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991.
Food Science and Biotechnology - Nineteen samples of Arabica and 14 of Robusta coming from various plantation were analysed by dynamic headspace capillary gas chromatography–mass spectrometry...  相似文献   
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In plant grana thylakoid membranes Photosystem II (PSII) associates with a variable number of antenna proteins (LHCII) to form different types of supercomplexes (PSII-LHCII), whose organization is dynamically adjusted in response to light cues, with the C2S2 more abundant in high-light and the C2S2M2 in low-light. Paired PSII-LHCII supercomplexes interacting at their stromal surface from adjacent thylakoid membranes were previously suggested to mediate grana stacking. Here, we present the cryo-electron microscopy maps of paired C2S2 and C2S2M2 supercomplexes isolated from pea plants grown in high-light and low-light, respectively. These maps show a different rotational offset between the two supercomplexes in the pair, responsible for modifying their reciprocal interaction and energetic connectivity. This evidence reveals a different way by which paired PSII-LHCII supercomplexes can mediate grana stacking at diverse irradiances. Electrostatic stromal interactions between LHCII trimers almost completely overlapping in the paired C2S2 can be the main determinant by which PSII-LHCII supercomplexes mediate grana stacking in plants grown in high-light, whereas the mutual interaction of stromal N-terminal loops of two facing Lhcb4 subunits in the paired C2S2M2 can fulfil this task in plants grown in low-light. The high-light induced accumulation of the Lhcb4.3 protein in PSII-LHCII supercomplexes has been previously reported. Our cryo-electron microscopy map at 3.8 Å resolution of the C2S2 supercomplex isolated from plants grown in high-light suggests the presence of the Lhcb4.3 protein revealing peculiar structural features of this high-light-specific antenna important for photoprotection.  相似文献   
995.
Alveolar macrophages are the first line of defence against detrimental inhaled stimuli. To date, no comparative data have been obtained on the inflammatory response induced by different carcinogenic mineral fibres in the three main macrophage phenotypes: M0 (non-activated), M1 (pro-inflammatory) and M2 (alternatively activated). To gain new insights into the different toxicity mechanisms of carcinogenic mineral fibres, the acute effects of fibrous erionite, crocidolite and chrysotile in the three phenotypes obtained by THP-1 monocyte differentiation were investigated. The three mineral fibres apparently act by different toxicity mechanisms. Crocidolite seems to exert its toxic effects mostly as a result of its biodurability, ROS and cytokine production and DNA damage. Chrysotile, due to its low biodurability, displays toxic effects related to the release of toxic metals and the production of ROS and cytokines. Other mechanisms are involved in explaining the toxicity of biodurable fibrous erionite, which induces lower ROS and toxic metal release but exhibits a cation-exchange capacity able to alter the intracellular homeostasis of important cations. Concerning the differences among the three macrophage phenotypes, similar behaviour in the production of pro-inflammatory mediators was observed. The M2 phenotype, although known as a cell type recruited to mitigate the inflammatory state, in the case of asbestos fibres and erionite, serves to support the process by supplying pro-inflammatory mediators.  相似文献   
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A new apparatus to measure the equilibrium solvent activity in a multiphase system containing a particulated polymer is presented. An experimental procedure to determine the monomer partitioning in typical emulsion copolymerization systems is developed; the method is devised in a way that no phase separation between water and swollen polymer particles is required in order to determine the monomer content in each phase. The analytical technique used is quantitative gas chromatography, either of the vapor or of the liquid phases. Different monomers (styrene, methyl methacrylate, and vinyl acetate) and polymeric matrices (polystyrene and methyl methacrylate–vinyl acetate copolymer) are examined both above and below saturation conditions (corresponding to intervals II and III of an emulsion polymerization process). The experimental results are compared with predictions of a literature model. © 1996 John Wiley & Sons, Inc.  相似文献   
998.
Monitoring the electrophysiology of living cells by micro/nano devices is a well-established technique in a large area of biomedical applications. The main fascination is the ability of these devices to perform, in real-time, non-invasive investigations of the physiological state of a cell population. In this work, we present a hybrid microsystem model to detect extracellular signals induced by cardiac cells (CDs). In particular, the bio-electronic junction established by interfacing cardiac cells to Carbon NanoTubes (CNTs) vertically grown on the surface of a metal microelectrode (MIC) was modeled to analyze the induced extracellular cell electrical activity. The simulation results strengthened the assumptions that CNTs, as electrical interfaces, enhance the amplitude and act on the shape of the recorded extracellular signals, compared to other microelectrode substrates.  相似文献   
999.
In this paper we propose a new method to detect the global scale of images with regular, near regular, or homogenous textures. We define texture “scale” as the size of the basic elements (texels or textons) that most frequently occur into the image. We study the distribution of the interest points into the image, at different scale, by using our Keypoint Density Maps (KDMs) tool. A “mode” vector is built computing the most frequent values (modes) of the KDMs, at different scales. We observed that the mode vector is quasi linear with the scale. The mode vector is properly subsampled, depending on the scale of observation, and compared with a linear model. Texture scale is estimated as the one which minimizes an error function between the related subsampled vector and the linear model. Results, compared with a state of the art method, are very encouraging.  相似文献   
1000.
Conjugated polymers (CPs) are promising materials for fluorescence imaging application. However, a significant problem in this field is the unexplained abnormally low fluorescence brightness (or number of fluorescence photons detected per one excitation photon) exhibited by most of CP single chains in solid polymer hosts. Here it is shown that this detrimental effect can be fully avoided for short chains of polyfluorene‐bis‐vinylphenylene (PFBV) embedded in a host polymer matrix of PMMA, if the conjugated backbone is insulated by cyclodextrin rings to form a polyrotaxane (PFBV‐Rtx). Fluorescence kinetics and quantum yields are measured for the polymers in liquid solutions, pristine films, and solid PMMA blends. The fluorescence brightness of PFBV‐Rtx single chains dispersed in a solid PMMA is very close to that expected for a chain with 100% fluorescence quantum yield, while the unprotected PFBV chains of the same length possess 4 times lower brightness. Despite this, the fluorescence decay kinetics are the same for both polymers, suggesting the presence of static or ultrafast fluorescence quenching in the unprotected polymer. About 80% of an unprotected PFBV chain is estimated to be completely quenched. The hypothesis is that the cyclodextrin rings prevent the quenching by working as ‘bumpers’ reducing the mechanical forces applied by the host polymer to the conjugated backbone and help retaining its conformational freedom. While providing a recipe for making CP fluorescence bright at the single‐molecule level, these results identify a lack of fundamental understanding in the community of the influence of the environment on excited states in conjugated materials.  相似文献   
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