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991.
Mannitol represents a major end product of photosynthesis in brown algae (Phaeophyceae), and is, with the β-1,3-glucan laminarin,
the main form of carbon storage for these organisms. Despite its importance, little is known about the genes and enzymes responsible
for the metabolism of mannitol in these seaweeds. Taking benefit of the sequencing of the Ectocarpus siliculosus genome, we focussed our attention on the first step of the synthesis of mannitol (reduction of the photo-assimilate fructose-6-phosphate),
catalysed by the mannitol-1-phosphate dehydrogenase (M1PDH). This activity was measured in algal extracts, and was shown to
be regulated by NaCl concentration in the reaction medium. Genomic analysis revealed the presence of three putative M1PDH
genes (named EsM1PHD1, EsM1PDH2 and EsM1PDH3). Sequence comparison with orthologs demonstrates the modular architecture of EsM1PHD1 and EsM1PDH2, with an additional N-terminal domain of unknown function. In addition, gene expression experiments carried out on samples
harvested through the diurnal cycle, and after several short-term saline and oxidative stress treatments, showed that EsM1PDH1 is the most highly expressed of these genes, whatever the conditions tested. In order to assess the activity of the corresponding
protein, this gene was expressed in Escherichia coli. Cell-free extracts prepared from bacteria containing EsM1PDH1 displayed higher M1PDH activity than bacteria transformed with an empty plasmid. Further characterisation of recombinant
EsM1PDH1 activity revealed its very narrow substrate specificity, salt regulation, and sensitivity towards an inhibitor of
SH-enzymes. 相似文献
992.
Brecknock S Dibbayawan TP Vesk M Vesk PA Faulkner C Barton DA Overall RL 《Planta》2011,234(4):749-758
Symplastic transport occurs between neighbouring plant cells through functionally and structurally dynamic channels called
plasmodesmata (PD). Relatively little is known about the composition of PD or the mechanisms that facilitate molecular transport
into neighbouring cells. While transmission electron microscopy (TEM) provides 2-dimensional information about the structural
components of PD, 3-dimensional information is difficult to extract from ultrathin sections. This study has exploited high-resolution
scanning electron microscopy (HRSEM) to reveal the 3-dimensional morphology of PD in the cell walls of algae, ferns and higher
plants. Varied patterns of PD were observed in the walls, ranging from uniformly distributed individual PD to discrete clusters.
Occasionally the thick walls of the giant alga Chara were fractured, revealing the surface morphology of PD within. External structures such as spokes, spirals and mesh were
observed surrounding the PD. Enzymatic digestions of cell wall components indicate that cellulose or pectin either compose
or stabilise the extracellular spokes. Occasionally, the PD were fractured open and desmotubule-like structures and other
particles were observed in their central regions. Our observations add weight to the argument that Chara PD contain desmotubules and are morphologically similar to higher plant PD. 相似文献
993.
994.
995.
The present study concerns three aspects of barley androgenesis: (1) the morphology and histology of the embryos during their
development, (2) the time course of fluorescent symplasmic tracers’ distribution, and (3) the correlation between symplasmic
communication and cell differentiation. The results indicate that barley embryos, which are developing via an androgenic pathway,
resemble their zygotic counterparts with respect to their developmental stages, morphology and histology. Analysis of the
distribution of the symplasmic tracers, HPTS, and uncaged fluorescein indicates the symplasmic isolation of (1) the protodermis
from the underlying cells of the late globular stage onwards, and (2) the embryonic organs at the mature stage of development. 相似文献
996.
Tarocystatin (CeCPI) from taro (Colocasia esculenta cv. Kaohsiung no. 1), a group-2 phytocystatin, shares a conserved N-terminal cystatin domain (NtD) with other phytocystatins but contains a C-terminal cystatin-like extension (CtE). The structure of the tarocystatin–papain complex and the domain interaction between NtD and CtE in tarocystatin have not been determined. We resolved the crystal structure of the phytocystatin–papain complex at resolution 2.03 Å. Surprisingly, the structure of the NtD–papain complex in a stoichiometry of 1:1 could be built, with no CtE observed. Only two remnant residues of CtE could be built in the structure of the CtE–papain complex. Therefore, CtE is easily digested by papain. To further characterize the interaction between NtD and CtE, three segments of tarocystatin, including the full-length (FL), NtD and CtE, were used to analyze the domain–domain interaction and the inhibition ability. The results from glutaraldehyde cross-linking and yeast two-hybrid assay indicated the existence of an intrinsic flexibility in the region linking NtD and CtE for most tarocystatin molecules. In the inhibition activity assay, the glutathione-S-transferase (GST)-fused FL showed the highest inhibition ability without residual peptidase activity, and GST-NtD and FL showed almost the same inhibition ability, which was higher than with NtD alone. On the basis of the structures, the linker flexibility and inhibition activity of tarocystatins, we propose that the overhangs from the cystatin domain may enhance the inhibition ability of the cystatin domain against papain. 相似文献
997.
SAC9 is a putative phosphoinositide phosphatase in Arabidopsis thaliana involved in phosphoinositide signaling. sac9-1 plants have a constitutively stressed phenotype with shorter roots which notably accumulate phosphatidylinositol 4,5-bisphosphate
and its hydrolysis product inositol trisphosphate. We investigated the primary roots of sac9-1 seedlings at the cytological and ultrastructural level to determine the structural basis for this altered growth. Despite
the normal appearance of organelles and cytoplasmic elements, our studies reveal extreme abnormalities of cell wall and membrane
structures in sac9-1 primary root cells, regardless of cell type, position within the meristematic area, and plane of section. Cell wall material
was deposited locally and in a range of abnormal shapes, sometimes completely fragmenting the cell. Simple protuberances,
broad flanges, diffuse patches, elaborate folds, irregular loops and other complex three-dimensional structures were found
to extend randomly from the pre-existing cell wall. Abundant vesicles and excessive membrane material were associated with
these irregular wall structures. We argue that a perturbed phosphoinositide metabolism most likely induces these observed
abnormalities and hypothesize that a disorganized cytoskeleton and excessive membrane trafficking mediate the cell wall defects. 相似文献
998.
Stromules are stroma-filled tubules that extend from the plastids in all multicellular plants examined to date. To facilitate
the visualisation of stromules on different plastid types in various tissues of bread wheat (Triticum aestivum L.), a chimeric gene construct encoding enhanced yellow fluorescent protein (EYFP) targeted to plastids with the transit
peptide of wheat granule-bound starch synthase I was introduced by Agrobacterium-mediated transformation. The gene construct
was under the control of the rice Actin1 promoter, and EYFP fluorescence was detected in plastids in all cell types throughout the transgenic plants. Stromules were
observed on all plastid types, although the stromule length and abundance varied markedly in different tissues. The longest
stromules (up to 40 μm) were observed in epidermal cells of leaves, whereas only short beak-like stromules were observed on
chloroplasts in mesophyll cells. Epidermal cells in leaves and roots contained the highest proportion of plastids with stromules,
and stromules were also abundant on amyloplasts in the endosperm tissue of developing seeds. The general features of stromule
morphology and distribution were similar to those shown previously for tobacco (Nicotiana tabacum L.) and arabidopsis (Arabidopsis thaliana (L.) Heynh.). 相似文献
999.
1000.
In single-celled spores of the fern Ceratopteris richardii, gravity directs polarity of development and induces a directional, trans-cellular calcium (Ca2+) current. To clarify how gravity polarizes this electrophysiological process, we measured the kinetics of the cellular response
to changes in the gravity vector, which we initially estimated using the self-referencing calcium microsensor. In order to
generate more precise and detailed data, we developed a silicon microfabricated sensor array which facilitated a lab-on-a-chip
approach to simultaneously measure calcium currents from multiple cells in real time. These experiments revealed that the
direction of the gravity-dependent polar calcium current is reversed in less than 25 s when the cells are inverted, and that
changes in the magnitude of the calcium current parallel rapidly changing g-forces during parabolic flight on the NASA C-9 aircraft. The data also revealed a hysteresis in the response of cells in
the transition from 2g to micro-g in comparison to cells in the micro-g to 2-g transition, a result consistent with a role for mechanosensitive ion channels in the gravity response. The calcium current
is suppressed by either nifedipine (calcium-channel blocker) or eosin yellow (plasma membrane calcium pump inhibitor). Nifedipine
disrupts gravity-directed cell polarity, but not spore germination. These results indicate that gravity perception in single
plant cells may be mediated by mechanosensitive calcium channels, an idea consistent with some previously proposed models
of plant gravity perception. 相似文献