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1.
  • 1.1. Three DNA dependent RNA polymerases have been purified from chromatin and chloroplast fractions of wheat leaves.
  • 2.2. The purified enzymes were completely dependent on exogenous DNA after purification by glycerol gradient, DEAE-Sephadex and phosphocellulose chromatography.
  • 3.3. The nuclear enzymes, I and II, showed a strong preference for denatured nuclear DNA, whereas the chloroplast enzyme preferred denatured chloroplast DNA.
  • 4.4. The three enzymes require either Mg2+ or Mn2+ for activity.
  • 5.5. α-amanitin specifically inhibited RNA polymerase II but has no effect on polymerase I and chloroplast polymerase.
  • 6.6. Enzyme I is most active at very low ionic strength (0.10 mM KC1), whereas enzyme II and chloroplast enzyme show maximum activity at 150mM and 50 mM KC1 respectively.
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2.
  • 1.1. Continuous feeding of adult honeybees with a 2 M sucrose syrup results in an early increase of both trehalase and sucrase activities in haemolymph, followed by a trough at day 5, then a second phase of increasing sucrase activity.
  • 2.2. In the presence of chloramphenicol as an inhibitor of protein synthesis, the induction of trehalase activity is depressed but the very early increase of sucrase is not; by contrast, the second phase of increase in sucrase activity is delayed and depressed by the inhibitor.
  • 3.3. These results suggest that in the earlier phases of induction, the sucrase molecules constitute a part of the trehalase complex already present whereas the second phase corresponds to the synthesis of a more specific sucrase.
  • 4.4. New carbohydrates (di and trisaccharides) are produced which might be due to the transglycosylation properties of the induced enzymes.
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3.
  • 1.1. A standard procedure for lipid-extraction of lyophilized hen brain material is decribed.
  • 2.2. Nine carboxylesterase isoenzymes (EC 3.1.1.1) are identified in lipid-extracted lyophilized material (LELM) using kinetic analysis of organophosphate inhibition. Total phenyl valerate (PV) hydrolysing carboxylesterase activity in LELM is 43.3U.g−1
  • 3.3. Two carboxylesterase isoenzymes of LELM are classified as neurotoxic esterases (NTEA and NTEgB).
  • 4.4. Using n-octylglucoside 51% of the water-insoluble neurotoxic esterase activity from LELM are solubilized.
  • 5.5. Six carboxylesterase isoenzymes including NTEA (6.5 U-l−1) and NTEB (4.2 U-l−1) are present in the solubilized preparation.
  • 6.6. Throughout purification and separation steps carboxylesterase isoenzymes are identified by their rate constants for the reaction with organophosphorus inhibitors.
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4.
  • 1.1. In lobster hepatopancreas, extracellular protreases cause the inactivation of glycogen phosphorylase.
  • 2.2. The proteolysis of glycogen phosphorylase purified from rabbit muscle by these proteases has been shown by SDS-polyacrylamide gel electrophoresis.
  • 3.3. A cell isolation technique has allowed us to remove proteases of extracellular digestion and to measure glycogen phosphorylase activity in lobster hepatopancreas.
  • 4.4. The glycogen phosphorylase activity seems to be mainly associated with R cells while it could not be detected in B cells.
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5.
  • 1.1. Metabolic rates and adenine nucleotide content of liver and kidney from hibernating ground squirrels were measured and compared to rats to study the biochemical adaptation to hibernation.
  • 2.2. High rates of renal and hepatic gluconeogenesis were observed in squirrels, particularly from propionate and glycerol compared to rat.
  • 3.3. During hibernation and starvation soluble phosphoenolpyruvate carboxykinase activity was increased in both liver and kidney.
  • 4.4. Although metabolic rates are decreased during hibernation the results suggest that the enzymic complement is maintained at high activity even during torpor.
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6.
  • 1.1. Extensive digestion of nuclei with micrococcal nuclease (MNase), commonly used in the analysis of chromatin structure, results in the production of mono- and dinucleosomal chromatin fragments.
  • 2.2. Digestion of nuclei from a range of cell types with low enzyme concentrations solubilized high molecular weight polynucleosomal fragments, some ⪢ 22 kb long.
  • 3.3. Such digestion conditions also resulted in extensive solubilization of nascent RNA which contributed considerably to the nucleic acid content of the soluble fraction.
  • 4.4. We conclude that the contribution of RNA to total nucleic acid content of the soluble fraction should be taken into consideration when nuclei are digested with low concentrations of MNase.
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7.
  • 1.1. The ontogeny of type I and type III deiodinase activities was studied in embryonic and posthatch chicks.
  • 2.2. Hepatic type I activity showed a 3-fold increase up to the period of pipping and hatching and decreased slowly thereafter.
  • 3.3. Hepatic type III activity increased by 3-fold from E14 to E17 and decreased more than 10-fold from E17 to CO. Posthatch levels were very low.
  • 4.4. Type I activity in the kidney decreased slowly after hatching while type III activity was very low over the whole period studied.
  • 5.5. Developmental changes during the late embryonic period suggest a causal relationship between the increase in plasma GH and T3 levels and the decrease in hepatic type III activity.
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8.
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Highlights
  • •Novel PTMs detected in native yeast exosome, RNA polymerase II and proteasome.
  • •MD based approach outperforms published tools in predicting PTMs stability effect.
  • •Dynamical approach reveals long range effects of PTMs on subunits binding.
  • •Acetylations may have a role in local stabilization of protein complex formation.
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9.
  • 1.1. Pyruvate dehydrogenase complex (PDC) activity was measured in several tissues of rats fed for 7 or 15 days on control, or high-sucrose or high-fat diets.
  • 2.2. Total activity in adipose tissue increased in the three groups 3–4-fold as compared with chow-fed animals in the first week. Total activity was 60% lower in rats fed the diet containing 22% corn oil for 2 weeks.
  • 3.3. Hepatic total and PDCa activities were 50–80% higher in rats fed the sucrose diet for 7 or 15 days and decreased 30–40% in those fed on the high-fat diet for 2 weeks.
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10.
  • 1.1. The addition of cAMP to stimulating solutions of NaCl, fructose (furanose sugar), sucrose, or glucose (pyranose sugars) decreases the responsiveness of labellar chemosensilla in Phormia.
  • 2.2. The addition of ATP, while decreasing the responsiveness to NaCl or fructose enhances the responsiveness to glucose and sucrose.
  • 3.3. The inhibiting effect of ATP on NaCl or fructose responses is suppressed by GDPßS, an inhibitor of adenylate cyclase (and thus of cAMP synthesis); moreover GDPßS further enhances the increase in response due to ATP when added to the sucrose or glucose solutions.
  • 4.4. Results suggest a possible involvement of cAMP and ATP in the taste reception mechanism in the blowfly.
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11.
12.
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Highlights
  • •New MALDI MS imaging sample preparation workflow reveals tissue protease activity.
  • •Differential time- and inhibitor concentration-dependence confirm active proteases.
  • •Mouse gastric tumor displays high protease activity compared to surrounding tissue.
  • •Proteomic data and biochemical protease activity assay support MALDI MSI results.
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13.
  • 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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14.
  • 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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15.
  • 1.1. A simple procedure for isolation of high molecular weight genomic DNA, and RNA, from Streptococcus sobrinus OMZ176 is described.
  • 2.2. Cell cultures were grown aerobically for 10 hr.
  • 3.3. Spheroplast formation and lysis was achieved by mutanolysin/lysozyme-dependent digestion of the cell wall, followed by N-lauroylsarcosinate-mediated lysis.
  • 4.4. Nucleic acids were isolated directly from cell-lysates using cesium-trifluoroacetate (CsTFA) densitygradient centrifugation.
  • 5.5. Three different centrifugation regimes were tested: self-generated density gradients in a fixed angle rotor; self-generated density-gradients in a swinging-bucket rotor; pre-formed density-gradients in a swinging-bucket rotor.
  • 6.6. Genomic DNA isolated by the CsTFA-procedure was found to have higher purity as compared to genomic DNA isolated in a conventional CsCl gradient.
  • 7.7. Isolated DNA was shown to be of a quality suitable for applications in molecular biology.
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16.
  • 1.1. The desaturation and elongation of linoleic acid has been studied in homogenates and in subfractions of ovine placental tissue.
  • 2.2. The reaction was characterized in terms of pH and temperature optima, time course and protein concentration.
  • 3.3. Activity was found to be confined to the 11,000g supernatant fraction of the tissue and the results suggest that the enzymes are membrane bound.
  • 4.4. The cytosolic fraction and ATP were required for full activity and the reaction was inhibited by cyanide.
  • 5.5. The properties of the reaction are compared with those of other desaturation systems and their implications with regard to possible reaction mechanisms are discussed.
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17.
  • 1.1. Subcellular fractions of rat liver were assayed for PLA2 activity.
  • 2.2. The PLA2 assay measures the release of [3 H]oleic acid from phospholipids, using labeled E. coli as substrate.
  • 3.3. Nuclear fractions contained PLA2 activity, which was Ca2+ dependent and could not be explained from mitochondrial, microsomal or plasma membrane contamination.
  • 4.4. The Vmax value of nuclear PLA2 is 0.30 ± 0.04 pmol oleic acid/min/mg protein; its Km value is 0.86±0.12μM, similar to that of mitochondrial PLA2.
  • 5.5. We conclude that rat liver nuclei contain PLA2 activity.
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18.
  • 1.1. A comparative study of the proteolytic activity in four different sections of the digestive tracts of the European sea bass (Dicentrarchus labrax) and hybrid striped bass (Morone chrysops × M. saxatilis) reared in freshwater revealed minor differences between these fish.
  • 2.2. Tryptic activity plays a major role in the proteolytic process in both fish.
  • 3.3. The activity of seven intestinal proteolytic enzymes was detected utilizing a combination of specific substrates and inhibitors.
  • 4.4. High levels of proteolytic activity were detected in both the proximal and distal sections of the fish intestine at a high pH range (9–10).
  • 5.5. In situ monitoring of pH levels revealed a lower pH level in the intestinal proximal section of hybrid striped bass compared with the distal section.
  • 6.6. In contrast, higher pH levels were detected at the proximal compared with the distal sections of D. labrax intestine.
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19.
  • 1.1. Rabbit cDNA probes for H and M lactic dehydrogenase subunits were used to monitor mRNA levels in different muscle types during growth.
  • 2.2. At the same time, lactic dehydrogenase activity and relative quantities of H and M protein subunits were measured.
  • 3.3. The main results are that mRNA abundance depends on muscle type and age, and mRNA abundance is not correlated with enzymatic activity.
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20.
  • 1.1. Lactate dehydrogenase in ovine tissues was separated by electrophoresis, one dimensional isoelectric focusing (IEF) and a two dimensional technique.
  • 2.2. Tissues showed five zones of enzyme activity consisting of multiple bands after IEF.
  • 3.3. The IEF zymograms were unique for each tissue and differed from those of other species.
  • 4.4. Two dimensional separation revealed that the five zones of activity observed on IEF corresponded to the five isoenzymes separable by conventional electrophoresis.
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