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1.
Purification and partial characterization of pyruvate decarboxylase from Oryza sativa L 总被引:2,自引:0,他引:2
Pyruvate decarboxylase(PyrDC) was purified from rice bran to a specific activity of 1 mu kat/mg and partially characterized. The holoenzyme is a tetramer of two types of subunits with molecular masses 64 kDa and 62 kDa. Purified rice PyrDC exhibits positive cooperative kinetics with respect to pyruvate and functions with a significant lag phase. When compared to other plant PyrDC, the lag phase was shorter at low pyruvate concentrations and the S0.5 was smaller. The optimum pH (6.25) was also less acidic and the enzyme retained 30% of its maximal activity at neutral pH. In contrast to other plant PyrDC, rice PyrDC could be active at the onset of anoxia and would be activated by small changes in pyruvate concentration. 相似文献
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3.
Lactate Dehydrogenase in Oryza sativa L. Seedlings and Roots: Identification and Partial Characterization 总被引:4,自引:4,他引:0 下载免费PDF全文
A lactate dehydrogenase activity is present in rice (Oryza sativa L.) seedlings and roots. Under aerobic conditions, lactate dehydrogenase activity is barely detectable in rice seedlings and is very low in rice roots. In 30 day old roots, the activity is increased two to three times by an anoxic or hypoxic treatment and can be detected on immunoblots by an antiserum raised against barley lactate dehydrogenase. The activity present in aerobic seedlings was partially purified. The native enzyme has a molecular mass of 160 kilodaltons, and is a tetramer of 2 subunit (38 and 39 kilodaltons) randomly associated. Studies of substrate specificity, native gel electrophoresis, and immunoblot analysis indicate that the partially purified enzyme is a typical lactate dehydrogenase. However, no increase of lactate dehydrogenase activity or protein was observed in seedlings transferred to anoxia. 相似文献
4.
J M Montserrat T Ricard M Mateu J Roca R Rodríguez-Roisín 《Revista Espanola de Fisiología》1991,47(4):193-199
To investigate the factors that modulate exercise performance at extreme altitude, the role of the following variables was analyzed in 16 climbers: 1) ventilatory response to chemical stimuli (hypoxia and hypercapnia); and, 2) maximum exercise performance while breathing room air and during acute hypoxia (F1O2, 0.11). Seven climbers (elite climbers, AE) had previously ascended to 8,000 m or more above sea level, and 9 (A) had never achieved such extreme altitude. Then healthy sedentary subjects (C) of similar age (31.1 +/- 6.0 SD years) were used as control group. Elite climbers showed higher ventilatory responses to both transient hypoxia (-0.49 +/- 0.13 L x min-1 x %-1) (p less than 0.05) and progressive hypoxia (-0.47 +/- 0.13 L x min-1 x %-1) than C (-0.33 +/- 0.14 and -0.30 +/- 0.15 L x min-1 x %-1, respectively). By contrast, no differences were observed between the two groups of climbers. The ventilatory response to hypercapnia was higher in AE (3.04 +/- 1.03 L x min-1 mmHg-1) compared to A (1.85 +/- 0.73 L x min-1 mmHg-1) (p less than 0.05) but similar to that observed in C. Breathing 11% O2, maximum workload and oxyhemoglobin desaturation during maximum exercise were similar in both groups of climbers. Additionally, the ventilatory response to hypoxia did not correlate with maximum workload (F1O2, 0.11), maximal ventilation during exercise (F1O2, 0.11), nor with the altitude score. The present study supports previous reports that inform about the role of the ventilatory response to hypoxia in the exercise performance at high altitude.(ABSTRACT TRUNCATED AT 250 WORDS) 相似文献
5.
Proteolytic cleavage of the E2 glycoprotein of murine coronavirus: activation of cell-fusing activity of virions by trypsin and separation of two different 90K cleavage fragments. 总被引:31,自引:23,他引:8 下载免费PDF全文
In the murine coronavirus mouse hepatitis virus, a single glycoprotein, E2, is required both for attachment to cells and for cell fusion. Cell fusion induced by infection with mouse hepatitis virus strain A59 was inhibited by the addition of monospecific anti-E2 antibody after virus adsorption and penetration. Adsorption of concentrated coronavirions to uninfected cells did not cause cell fusion in the presence of cycloheximide. Thus, cell fusion was induced by E2 on the plasma membrane of infected 17 Cl 1 cells but not by E2 on virions grown in these cells. Trypsin treatment of virions purified from 17 Cl 1 cells quantitatively cleaved 180K E2 to 90K E2 and activated cell-fusing activity of the virions. This proteolytic cleavage yielded two different 90K species which were separable by sodium dodecyl sulfate-hydroxyapatite chromatography. One of the trypsin cleavage products, 90A, was acylated and may be associated with the lipid bilayer. The other, 90B, was not acylated and yielded different peptides than did 90A upon limited digestion with thermolysin or staphylococcal V8 protease. Thus, the cell-fusing activity of a coronavirus required proteolytic cleavage of the E2 glycoprotein, either by the addition of a protease to virions or by cellular proteases acting on E2, which was transported to the plasma membrane during virus maturation. There is a striking functional similarity between the E2 glycoprotein of coronavirus, which is a positive-strand RNA virus, and the hemagglutinin glycoprotein of negative-strand orthomyxoviruses, in that a single glycoprotein has both attachment and protease-activated cell-fusing activities. 相似文献
6.
Jacques Ricard Jacques Vergne Jean-Luc Decout Marie-Christine Maurell 《Journal of molecular evolution》1996,43(4):315-325
A polyallylamine carrying long hydrophobic dodecyl groups and adenine residues as side chains (PALAD C12) may be able to catalyze the hydrolysis ofN-carbobenzoxy-l-alaninep-nitrophenyl ester (N-Cbz-Ala) as well asp-nitrophenyl acetate (pNPA). The progress curve of hydrolysis of the former displays a long lag and apparently no steady state.
After this transient the rate falls off due to the accumulation of the products. Conversely, the hydrolysis ofp-nitrophenyl acetate displays classical burst kinetics followed by a slow decline of the reaction rate.
Theoretical considerations show that a steady state may be expected to occur only if the concentration of the free catalyst
is very small during the reaction. This condition is sufficient to allow the rate of disappearance of the substrate to be
equal to the rate of appearance of the products, which is precisely a condition for the existence of a steady state. If the
catalyst is poorly active and has a loose affinity for its substrate and product, the measurement of a significant reaction
rate will require a much larger concentration of the catalyst. Therefore, under these conditions, one cannot expect a steady
state to occur. The mathematical expression of the error made in the steady-state assumption has been derived. This error
increases with the catalyst concentration and decreases if the affinity of the substrate for the catalyst is high. Therefore
the lack of steady state is associated with the affinity (or the dissociation) of the substrate and the product for the catalyst.
When this affinity is low, the free concentration of the catalyst during the reaction is high and one cannot expect a steady
state to occur. This is precisely what takes place with N-Cbz-Ala.
A mathematical expression of the rate of hydrolysis of N-Cbz-Ala and of any reactant that displays this type of kinetics may
be derived at the end of the transient when the rate is close to its maximum value. Under these conditions the rate cannot
follow classical Michaelis-Menten kinetics and displays positive cooperativity.
It may therefore be speculated that primordial template-like catalysts that were displaying a poor affinity for their substrates
and products were already exhibiting apparent positive cooperativity in the kinetic reactions they were able to catalyze.
Correspondence to: J. Ricard 相似文献
7.
8.
The effects of inorganic mercury (HgII) and methylmercury (MeHg) on the colonization of artificial substrates by periphytic
diatoms were studied using indoor freshwater microcosms. These consisted of a mixed biotope– water column + natural sediment
– with rooted macrophyte cuttings (Elodea densa) and benthic bivalve molluscs (Corbicula fluminea).The periphyton was collected
on glass slides in the water column after 34and 71 days. The two Hg sources were introduced either by daily additions to the
water column, or once at the beginning into the sediment, using two nominal concentrations: water column, 0.5 μgL-1 and 2 μg L-1 for both compounds: sediment, 0.5 mg kg-1 (fw) and 2 mgkg-1 (fw) for MeHg and 1 mg kg-1 (fw) and 10 mgkg-1 (fw) for HgII. Several complementary criteria were used to analyse the structural and functional perturbations induced: cell
density, species richness, diatom size, relative abundance. Exposure to MeHg added to the water column resulted in reduced
cell density and changes in species composition with enhancement of e.g. Fallacia pygmaea or Nitzschia palea; inorganic Hg
had less effect on the population structure. After contamination via the sediment, the effects of the two compounds were less
pronounced than for the water source.
This revised version was published online in August 2006 with corrections to the Cover Date. 相似文献
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10.
Thioredoxin activation of phosphoribulokinase in a chloroplast multi-enzyme complex. 总被引:1,自引:0,他引:1
The activation process of spinach phosphoribulokinase by thioredoxin f has been studied with the enzyme in a free, isolated state, or integrated in a multi-enzyme complex. The time periods required for enzyme activation are always smaller and the maximal enzyme velocities are always greater when chloroplast phosphoribulokinase is included in the multi-enzyme complex than when it is in the isolated state. Comparative kinetic studies show that phosphoribulokinase extracted from the complex behaves exactly as in the isolated state. The reduced form of the kinase, whatever it has been included in the complex or isolated from the chloroplasts, are deactivated by oxidized thioredoxins. In the absence of thioredoxin f however, the reduced form of the isolated enzyme undergoes spontaneous oxidation whereas the reduced kinase included in the multi-enzyme complex is stable. 'Unspecific' proteins such as bovine serum albumin do not provide any protection of the kinase against autooxidation, whereas 'homologous' specific proteins such as ribulose-1,5-bisphosphate carboxylase/oxygenase dramatically decrease the rate of this autooxidation process. These results therefore support the view that interactions between phosphoribulokinase and the other components of the multi-enzyme complex play an important role in the modulation of the activity of this enzyme. The possible part of these interactions in the control of the Calvin cycle is discussed. 相似文献