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31.
杜康宁 《中国脊柱脊髓杂志》1988,(4)
本文讨论用“包络一轨迹”法设计的修正齿形链的传动特性,并提出了完善齿形修正设计的方法,基本上实现消除链传动申的“多边形效应”。 相似文献
32.
33.
Preparation and characterization of porous beta-tricalcium phosphate/collagen composites with an integrated structure 总被引:11,自引:0,他引:11
Porous beta-tricalcium phosphate (TCP)/collagen composites with different beta-TCP/collagen weight ratio were prepared. The influences of the preparation conditions on the microstructure of porous composite and the joint status of beta-TCP particles with collagen fibrils were characterized by X-ray diffractometer, scanning electron microscopy and transmission electron microscopy. The results showed: (1) an acid treatment could effectively disassemble collagen fibrils; (2) in the resulting porous composites, beta-TCP particles homogenously existed on the skeleton of the collagen fibril network and bonded tightly to both the fibrils and themselves. The tight bonding formation could be due to the reaction between Ca ions in the particles and carboxyl groups in collagen polypeptide chains and due to the reprecipitation of partially dissolved beta-TCP during synthesis. The tight bonding between beta-TCP particles and collagen fibrils in the composites demonstrated an integrated structure, which was reproducible when beta-TCP/collagen ratio ranged from 2 to 4. Such integrated structure would make significant contributions in reliably tailoring properties of the porous composites by varying beta-TCP content. In addition, the porous composites had large porosity (approximately 95%) and appropriate pore size (approximately 100 microm), showed no negative impact in cytotoxicity assay and complete bone tissue regeneration after 12 weeks in animal test. 相似文献
34.
Alpha-smooth muscle actin as a marker for soft tissue tumours: a comparison with desmin 总被引:1,自引:0,他引:1
The immunoreactivity of a range of vascular and non-vascular smooth muscle tumours, rhabdomyosarcomas, and non-myoid lesions has been examined with the use of a monoclonal antibody to smooth muscle-specific actin and the muscle intermediate filament, desmin. In all cases of smooth muscle-derived tumours, the alpha-actin antibody yielded superior results. Staining of the myofibroblasts of fibromatoses was also seen. In contrast to desmin, immunoreactivity was not exhibited by rhabdomyosarcomas. We propose that this monoclonal antibody to alpha-smooth muscle actin is a useful addition to the panel of reagents used for the characterization of soft tissue proliferations and tumours. The technical aspects of the application of this monoclonal antibody to immunohistochemistry are discussed. 相似文献
35.
A novel active L1 retrotransposon subfamily in the mouse 总被引:8,自引:1,他引:8
Unlike human L1 retrotransposons, the 5' UTR of mouse L1 elements contains tandem repeats of approximately 200 bp in length called monomers. Multiple L1 subfamilies exist in the mouse which are distinguished by their monomer sequences. We previously described a young subfamily, called the T(F) subfamily, which contains approximately 1800 active elements among its 3000 full-length members. Here we characterize a novel subfamily of mouse L1 elements, G(F), which has unique monomer sequence and unusual patterns of monomer organization. A majority of these G(F) elements also have a unique length polymorphism in ORF1. Polymorphism analysis of G(F) elements in various mouse subspecies and laboratory strains revealed that, like T(F), the G(F) subfamily is young and expanding. About 1500 full-length G(F) elements exist in the diploid mouse genome and, based on the results of a cell culture assay, approximately 400 G(F) elements are potentially capable of retrotransposition. We also tested 14 A-type subfamily elements in the assay and estimate that about 900 active A elements may be present in the mouse genome. Thus, it is now known that there are three large active subfamilies of mouse L1s; T(F), A, and G(F), and that in total approximately 3000 full-length elements are potentially capable of active retrotransposition. This number is in great excess to the number of L1 elements thought to be active in the human genome. 相似文献
36.
酵母双杂合系统AD端阴离子交换蛋白C-末端表达质粒的构建 总被引:2,自引:0,他引:2
利用PCR方法,从阴离子交换蛋白1(AE1)全长cDNA中扩增出约350bp c末端cDNA片段,测序后将其克隆至pGADT7载体上,用醋酸锂法构建好的pADT7-AE1-c末端转染酵母菌HA109,观察其在选择性培养基上的表达情况。结果表明,获得了530bp AE1c-末端cDNA,pGADT7-AE1-c末端对酵母无毒性,不能激活检测基因,可作为酵母双杂合系统中的靶基因。 相似文献
37.
Slobodan Jarić Dušan Ristanović Daniel M. Corcos 《European journal of applied physiology》1989,59(5):370-376
Summary Kinematic variables of the vertical jump (jumping height, jump phase durations and joint angles) were measured on 39 male
physical education students. In addition, kinetic parameters of the hip and knee extensors, and of the plantar flexors (maxima
voluntary force and its rate of development) were recorded on the same subjects, in isometric conditions. The results demonstrated
significant positive correlations between kinetic parameters of the active muscle groups and jumping height (r=0.217−0.464). The dominant effect on these correlations was due to the knee extensors. Correlations between these parameters
and the duration of the jump phases were much weaker. Correlation coefficients between kinetic parameters and limb angles
in the lowest body position showed that fast force production in one muscle group was related to a significant decrease in
the joint angles of distant body segments. Multiple correlation coefficients between leg extensor parameters and kinematic
variables (ranging between 0.256 for the duration of the counter-movement phase and 0.616 for jump height) suggested that
kinetic parameters could explain more than a quarter of the variability of this complex human movement. Therefore, the conclusion
was drawn that an extended set of measurements of the relevant musculo-skeletal system parameters could predict a considerable
amount of the variability of human movement. However, high correlation coefficients between the same kinetic parameters of
different muscle groups suggest that not all active muscle groups have to be included in the measurements. 相似文献
38.
Zebrafish SmyD1 is a SET and MYND domain-containing protein that plays an important role in myofiber maturation and muscle contraction. SmyD1 is required for myofibril organization and sarcomere assembly during myofiber maturation. Whole-mount in situ hybridization revealed that smyd1 mRNAs are specifically expressed in skeletal and cardiac muscles in zebrafish embryos. However, it is unknown if smyd1 is expressed in other striated muscles, such as cranial and fin muscles, and moreover, the regulatory elements required for its muscle-specific expression. We report here the analyses of smyd1 expression using smyd1-gfp transgenic zebrafish. smyd1-gfp transgenic zebrafish were generated using the 5.3-kb smyd1 promoter and its 5'-flanking sequence. GFP expression was found in the skeletal and cardiac muscles of smyd1-gfp transgenic embryos. GFP expression appeared stronger in slow muscles than fast muscles in transgenic zebrafish larvae. In addition, GFP expression was also detected in cranial and fin muscles of smyd1-gfp transgenic zebrafish larvae. In situ hybridization confirmed smyd1 mRNA expression in these tissues, suggesting that the expression of the smyd1-gfp transgene recapitulated that of the endogenous smyd1 gene. Deletion analysis revealed that the 0.5-kb sequence in the proximal promoter of smyd1 was essential for its muscle specificity. Together, these data indicate that smyd1 is specifically expressed in most, if not all, striated muscles, and the muscle specificity is controlled by the 5.3-kb promoter and flanking sequences. 相似文献
39.
Rigor and resistance to stretch in vertebrate smooth muscle 总被引:2,自引:0,他引:2
40.
Human malignant glioma grown in athymic nude mice (NHG-1) and three freshly resected human solid gliomas were used in the study of factors influencing the direct preparation (DP) for chromosome analysis of human solid tumors. The results showed that: 1) the length of time after the blood supply was obstructed was a major factor in reducing the success rate of DP, i.e., a 2-hour delay resulted in a significantly lowered metaphase number and after 4 hours almost no metaphases could be seen; 2) preserving tumor cells at 4 degrees C may prolong the time limit to about 4 hours; 3) culture medium (RPMI 1640 and Eagle MEM) and bovine calf serum concentration (0%, 10%, 20%, and 30%) did not influence the success rate significantly; 4) colchicine concentration (0.025 micrograms/mL, 0.05 micrograms/mL, 0.1 micrograms/mL) and time of treatment (30 min, 90 min, or 180 min) mainly affected the quality of chromosomes observed but had little effect on the quantity of metaphases that might be obtained. Based on these results, we had a success rate of more than 80% in 72 xenografts and 22 human brain tumors. 相似文献