoproteins (LDL) and the efficiency of tumour targeting by some classes of photosensitizers, such as differently sulphonated porphyrins and phthalocyanines, haematoporphyrin dialkylethers and unsubstituted phthalocyanines and naphthalocyanines.
• 3.3. In all cases, LDL-carried photosensitizers are preferentially released to malignant cells; hence, direct cell damage appears to be the major determinant of tumour damage consequent to photodynamic therapy.
• 4.4. Present evidence suggests that the LDL-associated photosensitizer is accumulated by tumour cells largely via a receptor-mediated endocytotic process.
• 5.5. Thus, the use of delivery systems for orientating a systemically injected photosensitizer towards lipoproteins has been explored; promising results have been obtained by incorporation of the dye into liposomal vesicles, oil emulsions or inclusion complexes, as well as by precomplexation of the dye with LDL.
• 6.6. Moreover, a suitable choice of the chemical constituents of the delivery system and the experimental conditions allows one to modulate the photosensitizer distribution among the different lipoproteins.
• 7.7. The occurrence of tumour-targeting strategies other than the LDL pathway is briefly discussed.

     

Anaerobic uptake and utilization of glycine-2-14C by the estuarine bivalve Rangia cuneata at three salinities

• 1.1. During facultative anaerobiosis Rangia cuneata acclimated at 5, 10 and 15‰ were injected with 0.1 μCi glycine-2-¹⁴C into the pallial fluid and incubated for 3, 12, 24 and 72 h.
• 2.2. Rangia rapidly accumulated glycine from the pallial fluid.
• 3.3. Accumulation was not significantly different at 5, 10 and 15‰.
• 4.4. Glycine was only metabolized into proteins, and at a slow rate which increased as salinity decreased.
• 5.5. Glycine was not involved in production of ATP during facultative anaerobiosis.
• 6.6. Results suggest both a general decrease in ATP utilization and selective inhibition of certain pathways in order to conserve ATP for the more essential pathways.

     

Morphology of leech retzius cells demonstrated by intracellular injection of horseradish peroxidase

• 1.1. The neuronal geometry of Retzius (R) cells in two species of leech (Hirudo medicinalis and Haemopis sanguisuga) was investigated by intracellular injection of horseradish peroxidase.
• 2.2. Each R cell sends major branches into the ipsilateral segmental nerves and, via the ipsilateral connectives, into the anterior and posterior adjacent ganglia.
• 3.3. No structural connection between the proximal axons of the two R cells could be detected, although numerous dendrites were demonstrated, some of which extended across the midline of the ganglion.
• 4.4. No major differences were found between the R cell morphology of the two species.

     

NADPH/NADP ratio could regulate the glyoxylate cycle in Tetrahymena pyriformis

• 1.1. The glyoxylic acid cycle pathway could be regulated through the modulation of the isocitrate dehydrogenase-NADP activity. This enzyme is inhibited by NADPH.
• 2.2. The effect on the glyoxylate cycle flux of variations in the rate of the NADPH-consuming pathways has been studied.
• 3.3. Increase in the rate of NADPH-consuming activity by addition of H₂O₂ produces inhibition of the glyoxylate cycle and decrease in the NADPH/NADP ratio.
• 4.4. These results suggest that the glyoxylate flux in Tetrahymena could be modulated by regulation of NADP-dependent isocitrate dehydrogenase by the NADPH/NADP ratio.

     

Effect of lindane on phosphatidylinositol synthesis by cerebral cortex after acute and subchronic treatment

• 1.1. The incorporation of myo-[2-³H]inositol into phosphatidylinositols was unmodified in brain cortex miniprisms from convulsant rats.
• 2.2. However, the incorporation had increased by 300–400% in non convulsant rats which had received the same amount of lindane at a lower concentration.
• 3.3. This result suggests that phosphatidylinositols are implicated in the convulsion syndrome.
• 4.4. Experiments with lindane added in vitro were performed with both subchronically lindane intoxicated and untreated rats.
• 5.5. The results show an interesting lack of parallelism.
• 6.6. This might indicate the development of some resistance to the effects of lindane, possibly as the result of complex compensatory changes in inositol lipid biosynthesis.

     

Pyrimidine degradation in tomato cell suspension cultures and in Euglena gracilis—localization of enzymes

• 1.1. Subcellular location of dihydropyrimidinase and NCβA-amidohydrolase2 was studied in a cell suspension culture of tomato (Lycopersicon esculentum cv. Lukullus) and in Euglena gracilis.
• 2.2. By differential centrifugation, crude extracts were separated into ten fractions. Activities of both enzymes were found mainly in cytosolic fractions marked by EDH (tomato) and glu-6-P-DH (E. gracilis).
• 3.3. A cytosolic location was also found by a 20–60% and a 17.5–30% sucrose density gradients.
• 4.4. Using mitochondrial marker enzymes such as fumarase, SDH, CS and MDH, a mitochondrial occurrence of both enzymes or their release from mitochondria can be excluded by sucrose gradient centrifugations. This can also be achieved using purified mitochondria prepared from tomato cells by two subsequent sucrose gradients.
• 5.5. A possible vacuolar location of dihydropyrimidinase and NCβA-amidohydrolase was excluded by comparing their activities in isolated protoplasts and purified vacuoles which were characterized by their marker enzyme α-mannosidase.
• 6.6. A nuclear location of both enzymes and/or their release from the nucleus during procedures used cannot be excluded.
• 7.7. The results are discussed in relation to subcellular location to other pyrimidine-metabolizing enzymes in plant cells.

     

Haematology of the australian eastern quoll,Dasyurus viverrinus

• 1.1. A variety of haematological parameters were determined in adult Dasyurus viverrinus.
• 2.2. Haemoglobin and red cell counts were high with a very low mean cell volume.
• 3.3. Basophils are absent but the eosinophils contain small numbers of basophilic granules which may indicate a dual role for this cell.
• 4.4. “Ring Form” leucocytes are present.
• 5.5. Three types of red cell picture could be identified, some animals showing large numbers of spherocytes, spicule cells, and inclusion bodies.
• 6.6. These cells resemble those found in some inherited human haemolytic anaemias but there was no evidence of haemolysis in the animals.
• 7.7. An alkali resistant haemoglobin component is present.