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1.
  • 1.1. Electrophoretic separation of the hemoglobin of healthy adult Triturus cristatus reveals four components.
  • 2.2. Isoelectric focusing of the samee hemolysates in various commercial ampholytes of different chemical composition and pH range results in the separation of eight individual hemoglobin bands.
  • 3.3. The bands obtained by electrophoresis are not homogeneous as revealed by individual gel electrofocusing. They finally separate into the same eight components, as in the whole hemolysate.
  • 4.4. From the above findings it is concluded that this species has not four but eight individual hemoglobin molecular forms.
  • 5.5. Our results demonstrate lack of hemoglobin polymorphism in this species.
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2.
  • 1.1. Ultrastructural examination of the central terminals of sensory afferent neurons in both invertebrates and vertebrates demonstrates that the synapses that form the substrate for presynaptic inhibition and facilitation are almost universally present.
  • 2.2. Presynaptic modulation of afferent input acts in many ways which tailor the inflow of sensory information to the behaviour of the animal, effectively providing a means of turning this on and off, or of combining information of the same or different modalities to refine responsiveness or clarify ambiguity.
  • 3.3. Presynaptic modulation may act in several different roles on the same afferent.
  • 4.4. A comparison of the mechanisms of presynaptic inhibition in different animals demonstrates the likelihood of a variety of common mechanisms,several of which may act simultaneously on the same terminal.These include changes in the conductance of the afferent membrane to Cl-, K+and Ca2+ions, in addition to less well understood mechanisms that directly affect transmitter release.
  • 5.5.A single transmitter can produce several effects on a terminal through the same or different receptors.
  • 6.6. Ultrastructural studies of afferent terminals reveal that only a proportion of boutons on a given afferent may receive presynaptic input and that this may depend on the region of the nervous system in which these are found or on the identity of the postsynaptic neurons contacted.
  • 7.7. The synaptic relationships of afferent terminals can be complex. In invertebrates different types of presynaptic neuron may interact synaptically,as may postsynaptic dendrites in vertebrates.
  • 8.8. Axons presynaptic to afferent terminals in vertebrates frequently synapse also with dendrites postsynaptic to the afferents.
  • 9.9. In both invertebrates and vertebrates reciprocal interactions between afferents and postsynaptic neurons are seen.
  • 10.10. Ultrastructural immunocytochemistry reveals the likely dominance of GABA as an agent of presynaptic inhibition but also demonstrates the possible presence of other transmitters some of whose roles are less completely understood.
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3.
  • 1.1. Proteins from crystalline styles of twelve species of bivalve mollusc were examined under different gel electrophoresis conditions and stained to reveal both protein and carbohydrate.
  • 2.2. Native extracts of styles produced relatively few protein bands, however denaturation with SDS resulted in much more complex zymograms.
  • 3.3. All species possessed several prominent high mol wt glycoproteins.
  • 4.4. Eulamellibranchia all had a major non-glycosylated protein at approx. 62,000 mol. wt.
  • 5.5. Most Filibranchia had a major non-glycosylated protein at 37,000–50,000 mol. wt.
  • 6.6. Eulamellibranchia were a much more homogeneous group than the Filibranchia.
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4.
  • 1.1. Basic nuclear proteins from spermatozoa of the three mollusc species belonging to the class Bivalvia have been analyzed using one- and two-dimensional electrophoresis.
  • 2.2. Four nuclear basic proteins have been purified and their amino acid compositions determined.
  • 3.3. In these spermatozoa histone-type proteins coexist with protamine-like proteins.
  • 4.4. The protamine-like proteins that have been studied show different electrophoretic behavior but in general are similar, with a high content of lysine, arginine, alanine and serine.
  • 5.5. Interspecific variability has been found for the H1-like histone.
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5.
  • 1.1. An SDS-PAGE study of the qualitative and quantitative differences in protein bands from haemolymph and ovaries of Spilostethus pandurus females treated with JH or chemically allatectomized with precocene II, has been done.
  • 2.2. The SDS-PAGE study of haemolymph revealed the occurrence of three female-specific proteins. In the ovary appeared three protein fractions (A, Band C) with mol. wts similar to those from haemolymph.
  • 3.3. The three female-specific proteins from the haemolymph, and the ovary bands B,C and D were absent in the samples from PII-treated females.
  • 4.4. JH accelerates ovary growth and the relative amounts of bands B, C and D were in relation to the physiological stage of the considered ovaries.
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6.
  • 1.1. Spectra of products obtained during dopa oxidation by mushroom tyrosinase in presence of cysteine or glutathione were recorded for the first minutes of the enzymatic reaction.
  • 2.2. Two isosbestic points were defined, indicating the existence of a constant ratio between the disappearance of dopa and the formation of cysteinyl- or glutathione-dopa.
  • 3.3. Matrix analysis of these spectra verified that there were two kinetically related absorbing species in solution, these being dopa and either cysteinyldopa or glutathione-dopa.
  • 4.4. This stoichiometry (1:1) was confirmed by measuring the lag period in dopachrome accumulation, arising from the presence of thiol.
  • 5.5. A kinetic approach has been proposed for the first steps, considered common, in the eumelanin and phaeomelanin biosynthesis pathway, thereby allowing us to establish a quantitative relation between the lag period and thiol concentration.
  • 6.6. This relation can be used as a simple kinetic method for thiol evaluation.
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7.
  • 1.1. The digestion proteases in five marine species (Atlantic halibut, Hippoglossus hippoglossus (L); Dover sole, Solea solea (L); turbot, Scophthalmus maximus, (L); European lobster, Hommarus gammaarus (L); and the giant prawn, Penaeus monodon) have been compared by biochemical methods.
  • 2.2. The pH profiles for the hydrolysis of casein by extracts from the digestive systems of each species showed different characteristics; extracts from adult halibut, turbot and sole exhibited strong pepsin-like activity; whereas this enzyme was absent in P. monodon and in sole larvae.
  • 3.3. Although lobster extracts, from either the hepatopancreas or the stomach, showed peaks at pH values of 5.8 and 2.5, this latter activity did not hydrolyse a specific substrate for pepsin.
  • 4.4. Halibut and turbot digestive extracts contained an activity optimal at pH values in the region of 5.0 resembling a cathepsin-like enzyme; an activity which was not evident in the other species under similar experimental conditions.
  • 5.5. Although all species possessed trypsin-like activity, the pH profiles of activity in the neutral to alkaline region were unique to each species.
  • 6.6. The significance of these results is considered with respect to the anatomical differences in the alimentary systems of these species.
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8.
  • 1.1. The chemical modifications of enzymes is a widely used technique to gain information about the number, type and location of aminoacid residues which are essential for activity. A number of these modifiers are unstable in aqueous solutions and act irreversibly.
  • 2.2. The kinetics of such systems have previously been studied under assumptions, some of which are either unnecessary or too restrictive.
  • 3.3. We replace these assumptions by others which are more realistic and less stringent.
  • 4.4. These assumptions allow us to derive analytical expressions for the evolution of all the species involved in the reaction.
  • 5.5. From the analytical expression for the time course of the product formation an experimental design and a kinetic data analysis allowing the easy characterization of these systems are suggested.
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9.
  • 1.1. Three calcium-binding proteins have been purified from Ehrlich ascites tumor cells.
  • 2.2. They were identified by amino acid sequence analysis on selected fragments obtained by tryptic digestion.
  • 3.3. The proteins belong to the annexin family and were identified as annexins II, III and V.
  • 4.4. Antibodies raised against the proteins were used to examine for their presence in a number of murine tissues.
  • 5.5. The occurrence was found to be in reasonable accordance with earlier reports.
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10.
  • 1.1. Soluble eye lens proteins of fifteen different Sparidae species were analysed.
  • 2.2. Species-specific electrophoretic and isoelectric focusing patterns were found.
  • 3.3. Significant differences in the distribution of β and γ-crystallin protein components were noted for all species.
  • 4.4. These data suggest that the Sparidae family may be a heterogenenous taxonomic group encompassing considerable genetic diferences and with different evolutionary histories.
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11.
This paper comments on: Low, B. S., Alexander, R. D., and Noonan, K.M. Human hips, breast, and buttocks: Is fat deceptive? Ethology and Sociobiology 8: 249-247, 1987. In it I argue that:
  • 1.1. Sexual selection has probably not been the most important selection pressure on
  • 2.female human body shape.
  • 3.2. Male humans in different cultures find different aspects of the female body attractive
  • 4.and therefore are unlikely to have exerted consistent directional sexual selection on
  • 5.the female body.
  • 6.3. Breast size is not correlated with lactation success.
  • 7.4. Visible hip width is not correlated with parturition success.
  • 8.5. Women would lower their fitness if they tried to deceive men about their internal
  • 9.pelvic dimensions.
  • 10.6. There are many alternative hypothesis to explain the existence of fat onwomen's
  • 11.breast, hips, and buttocks.
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12.
  • 1.1. A comparative examination of sarcoplasmic proteins of the two nominal European species of angler-fish, Lophius piscatorius and L. budegassa was carried out using isoelectric focusing techniques.
  • 2.2. Two protein bands differing in isoelectric point proved diagnostic for L. budegassa (pI 4.40 and pI 5.75) while a third characterized L. piscatorius (pI 4.65).
  • 3.3. These species-specific protein profiles provide a method of species discrimination independent of morphological criteria.
  • 4.4. Within-species heterogeneity of banding pattern suggested the presence of polymorphic gene loci of potential use in studies of population structure.
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13.
  • 1.1. The blue shrimp (Penaeus stylirostris) haemolymph is capable of agglutinating the red blood cells of several vertebrates to different titres. However, the haemagglutinin is considered non-specific because it is incapable of differentiating erythrocytes of human blood types A, B and O.
  • 2.2. Haemagglutinating activity and serum protein content were determined for male and female blue shrimp ranging in size from 8.5 to 16 cm. Haemagglutinating activity decreased significantly with animal size, while protein content was unaffected.
  • 3.3. The above finding is probably related to maturation of the immune system and could explain the higher susceptibility of young shrimp to parasitic and viral diseases.
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14.
  • 1.1. A kinetic analysis of the Michaelis-Menten mechanism for the case in which both the substrate and the product are unstable, either spontaneously or as the result of the addition of a reagent, has been made.
  • 2.2. The explicit time course equations of the immediate product and the species into which it subsequently is transformed have been derived under the conditions of rapid equilibrium and limiting substrate concentration.
  • 3.3. The validity of these equations has been checked using numerical simulations.
  • 4.4. The kinetic data analysis which we suggest is based on the time progress curves of the product or, in the case in which the product accumulation cannot be monitored experimentally, on the time progress curve of the species into which the immediate product is transformed.
  • 5.5. This analysis allows the determination of the rate and the equilibrium constants if adequate experimental results are available.
  • 6.6. We have chosen a numerical example, with which we illustrate the procedure of the kinetic data analysis by simulating some curves with assumed experimental errors.
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15.
  • 1.1. The utility of biochemical genetic methods of bird identification was investigated for some common species which create a hazard for commercial aviation in Ireland.
  • 2.2. Sixteen enzyme loci were assayed in eight species, using starch gel electrophoresis; three larids, three corvids and two columbids.
  • 3.3. Genera were distinguishable using all but two loci.
  • 4.4. Differences within genera were small, but all species except for the gulls Larus argentatus and L. marinus, could be identified using one or more loci.
  • 5.5. Arising from the success of the method using fresh specimens, a protocol for the electrophoretic identification of traumatized remains of strikes is suggested.
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16.
  • 1.1. A series of diesters of isohematoporphyrin (isoHp), from dimethyl to dioctyl were prepared according to Rimington et al. (1989b). Their optical absorption, fluorescence spectra and high performance liquid chromatography (HPLC) retention times were recorded.
  • 2.2. A plot of HPLC retention time against number of C atoms in the alcohol used for esterification was approximately linear at first then rising steeply from diamyl to diocyi ester, whether a gradient elution was used or only methanol: water, 95/5, at pH 7.5.
  • 3.3. Preparation of the diethers of isoHp was much more difficult than that of the corresponding derivatives of hematoporphyrin (Hp). Several different methods were investigated, varying both times and temperatures.
  • 4.4. These methods included reaction of isoHp or its demethyl ester with
    • 4.1.(i) a bromoalkane in presence of anhydrous K2CO3;
    • 4.2.(ii) reaction with bromoalkane and Ag2O;
    • 4.3.(iii) reaction of brominated-isoHp, prepared by using thionylbromide, with the selected alcohol, or corresponding sodium alcoholate;
    • 4.4.(iv) heating of isoHp alone with an alcohol containing 20% (w/v) H2SCO4 (temp. range from 45° to 118°C),
    • 4.5.(v) refluxing as in (iv) at the b.p. of the alcohol; and
    • 4.6.(vi) carrying out this reaction in refluxing ethyleneglycoldimethyl ether (b.p. 85°C) or diethyleneglycoldimethyl ether (b.p. 155°C).
  • 5.5. Some diether formation was observable by all these methods but yields were small, a considerable quantity of unreacted isoHp and other products remaining.
  • 6.6. Examined by HPLC, the diethers consistently afforded a forked peak which on thin layer chromatography was only resolved into two very closely associated bands by a solvent mixture carefully selected for development.
  • 7.7. On elution these materials had virtually identical optical absorption and fluoresence spectra.
  • 8.8. The nature of the association is discussed, atropisomers (Gottwald and Ullman, 1969) and possible stacked monomer: dimers (Abraham et al., 1963) being considered as possibilities.
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17.
  • 1.1. A potentiometric method for the assay of cholinesterase has been proposed and compared with a colorimetric assay.
  • 2.2. Main kinetic parameters of cholinesterase from Hypostomus punctatus brain were determined indicating that true acetylcholinesterase is by far the predominant enzyme in the brain of this fish.
  • 3.3. We have compared our data with published results described from other fish species.
  • 4.4. The enzyme inhibition achieved after 3 hr incubation of brain homogenates with ethyl-parathion have indicated that this enzyme shows a characteristic organophosphorous sensitive behavior.
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18.
  • 1.1. Among the digestive enzymes synthesized by pancreas, lipase is the principle lipolytic enzyme which hydrolyses dietary glycerides.
  • 2.2. For its action it requires a coenzyme, colipase.
  • 3.3. The molecular mechanisms of the interaction of these two are not fully understood.
  • 4.4. Further, molecular events that regulate and influence lipid absorption are ill denned.
  • 5.5. The rabbit is the conventional animal model for the study of lipid absorption. We have undertaken the molecular cloning, and characterization of rabbit pancreatic colipase, the coenzyme for pancreatic lipase.
  • 6.6. Colipase has been cloned from a gt 11 library of an adult rabbit pancreatic cDNA by probing with an oligonucleotide derived from human colipase sequence.
  • 7.7. The total reading frame consists of 321 nucleotides coding for 90 amino acids of the functional protein and 17 nucleotides of the leader peptide.
  • 8.8. Northern blot analysis revealed a distinct band around 0.5kb. Comparison with other species revealed an over all homology of 75% at the nucleotide level.
  • 9.9. At the amino acid level highest conservation is observed at the lipase-binding region (AA 53–73).
  • 10.10. Rabbit enzyme also retained the N-terminal pentapeptide of it preform.
  • 11.11. The regions of homology and conservation may aid to define the sites of interaction of colipase with lipase.
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19.
  • 1.1. We studied the morphology and contractile properties in marginal sphincters isolated from anemones from different environments.
  • 2.2. Sphincters from specimens from protected areas are ovoid or roughly square shape. Oval sphincters have increased number of mesogloeal branches and the main axis is thickened. Roughly square sphincters have irregular borders, mesogloeal axes of uniform thickness and homogeneous branching.
  • 3.3. Specimens from exposed areas have sphincters with an ovoid shape and dichotomous branching.
  • 4.4. Sphincters of specimens from partially protected areas show transition forms.
  • 5.5. Under stimulation with KCl at different concentrations, sphincters of anemones from exposed environments contract faster and develop higher isometric forces than muscles isolated from specimens of protected areas.
  • 6.6. It was concluded that sphincters of anemones from different environments have a morphology and a physiological response adapted to the milieu.
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20.
  • 1.1. Cholesterol metabolism has been characterized in three species of New World primates, the cotton-top tamarin, the saddle-back tamarin, and the squirrel monkey.
  • 2.2. When fed a diet containing cholesterol, the three species exhibited differing responses of plasma cholesterol levels.
  • 3.3. Dietary cholesterol absorption was determined and plasma cholesterol die-away kinetics were analyzed in terms of a two-pool model.
  • 4.4. The results of the analyses of cholesterol turnover are consistent with the observed species-specific differences in plasma cholesterol values and cholesterol absorption.
  • 5.5. Cholesterol metabolism differs between the two tamarin species, as well as between the tamarins and the squirrel monkey.
  • 6.6. Implications of species-specific differences between tamarin species are discussed in terms of the use of tamarin species as animal models for comparative studies of cholesterol metabolism and the etiology of cancer and cardiovascular disease.
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