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1.
  • 1.1. Digestive protease, lipase, and amylase of Stage I larvae of the American lobster Homarus americanus are characterized.
  • 2.2. A sensitive method for detection of crustacean lipase was developed using an latroscan which combines thin-layer chromatography and flame ionization detection to quantify free fatty acids generated by lipase digestion.
  • 3.3. pH optima of the three enzymes occurred at or near the pH of gastric fluid.
  • 4.4. A time course study demonstrated slight increases in protease and amylase activities during the first larval stage, regardless of whether the lobsters were fed or not, whereas lipase activity was constant.
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2.
  • 1.1. The hydrocarbon composition of different cuticular regions (pronotum, legs, abdominal tergites and sternites, pleural membrane) was determined for adult female crickets (Acheta domesticus).
  • 2.2. Hydrocarbon groups included n-alkanes, 2-methylalkanes, long-chain internally branched monomethyl- and dimethyalkanes, n-alkenes, 2-methylalkenes and alkadienes.
  • 3.3. Saturated hydrocarbons were more abundant than unsaturated hydrocarbons and branched saturates more abundant than n-alkanes in all regions of the cuticle examined.
  • 4.4. Except for a higher percentage of n-alkanes in the pleural membrane (soft cuticle), little difference was noted in compositional patterns or relative amounts of individual molecules from the different cuticular regions.
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3.
  • 1.1. Male crickets Gryllus bimaculatus show a drastic change in circadian rhythm from nymphal diurnality to adult nocturnality, in association with an increase in activity level several days after the imaginai moult.
  • 2.2. The corpora allata implantation into male 7th or 8th instar nymphs produced supernumerary instar nymphs in about 30% of the implanted animals, but did not affected the normal development in the remaining animals.
  • 3.3. The majority of the supernumerary instar nymphs were diurnal and sexually inactive, although their internal reproductive organs appeared to be fully mature.
  • 4.4. The supernumerary instar nymphs became nocturnal with an increase in activity level several days after the imaginai (9th) moult.
  • 5.5. The roles of the nervous system in the regulation of the rhythm reversal are discussed.
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4.
  • 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.
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5.
  • 1.1. Metabolic rate (MR) and water budget (WB) components of cave and camel crickets are directly related to size and temperature.
  • 2.2. MR increases most rapidly with size for insects in general followed by cave crickets (females > males), and lastly, camel crickets (no sex differences).
  • 3.3. Metabolic thermal sensitivity of cave crickets (males > females) is much greater than camel crickets.
  • 4.4. WB components parallel MR relations.
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6.
  1. Specific activity of amylase, cellulase, protease and lipase in the intestines of the air-breathing catfish, Clarias batrachus (Linn.) has been studied.
  2. Excepting amylase and protease, the activity of lipase and cellulase showed practically no changes with change in the nutritional status of the diets.
  3. pH optima of all enzymes were between 6.9 and 7.6
  4. There is reason to believe from cellulase and high amylase activity in the intestine of the species that its culture operation could be done more economically by giving them a supplementary diet from indigeneously available raw material particularly from plant origin.
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7.
  • 1.1. The optimal pH of maltase of the house cricket was 5.6 and the optimal temperature was 40°C. The apparent activation energy was 5300 cal/mol
  • 2.2. The 50% inactivation time for maltase at 50°C was 69 min and the 50% inhibition concentration for mercuric chloride was 163μmole.
  • 3.3. Maltase was only produced by the caecal tissues but its highest activity was found in the foregut lumen and after 5 days of starvation, only 44.6% of the total maltase activity remained.
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8.
  • 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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9.
  • 1.1. The plasma membrane of slime-forming, encapsulated Streptococcus cremoris from “viili” was isolated in hypotonie conditions in the presence of lysozyme (EC 3.2.1.17) using density gradient centrifugation as the last purification step.
  • 2.2. The membrane yield was 15.8% of wet weight cells and the preparation contained 64.4% protein. 19.1% carbohydrate, 5.8% aminosugars, 5.1% RNA and 0.07% DNA.
  • 3.3. Buffered 1% (w/v) Triton X-100 solubilized 33.6% of membrane proteins. The number of polypeptides detected by SDS-polyacrylamide gel electrophoresis was 59 when the membrane was isolated without a protease inhibitor and 44 in the presence of a protease inhibitor.
  • 4.4. The molecular weights of the polypeptides varied from 13,500 to 100,000.
  • 5.5. Ultrathin-layer electrofocusing analysis revealed the range of protein pi values to be between 3.50 and 5.85 concerning 77.3% of proteins and between pI 5.85 and 8.15 concerning 18.2% of proteins.
  • 6.6. The isoelectric point of the only basic protein component was 9.3.
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10.
  • 1.1. Crude extract of the whole digestive tract from the brown shrimp (P. californiensis) was investigated for digestive amylase activity.
  • 2.2. Considerable amylase activity was found at pH 6.5–8.0, with optimum pH at around 7.5.
  • 3.3. Optimum temperature was found between 30–40°C, similar to amylases from other crustaceans.
  • 4.4. Amylase activity was highly halotolerant, having 50% maximum activity at 3 M NaCl.
  • 5.5. Maximum amylase activity was found at 0.01 M NaCl.
  • 6.6. Amylase activity was partially inhibited by the divalent ions Hg2+, Zn2+, Cu2+ and Cr2+.
  • 7.7. Mg2+ and Ca2+ ions seemed to enhance amylase activity.
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11.
  • 1.1. Detergent solubilisation of particulate rat liver low Km cyclic AMP phosphodiesterase in the presence of protease inhibitors yields a form of the enzyme with a larger molecular weight than the form solubilised by protease treatment.
  • 2.2. The detergent solubilised enzyme could be partially purified by anion exchange chromatography.
  • 3.3. It displayed a marked tendency to precipitate from solution when detergent was removed.
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12.
  • 1.1. AMP deaminase from Palaemon serratus tail muscle was partially purified by chromatography on cellulose phosphate.
  • 2.2. Muscle homogenates expressed very low enzyme activities and the presence of ATP was necessary to detect AMP deaminase. The specific activity and substrate affinity of the purified enzyme were also very low.
  • 3.3. The purified prawn muscle AMP deaminase was contaminated by contractile proteins, one of the major contaminants being actin.
  • 4.4. The enzyme displayed a very high affinity for actomyosin which was only partially abolished by pyrophosphate.
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13.
  • 1.1. A comparison of proteolytic and protease inhibitory activity, and ecdysteroid levels in body fluids was made between normal larvae of the flesh fly, Sarcophaga bullata, and those that had been water-stressed for two days.
  • 2.2. The course of proteolytic activity in water stressed flies decreases 6 hr after beginning the experiment and remains low in comparison with control flies.
  • 3.3. The course of protease inhibitors exhibits a mirror image pattern to proteases.
  • 4.4. Ecdysteroid pattern shows two peaks in control animals: minor at 24 hr and major at pupariation, in experimental animals: at 1 hr, at 6 hr and at white pupal stage.
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14.
  • 1.1. Ovaries of Therobia domestica, dissected from inseminated females and incubated with tritiated amino acids, synthesize labeled proteins, the major fraction of which is indistinguishable from the major vitellogenin secreted by the fat body, when considering the electrophoretic mobility, the polypeptide composition and the immunoreactivity.
  • 2.2. Peptide mapping, using two different proteases, shows a striking structural similarity between the proteins of both origins and reveals interrelationships between their subunits.
  • 3.3. The ovary synthesizes the 210–212 kD precursors of the major vitellogenin, as does the fat body, and processes them intensively into smaller subunits (176–182, 57 and 46 kD). The follicle cells are tentatively nominated for both roles.
  • 4.4. The quantitative contribution of the two ovaries to the vitellogenin pool was found to be much higher than that of the fat body.
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15.
  • 1.1. Biliverdin reductase from the liver of eel, Anguilla japonica was characterized and purified with a novel enzymatic staining method on polyacrylamide electrophoretic gel.
  • 2.2. This enzyme could use both NADPH and NADH as coenzyme. The Km of NADPH was 5.2 μM, while that of NADH was 5.50 μM.
  • 3.3. The optimum reaction pH for using HADPH as coenzyme was 5.3. That for NADH was 6.1. The optimum reaction temperature is 37°C.
  • 4.4. When NADPH was used as coenzyme, the Km of biliverdin was 0.6 μM. When NADH was used as coenzyme, the Km of biliverdin was 7.0 μM.
  • 5.5. The activity of the enzyme was inhibited by the concentration of biliverdin. Also, the potency of the enzyme was much less than that of the analogous enzyme isolated from mammals.
  • 6.6. This is a fairly stable enzyme with a mol. wt around 67,000. Its estimated pI was pH 3.5–4.0.
  • 7.7. This is the first time biliverdin reductase has been isolated and characterized from a vertebrate other than mammals. The property of it is quite different from that of mammals.
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16.
  • 1.1. Proteolytic, lipolytic, amylolytic and cellulolytic activities were studied in adults of the phytophagous beetle, Hydromedion sparsutum, indigenous to the sub-Antarctic island of South Georgia.
  • 2.2. Gastric enzyme activities were measured at experimental temperatures of 5–40°C and results were compared with those obtained from two thermophilic insects, Gryllus bimaculatus and Tenebrio molitor.
  • 3.3. Protease and lipase activities in Hydromedion were 10–15 times lower than in Gryllus and Tenebrio.
  • 4.4. In the temperature range of 5–15°C, α-amylase activity from Hydromedion was only slightly lower than that from Gryllus.
  • 5.5. Hydromedion gut homogenates exhibited a distinct cellulolytic activity, even at a low temperature of 5°C.
  • 6.6. Cellulolytic activity in the digestive tract of Hydromedion was confirmed by the evolution of 14CO2 after consumption of labelled cellulose.
  • 7.7. The thermal properties of digestive enzymes agree well with the role of Hydromedion as primary decomposer in its ecosystem.
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17.
  • 1.1. Three methods of recuperating and preserving enzyme activity from freshly-caught langostilla were assessed. In the pressing and acetone extract methods, the recovered specific activity was similar.
  • 2.2. Protease activity was higher between 6.5 and 8 pH, and was sensitive to high temperatures.
  • 3.3. In PAGE and serine inhibition assays, one fraction resembled bovine trypsin.
  • 4.4. The composition of proteins and molecules bearing protease activity from the hepatopancreas and stomach of both fed and starved animals was similar, indicating proteases are not induced but constitutive.
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18.
  • 1.1. An elastase-like enzyme was purified from the pyloric caeca of rainbow trout by hydrophobic interaction, cation exchange and gel-filtration chromatography.
  • 2.2. The approximate molecular weight of the elastase was 27 kDa and the isoelectric point was remarkably basic.
  • 3.3. The pH optimum of this enzyme was 8.0, when assayed with Succinyl-Ala-Ala-Ala-p-Nitroanilide.
  • 4.4. When assayed with Succinyl-Ala-Ala-Ala-p-Nitroanilide, the enzyme activity had a temperature optimum of 45°C, and the enzyme was stable up to this temperature.
  • 5.5. The trout elastase exhibited a higher specific activity than porcine elastase against Succinyl-Ala-Ala-Ala-p-Nitroanilide and elastin-orcein.
  • 6.6. The trout elastase was inhibited by elastatinal, PMSF, TPCK, SBTI and Bowman-Birk inhibitor.
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19.
  • 1.1. Lipoprotein lipase (LPL) was isolated from five rat tissues: white adipose, skeletal muscle, cardiac muscle, mammary gland and lung.
  • 2.2. Specific activity of the preparations varied from 75 U/mg for skeletal muscle and 720 U/mg for adipose.
  • 3.3. The preparations were further analysed using SDS-PAGE and a single component identified. The mol. wt of 61,000 Da of this component was consistent for all five of the tissue sources.
  • 4.4. Significant differences in the values of the isoelectric points of the enzyme species were revealed. The values varied from 7.23 (SEM 0.022) for cardiac and lung to 7.51 (SEM 0.037) for mammary.
  • 5.5. Two-dimensional electrophoresis, using isoelectric focusing in the first dimension and SDS-PAGE in the second revealed differences in the patterns of stained material derived from the five tissue sources.
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20.
  • 1.1. Equine plasma contains lipoproteins corresponding to very low density (VLDL), low density (LDL) and high density lipoproteins (HDL).
  • 2.2. HDL accounts for approximately 60% of plasma lipoprotein mass and consists of a single population of particles.
  • 3.3. LDL is heterogeneous comprising three discrete subfractions.
  • 4.4. Two proteins are found in the region of apolipoprotein (apo) B-100 in VLDL and LDL and a third similar to apo B-48 is in VLDL.
  • 5.5. Lecithin:cholesterol acyl transferase is active in plasma and hepatic lipase and lipoprotein lipase are evident in post-heparin plasma.
  • 6.6. There is no significant cholesteryl ester transfer protein activity.
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