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361.
362.
The yeast GLC7 gene required for glycogen accumulation encodes a type 1 protein phosphatase. 总被引:10,自引:0,他引:10
Z H Feng S E Wilson Z Y Peng K K Schlender E M Reimann R J Trumbly 《The Journal of biological chemistry》1991,266(35):23796-23801
The glc7 mutant of the yeast Saccharomyces cerevisiae does not accumulate glycogen due to a defect in glycogen synthase activation (Peng, Z., Trumbly, R. J., and Reimann, E.M. (1990) J. Biol. Chem. 265, 13871-13877) whereas wild-type strains accumulate glycogen as the cell cultures approach stationary phase. We isolated the GLC7 gene by complementation of the defect in glycogen accumulation and found that the GLC7 gene is the same as the DIS2S1 gene (Ohkura, H., Kinoshita, N., Miyatani, S., Toda, T., and Yanagida, M. (1989) Cell 57, 997-1007). The protein product predicted by the GLC7 DNA sequence has a sequence that is 81% identical with rabbit protein phosphatase 1 catalytic subunit. Protein phosphatase 1 activity was greatly diminished in extracts from glc7 mutant cells. Two forms of protein phosphatase 1 were identified after chromatography of extracts on DEAE-cellulose. Both forms were diminished in the glc7 mutant and were partly restored by transformation with a plasmid carrying the GLC7 gene. Southern blots indicate the presence of a single copy of GLC7 in S. cerevisiae, and gene disruption experiments showed that the GLC7 gene is essential for cell viability. The GLC7 mRNA was identified as a 1.4-kilobase RNA that increases 4-fold at the end of exponential growth in wild-type cells, suggesting that activation of glycogen synthase is mediated by increased expression of protein phosphatase 1 as cells reach stationary phase. 相似文献
363.
We have cloned and sequenced the 2175-nucleotide, full-length cDNA for the mouse 46-kDa Man 6-P receptor (46MPR) and studied its functional properties in stably transfected mouse L cells which do not express the insulin-like growth factor-II receptor/mannose 6-phosphate receptor (IGF-IIR/MPR). The 278-amino acid sequence deduced from the cDNA for the murine 46MPR shows 19 amino acid differences from that of the human 46MPR, none of which are found in the 68-amino acid cytoplasmic tail. Binding of ligand to the murine 46MPR in permeabilized cells showed a pH optimum of 6.5, was completely inhibited by Man 6-P, and was stimulated by divalent cations. Mn2+ was more effective than Ca2+ or Mg2+. Endocytosis was demonstrated at pH 6.5 and was stimulated 4-7-fold by Mn2+. In its responsiveness to divalent cations and its preference for Mn2+, the murine 46MPR resembled the bovine 46MPR more than the human 46MPR. It was even less efficient than the human receptor in its ability to mediate endocytosis in transfected murine cells. It was also no more efficient than the human 46MPR in correcting the sorting defect of IGF-IIR/MPR-deficient mouse L cells. We conclude that the previously observed relative inefficiency of the human 46MPR in sorting enzymes to lysosomes in murine cells is a property of the 46MPR itself and not a manifestation of studying its expression in a heterologous cell line. 相似文献
364.
365.
Kashin-Beck disease is an endemic osteoarthropathy in China which may lead to skeletal deformation and dwarfism. We have analysed articular cartilage from two patients and found an accumulation of the precursor molecule, pro-pN-collagen II (pN, peptide attached at the amino-terminus) which was not present in extracts of control fetal cartilage. In addition, collagen II isolated from the same tissue by limited pepsin digestion had a decreased electrophoretic mobility, increased proline hydroxylation and decreased thermal stability. Previously, a genetic defect in pro-pN-collagen-I processing has been described in calf and sheep (dermatosparaxis) and man (Ehlers-Danlos, type VII) which caused an extreme fragility of the skin [Lenaers, A., Ansay, M., Nusgens, B.V. & Lapière, C.M. (1971) Eur. J. Biochem. 23, 533-541; Helle, O. & Nes, N.J. (1972) Acta Vet. Scand. 13, 443-445; Lichtenstein, J.R., Martin, G.R., Kohn, L.D., Byers, P.H. & McKusick, V.A. (1973) Science 182, 298-300]. Accordingly, one may assume that the impaired conversion of pro-pN-collagen II to collagen II and the structural alteration of collagen II, presumably caused by fulvic acid and other environmental factors, play an important role in the pathogenesis of Kashin-Beck disease. 相似文献
366.
本文着重分析了广西城市和农村脑血管病发病情况的差异。我们发现城市CVD发病率、患病率明显高于农村,但是农村CVD的死亡率高于城市,其中我们对其原因作了初步的探讨。 相似文献
367.
采用纤维素黄原酸酯——过氧化氢构成氧化还原体系,把丙烯酰胺接枝到蔗渣纤维浆泊上。探讨了引发剂用量、初始pH值、单体比、反应温度、反应时间诸因素对接枝共聚反应的影响。 相似文献
368.
一类含间隙分布时滞的种群增长模型的稳定性 总被引:4,自引:0,他引:4
本文首先利用间隙分布时滞函数来建立更为符合实际的种群增长模型,然后运用两种不同的方法,对其平衡位置的局部稳定性进行了全面的讨论,得出了局部渐近稳定的充分必要条件,在参数平面上划分出了稳定和不稳地的区域。 相似文献
369.
广东鹤山亚热带丘陵人工林群落分析:Ⅳ 针叶林 总被引:2,自引:0,他引:2
本文研究14年林龄的马尾松人工群落和5年林龄的人工湿地松群落。通过研究这两个针叶林造林后的生境变化和现有群落的生物量、生长量、叶面积指数以及垂直生物量结构等,揭示其群落学特征,为林业实践提供理论依据。 相似文献
370.
肠球菌是宿主肠道中正常G~ 球菌,目前已成为医源性感染的重要致病菌。临床上有30%肠球菌感染患者感染源不明,拟肠道来源可能性最大。本文给小鼠肌注灭滴灵3日,造成动物肠系膜淋巴结(MLN)肠球菌的感染率为40%;肌注灭滴灵加口服链霉素,MLN的感染率上升为90%,肝脾内脏中的感染率为83%;联合使用上述抗生素合并25%体表面积烧伤,动物发生致死性肠球菌性肠源性感染,动物诸内脏中肠球菌感染的检出率均高达100%。本研究证明肠球菌感染可以是肠源性的。 相似文献