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1.
The microcapsule artificial kidney was used in the treatment of three patients with acute drug intoxication. The apparatus contains 300 g. of microencapsulated activated charcoal with a total membrane area available for diffusion of more than 2m.2 The membrane thickness is only 500 A. These properties make possible a compact artificial kidney whose efficiency for the removal of uremic metabolites and drugs is much higher than standard hemodialysis apparatus. The microcapsules are made blood-compatible by coating with human albumin. A roller pump was used to propel the blood through the microcapsule artificial kidney at a flow rate of 300 ml./min. for two to three hours. The clearance values for glutethimide, methyprylon and methaqualone were much higher than those achieved by standard hemodialysis. Hemoperfusion quickly lowered the drug level in the blood with resulting clinical improvement.  相似文献   

2.
Studies of 3H-PGE1 binding in hamster uterus were conducted with tissue fractions isolated after incubation of tissue slices in media containing 3H-PGE1, or in a total system, in which 3H-PGE1 was incubated directly with isolated uterine tissue fractions. Bound 3H-PGE1 was seperated from unbound 3H-PGE1 by gel column chromatography or by treatment with activated charcoal. The effects of the non-ionic detergent Triton X-100 on binding were measured in both incubation systems.The presence of a specific binding-protein for 3H-PGE1 in hamster myometrium was demonstrated . The binding-protein was associated with a membrane fraction of the myometrial cell and was dependent on the integrity of membrane structure for binding specificity. The binding-protein was stabilized by association with its ligand, 3H-PGE1, and binding was irreversible .  相似文献   

3.
To address the questions of whether allocation of carbohydrates to roots is influenced by ionic form of nitrogen absorbed and whether allocation of carbohydrates to roots in turn influences proportionality between NH4+ and NO3? uptake from mixed sources, NH4+ and NO3? were supplied separately to halves of a split-root hydroponic system and were supplied in combination to a whole-root system. Dry matter accumulation in the split-root system was 18% less in the NH4+-fed axis than in the NO3?-fed axis. This, however, does not indicate that partitioning of carbohydrate between the two axes was different. Most of the reduction in dry matter accumulation in the NH4+-fed axis can be accounted for by the retransport of CH2O equivalents from the root back to the shoot with amino acids produced by NH4+ assimilation. Uptake of NH4+ or NO3? by the respective halves of the split-root system was proportional to the estimated allocation of carbohydrate to that half. When NH4+ and NO3? were supplied to separate halves of the split-root system, the cumulative NH4+ to NO3? uptake ratio was 0.81. When supplied in combination to the whole-root system, the cumulative NH4+ to NO3? uptake ratio was 1.67. Thus, while the shoot may affect total nitrogen uptake through the export of carbohydrates to roots, the shoot (common for halves of the split-root system) apparently does not exert a direct effect on proportionality of NH4+ and NO3? uptake by roots. For whole roots supplied with both NH4+ and NO3?, the restriction in uptake of NO3? may involve a stimulation of NO3? efflux rather than an inhibition of NO3? influx. While only the net uptake of NH4+ and NO3? was measured by ion chromatography, monitoring at approximately hourly intervals during the first 3 days of treatment revealed irregularly occurring intervals of both depletion (net influx) and enrichment (net efflux) in solutions. In the case of NH4+, numbers of net efflux events were similar (21 to 24 out of 65 sequential sampling intervals) whether NH4+ was supplied with NO3? to whole-root systems or separately to an axis of the split-root system. In the case of NO3?, however, the number of net efflux events increased from 8 when NO3? was supplied to a separate axis of the split-root system to between 19 and 24 when NO3? was supplied with NH4+ to whole-root systems.  相似文献   

4.
Alfalfa (Medicago sativa L.) N-sufficient plants were fed 1·5 mM N in the form of NO3, NH4+ or NO3 in conjunction with NH4+, or were N-deprived for 2 weeks. The specific activity of phosphoenolpyruvate carboxylase (PEPC) from the non-nodulated roots of N-sufficient plants was increased in comparison with that of N-deprived plants. The PEPC value was highest with NO3 nutrition, lowest with NH4+ and intermediate in plants that were fed mixed salts. The protein was more abundant in NO3-fed plants than in either NH4+- or N mixed-fed plants. Nitrogen starvation decreased the level of PEPC mRNA, and nitrate was the N form that most stimulated PEPC gene expression. The malate content was significantly lower in NO3-deprived than in NO3-sufficient plants. Root malate accumulation was high in NO3-fed plants, but decreased significantly in plants that were fed with NH4+. The effect of malate on the desalted enzyme was also investigated. Root PEPC was not very sensitive to malate and PEPC activity was inhibited only by very high concentrations of malate. Asparagine and glutamine enhanced PEPC activity markedly in NO3-fed plants, but failed to affect plants that were either treated with other N types or N starved. Glutamate and citrate inhibited PEPC activity only at optimal pH. N-nutrition also influenced root nitrate and ammonium accumulation. Nitrate accumulated in the roots of NO3- and (NO3 + NH4+)-fed plants, but was undetectable in those administered NH4+. Both the nitrate and the ammonium contents were significantly reduced in NO3- and (NO3 + NH4+)-starved plants. Root accumulation of free amino acids was strongly influenced by the type of N administered. It was highest in NH4+-fed plants and the most abundant amides were asparagine and glutamine. It was concluded that root PEPC from alfalfa plants is N regulated and that nitrate exerts a strong influence on the PEPC enzyme by enhancing both PEPC gene expression and activity.  相似文献   

5.
The effect of NO2 fumigation on root N uptake and metabolism was investigated in 3-month-old spruce (Picea abics L. Karst) seedlings. In a first experiment, the contribution of NO2 to the plant N budget was measured during a 48 h fumigation with 100mm3m?3 NO2. Plants were pre-treated with various nutrient solutions containing NO2 and NH4+, NO3? only or no nitrogen source for 1 week prior to the beginning of fumigation. Absence of NH4+ in the solution for 6d led to an increased capacity for NO3? uptake, whereas the absence of both ions caused a decrease in the plant N concentration, with no change in NO3? uptake. In fumigated plants, NO2 uptake accounted for 20–40% of NO3? uptake. Root NO3? uptake in plants supplied with NH4+plus NO3? solutions was decreased by NO2 fumigation, whereas it was not significantly altered in the other treatments. In a second experiment, spruce seedlings were grown on a solution containing both NO2 and NH4+ and were fumigated or not with 100mm3m?3 NO2 for 7 weeks. Fumigated plants accumulated less dry matter, especially in the roots. Fluxes of the two N species were estimated from their accumulations in shoots and roots, xylem exudate analysis and 15N labelling. Root NH4+ uptake was approximately three times higher than NO3? uptake. Nitrogen dioxide uptake represented 10–15% of the total N budget of the plants. In control plants, N assimilation occurred mainly in the roots and organic nitrogen was the main form of N transported to the shoot. Phloem transport of organic nitrogen accounted for 17% of its xylem transport. In fumigated plants, neither NO3? nor NH4+ accumulated in the shoot, showing that all the absorbed NO2 was assimilated. Root NO3? reduction was reduced whereas organic nitrogen transport in the phloem increased by a factor of 3 in NO2-fimugated as compared with control plants. The significance of the results for the regulation of whole-plant N utilization is discussed.  相似文献   

6.
Similarly to higher plant root systems, Chlamydomonas reinhardtii Dangeard (UTEX 90) cells exhibited biphasic NO3? uptake kinetics. The uptake pattern was similar in cells cultured in 10 mM NO3? (NO3?-grown), 0.25 mM NO3? (N-limited) or 10 mM NO3? followed by an 18-h period of N-deprivation (N-starved). In all cell types there was an apparent phase transition in uptake at 1.1 mM NO3?, although there were variations in the uptake Vmax of both isotherms. The rate of uptake via isotherm 0 ([NO3?]<1.1 mM) in N-limited cells was higher than that of either NO3?-grown or N-starved cells. In contrast, NO3?-grown and N-limited cells exhibited comparable Vmax values when supplied with 1.1 to 1.8 mM NO3? (isotherm 1). When supplied with 1.6 mM NO3?, both N-limited and N-starved cells exhibited enhanced linear uptake after 60 min of incubation. We ascribed this to an induction phenomenon. This trend was not observed when NO3?-grown cells were supplied with 1.6 mM NO3?, or when N-limited and N-starved cells were supplied with 0.6 mM NO3?. The ‘inducible’ aspect of uptake by N-limited cells was blocked by cycloheximide (10 mg l?1), but not by actinomycin D (5 mg l?1), thus indicating the involvement of a translational or post-translational event. To investigate this phenomenon further, we analysed the cell proteins of N-limited cells supplied with either 0.6 or 1.6 mM NO3? for 90 min, using two-dimensional gel electrophoresis. Comparison of protein profiles enabled the identification of a single cell membrane-associated polypeptide (21 kDa, pI ca 5.5) and ten soluble fraction polypeptides (17–73 kDa, pI ca 5.0 to 7.1) unique to the high NO3? treatment. We propose that the ‘inducible’ portion of NO3? uptake may provide the means by which C. reinhardtii cells regulate uptake in accordance with assimilatory capacity.  相似文献   

7.
Transport of a nitrate analogue, 36Cl-ClO3, was examined in two diatoms, Skeletonema costatum (Greve.) Cleve and Nitzschia closterium (Ehrenb) W. Sm. A dinoflagellate, Gonyaulax polyedra did not transport ClO3. Transport of 36Cl-ClO3 by diatoms appeared to be active and showed saturation kinetics. The data were fitted by Michaelis-Menten equation at all but the lowest chlorate concentrations (where plots of S vs. v showed a slight concave bend). Affinity of cells for nitrate was considerably higher than for chlorate. The Ki for nitrate inhibition of chlorate transport was calculated assuming competitive inhibition. Light had little or no effect on chlorate transport. Pulse-chase experiments demonstrated that (1) ClO3 (hence NO3) was stored in two intracellular compartments of equal size, (2) internal ClO3 was exchangeable with external ClO3 (rates of efflux and influx were measured), and (3) efflux of intracellular ClO3 showed transient states following a chase of ClO3 or NO3 which stabilized after 10–20 min. Transport of chlorate was a function of growth phase.  相似文献   

8.
[3H]gibberellin A9 was applied to shoots or seed parts of G2 pea to produce radiolabeled metabolites. These were used as markers during purification for the recovery of endogenous GA9 and its naturally occurring metabolites. GA9 and its metabolites were purified by HPLC, derivatized and examined by GC-MS. Endogenous GA9, GA20, GA29 and GA51 were identified in pea shoots and seed coats. GA51-catabolite and GA29-catabolite were also detected in seed coats. GA70 was detected in seed coats following the application of 1 g of GA9. Applied [3H]GA9 was metabolized through both the 13-hydroxylation and 2-hydroxylation pathways. Labeled metabolites were tentatively identified on the basis of co-chromatography on HPLC with endogenous compounds identified by GC-MS. In shoots [3H]GA51 and [3H]GA51-catabolite were the predominant metabolites after 6 hrs, but by 24 hrs there was little of these metabolites remaining, while [3H]GA29-catabolite and an unidentified metabolite predominated. In seed coats [3H]GA51 was the initial product, later followed by [3H]GA51-catabolite and an unidentified metabolite (different from that in shoots), with lesser amounts of [3H]GA20, [3H]GA29 and [3H]GA29-catabolite. [3H]GA70 was a very minor product in both cases. [3H]GA9 was not metabolized by pea cotyledons.Edited by T.J. Gianfagna.Author for correspondence  相似文献   

9.
Cell growth and tRNA-lys4 synthesis in mouse 3T3 cells   总被引:2,自引:0,他引:2  
The RPC-5 chromatographic profiles of lys-tRNA were analyzed during the growth of 3T3 cells in culture. An inverse relationship was seen between tRNA2lys and tRNA4lys which was markedly influenced by medium changes. This interchange of tRNA2lys and tRNA4lys could be controlled by altering the levels of serum in the medium, or more precisely by altering the serum to cell ratio. A different change in lys-tRNA distribution was seen when the cells reached confluency. The amounts of tRNA2lys, tRNA3lys and tRNA4lys all decreased with a corresponding increase in either tRNA5lys or tRNA6lys. An identical change in lys-tRNA could be produced by shifting sparse cells into a medium containing 10% calf plasma instead of 10% serum. Both tRNAlys profiles and cell growth were returned to normal when the cells were returned to medium with 10% fetal calf serum (FCS) or 10% calf plasma and fibroblast growth factor (FGF). A third alteration in tRNAlys profiles was seen by the addition of cAMP to the cultures. A decrease in tRNA5lys and a corresponding increase in tRNA6lys was seen upon the addition of 10?3 M db-cAMP and was accentuated by the simultaneous addition of 10?3 M methyl isobutylxanthine.These data are consistent with an ordered sequence of tRNAlys modification involving tRNA2lys, tRNA3lys, tRNA4lys, tRNA5Blys and tRNA6lys. Several of the factors which control proliferation appear to control the activity of different tRNA-modifying enzymes in this tRNAlys pathway thereby controlling the levels of tRNA4lys, a tRNA previously shown to correlate directly with the proliferative rate of cells.  相似文献   

10.
Relationships among growth, N accumulation and assimilation were investigated in Chrysanthemum morifolium Ramat cv. Fiesta in experiments testing the effects of varying levels of NO–33supply and of increasing NH+4 added to a constant level of NO–33 Flowing solution culture systems were used to provide NO?3at concentrations of 0.03 to 5.0 mol m–3 and NH+4 levels from 0.05 to 0.3 mmol m–3 added to 0.1 mol m–3NO?3. Rates of growth, N absorption, accumulation, distribution and utilization were estimated by regression analysis of data obtained from sequential plant harvests, and rates of NO?3 and NH?4 net uptake were estimated from solution depletion. A sustained ambient NO?3 concentration of 0.03 mol m–3 was evidently adequate to support growth, since relative growth rates were not affected by increasing NO?3 supply from 0.03 to 1.0 mol m–3, nor from 0.25 to 5.0 mol m–3, in separate experiments. Shoot growth rates were stimulated by NH4 added to NO?3 one experiment, but not when the experiment was repeated under ambient conditions less favorable to growth. Relative accumulation rates for total N increased with increasing NO?3 and with NH+4added to NO?3 A constant proportion of NO?3 taken up was reduced when NO?3 alone was supplied. Both the proportion of total N taken up as NO?3 and the proportion of NO?3 reduced decreased with increasing NH+3 added to NO?3 NH+4 uptake apparently must exceed a threshold of about 30% of the total uptake to inhibit NO?3 uptake. Utilization of N in chrysanthemum was apparently limited by redistribution since relative accumulation rates for total N were equal to or greater than relative growth rates, in contrast to results reported for several other species. Results of this study and other information support the postulate that NH+4 added to NO?3might stimulate growth by increasing transport of reduced N from roots to shoots, thus increasing the supply of reduced N available to support growth of shoot meristems.  相似文献   

11.
The BaZrSi3O9:Cr3+ phosphors were prepared by a high temperature solid state method. Their structures were confirmed with XRD and their luminescence properties were investigated. Under excitation at 455 nm, BaZrSi3O9:Cr3+ phosphors exhibited a broad near infrared emission band peaked at 800 nm, which was assigned to the 4T24A2 transition of Cr3+. The near infrared emission intensity reached a maximum at Cr3+ concentration of 0.7%. There was a concentration quenching phenomenon of Cr3+ in BaZrSi3O9 matrix and the corresponding concentration quenching mechanism was investigated. With efficient near infrared emission in the range of 700–1000 nm, BaZrSi3O9:Cr3+ phosphors may find applications in solar energy conversion.  相似文献   

12.
Tropospheric ozone (O3) decreases photosynthesis, growth, and yield of crop plants, while elevated carbon dioxide (CO2) has the opposite effect. The net photosynthetic rate (P N), dark respiration rate (R D), and ascorbic acid content of rice leaves were examined under combinations of O3 (0, 0.1, or 0.3 cm3 m−3, expressed as O0, O0.1, O0.3, respectively) and CO2 (400 or 800 cm3 m−3, expressed as C400 or C800, respectively). The P N declined immediately after O3 fumigation, and was larger under O0.3 than under O0.1. When C800 was combined with the O3, P N was unaffected by O0.1 and there was an approximately 20 % decrease when the rice leaves were exposed to O0.3 for 3 h. The depression of stomatal conductance (g s) observed under O0.1 was accelerated by C800, and that under O0.3 did not change because the decline under O0.3 was too large. Excluding the stomatal effect, the mesophyll P N was suppressed only by O0.3, but was substantially ameliorated when C800 was combined. Ozone fumigation boosted the R D value, whereas C800 suppressed it. An appreciable reduction of ascorbic acid occurred when the leaves were fumigated with O0.3, but the reduction was partially ameliorated by C800. The degree of visible leaf symptoms coincided with the effect of the interaction between O3 and CO2 on P N. The amelioration of O3 injury by elevated CO2 was largely attributed to the restriction of O3 intake by the leaves with stomatal closure, and partly to the maintenance of the scavenge system for reactive oxygen species that entered the leaf mesophyll, as well as the promotion of the P N.  相似文献   

13.
The distribution of NO3? reduction between roots and shoots was studied in hydro-ponically-grown peach-tree seedlings (Prunus persica L.) during recovery from N starvation. Uptake, translocation and reduction of NO3?, together with transport through xylem and phloem of the newly reduced N were estimated, using 15N labellings, in intact plants supplied for 90 h with 0.5 mM NH4+ and 0.5, 1.5 or 10 mM NO3?. Xylem transport of NO3? was further investigated by xylem sap analysis in a similar experiment. The roots were the main site of NO3? reduction at all 3 levels of NO3? nutrition. However, the contribution of the shoots to the whole plant NO3? reduction increased with increasing external NO3? availability. This contribution was estimated to be 20, 23 and 42% of the total assimilation at 0.5, 1.5 and 10 mM NO3?, respectively. Both 15N results and xylem sap analysis confirmed that this trend was due to an enhancement of NO3? translocation from roots to shoots. It is proposed that the lack of NO3? export to the shoots at low NO3? uptake rate resulted from a competition between NO3? reduction in the root epidermis/cortex and NO3? diffusion to the stele. On the other hand, net xylem transport of newly reduced N was very efficient since ca 70% of the amino acids synthesized in the roots were translocated to the shoots, regardless of the level of NO3? nutrition. This net xylem transport by far exceeded the net downward phloem transport of the reduced N assimilated in shoots. As a consequence, the reduced N resulting from NO3? assimilation, principally occurring in the roots, was mainly incorporated in the shoots.  相似文献   

14.
15.
A series of Bi3+,Eu3+‐doped BaMoO4 phosphors was synthesized using a hydrothermal method. The crystal structure, morphology and optical properties of the phosphors were studied using X‐ray diffraction (XRD), scanning electron microscope (SEM) and photoluminescence (PL) measurements. Three different particle morphologies were detected in the SEM observation. The energy dispersive spectroscopy (EDS) results indicated that the solubility of Bi3+ in spherical or rugby‐like BaMoO4 particles was very low and the excess Bi3+ element was cumulated in the irregular particles. Characteristic emissions of Eu3+ ions (5D0 → 7FJ; J = 0, 1, 2, 3, 4) were observed under excitation in ultraviolet (UV) light, with the most intense transition being the 5D0 → 7F2 transition. Energy transfer from MoO42? and Bi3+ to Eu3+ can be readily achieved. Red emission intensity of Eu3+ was enhanced by a factor of two by co‐doping with a small amount of Bi3+. Optical properties as a function of Bi3+ content were studied and the optimum Bi3+ content in BaMoO4 nanocrystals was determined to be 0.4 mol%.  相似文献   

16.
Kende H  Hahn H  Kays SE 《Plant physiology》1971,48(6):702-706
Nitrate reductase activity in excised embryos of Agrostemma githago increases in response to both NO3 and cytokinins. We asked the question whether cytokinins affected nitrate reductase activity directly or through NO3, either by amplifying the effect of low endogenous NO3 levels, or by making NO3 available for induction from a metabolically inactive compartment. Nitrate reductase activity was enhanced on the average by 50% after 1 hour of benzyladenine treatment. In some experiments, the cytokinin response was detectable as early as 30 minutes after addition of benzyladenine. Nitrate reductase activity increased linearly for 4 hours and began to decay 13 hours after start of the hormone treatment. When embryos were incubated in solutions containing mixtures of NO3 and benzyladenine, additive responses were obtained. The effects of NO3 and benzyladenine were counteracted by abscisic acid. The increase in nitrate reductase activity was inhibited at lower abscisic acid concentrations in embryos which were induced with NO3, as compared to embryos treated with benzyladenine. Casein hydrolysate inhibited the development of nitrate reductase activity. The response to NO3 was more susceptible to inhibition by casein hydrolysate than the response to the hormone. When NO3 and benzyladenine were withdrawn from the medium after maximal enhancement of nitrate reductase activity, the level of the enzyme decreased rapidly. Nitrate reductase activity increasd again as a result of a second treatment with benzyladenine but not with NO3. At the time of the second exposure to benzyladenine, no NO3 was detectable in extracts of Agrostemma embryos. This is taken as evidence that cytokinins enhance nitrate reductase activity directly and not through induction by NO3.  相似文献   

17.
Role of Chemotaxis in the Ecology of Denitrifiers   总被引:4,自引:2,他引:2       下载免费PDF全文
A modification of the Adler capillary assay was used to evaluate the chemotactic responses of several denitrifiers to nitrate and nitrite. Strong positive chemotaxis was observed to NO3 and NO2 by soil isolates of Pseudomonas aeruginosa, Pseudomonas fluorescens, and Pseudomonas stutzeri, with the peak response occurring at 10−3 M for both attractants. In addition, a strong chemoattraction to serine (peak response at 10−2 M), tryptone, and a soil extract, but not to NH4+, was observed for all denitrifiers tested. Chemotaxis was not dependent on a previous growth on NO3, NO2, or a soil extract, and the chemoattraction to NO3 occurred when the bacteria were grown aerobically or anaerobically. However, the best response to NO3 was usually observed when the cells were grown aerobically with 10 mM NO3 in the growth medium. Capillary tubes containing 103 M NO3 submerged into soil-water mixtures elicited a significant chemotactic response to NO3 by the indigenous soil microflora, the majority of which were Pseudomonas spp. A chemotactic strain of P. fluorescens also was shown to survive significantly better in aerobic and anaerobic soils than was a nonmotile strain of the same species. Both strains had equal growth rates in liquid cultures. Thus, chemotaxis may be one mechanism by which denitrifiers successfully compete for available NO3 and NO2, and which may facilitate the survival of naturally occurring populations of some denitrifiers.  相似文献   

18.
Abstract: Specific binding of tritiated dopamine, spiperone, and N-propylnorapomorphine was examined in subcellular fractions from bovine caudate nucleus. All fractions contained at least two sets of specific binding sites for [3H]spiperone (KD 1aPP= 0.2 nM, KD 2aPP= 2.2 nM), the higher affinity sites accounting for one-third to one-eighth of the total. [3H]Spiperone binding was slightly enriched over the total particulate fraction in P2, P3, SPM, and a crude fraction of synaptic mitochondria. A microsomal subfraction (P3B2) exhibited the highest specific binding capacity obtained, representing a fourfold enrichment over the total particulate fraction. [3H]Dopamine exhibited apparent binding to a single class of high-affinity sites in all fractions examined (KDaPP= 4.0 nM). A greater than twofold enrichment was observed in all fractions except myelin and P3, with a fivefold enrichment in SPM and P3B2. At least two classes of receptors were labeled by [3H]-N-propylnorapomorphine (KD 1aPP= 0.55 nM, KD 2aPP= 20 nM), using 50 nM-spiperone together with 100 nM-dopamine to define nonspecific binding. Although binding to the higher affinity site was displaced by spiperone, and lower affinity binding by dopamine, comparison of receptor densities with values obtained by using [3H]spiperone and [3H]dopamine directly suggested that [3H]-N-propylnorapomorphine labeled additional sites. We have also examined a postsynaptic membrane (PSM) fraction obtained from SPM by successive extraction with salt and EGTA followed by sonication and separation on a density gradient. [3H]Spiperone binding in PSM was enriched two- to threefold over unfractionated SPM with a concomitant decrease in [3H]dopamine binding. The enrichment in spiperone receptors was almost entirely due to an increase in the number of lower affinity binding sites, suggesting that these sites may be associated with the postsynaptic membrane.  相似文献   

19.
Barley (c.v. Himalaya) aleurone layers were incubated in [3H]gibberellin A1 (GA1) at low temperatures. At 3 and 4 C, 3H-activity was steadily accumulated in aleurone layers, and this accumulation was correlated with significant [3H]GA1 metabolism. At 1 and 1.5 C, metabolism could not be detected, and at these temperatures aleurone layers equilibrated with the [3H]GA1 concentration in the incubation medium. At equilibrium, the total amount of 3H-activity per unit volume in the aleurone layers was higher than in the incubation medium. Aleurone layers incubated at 0.5 C for 72 hours with [3H]GA1 in the presence of saturating levels of carrier GA1 consistently retained lower levels of 3H-activity than when incubated in [3H]GA1 alone. The retention of [3H]GA1 was unaffected by saturating levels of carrier GA8. GA1 retained by barley aleurone layers that were incubated at 0.5 C for 72 hours was able to induce α-amylase synthesis when aleurone layers were subsequently washed and transferred to a gibberellin-free medium at 25 C.  相似文献   

20.
Transport of a nitrate analogue, 36Cl-ClO3, was examined in two diatoms, Skeletonema costatum (Greve.) Cleve and Nitzschia closterium (Ehrenb) W. Sm. A dinoflagellate, Gonyaulax polyedra did not transport ClO3. Transport of 36Cl-ClO3, by diatoms appeared to be active and showed saturation kinetics. The data were fitted by Michaelis-Menten equation at all but the lowest chlorate concentrations (where plots of S vs. v showed a slight concave bend). Affinity of cells for nitrate was considerably higher than for chlorate. The Ki for nitrate inhibition of chlorate transport was calculated assuming competitive inhibition. Light had little or no effect on chlorate transport. Pulse-chase experiments demonstrated that (1) ClO3 (hence NO3) was stored in two intracellular compartments of equal size, (2) internal ClO3 was exchangeable with external ClO3 (rates of efflux and influx were measured), and (3) efflux of intracellular ClO3 showed transient states following a chase of ClO3 or NO3 which stabilized after 10–20 min. Transport of chlorate was a function of growth phase.  相似文献   

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