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991.
Four farms that group-housed sows from 2 weeks of lactation until weaning (G-farms) and 3 farms that kept the sows individually penned throughout the 5 to 6-week-long lactation period (C-farms), were compared in terms of sow health. All sows were crossbred Swedish Yorkshire × Swedish Landrace. The daily food ration was similar on all farms except during the group-housing period, when G-farm sows were fed ad libitum. Sows were grouped in the breeding section and kept grouped on deep litter in the dry sow section on all farms. Individual health examinations were performed at the time of weaning (±4 days) on 179 G-farm sows and on 167 C-farm sows. Teat- and udder skin wounds occurred less frequently (p<0.001) in G-farm sows than in C-farm sows. In addition, preweaning atrophy of all mammary glands occurred in 6.6% of the G-farm-sows but not in a single C-farm sow (p<0.001). This indicates that sow-piglet interactions decrease when sows are group housed. However, these differences did not occur in primiparous sows, suggesting that the relation between the primiparous sow and her litter is not affected. Mastitis frequency was the same in the 2 systems. Moreover, the frequency of locomotor disorders was the same in the 2 groups, and hoof overgrowth was common in both systems. These similarities could be due to the fact that all farms group housed dry sows on deep litter. A strong relation (p<0.001) between hoof overgrowth and locomotor disorders was evident. Low access to food due to low rank among primiparous group-housed sows was indicated by a lower (p<0.05) backfat thickness compared with multiparous sows, and a higher (p<0.001) frequency of skin wounds compared with individually housed primiparous sows.  相似文献   
992.
Summary Brugmansia candida hairy roots, obtained by infection withAgrobacterium rhizogenes LBA 9402, exhibit, after subculturing in liquid media, a tendency towards dedifferentiation. It has been found that the following strategies can be applied to inhibit this dedifferentiation and preserve normal root morphology: (a) lowering both the mineral and sucrose concentration in the media employed so as to diminish osmotic stress (a condition to which these roots appear to be particularly susceptible); (b) employing antiauxins in appropriate concentrations; and (c) maintaining the hairy roots on solid media prior to use in production processes in liquid media. The first strategy suggested does not favor alkaloid productivity, but in this case a two-step method could be attempted: biomass with normal root morphology could be obtained in a first stage using low sucrose concentrations, and in a second stage, sucrose could be increased in order to achieve higher productivity. In all the clones ofB. candida obtained, alkaloid production was biased towards scopolamine.  相似文献   
993.
Northern blot hybridizations with a probe complementary to a 275-nt circular RNA isolated from carnation plants revealed that this RNA co-exists in vivo with minor amounts of other small circular RNAs. Sequencing of cDNA clones of nine RNA species demonstrated deletions and duplications of the predominant 275-nt RNA. Minor sequence heterogeneities were observed at the crossover sites. Deletions mapped to three arms of the cruciform structure of lowest free energy obtained previously for the parental 275-nt RNA, whereas repeats encompassed mostly regions of the arm where deletions were not found. Some of the deleted and duplicated regions corresponded to sequences forming part of the two hammerhead structures involved in the in vitro self-cleavage of the plus and minus strands of the 275-nt RNA. A copy choice model is proposed for the emergence of deletions and duplications, where the RNA polymerase with the nascent strand dissociates from the template at regions rich in secondary and possibly tertiary structures, and reinitiates synthesis at different upstream and downstream positions.  相似文献   
994.
A Bacillus subtilis mutant spnA95 was isolated as resistant at 30 degrees C to the protein kinase C (PKC) inhibitor, sphinganine, and temperature sensitive for growth. As deduced by flow cytometry measurements, the mutant has a 35% reduced initiation mass at permissive temperature, resulting in initiation of DNA replication much earlier in the cell cycle than in the wild type. This modification is accompanied by a change in cell size, as determined by phase-contrast microscopy and flow cytometry. Therefore, this strain displays the characteristics of a novel cell clock mutant. spnA is a newly identified gene in B.subtilis and was shown to encode a cysteinyl-tRNA synthetase. At non-permissive temperature, the mutant was defective in the synthesis of P70, a protein with several characteristics of PKC (a cysteine-rich protein). As one possibility, we propose that the altered timing of replication may be due to the reduced synthesis of specific cysteine-rich proteins normally involved in controlling chromosomal replication initiation in B. subtilis.  相似文献   
995.
996.
Structure and function of the b/HLH/Z domain of USF.   总被引:32,自引:5,他引:27       下载免费PDF全文
  相似文献   
997.
Genomic polymorphism in the T-even bacteriophages.   总被引:11,自引:0,他引:11       下载免费PDF全文
F Repoila  F Tétart  J Y Bouet    H M Krisch 《The EMBO journal》1994,13(17):4181-4192
We have compared the genomes of 49 bacteriophages related to T4. PCR analysis of six chromosomal regions reveals two types of local sequence variation. In four loci, we found only two alternative configurations in all the genomes that could be analyzed. In contrast, two highly polymorphic loci exhibit variations in the number, the order and the identity of the sequences present. In phage T4, both highly polymorphic loci encode internal proteins (IPs) that are encapsidated in the phage particle and injected with the viral DNA. Among the various T4-related phages, 10 different ORFs have been identified in the IP loci; their amino acid sequences have the characteristics of internal proteins. At the beginning of each of these coding sequences is a highly conserved 11 amino acid leader motif. In addition, both 5' and 3' to most of these ORFs, there is a approximately 70 bp sequence that contains a T4 early promoter sequence with an overlapping inversely repeated sequence. The homologies within these flanking sequences may mediate the recombinational shuffling of the IP sequences within the locus. A role for the new IP-like sequences in determining the phage host range is proposed since such a role has been previously demonstrated for the IP1 gene of T4.  相似文献   
998.
F Ventura  J Doody  F Liu  J L Wrana    J Massagué 《The EMBO journal》1994,13(23):5581-5589
Transforming growth factor-beta (TGF-beta) signals by contacting two distantly related transmembrane serine/threonine kinases called receptors I (T beta R-I) and II (T beta R-II). TGF-beta binds to T beta R-II, which is a constitutively active kinase and this complex recruits T beta R-I, causing its phosphorylation and signal propagation to downstream substrates. The biochemical properties of this interaction were analyzed with reconstituted receptor systems. T beta R-I and T beta R-II baculovirally expressed at high levels in insect cells have the ligand binding properties of receptors expressed in mammalian cells, and form a complex in which T beta R-I phosphorylation is dependent on the kinase activity of T beta R-II. Furthermore, T beta R-I and T beta R-II can form a complex in vitro, and their cytoplasmic domains can specifically interact in a yeast two-hybrid system. In vitro complex formation with catalytically active T beta R-II is necessary and sufficient for T beta R-I phosphorylation, which within this complex does not require the catalytic activity of T beta R-I, thus mimicking T beta R-I phosphorylation in intact cells. In addition, T beta R-I phosphorylated in vitro remains associated with T beta R-II. These results suggest that T beta R-I and T beta R-II have affinity for each other, however, the ligand is required for stable complex formation under physiological conditions. Once formed, this complex is sufficient for T beta R-I phosphorylation by T beta R-II.  相似文献   
999.
1000.
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