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11.
Mice were injected three times a day for 12 days with 300 micrograms/kg body weight of gastrin G17 or 37.5 Ivy dog U/kg body weight of CCK or saline. Other mice were also injected four times an hr for 1 hr with 7.5 micrograms/kg of gastrin, nine Ivy dog U/kg of CCK or saline; 1 hr before killing, they were injected with tritiated thymidine to evaluate the labelling indices in peptic, antral, duodenal, jejunal, and ileal mucosae. Four hours after the first injection of the two peptides, the peptic labelling indices increased while those of intestinal mucosa increased 8 hr after these injections. Long-term injections of CCK had a trophic effect on secretory cells of the digestive tract: the number of gastric zymogenic cells, Paneth cells, and the mucous cells of Brünner glands were hypertrophied. The pepsin, amylase, chymotrypsin, and lysozyme activities increased in stomach, exocrine pancreas, and intestine, respectively. Neither parietal cells nor intestinal enterocytes and hydrolase activities were affected. The trophic effect of long-term injections of gastrin is confirmed on parietal cells and exocrine pancreatic parenchyma and is demonstrated in Paneth cells. Confirming cytological results, pancreatic lipase and amylase activities and intestinal lysozyme activity were increased after gastrin. Although CCK and gastrin have a structural analogy, these two peptides did not affect the same cellular types. A specific action of CCK on the main secretory cells of the digestive mucosa is demonstrated.  相似文献   
12.
The tetracycline resistance determinant in transposon Tn10 consists of two genes, the tetA resistance gene and the tetR repressor gene, that are transcribed from divergent overlapping promoters. We determined the levels of pulse-labeled tet messenger RNA in Escherichia coli strains with the Tn10 tet genes on a multicopy plasmid. Addition of the inducer 5a,6-anhydrotetracycline results in a 270- to 430-fold increase in tetA mRNA and a 35- to 65-fold increase in tetR mRNA. As judged by the relative molar amounts of tetA and tetR mRNA synthesized under maximally inducing conditions, the tetA promoter (tetPA) is 7 to 11 times more active than the two tetR promoters (tetPR1 and tetPR2) combined. We characterized ten mutations in tetPA, including nine single-base-pair substitutions and a 30-base-pair deletion. All of the single-base-pair changes reduce the agreement with the consensus sequence for promoters recognized by E. coli RNA polymerase. Mutations in highly conserved nucleotides result in a 200- to 600-fold reduction in tetPA activity in vivo. Unexpectedly, tetPA mutations reduce by two- to fourfold the combined activity in vivo of tetPR1 and tetPR2, in spite of their locations outside the -35 and -10 regions of tetPR1 and tetPR2. For two tetPA mutations, the negative effect on tetPR activity was also demonstrated in tetR- tetPR-lacZ operon fusion strains, thus eliminating the possibility that it is due to variations in either plasmid copy-number or induction efficiency. The pleiotropic effects of tetPA mutations are discussed in terms of the expectation that the overlapping tet promoters compete for RNA polymerase.  相似文献   
13.
H Bertrand  B S Chan  A J Griffiths 《Cell》1985,41(3):877-884
The kalilo variants of Neurospora contain a cytoplasmic genetic factor that causes senescence. This factor is a 9.0 kb transposable element (kalDNA) that lacks nucleotide sequence homology with mtDNA and is inserted into the mitochondrial chromosome, often at sites located within the open reading frame in the intron-DNA of the mitochondrial 25S-rRNA gene. Genomes containing the "foreign" DNA insert accumulate during growth, and death occurs as the cells become deficient in functional large and small subunits of mitochondrial ribosomes. The kalDNA transposon may be an "activator" element that causes breaks in mtDNA. Nonsenescing [+] strains of Neurospora do not contain kalDNA.  相似文献   
14.
Summary The crude oil was degraded (80%) in continuous culturing and non sterile conditions by a mixed bacteria community. The fermentation process relies on a step of pre-emulsification of the substrate before it is introduced into the reactor. The emulsification indispensable for degrading crude oil is performed by the mixed bacteria community during its growth on hydrocarbons. On the other hand, the use of an ultrafiltration device allows the obtention of high cell concentrations (7.6 g·l-1) and high degradation rates.  相似文献   
15.
Résumé Les cellules du tissu glandulaire du testicule et de la glande interrénale de pleurodèle montrent les caractères généralement observés dans les cellules stéroïdogènes. Des différences existent entre les deux tissus. Le reticulum endoplasmique du tissu glandulaire est très développé et présent dans toutes les cellules qui sont d'aspect homogène. Au contraire, le tissu interrénal montre deux aspects cellulaires différents. Le premier se caractérise par un reticulum endoplasmique lisse relativement peu développé par rapport au tissu glandulaire, par des mitochondries petites et nombreuses, enfin par des liposomes denses et petits. Le deuxième aspect au contraire, se distingue par le petit nombre de mitochondries souvent géantes et à crêtes plus fréquemment organisées en faisceaux, par des liposomes nombreux de grandes dimensions et peu denses aux électrons.Le tissu glandulaire est très peu touché par l'hypophysectomie. Le reticulum persiste plusieurs mois comme d'ailleurs l'activité 5-3 -hydroxystéroïde deshydrogénase. Dans le tissu interrénal, la proportion des cellules d'aspects différents varie au profit des cellules à lipides abondants et à grandes mitochondries. L'activité 5-3 -hydroxystéroïde deshydrogénase est longtemps décelable.Le rôle du reticulum endoplasmique du tissu glandulaire est discuté en fonction des observations réalisées dans d'autres cellules stéroïdogènes à reticulum abondant. La signification des deux aspects cellulaires observés dans l'interrénale est discutée en relation avec les résultats expérimentaux obtenus en particulier chez le rat.Cette étude révèle que les critères d'activité d'une cellule stéroïdogène sont délicats à établir et doivent être différents d'un tissu à l'autre.
Tissues secreting steroid hormones in urodele amphibians
Summary The fine structure of testis glandular tissue and interrenal gland cells of Pleurodeles shows the general features observed in other steroïdogenic cells. Certain differences exist between the two tissues. The agranular endoplasmic reticulum of the glandular tissue cells is well developed and present in all cells of similar appearance. On the contrary, the interrenal tissue cells show two different features. The first is characterised by a poorly developed smooth endoplasmic reticulum, compared with that of the glandular tissue, by small and numerous mitochondria, and finally by small electron dense lipid droplets. The second feature is the small number of mitochondria often giant and with fascicles of straight tubular cristae and numerous large lipid droplets of low electron density.The effect of hypophysectomy on the glandular tissue cells seem very slight. The endoplasmic reticulum and the 5-3 -hydroxysteroid dehydrogenase activity persists for several months. In the interrenal tissue, the proportions of the two different cellular features are modified. Cells rich in lipids and with large mitochondria are more abundant. It is possible to demonstrate a 5-3 -hydroxysteroid dehydrogenase activity for a long time after hypophysectomy. The functional significance of the agranular endoplasmic reticulum is discussed in relation to some other observations on different steroidogenic cells with a well developed agranular endoplasmic reticulum. The significance of the two cellular features observed in the interrenal gland is discussed in connection with experimental data obtained in the frog and the rat.This study shows that it is difficult to define criteria of cellular activity, which probably differ from one tissue to another.
Equipe de Recherche associée au C. N. R. S. Cytologie Ultrastructurale n 129.  相似文献   
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A simple, reliable method was developed for measuring brain acetylcholine (ACh) turnover using HPLC methodology. Mice were injected intravenously with [3H]choline ([3H]Ch), and the turnover rate of ACh was calculated from the formation of [3H]ACh. Ch and ACh were separated from phosphorylcholine and from other radioactive compounds using tetraphenylboron extraction and counterion/reverse-phase chromatography. Endogenous Ch and ACh were quantified electrochemically through hydrogen peroxide production in a postcolumn reactor containing covalently bonded ACh esterase and Ch oxidase. Labeled Ch and ACh were quantified in the same sample by collecting the chromatographic fractions for radioactive content determinations. The method is rapid, well adapted to large series, and highly reproducible, with recoveries of 72.1% for Ch and 79.3% for ACh. The turnover value in mouse cerebral hemispheres was 16.02 nmol g-1 min-1 and decreased to 9.94 nmol g-1 min-1 in mice treated with oxotremorine.  相似文献   
19.
In the photosystem I of thylakoid membranes, the photoinduced electron transfer involves three iron-sulfur centers, A, B, and X. Among them, center X is characterized by very unusual spectroscopic and redox properties. Recent arguments have been presented in favor of a [2Fe-2S] structure for the clusters implicated in this center, but the number of these clusters is still a controversial question. By using an original EPR method, based on the differences in the relaxation properties of A, B, and X, we have determined the stoichiometry for the iron-sulfur clusters in photosystem I. Our measurements indicate that center X is composed of a single iron-sulfur cluster per P700. The possible implications of this result for the polypeptide composition of the core reaction center are discussed.  相似文献   
20.
The gene encoding a putative G protein-coupled receptor (HG10) was cloned from human genomic DNA by low stringency PCR and found to be homologous to the recently described rat bradykinin B2 receptor. The receptor was expressed in xenopus oocytes and stably transfected CHO cell lines. Binding studies demonstrated that HG10 encodes a high affinity BK receptor with an apparent Kd of 150 pM. Displacement by BK agonists and antagonists allowed the characterization of the receptor as a B2 subtype. Functional coupling to the Ca(2+)-phosphatidylinositol cascade was demonstrated in transfected CHO cells where inositol phosphates accumulation and intracellular calcium concentration were elevated in response to BK stimulation. The agonistic and antagonistic properties of BK analogs do not match strictly the pharmacological profile described for the rat or guinea pig B2 receptor subtypes or the putative B3 subtype. This discrepancy is attributed either to species variability or to differences in the coupling efficiency of receptors to the transduction cascade in different cell types. From our results, the existence of B3 receptors and of B2 subtypes appears questionable.  相似文献   
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