Synechococcus R-2 (PCC 1942) actively accumulates sulphate in the light and dark. Intracellular sulphate was 1.35 ± 0.23 mol m?3 (light) and 0.894 ± 0.152 mol m?3 (dark) under control conditions (BG-11 media: pHo, 7.5; [SO42?]o, 0.304 mol m?3). The sulphate transporter is different from that found in higher plants: it appears to be an ATP-driven pump transporting one SO42?/ATP [ΔμSO42?i,o=+ 27.7 ± 0.24 kJ mol?1 (light) and + 24 ± 0.34 kj mol?1 (dark)]. The rate of metabolism of SO42?at pHo, 7.5 was 150 ± 28 pmol m?2 s?1 (n = 185) in the light but only 12.8 ± 3.6 pmol m?2 s?1 (n = 61) in the dark. Light-driven sulphate uptake is partially inhibited by DCMU and chloramphenicol. Sulphate uptake is not linked to potassium, proton, sodium or chloride transport. The alga has a constitutive over-capacity for sulphate uptake [light (n= 105): Km= 0.3 ± 0.1 mmol m?3, Vmax, = 1.8 ± 0.6 nmol m?2 s?1; dark (n= 56): Km= 1.4 ± 0.4 mmol m?3, Vmax= 41 ± 22 pmol m?2 s?1]. Sulphite (SO32?) was a competitive inhibitor of sulphate uptake. Selenate (SeO42?) was an uncompetitive inhibitor. 相似文献
Synechococcus R-2 (PCC 7942) actively accumulated Cl? in the light and dark, under control conditions (BG-11 media: pHo, 7·5; [Na+]o, 18 mol m?3; [Cl?]o, 0·508 molm?3). In BG-11 medium [Cl?], was 17·2±0·848 mol m?3 (light), electrochemical potential of Cl? (ΔμCl?i,o) =+211±2mV; [Cl?]i= 1·24±0·11 mol m?3(dark), ΔμCl?i,o=+133±4mV. Cl? fluxes, but not permeabilities, were much higher in the light: ?Cl?i,o= 4·01±5·4 nmol m?2 s?1, PCl?i,o= 47±5pm s?1 (light); ?Cl?i,o= 0·395±0·071 nmol m?2 s?1, PCl?i,o= 69±14 pm s?1 (dark). Chloride fluxes are inhibited by acid pHo (pHo 5; ?Cl?i,o= 0·14±0·04 nmol m?2 s?1); optimal at pHo 7·5 and not strongly inhibited by alkaline pHo (pHo 10; ?Cl?1i,o= 1·7±0·14 nmol m?2 s?1). A Cl?in/2H+in coporter could not account for the accumulation of Cl? alkaline pHo. Permeability of Cl? is very low, below 100pm s?1 under all conditions used, and appears to be maximal at pHo 7·5 (50–70 pm s?1) and minimal in acid pHo (20pm s?1). DCCD (dicyclohexyl-carbodiimide) inhibited ?Cl?i,o in the light about 75% and [Cl?]i fell to 2·2±0·26 (4) mol m?3. Valinomycin had no effect but monensin severely inhibited Cl? uptake ([Cl?]i= 1·02±0·32 mol m?3; ?Cl?i,o= 0·20±0·1 nmol m?2 s?1). Vanadate (200 mmol m?3) accelerated the Cl? flux (?Cl?i,o= 5·28±0·64 nmol m?2 s?1) but slightly decreased accumulation of Cl? ([Cl?], = 13·9±1·3 mol m?3) in BG-11 medium but had no significant effect in Na+-free media. DCMU (dichlorophenyldimethylurea) did not reduce [Cl?], or ?Cl?i,o to that found in the dark ([Cl?]i= 8·41±0·76 mol m?3; ?Cl?i,o= 2·06±0·36 nmol m?2 s?1). Synechococcus also actively accumulated Cl? in Na+-free media, [Cl?]i was lower but ΔΨi,o hyperpolarized in Na+-free media and so the ΔμCl?i,o was little changed ([Cl?]i= 7·98±0·698 mol m?3; ΔμCl?i,o=+203±3 mV). Net Cl? uptake was stimulated by Na+; Li+ acted as a partial analogue for Na+. Synechococcus has a Na+ activated Cl? transporter which is probably a primary 2Cl?/ATP pump. The Cl? pump is voltage sensitive. ΔμCl?i,o is directly proportional to ΔΨi,o(P»0·01%): ΔμCl?i,o= -1·487 (±0·102) ×ΔΨi,o, r= -0·983, n= 31. The ΔμCl?i,o increased (more positive) as the Δμi,o became more negative. The ΔμCl?i,o has no known function, but might provide a driving force for the uptake of micronutrients. 相似文献
The kinetics of the light-driven Cl? uptake pump of Synechococcus R-2 (PCC 7942) were investigated. The kinetics of Cl? uptake were measured in BG-11 medium (pHo, 7·5; [K+]o, 0·35 mol m?3; [Na+]o, 18 mol m?3; [Cl?]o, 0·508 mol m?3) or modified media based on the above. Net36Cl? fluxes (?Cl?o,i) followed Michaelis-Menten kinetics and were stimulated by Na+ [18 mol m?3 Na+ BG-11 ?Cl?max= 3·29±0·60 (49) nmol m?2 s?1 versus Na+-free BG-11 ?Cl?max= 1·02±0·13 (54) nmol m?2 s?1] but the Km was not significantly different in the presence or absence of Na+ at pHo 10; the Km was lower, but not affected by the presence or absence of Na+ [Km = 22·3±3·54 (20) mmol m?3]. Na+ is a non-competitive activator of net ?Cl?o,i. High [K+]o (18 mol m?3) did not stimulate net ?Cl?o,i or change the Km in Na+-free medium. High [K+]o (18 mol m?3) added to Na+ BG-11 medium decreased net ?Cl?o,i [18 mol m?3K+ BG-11; ?Cl?max= 2·50±0·32 (20) nmol m?2 s?1 versus BG-11 medium; ?Cl?max= 3·35±0·56 (20) nmol m?2 s?1] but did not affect the Km 55·8±8·100 (40) mmol m?3]. Na+-stimulation of net ?Cl?o,i followed Michaelis-Menten kinetics up to 2–5 mol m?3 [Na+]o but higher concentrations were inhibitory. The Km for Na+-stimulation of net ?Cl?o,i [K1/2(Na+)] was different at 47 mmol m?3 [Cl?]o (K1/2[Na+] = 123±27 (37) mmol m?3]. Li+ was only about one-third as effective as Na+ in stimulating Cl? uptake but the activation constant was similar [K1/2(Li+) = 88±46 (16) mmol m?3]. Br? was a competitive inhibitor of Cl? uptake. The inhibition constant (Ki) was not significantly different in the presence and absence of Na+. The overall Ki was 297±23 (45) mmol m?3. The discrimination ratio of Cl? over Br? (δCl?/δBr?) was 6·38±0·92 (df = 147). Synechococcus has a single Na+-stimulated Cl? pump because the Km of the Cl? transporter and its discrimination between Cl? and Br? are not significantly different in the presence and absence of Na+. The Cl? pump is probably driven by ATP. 相似文献
The electrical properties of the egg of the medaka, Oryzias latipes, were studied before, during, and after fertilization. The resting potential of the unfertilized egg averaged ?39 ± 9 mV in Yamamoto's Ringers (Y. Ringers), but 20% of the values were between ?50 and ?60 mV. Fertilization triggers a small depolarization of 4 ± 3 mV in 10% Y. Ringers with an average duration of 20 ± 10 sec. The amplitude of this depolarization is independent of [Na+]o, [Ca2+]o, and [Cl?]o, so it appears to be due to a nonspecific leak triggered by sperm-egg fusion. The depolarization is followed by a longer hyperpolarizing phase with an average amplitude of 31 ± 12 mV. Recovery from this hyperpolarization has a fast phase lasting 155 ± 18 sec, followed by a slower phase which reaches a steady average membrane potential of ?19 ± 1 mV by 9 min after fertilization. The membrane resistance falls 10-fold during the first 2 min after fertilization, from 40 (1520 kΩ-cm2) to 3 MΩ. This is largely due to an increase in the K+ conductance. At the peak of the hyperpolarization, the membrane potential exhibits a 28 mV/decade [K+]o dependence and a 6 mV/decade [Na+]o dependence. The membrane resistance slowly recovers over the next 8 min to a value about 30% larger than before fertilization. The relation of current vs voltage was linear before, during, and after fertilization and indicated a reversal potential of ?98 ± 20 mV for the hyperpolarization peak. The egg's capacitance averaged 0.04 ± 0.01 μF (0.9 μF/cm2) before fertilization and approximately doubles within 90 sec after fertilization. It then decreases over a 9-min period, reaching a value 25% smaller than before fertilization. 相似文献
Batch growth characteristics of various organisms were determined on a number of pairs of sugars to find a stable system showing clear-cut classical diauxie. The system selected for further study was a strain of Klebsiella (Acrobacter) aerogenes, NCIB 8021 growing on a mixture of glucose and maltose in minimal salts medium at 30°C. This showed a specific growth rate (μ) of 1.19 ± 0.03 hr.?1 on 0.01% (w/v) glucose, followed by a diauxie lag of 0.73 ± 0.04 hr and then further growth on 0.01% (w/v) maltose at μ = 0.60 ± 0.03 hr?1. This system was applied to a two-stage continuous, stirred, aerated fermentor system, with working volumes of 1.85 and 2.77 liters, respectively, and growth was followed (mainly by optical density, referred to dry weights and viable counts) and also the concentrations of the sugars were measured. Except at the very highest flow rates, glucose was immediately and virtually completely consumed, but the utilization of maltose showed interesting variations: (a) At low feed rates between 0.09 and 0.4 vol./hr. exactly the same response was found with mixed sugars as with double concentration glucose, showing that the organism was able to metabolize maltose as well and as quickly as glucose. (b) At medium feed rates of 0.46 to 1.03 vol./hr. two deviations were observed, both of which increased as the dilution rate increased: the system showed a time lag on maltose before the cell population began to rise and the volume of medium used before the steady state was established was greater than predicted, (c) At fast feed rates, approaching “washout” condition of 1.055 to 1.135 vol./hr. the first culture vessel showed no reaction to a step change which included maltose, although, of course, with doubled glucose it responded immediately. The second vessel, however, quickly metabolized the overflow maltose, and showed a steady increase of cell population to the theoretical steady state. These results may have significance for industrial systems using complex commercial substrates. 相似文献
A method is described for measuring total CO2 and HCO3? in tissues rapidly frozen in liquid nitrogen. The method is a modification of the procedure of D. D. Van Slyke and J. M. Neill (1924, J. Biol. Chem.61, 523–573) for use with freeze-clamped tissue where anoxic changes have not occurred. The HCO3? content exclusive of tissue CO2 in fed rats was found to be: liver, 19.4 ± 1.0; brain, 20.2 ± 0.9; thigh, 16.2 ± 0.8; and heart, 15.4 ± 1.4 μmol/g. 相似文献
Depression, a severe mental disease, is greatly difficult to treat and easy to induce other neuropsychiatric symptoms, the most frequent one is cognitive impairment. In this study, a series of novel vilazodone-tacrine hybrids were designed, synthesized and evaluated as multitarget agents against depression with cognitive impairment. Most compounds exhibited good multitarget activities and appropriate blood-brain barrier permeability. Specifically, compounds 1d and 2a exhibited excellent 5-HT1A agonist activities (1d, EC50?=?0.36?±?0.08?nM; 2a, EC50?=?0.58?±?0.14?nM) and 5-HT reuptake inhibitory activities (1d, IC50?=?20.42?±?6.60?nM; 2a, IC50?=?22.10?±?5.80?nM). In addition, they showed moderate ChE inhibitory activities (1d, AChE IC50?=?1.72?±?0.217?μM, BuChE IC50?=?0.34?±?0.03?μM; 2a, AChE IC50?=?2.36?±?0.34?μM, BuChE IC50?=?0.10?±?0.01?μM). Good multitarget activities with goodt blood-brain barrier permeability of 1d and 2a make them good lead compounds for the further study of depression with cognitive impairment. 相似文献
This study investigated the action of enprostil, a synthetic analog of PGE2, on gastric HCO3− secretion in humans and on duodenal HCO3− secretion in the anesthetized rat. A previously validated 2-component model was used to calculate gastric HCO3− and H+ secretion in 10 human subjects. Compared to placebo, a single 70 μg oral dose of enprostil increased basal gastric HCO3− secretion from 1810 +- 340 to 3190 ± 890 μmol/hr (P < 0.05). In addition, enprostil reduced basal gastric H+ secretion from 5240 ± 1140 to 1680 ± 530 μmol/hr (P < 0.02). Enprostil also increased HCO3− and reduced H+ secretion during intravenous pentagastrin infusion. In the rat, duodenal HCO3− secretion was measured by direct titration in situ using perfused segments of duodenum just distal to the Brunner gland area dn devoid of pancreatic and biliary secretions. Addition of enprostil(10 μg/ml) to the duodenal bathing solution increased duodenal HOC3− secretion from 6.3 ± 1.3 to 15.1 ± 2.0 μmol/cm·hr (P < 0.01, n = 6). The stimulatory action of enprostil on duodenal HCO3− secretion at 10 μg/ml was comparable in magnitude and duration to that of 10 μg/ml natural PGE2. In summary, the PGE2 analog enprostil stimulated gastroduodenal HCO3− secretion, effects which may be beneficial in protection of the gastroduodenal mucosa against luminal acid. 相似文献
The following procedure is recommended: Fix ces-todes and trematodes (while held flat between glass slides) 0.5–2.0 hr. in the following mixture: formalin, 15; acetic acid (gl.), 5; glycerol, 10; 95% ethyl alcohol, 24; distilled H2O, 46; all proportions by volume. After freeing them from the slides, wash thoroughly in running water and stain immediately thereafter. Stock staining solution: ferric ammonium alum (violet cryst.), 2 g.; distilled H2O (cold) 100 ml.; after solution, add 2 ml. concentrated H2SO4, bring to a boil; add 1 g. coelestin blue B (Nat. Aniline), boil 3–5 min.; cool and add 10 ml. absolute methyl alcohol and 10 ml. glycerol. Dilute 1 vol. with 3 vol. distilled H20 for use. Stain 5–30 min., depending on size of specimens. Wash with 2 changes 0.5 hr. each of distilled H2O, then 50% isopropyl alcohol 12–16 hr., 50% isopropyl alcohol 2 hr., followed by graded isopropyl alcohol for dehydration. Ether: ethyl alcohol (equal parts), 1 hr., is followed by embedding in celloidin in a sheet just thick enough to cover the specimens. Trim embedded specimens and dehydrate with isopropyl alcohol, 80%, 90% and absolute. Clear in beechwood creosote. Mount in balsam with cover glasses that overlap the edges of the celloidin 1–2 mm. While drying at 37°C, refill edges of mount with fresh balsam as needed. When dry, remove excess balsam and ring the edges with ordinary gloss enamel paint. 相似文献
Abstract: Neuroleptics, which are potent dopamine receptor antagonists, are used to treat psychosis. In the striatum, dopamine subtype-2 (D2) receptors interact with high-affinity adenosine subtype-2 (A2a) receptors. To examine the effect of various neuroleptics on the major subtypes of striatal dopamine and adenosine receptors, rats received 28 daily intraperitoneal injections of these drugs. Haloperidol (1.5 mg/kg/day) increased the density of striatal D2 receptors by 24% without changing their affinity for [3H]sulpiride. Haloperidol increased the density of striatal A2a receptors by 33% (control, 522.4 ± 20.7 fmol/mg of protein; haloperidol, 694.6 ± 23.6 fmol/mg of protein; p < 0.001) without changing their affinity for [3H]CGS-21680 (control, 19.2 ± 2.2 nM; haloperidol, 21.4 ± 2.3 nM). In contrast, haloperidol had no such effect on striatal dopamine subtype-1 (D1) and adenosine subtype-1 (A1) receptors. Binding characteristics and the pharmacological displacement profile of the increased [3H]CGS-21680 binding sites confirmed them as A2a receptors. Comparing different classes of neuroleptics showed that the typical neuroleptics haloperidol and fluphenazine (1.5 mg/kg/day) increased D2 receptor densities, whereas the atypical neuroleptics sulpiride (100 mg/kg/day) and clozapine (20 mg/kg/day) did not (control, 290.3 ± 8.7 fmol/mg of protein; haloperidol, 358.1 ± 6.9 fmol/mg of protein; fluphenazine, 381.3 ± 13.6 fmol/mg of protein; sulpiride, 319.8 ± 18.9 fmol/mg of protein; clozapine, 309.2 ± 13.7 fmol/mg of protein). Similarly, the typical neuroleptics increased A2a receptor densities, whereas the atypical neuroleptics did not (control, 536.9 ± 8.7 fmol/mg of protein; haloperidol, 687.9 ± 28.0 fmol/mg of protein; fluphenazine, 701.1 ± 31.6 fmol/mg of protein; sulpiride, 563.3 ± 27.2 fmol/mg of protein; clozapine, 550.9 ± 40.9 fmol/mg of protein). There were no differences in affinities for [3H]CGS-21680 or [3H]sulpiride among the various treatment groups. This study demonstrates that typical neuroleptics induce comparable up-regulation in both striatal D2 and A2a receptors. Thus, A2a receptors might be a pharmacologic target for the development of novel therapeutic strategies to minimize the adverse effects of antipsychotic treatment. 相似文献
This study was conducted to investigate the ecotoxicological effects of exposure to copper oxide nanoparticles (CuO NPs) on the gill of the swan mussel Anodonta cygnea using several approaches including qualitative and quantitative histopathology, ultra-morphology (scanning electron microscopy [SEM]) and measures of clearance rate (CR) and bioaccumulation of CuO NPs. Histological alterations in mussels exposed to 0.25 (T1), 2.5 (T2) and 25.0?µg L?1 (T3) CuO NPs for 12 days include changes in the length and form of gill lamellae, changes in inter-lamellar spaces, epithelial hyperplasia, atrophy and tissue rupture. Ultra-morphological changes following CuO NP exposure included epithelial hyperplasia and hypertrophy, epithelial lifting, tissue rupture (water channel fusion) and extensive necrosis of the gill surfaces. IGill (gill damage severity) index values for both histopathological and ultra-morphological data were significantly (P?0.05) higher in T3. The CR of mussels was significantly (P??1 g?1 dry weight]) in comparison to controls (CR?=?108?±?47.14 [L min?1 g?1 dry weight]). CuO NPs accumulated in exposed mussels at all exposure concentrations until day 4, but there was no further change in accumulation levels by the end of the exposure period. The accumulated content of CuO NPs was significantly (P??1 exposure concentration. Based on these results, significant accumulation of CuO NPs in the gills of swan mussel could affect histological and ultra-structural characteristics of this organ and consequently have deleterious impacts on its filtration activity. 相似文献
Measurements of ppm (v/v) level COg concentration is conveniently performed by its preconcentration in alkaline absorber solution of Ag+-(4)- HCO2-C6H4-SO2NH2 complex, followed by a spectral measurement of the reduced silver sol. In this study, the transitory nature of this latter species and its subsequent real-time transformation to silver nanoparticle are presented. These results were based on spectral measurements made under varying concentrations of alkali, (4)-HCO2-C6H4-SO2NH2, and Ag+ in the absorber solution, and in the presence of a wide range of sampled COg concentration. The initially created light yellow colored sol with its broad absorption profile peaking at 380 nm and absorption coefficient 3500?±?300 cm?1 M?1 (related to the amount of sampled [COg] as standardized by gas chromatographic analysis) changed into the characteristic yellow orange nanoparticle with its plasmon band peak absorption at 425 nm and absorption coefficient 6350?±?300 cm?1 M?1. Under different sampling conditions, the respective first-order conversion rates varied between 0.03 and 0.15 h?1, whereas simultaneous dynamic light scattering measurements revealed steady growth of the averaged particle size ranging from 60 to 300 nm. 相似文献
We measured resting metabolic rate (RMR), tidal volume (VT), breathing frequency (fR), respiratory flow, and end-expired gases in rough-toothed dolphins (Steno bredanensis) housed in managed care after an overnight fast and 1–2 hr following a meal. The measured average (± standard deviation) VT (4.0 ± 1.3 L) and fR (1.9 ± 1.0 breaths/min) were higher and lower, respectively, as compared with estimated values from both terrestrial and aquatic mammals, and the average VT was 43% of the estimated total lung capacity. The end-expired gas levels suggested that this species keep alveolar O2 (10.6% or 80 mmHg) and CO2 (7.6% or 57 mmHg), and likely arterial gas tensions, low and high, respectively, to maximize efficiency of gas exchange. We show that following an overnight fast, the RMR (566 ± 158 ml O2/min) was 1.8 times the estimated value predicted by Kleiber for terrestrial mammals of the same size. We also show that between 1 and 2 hr after ingestion of a meal, the metabolic rate increases an average of 29% (709 ± 126 ml O2/min). Both body mass (Mb) and fR significantly altered the measured RMR and we propose that both these variables should be measured when estimating energy use in cetaceans. 相似文献
A new flavoalkaloid racemate, leucoflavonine (1), together with its flavonoid precursor pectolinarigenin (2), was isolated from the leaves of Leucosceptrum canum collected from Tibet. Its structure was established by comprehensive spectroscopic analysis. Chrial separation of the enantiomers of 1 was achieved, and their absolute configurations were determined as S-(+)- and R-(?)-leucoflavonines ((+)-1a and (?)-1b) by comparison of their computational and experimental optical rotations. Biological assays indicated that both (+)-1a and (?)-1b exhibited inhibitory activity against acetylchlorinesterase (AChE) in vitro (IC50?=?68.0?±?8.6 and 18.3?±?1.8?μM, respectively). Moreover, (?)-1b displayed cytotoxicity against human hepatoma cells HepG2 (IC50?=?52.9?±?3.6?μM), and inhibited the production of interleukelin-2 (IL-2) in Jurkat cells (IC50?=?16.5?±?0.9?μM), while (+)-1a showed no obvious activity in these assays. 相似文献
The present study was aimed at determining total phenolic and flavonoid contents and studying the antioxidant activity of ginger (Zingiber officinale Rosc.) rhizome and callus, 6-gingerol and 6-shogaol and callus treated with elicitors. Petroleum ether (PE) and chloroform: methanol (1:1, v/v) (CM) extracts were prepared by maceration. Highest total phenolic content was obtained from the CM extract (60.34?±?0.43?mg gallic acid/g) of rhizome while callus showed lower content detected in the CM extract (33.6?±?0.07?mg gallic acid/g). Flavonoids were only detected in rhizome (CM extract 40.25?±?0.21?mg quercetin/g). Both rhizome extracts exhibited good antioxidant activity with higher activity recorded in PE extract (IC50 value 8.29?±?1.73?μg/mL). Callus extracts revealed lower antioxidant activity (IC50 value 1265.49?±?59.9?μg/mL obtained from CM extract). 6-gingerol and 6-shogaol displayed high antioxidant activity in both assays with IC50 4.85?+?0.58DPPH and 5.35?±?0.33ABTS μg/mL for the former and IC50 7.61?±?0.81DPPH and IC50 7.05?±?0.23ABTS μg/mL for the latter. Treatment of callus with elicitors showed significant (p?<?0.05) effects in enhancing phenolic content and related antioxidant activity. The highest significant increase in phenolic content (37% and 34%) and antioxidant activity in DPPH assay (34% and 30%) was observed in callus treated with 100?mg/L yeast extract and 50?mg/L salicylic acid respectively. Therefore, studying the effect of the elicitation of ginger cultured tissues in phenolic accumulation would be of immense importance for pharmacological, cosmetic and agronomic industries. 相似文献
A single dose of tritiated estradiol-17β (3H-E2β) was injected i.v. into 5 high egg producing White Leghorn hens, 31 weeks of age, at 19.2 ± 2.1 (mean ± S.D.) hr before oviposition. Blood (2 ml) was sampled at approximately 5 min intervals over 40 min. Whenever possible, metabolites were monitored and identified by the double isotope technique with the addition of the corresponding 14C-labelled standards to plasma prior to analysis. The metabolic half-life and clearance rate of 3H-E2β in plasma were 10.9 ± 1.9 min and 118 ± 18 ml/min/kg body weight, respectively. The calculated production rate of E2β at 19.2 hr before oviposition was 19.5 ± 5.7 ng/min based on the plasma level (93±22 pg/ml) measured at that time. The relative concentrations (% of plasma radioactivity) of the major metabolites isolated at 5.7 ± 0.6 min post injection were, in descending order: estradiol-17β-3-sulfate (E2β-3S : 14.9 ± 2.7), estradiol-17α-3-sulfate (E2α-3S; 5.7 ± 0.3), estrone (E1; 4.6 ± 0.5), estrone sulfate (E1S; 2.2 ± 0.5), and estradiol-17 α (E2α; 1.2 ± 0.4). As time proceeded, the relative concentration of E2α-3S gradually increased so that by 43.2 ± 1.0 min it became the most abundant identifiable metabolite (12.3 ± 1.1) followed by E2β-3S (9.1 ± 1.7), E2S (1.2 ± 0.6), E1 (0.7 ± 0.4) and E2α (0.3 ± 0.2). These findings are consistent with the view that one of the major pathways of E2β metabolism in the circulation of the hen is via E2β E2β?3S ?E1S E2α-3S. 相似文献
1. Acute toxicity effects of diazinon on European eel (Anguilla anguilla) were examined using short-term exposures in static conditions.2. The lc50 values found were: 0.16, 0.11, 0.09 and 0.08 mg/1 at 24, 48, 72 and 96 hr exposure, respectively.3. Eels were exposed to 0.056 mg/l of diazinon and the bioaccumulation and elimination of this insecticide in liver, muscle, gill and blood tissues were studied.4. BCF were 800 in liver, 1600 in muscle tissue and 2300 and 2730 in gill and blood tissue, respectively.5. The BCF1 were 0.30 for liver, 0.60 for muscle and 0.84 for gill. Higher accumulation capacity of the gill was observed for the first hour of exposure.6. Diazinon elimination from the selected tissues was rapid, diazinon levels were not detected in any tissue after 24 hr in clean water.7. The excretion rate constants (K2) of this insecticide were 0.023 hr−1 for liver, 0.005 hr−1 for gill and 0.019 −1 for muscle.8. Diazinon half-lives were calculated as 30.6, 32.2 and 38.3 hr for liver, muscle and gill, respectively. 相似文献
The reaction of β-galactosidase ( K12) with -nitrophenyl-β--galactoside has been investigated over the temperature range +25° to ?30° using 50% aqueous dimethyl sulfoxide as solvent. At temperatures below ?10° turnover becomes very slow and a burst of -nitrophenol is observed. Such a burst indicates the existence of a galactosyl-enzyme intermediate whose breakdown is rate-limiting and provides a means of determining the active site normality. The Arrhenius plot for turnover is linear in the ?25 to +25° range with Ea = 26 ± 3 kcal/mole. The presence of the 50% DMSO had no effect on Km but caused a small decrease in Kcat. 相似文献
Closure of atrial septal defects (ASD) prevents pulmonary hypertension, right heart failure and thromboembolic stroke. The exact timing for ASD closure is controversial.
Methods
In a prospective study to address the question whether unapparent pulmonary hypertension can be revealed prior to right ventricular (RV) remodelling, patients were investigated before and 6, 12, and 24 months after ASD closure using exercise stress echocardiography (ESE) and ergospirometry (n?=?24).
Results
At rest, RV systolic pressure (RVSP) was normal in 58.8 %, slightly elevated in 26.5 %, and moderately elevated in 11.8 %. One patient showed severe pulmonary hypertension. During ESE, all patients with normal RVSP at rest exhibited an increase (25.7?±?1.2 mmHg vs. 45.3?±?2.3 mmHg, p?<?0.001). After closure the RVSP was lower, both at rest and ESE. RV diameters decreased too. Tricuspid annulus plane systolic excursion (TAPSE) at rest remained lower after closure (24.0?±?0.9 vs. 22.0?±?0.9 mm, p?<?0.05). TAPSE in ESE was elevated, and stayed stable after closure (30.1?±?1.8 mm vs. 29.3?±?1.6 mm). Before closure, RV systolic tissue velocities (sa) at rest were normal and decreased after closure (14.0?±?1.0 cm/s vs. 11.5?±?0.7 (6 month) vs. 10.6?±?0.5 cm/s (12 month), p?<?0.05). During ESE, sa velocity was similar before and after closure (23.0?±?1.3 cm/s vs. 23.3?±?1.9 cm/s). Maximal oxygen uptake (VO2/kg) did not differ between baseline and follow-ups.
Conclusion
Latent pulmonary hypertension may become apparent in ESE. ASD closure leads to a significant reduction in this stress-induced pulmonary hypertension and to a decrease in the right heart diameters indicating reverse RV remodelling. RV functional parameters at rest did not improve. The VO2/kg did not change after ASD closure. 相似文献
Bats in hot roosts experience some of the most thermally challenging environments of any endotherms, but little is known about how heat tolerance and evaporative cooling capacity vary among species. We investigated thermoregulation in three sympatric species (Nycteris thebaica, Taphozous mauritianus and Sauromys petrophilus) in a hot, semi-arid environment by measuring body temperature (Tb), metabolic rate and evaporative water loss (EWL) at air temperatures (Ta) of 10?C42?°C. S. petrophilus was highly heterothermic with no clear thermoneutral zone, and exhibited rapid increases in EWL at high Ta to a maximum of 23.7?±?7.4?mg?g?1?h?1 at Ta????42?°C, with a concomitant maximum Tb of 43.7?±?1.0?°C. T. mauritianus remained largely normothermic at Tas below thermoneutrality and increased EWL to 14.7?±?1.3?mg?g?1?h?1 at Ta????42?°C, with a maximum Tb of 42.9?±?1.6?°C. In N. thebaica, EWL began increasing at lower Ta than in either of the other species and reached a maximum of 18.6?±?2.1?mg?g?1?h?1 at Ta?=?39.4?°C, with comparatively high maximum Tb values of 45.0?±?0.9?°C. Under the conditions of our study, N. thebaica was considerably less heat tolerant than the other two species. Among seven species of bats for which data on Tb as well as roost temperatures in comparison to outside Ta are available, we found limited evidence for a correlation between overall heat tolerance and the extent to which roosts are buffered from high Ta. 相似文献
