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81.
Evaluation of major genetic loci contributing to inbreeding depression for survival and early growth in a selfed family of Pinus taeda 总被引:1,自引:0,他引:1
Remington DL O'Malley DM 《Evolution; international journal of organic evolution》2000,54(5):1580-1589
The magnitude of fitness effects at genetic loci causing inbreeding depression at various life stages has been an important question in plant evolution. We used genetic mapping in a selfed family of loblolly pine (Pinus taeda L.) to gain insights on inbreeding depression for early growth and viability. Two quantitative trait loci (QTLs) were identified that explain much of the phenotypic variation in height growth through age 3 and may account for more than 13% inbreeding depression in this family. One of these QTLs maps to the location of cad-nl, a lignin biosynthesis mutation. Both QTLs show evidence of overdominance, although evidence for true versus pseudo-overdominance is inconclusive. Evidence of directional dominance for height growth was noted throughout the genome, suggesting that additional loci may contribute to inbreeding depression. A chlorophyll-deficiency mutation, spf did not appear to be associated with growth effects, but had significant effects on survival through age 3. Previously identified embryonic viability loci had little or no overall effect on germination, survival, or growth. Our results challenge, at least in part, the prevailing hypothesis that inbreeding depression for growth is due to alleles of small effect. However, our data support predictions that loci affecting inbreeding depression are largely stage specific. 相似文献
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有关束长蝽科若虫期的报道很少,其中束长蝽亚科尤其如此,迄今只有Malcus flavidipes Stal一种曾有详细描述。本文首次记述Malcus sinicus Syts(5龄),M.elongatus Stys(5龄和4龄)以及Chauliops bisonotula Banks(5龄)的若虫,并记录寄主植物。对于腺毛系统及其系统学意义进行了讨论。 相似文献
83.
黄单胞杆菌XC—82,R5二步发酵工艺研究 总被引:2,自引:0,他引:2
通过对黄单胞杆菌XC-82,R5株的黄原胶二步发酵工艺研究,针对菌株在生长时期与产胶时期不同培养条件的需求,确定了两个阶段各自适宜的培养基组成,温度,pH值条件,实验表明,当流加稀释率为5时,二步发酵生产可达到了较高水平,其产胶量较传统的间歇发酵提高31%。 相似文献
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枫香因其树形优美,入秋后叶色红艳或橙黄,极具观赏价值,是优良的景观生态树种。为了解枫香叶片变色及其次级代谢过程的遗传基础,该文以枫香5个叶片变色期叶片混合样品为材料,利用单分子实时测序技术(PacBio平台)对其进行全长转录组测序。结果表明:(1)全长转录组测序共获得41.04 Gb的高质量数据,从中鉴定出全长非嵌合序列563 180条,通过聚类和去冗余,获得27 269条高质量全长转录本。在27 269条全长转录本中预测到2 035条长链非编码RNA(lncRNA),并检测出14 892个简单重复序列(SSR)位点和1 856个转录因子。(2)基因注释结果表明,NR、GO、COG、KEGG 等8个数据库共注释了24 857条转录本,KEGG数据库共获得了124个条代谢途径,主要有核糖体、碳代谢、氨基酸生物合成等,在类黄酮和叶绿素代谢途径中分别有49和71个转录本参与。上述结果初步揭示了枫香叶片变色期转录组信息以及功能特性,为后续研究枫香叶片变色分子机制、色素代谢合成途径和调控、相关功能基因克隆以及叶色改良提供基础数据。 相似文献
85.
Michael A. Proschan 《Biometrical journal. Biometrische Zeitschrift》2009,51(2):348-357
Adaptive clinical trials are becoming very popular because of their flexibility in allowing mid‐stream changes of sample size, endpoints, populations, etc. At the same time, they have been regarded with mistrust because they can produce bizarre results in very extreme settings. Understanding the advantages and disadvantages of these rapidly developing methods is a must. This paper reviews flexible methods for sample size re‐estimation when the outcome is continuous. 相似文献
86.
Benjamin Bertin Yoan Renaud Rajaguru Aradhya Krzysztof Jagla Guillaume Junion 《Journal of visualized experiments : JoVE》2015,(103)
Measuring levels of mRNAs in the process of translation in individual cells provides information on the proteins involved in cellular functions at a given point in time. The protocol dubbed Translating Ribosome Affinity Purification (TRAP) is able to capture this mRNA translation process in a cell-type-specific manner. Based on the affinity purification of polysomes carrying a tagged ribosomal subunit, TRAP can be applied to translatome analyses in individual cells, making it possible to compare cell types during the course of developmental processes or to track disease development progress and the impact of potential therapies at molecular level. Here we report an optimized version of the TRAP protocol, called TRAP-rc (rare cells), dedicated to identifying engaged-in-translation RNAs from rare cell populations. TRAP-rc was validated using the Gal4/UAS targeting system in a restricted population of muscle cells in Drosophila embryos. This novel protocol allows the recovery of cell-type-specific RNA in sufficient quantities for global gene expression analytics such as microarrays or RNA-seq. The robustness of the protocol and the large collections of Gal4 drivers make TRAP-rc a highly versatile approach with potential applications in cell-specific genome-wide studies. 相似文献
87.
Continuous removal of endocrine disruptors by versatile peroxidase using a two‐stage system
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Roberto Taboada‐Puig Thelmo A. Lu‐Chau Gemma Eibes Gumersindo Feijoo Maria T. Moreira Juan M. Lema 《Biotechnology progress》2015,31(4):908-916
The oxidant Mn3+‐malonate, generated by the ligninolytic enzyme versatile peroxidase in a two‐stage system, was used for the continuous removal of endocrine disrupting compounds (EDCs) from synthetic and real wastewaters. One plasticizer (bisphenol‐A), one bactericide (triclosan) and three estrogenic compounds (estrone, 17β‐estradiol, and 17α‐ethinylestradiol) were removed from wastewater at degradation rates in the range of 28–58 µg/L·min, with low enzyme inactivation. First, the optimization of three main parameters affecting the generation of Mn3+‐malonate (hydraulic retention time as well as Na‐malonate and H2O2 feeding rates) was conducted following a response surface methodology (RSM). Under optimal conditions, the degradation of the EDCs was proven at high (1.3–8.8 mg/L) and environmental (1.2–6.1 µg/L) concentrations. Finally, when the two‐stage system was compared with a conventional enzymatic membrane reactor (EMR) using the same enzyme, a 14‐fold increase of the removal efficiency was observed. At the same time, operational problems found during EDCs removal in the EMR system (e.g., clogging of the membrane and enzyme inactivation) were avoided by physically separating the stages of complex formation and pollutant oxidation, allowing the system to be operated for a longer period (~8 h). This study demonstrates the feasibility of the two‐stage enzymatic system for removing EDCs both at high and environmental concentrations. © 2015 American Institute of Chemical Engineers Biotechnol. Prog., 31:908–916, 2015 相似文献
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