Comparative Biochemistry and Physiology Part B: Comparative Biochemistry最新文献

Mechanical properties of catch connective tissue are greatly affected by its ionic environment. In order to understand the role of ions, a preparation was developed in which cellular activities were suppressed by treatment with 1% Triton X-100.

The material used was body-wall dermis of the sea cucumber Holothuria leucospilota Brandt.

The effects of the main cations in seawater (H⁺, Na⁺, K⁺, Ca²⁺, Mg²⁺) on the creep viscosity of the Triton model were compared with those of intact dermis.

The comparison distinguished the site of action of ions. K⁺ had its main effect on cells that control the catch mechanism, whereas Ca²⁺ worked directly on extracellular materials. H⁺, Na⁺ and Mg²⁺ had both effects.

Peroxisomes were isolated from liver tissue of control and clofibrate-treated adult male NMRI mice and Sprague-Dawley rats. Phospholipids, cholesterol, triglycerides and free fatty acids were measured in the peroxisomes. The fatty acid profiles of the phosphatidylethanolamine, the phosphatidylcholine, the triglyceride and the free fatty acid fractions were also analyzed. Phosphatidylethanolamine was the dominating phospholipid in peroxisomes from untreated animals. The fatty acid profiles of phosphatidylethanolamine, free fatty acids and triglycerides were similar for untreated mice and rats but differences between the species were observed in the pattern derived from phosphatidylcholine. Phosphatidylcholine was the most abundant phospholipid after clofibrate treatment. Clofibrate treatment caused an increase in the concentrations of phospholipids and unsaturated long-chain fatty acids and a decrease in the concentrations of triglycerides, free fatty acids, cholesterol and shorter saturated fatty acids.

Insect transposable elements occur as intracellular parasitic DNA sequences which are amplified in genomes either by a pure DNA replication mechanism, or for the most frequent elements, via reverse transcription of an RNA intermediate. Due to their structural properties and their coding potential, many of them are potentially able to invade the chromosomes. However, selection pressures and evolution have apparently established true host-parasite relationships between these “selfish” sequences and the genomes which harbour them. Transposable elements seem to be expressed only occasionally, upon stimulation by genetic or environmental factors or in situations of “genomic shocks” induced by stresses. Such an activation of a given entity in the germline will result in the amplification and dispersion of daughter copies into the host genome. This appears to have occurred recently in mosquito chromosomes for the Juan retroposons: they have been probably amplified from one master element present in a unique population which has since spread worldwide. Horizontal transfers between species might also contribute to the spread of some elements, a fact which can restrict the use of recombinant organisms in the field. There is strong evidence that transposable elements are responsible for variability and biodiversity of insect populations. For example, in Culex pipiens mosquitoes, transposition events are responsible for polymorphism in the region of the esterase B gene locus and for insecticide resistance properties. Because they may affect the biological properties of individuals carrying them, transposable elements can be tools for the development of efficient genetical control methods of pest species.

The molecular mechanisms evolved in adaptation of cellular membranes to low temperatures have been studied.

The lipid composition of membranes from digestive gland cells of two Pectinidae living at different temperatures such as Adamussium colbecki (Smith, 1902), an Antarctic mollusc, and Pecten jacobaeus L., from the Mediterranean Sea, has been compared.

Our results demonstrate that cold adaptation of the membranes from Pectinidae digestive gland cells mainly implies the regulation of the ratio of short/long and straight/branched fatty acid chains and of the cholesterol content of membranes

GTP has been shown to inhibit AlF₄⁻-stimulated, and to activate forskolin-stimulated adenylyl cyclase activity in the presence of Mg²⁺ in cell membranes from human embryonic kidney 293 cells. The maximal inhibitory response of AlF₄⁻-stimulated adenylyl cyclase activity by GTP was not dependent on the concentration of Mg²⁺, but was so in the case of forskolin-activated activity at all forskolin concentrations assayed. Mn²⁺ ions stimulated AlF₄⁻- or forskolin-activated adenylyl cyclase activity to a greater extent than Mg²⁺. The inhibition of AlF₄⁻-stimulated cyclase by GTP was still observed with Mn²⁺, but the activation of forskolin-stimulated cyclase by GTP was not. When assayed together, Mn²⁺ and Mg²⁺ showed non-additive behaviours with respect to the amount of cyclic AMP formed after AlF₄⁻-stimulation of adenylyl cyclase. The temperature dependence of the activation of adenylyl cyclase by forskolin, AlF₄⁻ or under basal conditions was observed to be somehow different in the presence of Mn²⁺ than in the presence of Mg²⁺ ions. Cholera toxin treatment produced a markedly increased cyclase activity, specially when assayed with AlF₄⁻. In the case of forskolin-activated adenylyl cyclase, UTP and CTP were unable to reproduce the cyclase activation detected with GTP. However, in the case of AlF₄⁻-stimulated adenylyl cyclase, UTP was as good as GTP at inhibiting cyclase activity, and CTP virtually eliminated the activation of the cyclase with AlF₄⁻.

Previously we have shown that the measurable soluble sialyltransferase (STase) activity released into the medium during the incubation of rat jejunal slices was dependent upon the presence of a heparin-binding fraction (HBF) from heat-inactivated serum or a trypsin-binding protein (TBP) isolated from HBF. Both HBF and TBP were able to inhibit trypsin and plasmin. The measurement of galactosyltransferase (GTase) activity which was also released in incubations was not dependent on HBF or TBP. The present study is directed towards further exploring the relationship between STase activity and protease inhibitory activity. Heat-inactivated serum from turpentine-treated rats (HTS), had higher plasmin-trypsin-inhibitory (HTS) activities compared to heat-inactivated serum from control rats (HCS). When HTS was used to supplement jejunal incubations, there was a 25–40% increase in the measurable STase activity in the incubation medium compared to similar incubations carried out in buffer alone. In contrast, with HCS the increase was 10–15%. During incubations with hepatocytes, STase activity detected in the incubation medium was increased with the incubation buffer was supplemented with HTS compared to incubations supplemented with HCS. Serum antiproteolytic activity was higher in turpentine rats compared to controls. Incubation of serum at 37°C led to a progressive decrease in plasmin-trypsin-inhibitory and STase activities. TBP a plasmin and trypsin inhibitor was able to prevent the decrease in STase activity. Overall, serum STase activity was higher in the turpentine treated rats. In contrast, GTase activity in serum as well as that detected in the medium during jejunal and hepatocyte incubations was not dependent on protease inhibitory activity. The results show that there is a relationship between soluble STase and plasmin-trypsin-inhibitory activities.

Erythrocyte aspartate aminotransferase (AST) and alanine aminotransferase (ALT) activities are often used as indices of vitamin B-6 nutritional status; however, results using a mixed population of erythrocytes can be qulte variable. Erythrocytes from two strains of mice (Mus domesticus), A/Ibg and DBA/Ibg, were separated according to age by centrifugation through discontinuous Percoll density gradients into three fractions: top (least dense, youngest), middle and bottom (most dense, oldest). A sufiicient yield of age-fractionated erythrocytes was obtained from a single mouse for all of the enzyme measurements. The activities of AST, ALT and three age-marker enzymes, pyruvate kinase, acetylcholinesterase and hexokinase, were found to be significantly higher in the youngest cell fractions, and declined in the older, more dense fractions. A mice had significantly lower AST and ALT activities in the age separated fractions than did DBA mice. The measurement of enzyme activities in low density, young cells may be especially useful in studies involving conditions in which the proportion of young erythrocytes may be elevated with respect to the entire erythrocyte mass.

Lipids and proteins in the Rathke's gland secretions of the North American mud turtle (Kinosternon subrubrum, Kinosternidae) were analyzed by gas chromatography-mass spectrometry (GC-MS) and SDS-polyacrylamide gel electrophoresis (SDS-PAGE), respectively. Analysis by GC-MS indicates 2,3-dihydroxypropanal and C₃–C₂₄ free or esterified fatty acids. Analysis by SDS-PAGE indicates a major protein component with an approximate molecular mass of 60 kDa and minor components ranging from ca. 23 to 34 kDa. The major component of K. subrubrum glandular secretions exhibits a mobility that matches that of the Kemp's ridley sea turtle (Lepidochelys kempi, Cheloniidae), suggesting that these proteins are evolutionarily conserved.

The flight muscle of adult desert locusts, Schistocerca gregaria, contains a fatty acid binding protein (FABP) that is homologous to mammalian M-FABP (cardiac FABP). In spite of the evolutionary distance between invertebrates and vertebrates, locust muscle FABP is similar to cardiac FABP in its amino acid sequence, structure, and binding behavior. While cardiac FABP is present already in the prenatal period, locust FABP is an adult specific protein; its expression is directly linked to metamorphosis. A correlation seems to exist between fatty acid oxidative capacity and FABP content in both locust and mammals. To accomplish the higher metabolic rate encountered during migratory flight, locust flight muscle cytosol contains more than three times as much FABP as that in mammalian heart. Increased fatty acid utilization by exercise or endurance training apparently induces FABP expression. Similarities and differences between vertebrate and invertebrate M-FABP are discussed in light of the proposed functions of muscle FABP as fatty acid transporter and cytoprotectant.

Lipids and phospholipids (both plasmalogen and alkyl forms) of the freshwater sponge Lubomirskia baicalensis and the sponge's gammarid parasite Brandtia (Spinacanthus) parasitica were examined. Composition of alkenyl-acyl (plasmalogen), alkylacyl and diacyl forms of major phospholipid classes, phosphatidylethanolamine and phosphatidylcholine were determined. One hundred and eighty-three fatty acids were identified by GC-MS: 46 saturated, 55 monoenoic, 35 dienoic, 25 trienoic and 22 tetra-, penta- and hexaenoic. The freshwater sponges, belonging to the family Lubomirskiidae, were shown to contain unusual long-chain fatty acids: anteiso-5, 9–28:2, branched-5, 9–29:2, 5,9,23–29:3, 5,9,23–30:3, 15,18,21,24–30:4 and 15,18,21,24,27–30:5. Some from these fatty acids were found in lipids of the amphipod parasite.