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31.
Reiser, Peter J., William O. Kline, and Pal L. Vaghy.Induction of neuronal type nitric oxide synthase in skeletal muscle by chronic electrical stimulation in vivo. J. Appl. Physiol. 82(4): 1250-1255, 1997.Fast-twitch skeletal muscles contain more neuronal-type nitricoxide synthase (nNOS) than slow-twitch muscles because nNOS is presentonly in fast (type II) muscle fibers. Chronic in vivo electricalstimulation of tibialis anterior and extensor digitorum longus musclesof rabbits was used as a method of inducing fast-to-slow fiber typetransformation. We have studied whether an increase in musclecontractile activity induced by electrical stimulation alters nNOSexpression, and if so, whether the nNOS expression decreases to thelevels present in slow muscles. Changes in the expression of myosinheavy chain isoforms and maximum velocity of shortening of skinnedfibers indicated characteristic fast-to-slow fiber type transformationafter 3 wk of stimulation. At the same time, activity of NOS doubled inthe stimulated muscles, and this correlated with an increase in theexpression of nNOS shown by immunoblot analysis. These data suggestthat nNOS expression in skeletal muscle is regulated by muscle activityand that this regulation does not necessarily follow the fast-twitchand slow-twitch pattern during the dynamic phase of phenotypetransformation.

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32.
Chromatography of soluble polyphenols of p-fluorophenylalanine-sensitive and -resistant tobacco cells revealed that the 10-fold increased level found in the resistant line was largely due to the accumulation of two unidentified polyphenols. The uptake of Phe-[U-14C] and Tyr-[U-14C] by the resistant line was ca 10 % that by the sensitive line. About 90 % of the phenylalanine-[14C] which was taken up by both cell lines could be accounted for as free phenylalanine in protein, soluble polyphenols or CO2. The fate of Tyr-[14C] was similar to that of phenylalanine except that the incorporation was into insoluble polymeric forms of polyphenols rather than into soluble polyphenols. The resistant line incorporated 9-times more phenylalanine-[14C] into soluble polyphenols than did the sensitive line. The different 14C-aromatic amino acid accumulation and incorporation patterns noted with the two cell lines indicates that there are different active pools. Differential uptake rates by the two cell lines might affect the distribution of the absorbed amino acid among the different pools.  相似文献   
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34.
In dissociated cells from chick embryos or from chick limb buds, acetylcholine (ACh) induced an increase in cellular levels of inositol 1,4,5-trisphosphate (Ins-P3) and of inositol 1,3,4,5-tetrakisphosphate (Ins-P4). The concentration of Ins-P3 was enhanced transiently, whereas the level of Ins-P4 remained elevated for at least 20 min after addition of ACh. In most cases the increase in Ins-P4 levels was more pronounced than that of Ins-P3 levels. The inhibition of the ACh-induced inositol-phosphate response by atropine (half-maximal inhibition at 10 nM) indicates the involvement of muscarinic receptors, which in chick embryo cells induce a transient rise and a following persistent elevation of cytosolic Ca2+ activity (G. Oettling et al. (1989) J. Dev. Physiol. 12, 85-94). Adenosine 5'-triphosphate (ATP) elicited a similar transient rise in cytosolic Ca2+ activity, however, without a subsequent plateau. ATP also caused an increase in inositol-oligophosphate levels. Thus, both muscarinic and purinergic receptors in chick embryo cells are coupled to phospholipase C. The enzymatically formed Ins-P3 mediates the release of Ca2+ from internal stores. The Ca2+ signal could be involved in embryonic cell migration during morphogenesis.  相似文献   
35.
An intracellular aryl-alcohol dehydrogenase (previously referred to as aryl-aldehyde reductase) was purified from the white-rot fungus Phanerochaete chrysosporium. The enzyme reduced veratraldehyde to veratryl alcohol using NADPH as a cofactor. Other aromatic benzaldehydes were also reduced, but not aromatic ketones. Methoxy-substituted rings were better substrates than hydroxylated ones. The enzyme was also able to reduce a dimeric aldehyde (4-benzyloxy-3-methoxybenzaldehyde). The highest reduction rate was measured when 3,5-dimethoxybenzaldehyde was used as a substrate. On SDS/PAGE the purified enzyme showed one major band with a molecular mass of 47 kDa, whereas gel filtration suggested a molecular mass of 280 kDa. Polyclonal antibodies raised against the gel purified 47-kDa protein were able to immunoprecipitate the aryl-alcohol dehydrogenase indicating that its activity possibly resides entirely in this protein fragment. The pI of the enzyme was 5.2 and it was most active at pH 6.1. The aryl-alcohol dehydrogenase was partially inhibited by typical oxidoreductase inhibitors.  相似文献   
36.
Zusammenfassung Pnoepyga immaculata n. sp. lebt im Areal der beiden anderenPnoepyga-Artenalbiventer (Hodgson 1837) undpusilla Hodgson 1845 und wurde durch ihren markant abweichenden Territorialgesang entdeckt. Sie besitzt eine kurze silberhelle Strophe aus kurzen, in gleichmäßigen Abständen gereihten Pfiff-Elementen, die in der Frequenz leicht abfällt. Neben der Stimme liegen die wesentlichen diagnostischen Merkmale nach jetzigem Kenntnisstand gegenüber sympatrischenalbiventer in wenig größerem Schnabel, der Fleckenlosigkeit von Oberseite, Kopf und Flügeldecken, gegenüberpusilla in den größeren Körperabmessungen, gegenüber sympatrischenalbiventer undpusilla im schwachen grünlichen Schimmer der Oberseite und in der länglichen Schuppung der Unterseite. Es bestehen keine Proportionsunterschiede zwischenimmaculata undalbiventer/pusilla einerseits wie auch nicht zwischen diesen beiden andererseits. Bis jetzt wurden 4 Belegstücke (SammlungenKoelz, Diesselhorst, Martens) und eine durch Bandaufnahme gesicherte Beobachtung zwischen Dhaulagiri in Mittelwest-Nepal bis nahe der Ost-Grenze Nepals bekannt.P. immaculata lebt zur Brutzeit in enger Nachbarschaft mitP. albiventer undP. pusilla, ist jedoch vonalbiventer vertikal getrennt bei nachgewiesenem Kontakt, vonpusilla durch Bevorzugung trockeneren Waldunterwuchses abseits von Bächen. Schon jetzt mußimmaculata als gefährdete Art eingestuft werden, da Waldvegetation in der zur Brutzeit bevorzugten Höhenstufe zwischen 2100 und 3100 m in Nepal weitgehend vernichtet worden ist.
Pnoepyga immaculata n. sp., a new ground living wren-babbler from the Nepal Himalayas (Timaliidae)
Summary P. immaculata n. sp. was discovered by its voice which strongly differs from the two other sympatric species,albiventer (Hodgson 1837) andpusilla Hodgson 1845. As a territorial song, it displays a silvery strophe arranged of short, more or less regularly spaced whistling notes (fig. 7a–d), slightly descending in pitch. The strophe is about 2 s long. Besides the distinct voice, the essential diagnostic characters in comparison toP. albiventer are the slightly larger bill, plain head, upper side and wing coverts (fig. 1a–d, 2, 4a–d), in comparison topusilla the larger body size (fig. 1i–m), in comparison to sympatricalbiventer andpusilla the slightly olive tinge of the upper side (against warm dark brown in both others, fig. 1e–m), and the more longish scaly feathers of the lower side (against stout scaly appearance in both others, fig. 1 a–d). These characters hold true at least in Central and Eastern Himalayan populations of the respective species. There do not exist proportional differences in the relations of any part of the body betweenimmaculata andpusilla and not between the latter ones as well. Heretofore, 4 museum specimens are known (Koelz Coll.,Diesselhorst Coll.,Martens Coll.) from West-central (Thakkhola, type locality) and East Nepal (Ting Sang La), 3 of them from the presumed breeding grounds (2100–3100 m), one from the winter quarters in the Terai lowlands. A field observation close to the Darjeeling border in far East Nepal is verified by a tape-recording.P. immaculata embarasses the biologist and systematist because it lives in close neighbourhood of the similar speciesalbiventer andpusilla. It must have been overlooked by its apparent scarcity and overall similarity to both other species of the genus. Slight ecological differences rather correspond to the vertical distribution ofalbiventer, which populates a higher forest belt. But both have already been found on territory at close range.P. pusilla inhabits different microbiotopes, especially the close proximity of running water in the same altitudinal belt asimmaculata. When discovered,P. immaculata is to be classified already as an endangered species. Forest vegetation of its preferred altitude is already greatly reduced in the Central and Eastern Nepal Himalayas. To get a more detailed information on its general distribution and biology in order to quickly arrange protected areas and thus to guarantee the survival ofP. immaculata, should be the urgent next step.


Results of the Himalaya Expeditions ofJ. Martens, No. 163. — For No. 162 see: Stuttgarter Beitr. Naturkde. (A) 453: 1–46, 1990.  相似文献   
37.
Summary The effects of cholesterol loading and depletion and of a 10% replacement of native phosphatidylcholine by dipalmitoyl phosphatidylcholine (di 16:0-PC) on kinetic properties of human red cell Na–Li exchange have been studied.Compared to control erythrocytes (cholesterol/phospholipid ratio (C/P=0.8–0.9)),V max of phloretin-sensitive Li uptake and of Li efflux stimulated by extracellular Na (Na o ) were reduced by 15–30% in cholesterol-loaded red cells (C/P=1.05–1.33). The apparentK m values for external Li (Li o ) and for internal Li (Li i ) were decreased by about one-third in these cells. Cholesterol depletion (C/P=0.7) exerted opposite effects on the kinetics of Na o -dependent Li efflux. On augmentingC/P from 0.66 to 1.0,V max of Na o -dependent Li efflux was reduced by about 30%; increasingC/P above 1.0 caused no further lowering ofV max. Li leakage rates monotonically decreased over the whole range ofC/P ratios examined (0.66–1.3). This indicates that Na–Li exchange and Li leak are differentially affected by cholesterol.Incorporation of di 16:0-PC (replacement of 3% of total red cell phospholipids) caused similar kinetic alterations of Na–Li exchange as a rise in membrane cholesterol by 20–50%. Notably, selective incorporation of di 16:0-PC into the outer monolayer increased both intra- and extracellular Li binding affinities of Na–Li exchange and lowered its maximum velocity. Thus, both di 16:0-PC enrichment and cholesterol loading exerted an uncompetitive type of transport inhibition. The results are in agreement with the hypothesis that the kinetic alterations of red cell Na–Li exchange seen in a subgroup of essential hypertensive patients could be due to subtle changes in the molecular species composition of individual phospholipids.  相似文献   
38.
In order to elucidate the regulation of the levels of free choline in the brain, we investigated the influence of chronic and acute choline administration on choline levels in blood, CSF, and brain of the rat and on net movements of choline into and out of the brain as calculated from the arteriovenous differences of choline across the brain. Dietary choline supplementation led to an increase in plasma choline levels of 50% and to an increase in the net release of choline from the brain as compared to a matched group of animals which were kept on a standard diet and exhibited identical arterial plasma levels. Moreover, the choline concentration in the CSF and brain tissue was doubled. In the same rats, the injection of 60 mg/kg choline chloride did not lead to an additional increase of the brain choline levels, whereas in control animals choline injection caused a significant increase; however, this increase in no case surpassed the levels caused by chronic choline supplementation. The net uptake of choline after acute choline administration was strongly reduced in the high-choline group (from 418 to 158 nmol/g). Both diet groups metabolized the bulk (greater than 96%) of newly taken up choline rapidly. The results indicate that choline supplementation markedly attenuates the rise of free choline in the brain that is observed after acute choline administration. The rapid metabolic choline clearance was not reduced by dietary choline load. We conclude that the brain is protected from excess choline by rapid metabolism, as well as by adaptive, diet-induced changes of the net uptake and release of choline.  相似文献   
39.
Continuous superfusion of rat glioma cells with medium containing bradykinin (from 0.2 nM) induced a transient hyperpolarization followed by regular hyperpolarizing oscillations of the membrane potential. Similar repetitive hyperpolarizing oscillations were caused by extracellularly applied bradykinin or muscarine or by intracellularly injected GTP-gamma-S. The frequency of the oscillations was 1 per minute at bradykinin concentrations ranging from 0.2 nM to 2 microM, but the amplitude and duration increased with rising peptide concentration. The muscarine-induced oscillations were blocked by atropine. In the presence of extracellular Ca2+, the substances thapsigargin, 2,5-di(tert-butyl)-1,4-benzohydroquinone (tBuBHQ), and ionomycin reversibly suppressed the bradykinin-induced oscillations. Thapsigargin and tBuBHA, which are known to block the Ca2+ ATPase of endoplasmic reticulum, caused a transient rise in cytosolic Ca2+ activity, monitored with Fura-2, in suspensions of rat glioma cells or of mouse neuroblastoma-rat glioma hybrid cells. After a transient Ca2+ rise caused by thapsigargin, tBuBHQ, or ionomycin, the Ca2+ response to bradykinin which is known to be due to release of Ca2+ from internal stores was suppressed. This indicates that thapsigargin and tBuBHQ deplete internal Ca2+ stores as already seen previously for ionomycin. Thus, the inhibition of the membrane potential oscillations by thapsigargin, tBuBHQ, and ionomycin indicates that the oscillations are associated with activation of InsP3-sensitive Ca2+ stores. In some cells composite oscillation patterns which consisted of two independent oscillations with different amplitudes that overlapped additively were seen. We discuss that this pattern and the concentration dependency of the oscillations could be due to "quantal" Ca2+ release from stores with different inositol 1,4,5-triphosphate sensitivities. Subsidence of the oscillations after omission of extracellular Ca2+ seems to be due to a lack of replenishment of the intracellular stores with Ca2+, which comes from the extracellular compartment.  相似文献   
40.
Construction and properties of K1 type killer wine yeasts   总被引:3,自引:0,他引:3  
Summary With the use of a protoplast fusion technique the killer character of K1 type was transferred into four industrial Saccharomyces wine yeasts. The prototrophic yeast strains active against standard sensitive and K2 killer Saccharomyces strains, resistant to K1 killer toxin were constructed with no changes in technological properties.  相似文献   
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