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为研究北柴胡种子内生菌的群落结构与多样性.采用Illumina Miseq高通量测序技术,分别对山西(BC_1)、黑龙江(BC_2)、河北(BC_3)和内蒙古(BC_4)的四个产地(4份)北柴胡种子的16S RNA V3-V4区和ITS1区扩增片段进行测序,并对内生细菌和内生真菌群落结构和多样性进行分析.结果表明,BC... 相似文献
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Suowei Wu Zhanwang Yu Fengge Wang Weihua Li Qingkai Yang Chunjiang Ye Yan Sun Demin Jin Jiuran Zhao Bin Wang 《DNA sequence》2008,19(3):357-365
Adenine phosphoribosyltransferase (APRT) is the key enzyme that converts adenine to adenosine monophosphate (AMP) in the purine salvage pathway. It was found that several different forms of APRT gene exist in plants, but no APRT gene in maize has been reported up to now. In this study, a novel maize APRT gene was cloned and characterized through a combination of bioinformatic, RT-PCR and RACE strategies. The full length of APRT cDNA sequence is 1202 nucleotides, with an ORF encoding 214 amino acid residues. Alignment of the deduced protein with that of other plant APRT genes indicates that the new gene is the form 2 of maize APRT, thus it was named ZmAPT2. Through basic local alignment search tool, search in the genomic survey sequence database of MaizeGDB, the putative genomic sequence of ZmAPT2 was obtained. Comparison of the cDNA and genomic sequence of the ZmAPT2 gene revealed that it contained seven exons and six introns. The locations of the introns within the maize ZmAPT2 coding region were consistent with those in the previously isolated APRTs of arabidopsis and rice. RT-PCR analysis showed that ZmAPRT was constitutively expressing in different organs under high temperature and salt stresses. Southern blot analysis indicated that at least three APRT genes existed in maize genome. These results confirmed that the novel maize ZmAPT2 gene was truly identified, and its potential role in maize growth and development was discussed. 相似文献
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This paper presents a kinetic model of phosphofructokinase-1 from Escherichia coli. A complete catalytic cycle has been reconstructed based on available information on the oligomeric structure of the enzyme and kinetic mechanism of its monomer. Applying the generalization of the Monod-Wyman-Changeux approach proposed by Popova and Sel'kov(35-37) to the reconstructed catalytic cycle rate equation has been derived. Dependence of the reaction rate on pH, magnesium, and effectors has been taken into account. Kinetic parameters have been estimated via fitting the rate equation against experimentally measured dependencies of initial rate on substrates, products, effectors, and pH available from the literature. The model of phosphofructokinase-1 predicts (1) cooperativity of binding both fructose-6-phosphate and ATPMg(2-), (2) significant inhibition of the enzyme resulting from an increase in total concentration of ATP under the condition of fixed concentration of Mg(2+) ions, and (3) dual effect of ADP consisting of allosteric activation and product inhibition of the enzyme. Moreover, the model developed can be used in the kinetic modeling of biochemical pathways containing phosphofructokinase-1. 相似文献
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Demin Wang Elizabeth C. Boylin Yoshiyuki Minegishi Renren Wen Edvard C. Smith James N. Ihle Mary Conley 《Immunogenetics》2001,53(7):550-556
Our recent studies using targeted gene disruption have shown that defects in phospholipase Cgamma2 (PLCgamma2) result in a B-cell abnormality that is very similar to that seen in Btk-deficient mice. Null mutations in either PLCG2 or BTK are associated with decreased numbers of mature B cells, failure to make antibodies to some T cell-independent antigens and the absence of CD5+ peritoneal B cells. Mutations in BTK in humans cause a more severe defect in B-cell development characterized by almost complete absence of B cells in the peripheral circulation, profound hypogammaglobulinemia and an inability to produce antibodies to any antigens. However, not all patients with severe defects in B-cell development have mutations in BTK or the components of the B-cell signal transduction complex. To explore the possibility that some patients with defects in B-cell development of unknown etiology might have mutations in PLCG2, we determined the genomic structure of this gene and established conditions to analyze the 32 exons of the gene and the flanking sequences by single-strand conformation polymorphism. Although 24 polymorphic variants of this gene were found in 35 patients, we did not identify any alterations that were likely to be the cause of disease. 相似文献
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基质金属蛋白酶及其抑制剂mRNA在正常及异位子宫内膜中的表达 总被引:1,自引:1,他引:0
目的:观察正常及异位子宫内膜中基质金属蛋白酶-1,-2(MMP-1,-2)和基质金属蛋白酶组织抑制剂-1(TIMP-1)基因表达的变化,以探讨其与子宫内膜异位症的关系。方法:应用原位技术,采用地高辛生物素标记的cDNA探针(MMP-1,MMP-2,TIMP-1)对子宫内膜异位症患者(EM组)的子宫内膜(14例)、异位病灶组织(20例)及非子宫内膜异位症患者(对照组)的子宫内膜(12例),分3批进行分子杂交检测,结果:3批结果相似。MMP-1,-2,TIMP-1mRNA在腺上皮细胞和间质细胞均有表达,EM组的子宫内膜MMP-1,-2及TIMP-1mRNA表达量与对照组无显著性差异(P>0.05),异位病灶组织的MMP-1,-2mRNA表达量明显高于对照组(P<0.05),而TIMP-1mRNA表达量则低于对照组(P<0.05)。结论:子宫内膜异位症患者的异位病灶中,存在MMP-1,-2和TIMP-1明显的平衡失调,这可能与子宫内膜异位症的发生、发展和不孕有关。 相似文献
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Principles of regulation on different levels of photosynthetic apparatus are discussed. Mathematical models of isolated photosynthetic reaction centers and general system of energy transduction in chloroplast are developed. A general approach to model these complex metabolic systems is suggested. Regulatory mechanisms in plant cell are correlated with the different patterns of fluorescence induction curve at different internal physiological states of the cells and external (environmental) conditions. Light regulation inside photosynthetic reaction centers, diffusion processes in thylakoid membrane, generation of transmembrane electrochemical potential, coupling with processes of CO2 fixation in Calvin Cycle are considered as stages of control of energy transformation in chloroplasts in their connection with kinetic patterns of fluorescence induction curves and other spectrophotometric data. 相似文献