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131.
N-ethylmaleimide (NEM) Lit 10-100 μ M led to a strong inhibition of the auxin-induced elongation growth of colcoptile segments, while fusicoccin-enhanced growth was not affected. Growth inhibition occurred only if NEM and auxin were allowed to act simultaneously. Preincubation of plant segments with NEM in the absence of auxin caused no inhibition of a subsequent growth stimulation by auxin, whenever NEM was removed before the application of IAA. However, preincubation with NEM plus auxin led to a remaining growth inhibition, which could not be reversed by a second auxin incubation in the absence of NEM. Fusicoccin added to NEM- plus auxin-treated segments was able to restore growth. It is suggested that auxin causes the unmasking of essential SH-groups of a protein to which NEM links covalently. thus inhibiting the growth process. This assumption was further supported by labeling experiments wish [14 C]-NEM using membranes of maize ( Zea mays L. cv. Inraplus) coleoptiles. Two membrane fractions (S2 = 480-1900 g; S4 = 4300-15000 g) revealed a significantly higher [14 C]-NEM labeling in the presence of auxin (2,4-diehlorophe-noxyacctic acid compared to 2,6 dichlorophenoxyacetic acid). This effect disappeared when the membranes were previously washed with EGTA [ethyleneglycolbis-(β-aminoethylether)-N,N,Nr',N'-tetraacetic acid]. The auxin-induced sensitization of coleoptilc segments against thiol-reagents and the auxin-induced expression of SH-groups of proteins of isolated membranes from coleoptiles arc suggested to be events involved in the primary action of auxins. 相似文献
132.
Suppression of ammonium uptake by nitrogen supply and its relief during nitrogen limitation 总被引:4,自引:0,他引:4
Barley ( Hordeum vulgare , cv. Triumph), wheat ( Triticum aestivum , cv. Kleiber) and oat ( Avena sativa , cv. Tarok) were grown until day 20 in nitrate-containing solutions or in nitrogen-free solutions for periods up to 8 days immediately prior to day 20. They then were exposed for 4 h to complete, nitrate-free solutions containing 0.5 or 2.0 mM ammonium (98 atom%15 N). In all 3 species in 2 experiments, net ammonium uptake was low in plants grown continuously in nitrate, and increased 3 to 4-fold with increasing nitrogen deprivation. Charge balance during net ammonium uptake was largely maintained by the sum of net potassium and net proton efflux. Variations in root ammonium concentration at the time of exposure to the ammonium solutions revealed no consistent pattern with net ammonium uptake, implying that a product of ammonium assimilation may serve as a negative effector for the uptake process. In nitrogen-replete plants, and in those deprived of nitrogen for 2 days, the amounts of endogenous 14 N-ammonium recovered in the ambient 15 N-ammonium solution during the 4-h uptake period were greater than the initial amounts of 14 N-ammonium present in the root tissue. Significant generation of 14 N-ammonium from endogenous organic nitrogen sources was thus evident in all 3 species. 相似文献
133.
During the senescence of detached first leaves of oat ( Avena sativa L. cv. Victory) seedlings (grown in continuous light) the protein is hydrolyzed and the proteases increase, but the expected simple relation between these two factors is not always realized. The present experiments examine the timing, the influence of light and darkness and the action of the protein synthesis inhibitors cycloheximide (CHI) and cordycepin. Transfer from dark to light delays the breakdown of both chlorophyll (Chl) and protein, but some residual proteolysis is ascribed to the enzyme initially present. Transfer to CHI resembles transfer to light, while the action of cordyceptin is similar but much weaker. Repeated determinations of the acid protease, which is the most active one and the first to appear, show that this enzyme is formed in the light about as rapidly as in the dark, though with different kinetics. In spite of this there is little proteolysis in light in the first 5 days. One possible explanation of that could be that protein is rapidly resynthesized in light, but treatment with [14 C]-leucine shows that such resynthesis is no faster in light than in darkness. It is therefore concluded that the protease initially does not have access to its substrates and, as a corollary, that the senescence process must be controlled by the gradual impairment of the vacuolar membrane, allowing protease to enter the cytosol and attack the proteins there and in the organelles. This concept is supported by many observations on the timing and on the known changes in membrane permeability during senescence. 相似文献
134.
Wild oat (Avena fatua L.) caryopses were germinated on moist filter paper and under water in the presence and absence of hydrogen peroxide (H2O2). The sequential growth and development of embryo parts were studied. Germination, as indicated by radicle emergence, was
least and slowest in caryopses submerged in deoxygenated water. The coleorhiza in such caryopses elongated much earlier than
the root, in contrast to the other treatments where the coleorhiza and the root emerged at about the same time. In caryopses
incubated on moist filter paper all embryo parts showed considerable growth. In H2O2 treated caryopses only the epicotyl showed substantial growth over the experimental period. In all treatments the first mitotic
peaks were noticed at the same period. The occurrence of these early nuclear divisions may be due to release of 4 C nuclei
from inhibition by the uptake of water during caryopsis imbibition. The mitosis continued in the radicle of the embryo in
those caryopses germinating on moist filter paper, indicating occurrence of DNA synthesis. In the other two treatments, however,
few divisions were detected. Here the early growth of the root, causing caryopsis germination, was due to cell elongation,
especially in the proximal part of the root. 相似文献
135.
The physiological basis of seed dormancy in Avena fatua III. Action of nitrogenous compounds 总被引:1,自引:0,他引:1
Sodium nitrate and nitrite (50–100 m M ) induced germination in three out of four genetically pure dormant lines of Avena fatua L. The sensitivity to these treatments was low immediately ater harvest and increased markedly after six months of dry after-ripening. The observation that a fourth dormant line failed to respond suggests at least two metabolic blocks may be involved in expression of dormancy. An inhibitor of gibberellin biosynthesis, 2-chloroethyl trimethylammonium chloride, completely inhibited the dormancy-breaking effect by nitrate and nitrite, indicating a requirement for gibberellin biosynthesis. Among reduced nitrogenous compounds, ammonium chloride and urea failed to break dormancy in all partly after-ripened lines, suggesting that nitrate and nitrite may induce germination through their ability to act as electron acceptors. The sensitivity to all nitrogenous compounds tested increased with the length of after-ripening indicating that the depth of the second dormancy block amy decrease with the time of after-ripening. Other reduced nitrogenous compounds, thiourea and hydroxylamine hydrochloride, promoted some germination in the least dormant, partially after-ripened lines. The function of these compounds as electron acceptors and their similarity in activity to the cytochrome oxidase inhibitor, sodium azide, is discussed with reference to dormancy and the possible involvement of the alternative pathway of respiration. 相似文献
136.
137.
Y. Koide H. Maeda K. Yamabe K. Naruishi T. Yamamoto S. Kokeguchi S. Takashiba 《Letters in applied microbiology》2010,50(4):386-392
Aim: To develop a detection assay for staphylococcal mecA and spa by using loop‐mediated isothermal amplification (LAMP) method. Methods and Results: Staphylococcus aureus and other related species were subjected to the detection of mecA and spa by both PCR and LAMP methods. The LAMP successfully amplified the genes under isothermal conditions at 64°C within 60 min, and demonstrated identical results with the conventional PCR methods. The detection limits of the LAMP for mecA and spa, by gel electrophoresis, were 102 and 10 cells per tube, respectively. The naked‐eye inspections were possible with 103 and 10 cells for detection of mecA and spa, respectively. The LAMP method was then applied to sputum and dental plaque samples. The LAMP and PCR demonstrated identical results for the plaque samples, although frequency in detection of mecA and spa by the LAMP was relatively lower for the sputum samples when compared to the PCR methods. Conclusion: Application of the LAMP enabled a rapid detection assay for mecA and spa. The assay may be applicable to clinical plaque samples. Significance and Impact of the Study: The LAMP offers an alternative detection assay for mecA and spa with a great advantage of the rapidity. 相似文献
138.
139.
Khwanchai Khucharoenphaisan Shinji Tokuyama Vichien Kitpreechavanich 《Mycoscience》2010,51(6):405-410
Highly thermostable β-xylanase produced by newly isolated Thermomyces lanuginosus THKU-49 strain was purified in a four-step procedure involving ammonium sulfate precipitation and subsequent separation on
a DEAE-Sepharose fast flow column, hydroxylapatite column, and Sephadex G-100 column, respectively. The enzyme purified to
homogeneity had a specific activity of 552 U/mg protein and a molecular weight of 24.9 kDa. The optimal temperature of the
purified xylanase was 70°C, and it was stable at temperatures up to 60°C at pH 6.0; the optimal pH was 5.0–7.0, and it was
stable in the pH range 3.5–8.0 at 4°C. Xylanase activity was inhibited by Mn2+, Sn2+, and ethylenediaminetetraacetic acid. The xylanase showed a high activity towards soluble oat spelt xylan, but it exhibited
low activity towards insoluble oat spelt xylan; no activity was found to carboxymethylcellulose, avicel, filter paper, locust
bean gum, cassava starch, and p-nitrophenyl β-d-xylopyranoside. The apparent K
m value of the xylanase on soluble oat spelt xylan and insoluble oat spelt xylan was 7.3 ± 0.236 and 60.2 ± 6.788 mg/ml, respectively.
Thin-layer chromatography analysis showed that the xylanase hydrolyzed oat spelt xylan to yield mainly xylobiose and xylose
as end products, but that it could not release xylose from the substrate xylobiose, suggesting that it is an endo-xylanase. 相似文献
140.