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1.
针对目前大多数人脸识别算法参数多、计算量大,难以部署到移动端和嵌入式设备中的问题,提出了一种基于改进MobileFaceNet的人脸识别方法。通过对MobileFaceNet模型结构的调整,将bottleneck模块优化为sandglass模块,改良深度卷积和逐点卷积的相对位置,适当增大sandglass模块的输出通道数,从而减少特征压缩时的信息丢失,增强人脸空间特征的提取。实验结果表明:改进后的方法在LFW测试数据集上准确率达99.15%,模型大小和计算量分别仅为原算法的61%和45%,验证了所提方法的有效性。  相似文献   
2.
高面板坝的变形对面板的安全运行有着特别重要的影响,国内外已建的高面板坝工程中,因坝体变形大导致防渗面板挤压破损,坝体渗漏量大的实例较多,不得不降低水库水位进行修复处理,造成较大的经济损失乃至给大坝的长期运行留下安全隐患。通过发生挤压破损的实例分析,发现变形控制缺乏系统性是发生面板挤压破损的主要因素,为预防面板破损,系统提出了“控制坝体总变形,转化有害变形,适应纵向变形”的坝体变形控制方法,并在使用软硬岩混合料筑坝的董箐面板堆石坝中得到的应用,取得了良好效果,该工程运行至今达十余年,未见面板有挤压破损迹象,该方法对建设200 m以上乃至300 m级超高面板坝具有重要借鉴意义。  相似文献   
3.
现代战场中的无线通信设备日益增多,精准获取个体信息已成为研究热点,但也是难点。针对通信电台,提出了一种分选识别技术。该技术从电台物理层特性出发,对其辐射信号的细微特征进行K-means聚类以实现分选,分选的同时提取各个个体的特征属性值,未知信号通过与特征属性值相关运算实现个体识别。该技术无需先验知识,无需训练运算,通过实验验证,其可行、高效,易于工程实现。  相似文献   
4.
The International Olive Council(IOC) is an international intergovernmental organization dedicated to olive oil and table olives, aiming at modernizing olive production, coordinating olive policies, improving the regulation of international trade, defending the quality of the olive sector and promoting olive oil and table olives to increase their consumption. The IOC grants recognition of laboratories and tasting panels in annual trials when they meet the conditions given in the decisions adopting the IOC certificate for laboratories for the physico–chemical testing of olive oil and laboratories for the sensory analysis of virgin olive oils. The IOC establishes analysis methods applying to olive oils and olive pomace oils for purity, quality and organoleptic assessment. The IOC elaborates guides of storage conditions for olive oils and olive pomace oils, of managing virgin olive oil tasting panels and of sensory testing laboratories. In future works, the IOC includes activities to identify analytical criteria for detecting fraud and guaranteeing the quality of olive oils and olive pomace oils.  相似文献   
5.
高效率地使用工程车辆是工程项目管理中节约成本的有效方法,无人监管环境下工程车辆的工况识别,是实现工程车辆高效率使用的有效手段。目前以GPS等技术为核心的车辆智能管理系统未对工程车辆进行工况识别,提出一种基于GRU循环神经网络的工程车辆工况识别方法,通过对工程车辆在不同工况下产生的音频信号进行分析,从中提取Mel倒谱系数作为主要特征,构建GRU循环神经网络模型进行训练和识别。实验结果表明,该方法可以实现对工程车辆工况的有效识别。  相似文献   
6.
《Ceramics International》2022,48(3):3495-3503
The photochromic phenomenon has been recently used as a fascinating technology in the development of highly efficient anti-counterfeiting materials with dual-mode security encoding of concurrent photochromism and fluorescence emission. Herein, we successfully developed lanthanide-doped aluminate nanoparticles (LAN)/polystyrene (PS) electrospun nanofibers as novel secure authentication films. Different ratios of lanthanide-doped aluminate nanoparticles were mixed with polystyrene-based copolymer solutions in N,N-dimethylformamide (DMF) and subjected to electrospinning to afford photochromic and fluorescent nanofibers. The generated electrospun nanofibers demonstrated a narrow diameter distribution, a smooth surface and well-defined morphological properties. The produced smart nanofibers were applied onto cellulose paper sheets to demonstrate a dual-mode secure strategy with a simple and rapid authentication. LAN was prepared in the nano-scale for better dispersion in PS, which guarantee the formation of transparent films. LAN was studied by transmission electron microscope (TEM) and X-ray diffraction (XRD). LAN displayed diameters of 5–12 nm. On the other hand, the fibrous diameters of LAN-PS samples were studied by scanning electron microscopy (SEM) to indicate diameters of 200–300 nm. The induced security marking was invisible (363 nm) under visible daylight turning into visible green (520 nm) color under ultraviolet irradiation demonstrating a bathochromic shift. Both excitation and emission displayed high intensities. The security marking was fully reversible under ultraviolet/visible irradiation cycles without fatigue. Those advantageous properties could be attributed to the high surface area of the chromogenic nanofibrous films to result in high absorption of light leading to strong optical dual-mode photo-responsiveness. The generated LAN-PS hybrid films showed improved hydrophobic properties with increasing LAN. The nanofibers showed transparency, stretchability and flexibility. The present strategy can be reported as an efficient technology to develop many anti-counterfeiting products toward a better market with social and economic values to avoid fake products.  相似文献   
7.
In present work, the development of macroporous monolithic layers bearing the artificial recognition sites toward L-phenylalanine has been carried out. The set of macroporous poly(2-aminoethyl methacrylate-co-2-hydroxyethyl methacrylate-co-ethylene glycol dimethacrylate) materials with average pore size ranged in 340–1200 nm was synthesized. The applicability of Hildebrand's and Hansen's theories for the prediction of polymer compatibility with porogenic solvents was evaluated. The dependences of average pore size on theoretically calculated parameters were plotted. The linear trend detected for Hansen's theory has indicated the high suitability of this approach to select appropriate porogens. The synthesized monolithic MIP layers were tested toward the ability to rebind phenylalanine-derivative in microarray format. The influence of such factors as average pore size of the material, the concentration of template molecule in polymerization mixture, interaction time of analyte with its imprinted sites on binding efficiency were studied. The developed materials demonstrated good analyte rebinding from buffer solution with recognition factors 2.5–3.4 depending on the MIP sample. The comparable rebinding efficiency was also detected when the analysis was carried using complex biological media. The selectivity of phenylalanine binding from the equimolar mixture of structural analogues was 81.9% for free amino acid and 91.2% for labeled one.  相似文献   
8.
Redox (reduction–oxidation) reactions control many important biological processes in all organisms, both prokaryotes and eukaryotes. This reaction is usually accomplished by canonical disulphide-based pathways involving a donor enzyme that reduces the oxidised cysteine residues of a target protein, resulting in the cleavage of its disulphide bonds. Focusing on human vitamin K epoxide reductase (hVKORC1) as a target and on four redoxins (protein disulphide isomerase (PDI), endoplasmic reticulum oxidoreductase (ERp18), thioredoxin-related transmembrane protein 1 (Tmx1) and thioredoxin-related transmembrane protein 4 (Tmx4)) as the most probable reducers of VKORC1, a comparative in-silico analysis that concentrates on the similarity and divergence of redoxins in their sequence, secondary and tertiary structure, dynamics, intraprotein interactions and composition of the surface exposed to the target is provided. Similarly, hVKORC1 is analysed in its native state, where two pairs of cysteine residues are covalently linked, forming two disulphide bridges, as a target for Trx-fold proteins. Such analysis is used to derive the putative recognition/binding sites on each isolated protein, and PDI is suggested as the most probable hVKORC1 partner. By probing the alternative orientation of PDI with respect to hVKORC1, the functionally related noncovalent complex formed by hVKORC1 and PDI was found, which is proposed to be a first precursor to probe thiol–disulphide exchange reactions between PDI and hVKORC1.  相似文献   
9.
10.
β-Glucan is widely distributed in various plants and microorganisms and is composed of β-1,3-linked d-glucose units. It may have a branched short or long side chain of glucose units with β-1,6- or β-1,4-linkage. Numerous studies have investigated different β-glucans and revealed their bioactivities. To understand the structure-function relationship of β-glucan, we constructed a split-luciferase complementation assay for the structural analysis of long-chain β-1,6-branched β-1,3-glucan. The N- and C-terminal fragments of luciferase from deep-sea shrimp were fused to insect-derived β-1,3-glucan recognition protein and fungal endo-β-1,6-glucanase (Neg1)-derived β-1,6-glucan recognition protein, respectively. In this approach, two β-glucan recognition proteins bound to β-glucan molecules come into close proximity, resulting in the assembly of the full-length reporter enzyme and induction of transient luciferase activity, indicative of the structure of β-glucan. To test the applicability of this assay, β-glucan and two β-glucan recognition proteins were mixed, resulting in an increase in the luminescence intensity in a β-1,3-glucan with a long polymer of β-1,6-glucan in a dose-dependent manner. This simple test also allows the monitoring of real-time changes in the side chain structure and serves as a convenient method to distinguish between β-1,3-glucan and long-chain β-1,6-branched β-1,3-glucan in various soluble and insoluble β-glucans.  相似文献   
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