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81.
A modified polyethylene glycol precipitation method for concentration of virus followed by a new method to recover nucleic acid was used to detect hepatitis A virus (HAV) and rotavirus (SA11) in shellfish (oysters and hard-shell clams) by hybridization tests. Infectious virus, seeded into relatively large quantities of shellfish, was recovered consistently, with greater than 90% efficiency as measured by either in situ hybridization (HAV) or plaque assay (rotavirus SA11). Viral nucleic acid for dot blot hybridization assays was extracted and purified from virus-containing polyethylene glycol concentrates. Separation of shellfish polysaccharides from nucleic acid was necessary before viral RNA could be detected by dot blot hybridization. Removal of shellfish polysaccharides was accomplished by using the cationic detergent cetyltrimethylammonium bromide (CTAB). Use of CTAB reduced background interference with hybridization signals, which resulted in increased hybridization test sensitivity. After polysaccharide removal, dot blot hybridization assays could detect approximately 10(6) physical particles (corresponding to approximately 10(3) infectious particles) of HAV and 10(4) PFU of SA11 rotavirus present in 20-g samples of oyster and clam meats. These studies show continuing promise for the development of uniform methods to directly detect human viral pathogens in different types of shellfish. However, practical applications of such methods to detect noncultivatable human viral pathogens of public health interest will require additional improvements in test sensitivity.  相似文献   
82.
Four fatty acids (FA, palmitic, myristic, decanoic, hexanoic) were individually conjugated to the N-terminus of the alpha-MSH fragment analog, H-Asp5-His6-D-Phe7-Arg8-Trp9-Lys10-NH2. This resulted in enhanced potency of the conjugates (compared to the unconjugated melanotropin analog) as determined in the lizard skin bioassay and in the mouse melanoma cell tyrosinase bioassay. The shorter conjugates of hexanoic and decanoic acid were at least equipotent to alpha-MSH in the lizard skin bioassay, whereas the longer myristoyl and palmitoyl analogs were 100 times less active. The myristoyl and palmitoyl conjugates exhibited a "creeping" potency in the lizard skin bioassay-that is, potency of the peptides increased with time in contact with the skins. These observations may be related to the more lipid nature of these FA-conjugates. In the tyrosinase assay, the conjugates were 10-100 times more active than alpha-MSH or the unconjugated analog. Each of the FA-melanotropic peptide conjugates exhibited prolonged (residual) melanotropic activity in both the lizard skin and melanoma cell bioassays. In other words, after removal of the melanotropin conjugates from contact with the skins or cells, responses were still manifested for hours or days thereafter. As little as 1 hr of contact with melanoma cells resulted in enhanced enzyme activity as measured 48 hr later. Since the conjugates, but not H-[Asp5, D-Phe7, Lys10]alpha-MSH5-10-NH2, exhibited prolonged activity, the conversion of reversible agonists to irreversible agonists was demonstrated.  相似文献   
83.
Chemotaxis is an important step in monocyte recruitment in inflammation, wound healing, and tumor growth. We reported previously that monocyte chemotactic activity secreted by malignant cells and normal smooth muscle cells is associated with a protein or family of proteins that are related to the monocyte-specific smooth muscle cell-derived chemotactic factor (SMC-CF) (Graves, D. T., Jiang, Y. L., Williamson, M. J., and Valente, A. J. (1989) Science 245, 1490-1493). Similar monocyte chemotactic proteins (MCP-1) produced by U-105MG human glioma cells have also been identified (Yoshimura, T., Robinson, E. A., Tanaka, S., Appella, E., Kuratsu, J., and Leonard, E. J. (1989) J. Exp. Med. 169, 1449-1459). We now report that the MCP-1 gene is expressed in MG-63 human osteosarcoma and vascular smooth muscle cells and that SMC-CF antiserum specifically immunoprecipitates proteins synthesized by U-105MG glioma cells. Experiments were undertaken to elucidate the processing pathway of MCP-1/SMC-CF-like proteins in each of these cell types. These experiments demonstrate that larger MCP-1/SMC-CF-like proteins are derived from a Mr = 9000 precursor. Post-translational modification involves the addition of O-linked carbohydrates and sialic acid residues. Differences in carbohydrate processing account for the heterogeneity in MCP-1/SMC-CF-like proteins produced by different cell types. Secretion of these proteins occurs rapidly following processing events in the endoplasmic reticulum-Golgi compartment.  相似文献   
84.
Retinal basement membrane (RBM), also called inner limiting membrane of retina, is constituted by extracellular matrix. It was reported that neurite outgrowth of a neuron was closely related to extracellular matrix, particularly the laminin. In this laboratory RBM was used as the optimal substrate for retinal cells in culture. We have studied the surface of RBM and its relation to neurite outgrowth by scanning electronmicroscopy and immunogold transmission electronmicroscopy. RBM could be separated by mechanical disruption of the retina mounted between 2 adhesive substrata (membrane filter and poly-L-lysine coated glass). The surface of RBM studied was the side of RBM facing the optic fiber layer and ganglion cell layer. Small particles densely distributed on surface of RBM (Plate I, Fig. 1 and 2) were shown to be chrysanthemum-like structures with radiative arms under the scanning electronmicroscopy (Plate I, Fig. 3 and 4). The radiative arms of RBM of 12-day old chick embryo (E 12) were more in number and longer in length than that of the 6-day old chick embryo (E 6). The axons of ganglion cell from E 6 retinal strip extended out very well on RBM (Plate I, Fig. 5). Growth cone was active with filopodia. The chrysanthemum-like structures changed to ball-particles when the RBM was cultured for 24 hr. Some of ball-particles lay over the growth cone, and some beside it. Over and beside the nerve fiber could also be seen some ball-particles. When many neurites grew on RBM, a lot of ball-particles were shown to be displaced and piled up (Plate I, Fig. 6). The whole amount RBM labeled by indirect immunogold staining of Müller glial cell could be observed by transmission electronmicroscopy. The gold particles wer located at the chrysanthemum-like structure of E 6 RBM (Plate II, Fig. 7) and E 12 RBM (Plate II, Fig. 8). It was suggested that those structures were the end foot of Müller glial cells. Staining of PBS control or mouse serum control was negative (Plate II, Fig. 9 and 10).(ABSTRACT TRUNCATED AT 250 WORDS)  相似文献   
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陈浩  王刚  王成  薛菲  成海  张亚楠 《生态学报》2024,44(4):1526-1538
了解野放丹顶鹤的运动模式、家域和栖息地选择的时间节律特征对丹顶鹤种群保护和栖息地管理尤为重要。基于GPS-GSM跟踪数据,综合运用3S技术、动态布朗桥模型、栖息地选择指数,研究了盐城海滨湿地野放丹顶鹤在不同生活周期的活动节律、家域的面积和重叠指数,以及栖息地选择。结果表明:(1)丹顶鹤日活动节律具有明显的周期性特征。丹顶鹤活动强度:育成期>越冬期>孵化期>育雏期,孵化期和育雏期日间活动强度平稳,育成期和越冬期呈“双峰”模式。(2)丹顶鹤95%家域面积均值介于(111.18±22.15)hm2—(621.28±105.77)hm2,育成期((621.28±105.77) hm2)>育雏期((226.83±54.86) hm2)>孵化期((112.40±7.72) hm2)>越冬期((111.18±22.15) hm2);核心家域面积均值介于(0.53±0.26)—(45.78±6.66) hm2,育成...  相似文献   
88.
王立国  朱海  叶炎婷  贺焱  宋薇 《生态学报》2024,44(2):625-636
旅游业碳中和的实现对于旅游业的绿色高质量发展和可持续发展至关重要。基于全国尺度以30个省份为分析单元,在承接团队前期关于旅游业碳达峰研究成果的基础上,借助土地利用数据、碳吸收系数和灰色预测模型分别测算与模拟了近20年和未来40年各省旅游业碳汇,通过旅游业碳中和指数反映旅游业碳排放和旅游业碳汇之间的动态变化,并利用空间自相关探索旅游业碳中和指数的时空差异。结果表明:(1)未来40年,我国省域旅游业碳汇总体呈现出"南北高,中间低"的空间分布特征,大多数省份的旅游业碳汇不断增长。东北部地区和长江流域以南各地区的旅游业碳汇较为富余,华东地区的山东、江苏和上海等省份的旅游业碳汇则相对匮乏。(2)不同情景中,低碳情景下的旅游业碳中和实现情况最好,有云南、四川和青海等7个省份在2060年之前实现了旅游业碳中和,而中等情景和基准情景下均仅有黑龙江和云南2个省份能够如期或提前实现。其中,西部和北部沿边省份的旅游业碳中和实现情况都要优于其它地区。(3)各省旅游业碳中和指数在未来40年的等级分区大致呈现出从Ⅰ级区逐步向Ⅴ级区转变的趋势,我国总体旅游业碳赤字率由2030年的96.67%逐渐降至2060年的76.67%。(4)未来40年,我国省域旅游业碳中和指数在空间上总体处于集聚态势,热点和冷点的空间分布特征较为明显,且演化趋势较为稳定。其中,热点区和次热点区主要分布在西北、西南、华南和东北地区,冷点区和次冷点区集中分布在华北、华中和华东地区。研究有效探讨了旅游业碳中和研究的理论与范式,并为中国旅游业碳中和的实现提供了一定的现实参考。  相似文献   
89.
Long noncoding RNAs (lncRNAs) play important roles in the spatial and temporal regulation of muscle development and regeneration. Nevertheless, the determination of their biological functions and mechanisms underlying muscle regeneration remains challenging. Here, we identified a lncRNA named lncMREF (lncRNA muscle regeneration enhancement factor) as a conserved positive regulator of muscle regeneration among mice, pigs and humans. Functional studies demonstrated that lncMREF, which is mainly expressed in differentiated muscle satellite cells, promotes myogenic differentiation and muscle regeneration. Mechanistically, lncMREF interacts with Smarca5 to promote chromatin accessibility when muscle satellite cells are activated and start to differentiate, thereby facilitating genomic binding of p300/CBP/H3K27ac to upregulate the expression of myogenic regulators, such as MyoD and cell differentiation. Our results unravel a novel temporal-specific epigenetic regulation during muscle regeneration and reveal that lncMREF/Smarca5-mediated epigenetic programming is responsible for muscle cell differentiation, which provides new insights into the regulatory mechanism of muscle regeneration.  相似文献   
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