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981.
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983.
The complete mitochondrial genome sequences were determined for two species of human hookworms, Ancylostoma duodenale (13,721 bp) and Necator americanus (13,604 bp). The circular hookworm genomes are amongst the smallest reported to date for any metazoan organism. Their relatively small size relates mainly to a reduced length in the AT-rich region. Both hookworm genomes encode 12 protein, two ribosomal RNA and 22 transfer RNA genes, but lack the ATP synthetase subunit 8 gene, which is consistent with three other species of Secernentea studied to date. All genes are transcribed in the same direction and have a nucleotide composition high in A and T, but low in G and C. The AT bias had a significant effect on both the codon usage pattern and amino acid composition of proteins. For both hookworm species, genes were arranged in the same order as for Caenorhabditis elegans, except for the presence of a non-coding region between genes nad3 and nad5. In A. duodenale, this non-coding region is predicted to form a stem-and-loop structure which is not present in N. americanus. The mitochondrial genome structure for both hookworms differs from Ascaris suum only in the location of the AT-rich region, whereas there are substantial differences when compared with Onchocerca volvulus, including four gene or gene-block translocations and the positions of some transfer RNA genes and the AT-rich region. Based on genome organisation and amino acid sequence identity, A. duodenale and N. americanus were more closely related to C. elegans than to A. suum or O. volvulus (all secernentean nematodes), consistent with a previous phylogenetic study using ribosomal DNA sequence data. Determination of the complete mitochondrial genome sequences for two human hookworms (the first members of the order Strongylida ever sequenced) provides a foundation for studying the systematics, population genetics and ecology of these and other nematodes of socio-economic importance. 相似文献
984.
Lakes N-1 and N-2 at the Arctic Long Term Ecological Research site at Toolik Lake, Alaska, U.S.A. were fertilized with nitrogen and phosphorus for 5 and 6 years, respectively. The response and recovery of the microplankton community (protozoans, rotifers and crustacean nauplii) differed in the two lakes. Microplankton biomass in Lake N-1 increased five-fold while that in Lake-N-2 only doubled, despite larger nutrient additions to N-2. Microplankton community structure in Lake N-1 shifted toward dominance by few taxa, while the community in Lake N-2 maintained diversity. Finally, the recovery of Lake N-1 to near prefertilization microplankton biomass levels was rapid, while Lake N-2 showed at least a 1-year lag in recovery. These differences appear to be related to differences in the structure of lake sediments. 相似文献
985.
Richard L. Johnson Paul C. Johnson Tim L. Johnson Neil R. Thomson Andrea Leeson 《Bioremediation Journal》2001,5(4):299-320
Groundwater pressure measurements during startup and shutdown of in situ air sparging (IAS) systems are used to diagnose air flow behavior below the water table. The magnitude of the pressure response provides insight into the permeability of the zone into which the air is flowing. The duration of elevated pressures during startup and reduced pressures during shutdown indicate the extent to which air is being trapped below the water table by lower-permeability layers. The pressure measurements can be easily and quickly repeated and as a result are useful for both pilot tests and for optimizing operating conditions of existing IAS systems. Whether used alone or in conjunction with other diagnostic tools, pressure measurements are an important tool for assessing IAS performance. 相似文献
986.
Dayle E. Saar Neil O. Polans Paul D. Sørensen Melvin R. Duvall 《Plant Molecular Biology Reporter》2001,19(3):249-260
PCR primers with broad applicability are useful in many molecular-based studies; however, their universality can compromise
results when DNA contaminants also are amplified. Eighty-one templates ofDahlia (Asteraceae), primarily extracted from native Mexican populations, were tested for the presence of fungal contaminants; out
of these, almost 1 in 7 templates (13.6%) was contaminated. In a second survey across 12 angiosperm families using material
collected in Illinois, fungal DNA contaminated over 60% of the templates analyzed. Endophytic fungi often are symptomless
symbionts living within the above-ground tissues of their angiosperm hosts and are not affected by surface sterilization techniques.
Recent studies have revealed their widespread occurrence and broad host range. We also present field strategies for obtaining
plant material to reduce the possibility of collecting infected leaves and a simple screening test for detecting fungal DNA
in angiosperm templates. 相似文献
987.
Julien O Chatterjee S Bjorndahl TC Sweeting B Acharya S Semenchenko V Chakrabartty A Pai EF Wishart DS Sykes BD Cashman NR 《Biochemistry》2011,50(35):7536-7545
The residue-specific urea-induced unfolding patterns of recombinant prion proteins from different species (bovine, rabbit, mouse, and Syrian hamster) were monitored using high-resolution (1)H nuclear magnetic resonance (NMR) spectroscopy. Protein constructs of different lengths, and with and without a His tag attached at the N-terminus, were studied. The various species showed different overall sensitivities toward urea denaturation with stabilities in the following order: hamster ≤ mouse < rabbit < bovine protein. This order is in agreement with recent circular dichroism (CD) spectroscopic measurements for several species [Khan, M. Q. (2010) Proc. Natl. Acad. Sci. U.S.A.107, 19808-19813] and for the bovine protein presented herein. The [urea](1/2) values determined by CD spectroscopy parallel those of the most stable residues observed by NMR spectroscopy. Neither the longer constructs containing an additional hydrophobic region nor the His tag influenced the stability of the structured domain of the constructs studied. The effect of the S174N mutation in rabbit PrP(C) was also investigated. The rank order of the regional stabilities within each protein remained the same for all species. In particular, the residues in the β-sheet region in all four species were more sensitive to urea-induced unfolding than residues in the α2 and α3 helical regions. These observations indicate that the regional specific unfolding pattern is the same for the four mammalian prion proteins studied but militate against the idea that PrP(Sc) formation is linked with the global stability of PrP(C). 相似文献
988.
Everett KL Buehler A Bunney TD Margineanu A Baxendale RW Vatter P Retlich M Walliser C Manning HB Neil MA Dunsby C French PM Gierschik P Katan M 《Molecular and cellular biology》2011,31(6):1240-1251
We performed analyses of the molecular mechanisms involved in the regulation of phospholipase Cγ2 (PLCγ2). We identified several regions in the PLCγ-specific array, γSA, that contribute to autoinhibition in the basal state by occlusion of the catalytic domain. While the activation of PLCγ2 by Rac2 requires stable translocation to the membrane, the removal of the domains required for membrane translocation in the context of an enzyme with impaired autoinhibition generated constitutive, highly active PLC in cells. We further tested the possibility that the interaction of PLCγ2 with its activator protein Rac2 was sufficient for activation through the release of autoinhibition. However, we found that Rac2 binding in the absence of lipid surfaces was not able to activate PLCγ2. Together with other observations, these data suggest that an important consequence of Rac2 binding and translocation to the membrane is that membrane proximity, on its own or together with Rac2, has a role in the release of autoinhibition, resulting in interfacial activation. 相似文献
989.
Diane C. Saunders Marcela Brissova Neil Phillips Shristi Shrestha John T. Walker Radhika Aramandla Greg Poffenberger David K. Flaherty Kevin P. Weller Julie Pelletier Tracy Cooper Matt T. Goff John Virostko Alena Shostak E. Danielle Dean Dale L. Greiner Leonard D. Shultz Nripesh Prasad Alvin C. Powers 《Cell metabolism》2019,29(3):745-754.e4
990.