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311.
报道了采自辽宁阜新,黑龙江镜泊湖和云南昆明的跳小蜂,即阔柄杜丝跳小蜂,新种Dusmetia latiscapa Xu,sp.nov、云南蚧狼跳小蜂,新种Gyranusoidea yunnanensis Xu,sp.nov.。对新种进行了详细描述。本也是杜丝跳小蜂属Dusmetia Mercet和蚧狼跳小蜂属Gyranusoidea Compere在我国分布的首次记录。阔柄杜丝跳小蜂,新种Dusmetia latiscapa Xu,sp.nov.寄主:粉蚧。分布:黑龙江(镜泊湖),辽宁(阜新)。本种与Dusmetia cardinalis Hoffer,1969相似,有以下几点区别:(1)本种索节第4节端部和第5、6节为白色,后索节3-6节为白色;(2)本种柄节长为宽的2.7倍,后柄节长为宽的5倍;(3)本种前翅完全退化,呈翅芽状,后前翅退化,末端尖;(4)前头胸腹呈现黑褐色,后呈红褐色。云南蚧狼跳小蜂,新种Gyranusoidea yunnanensis Xu,sp.nov.寄主:粉蚧。分布:云南(昆明)。本新种与Gyranusoidea hecale Noyes et Hayat 1988很相似,主要区别是新种:(1)触角窝与复眼之间有1褐色斑,后触角窝与复眼之间有1褐色线相连;(2)触角柄节细长,长为最宽处的5倍,后柄节膨大,长为最宽处的2.5—2.8倍;(3)触角柄节近端无白色环斑,后触角柄节近端有白色环斑。 相似文献
312.
Samuel S. KOIDE 《Cell research》2004,(3)
A cDNA, designated as rtSH3p13, was isolated from a rat testis cDNA library. It consists of 1463 bp nuclear acids, which encodes a protein of 312 amino acids and was assigned the GenBank accession number AF227439. The deduced rtSH3p13 protein is a truncated isoform of SH3p13 as a result of mRNA alternative splicing. It is mainly expressed in the rat testis, detected in spermatids at the steps 8-19 of spermiogenesis, and found around the acrosome. During postnatal development, rtSH3p13 appears on day 18 and reaches maximum on day 60. Further experimental results suggested that rtSH3p13 forms a complex with activated epidermal growth factor receptor (EGFR) and interacts with synaptojanin I. Surprisingly, similar to SH3 domain, the V region of rtSH3p13 also inhibits endocytosis in CHO cells. Our results reveal a link between an rtSH3p13-synaptojanin-clathrin complex-mediated formation of pits and the process of spermiogenesis. 相似文献
313.
茧蜂亚科已知有123个属(Quicke,1987),其中窄腹茧蜂属Angustibracon Quicke是Quicke(1987)根据分布在印度的1个种Bracon leptogaster Cameron重新组合为1个新属而建立,迄今已定名种仅此1种。我们整理广西茧蜂标本时,鉴定出该属1新种。这是本属种类在我国分布的首次报道,现将该属属征和新种形态记述如下。新种模式标本存湖南农学院昆虫标本室。 相似文献
314.
作者在整理1985年采集的麻蝇科标本中,发现所麻蝇属(SarcosolomoniaBaranov)1新种。模式标本分别保存于云南省卫生防疫站和军事医学科学院微生物流行病研究所。 相似文献
315.
I Feinkohl N Sattar P Welsh RM Reynolds IJ Deary MW Strachan JF Price;on behalf of the Edinburgh Type Diabetes Study 《PloS one》2012,7(9):e44569
Background
Type 2 diabetes mellitus is associated with risk of congestive heart failure (CHF), cognitive dysfunction and depression. CHF itself is linked both to poor cognition and depression. The ventricular N-terminal pro-brain natriuretic peptide (NT-proBNP) is a marker of CHF, suggesting potential as a marker for cognitive impairment and/or depression. This was tested in the Edinburgh Type 2 Diabetes Study (ET2DS).Methodology and Principal Findings
Cross-sectional analysis of 1066 men and women aged 60–75 with type 2 diabetes. Results from seven neuropsychological tests were combined in a standardised general cognitive ability factor, ‘g’. A vocabulary-based test estimated pre-morbid cognitive ability. The Hospital Anxiety and Depression Scale (HADS) assessed possible depression. After adjustment for age and sex, raised plasma NT-proBNP was weakly associated with lower ‘g’ and higher depression scores (ß −0.09, 95% CI −0.13 to −0.03, p = 0.004 and ß 0.08, 95% CI 0.04 to 0.12, p<0.001, respectively). Comparing extreme quintiles of NT-proBNP, subjects in the highest quintile were more likely to have reduced cognitive ability (within the lowest tertile of ‘g’) and ‘possible’ depression (HADS depression ≥8) (OR 1.80; 95% CI: 1.20, 2.70; p = 0.005 and OR 2.18; 95% CI: 1.28, 3.71; p = 0.004, respectively). Associations persisted when pre-morbid ability was adjusted for, but as expected were no longer statistically significant following the adjustment for diabetes-related and vascular co-variates (β −0.02, 95% CI −0.07 to 0.03, p>0.05 for ‘g’; β 0.03, 95% CI −0.02 to 0.07, p>0.05 for depression scores).Conclusion
Raised plasma NT-proBNP was weakly but statistically significantly associated with poorer cognitive function and depression. The prospective phases of the ET2DS will help determine whether or not NT-proBNP can be considered a risk marker for subsequent cognitive impairment and incident depression and whether it provides additional information over and above traditional risk factors for these conditions. 相似文献316.
317.
Ceres Fernández-Rozadilla Luisa de Castro Juan Clofent Alejandro Brea-Fernández Xavier Bessa Anna Abulí Montserrat Andreu Rodrigo Jover Rosa Xicola Xavier Llor Antoni Castells Sergi Castellví-Bel Angel Carracedo Clara Ruiz-Ponte for the Gastrointestinal Oncology Group of the Spanish Gastroenterological Association 《PloS one》2010,5(9)
Background
Colorectal cancer (CRC) is considered a complex disease, and thus the majority of the genetic susceptibility is thought to lie in the form of low-penetrance variants following a polygenic model of inheritance. Candidate-gene studies have so far been one of the basic approaches taken to identify these susceptibility variants. The consistent involvement of some signaling routes in carcinogenesis provided support for pathway-based studies as a natural strategy to select genes that could potentially harbour new susceptibility loci.Methodology/Principal Findings
We selected two main carcinogenesis-related pathways: Wnt and BMP, in order to screen the implicated genes for new risk variants. We then conducted a case-control association study in 933 CRC cases and 969 controls based on coding and regulatory SNPs. We also included rs4444235 and rs9929218, which did not fulfill our selection criteria but belonged to two genes in the BMP pathway and had consistently been linked to CRC in previous studies. Neither allelic, nor genotypic or haplotypic analyses showed any signs of association between the 37 screened variants and CRC risk. Adjustments for sex and age, and stratified analysis between sporadic and control groups did not yield any positive results either.Conclusions/Significance
Despite the relevance of both pathways in the pathogenesis of the disease, and the fact that this is indeed the first study that considers these pathways as a candidate-gene selection approach, our study does not present any evidence of the presence of low-penetrance variants for the selected markers in any of the considered genes in our cohort. 相似文献318.
Asian cultivated rice(Oryza sativa L.),an important cereal crop worldwide,was domesticated from its wild ancestor 8000 years ago.During its long-term cultivation and evolution under diverse agroecological conditions, Asian cultivated rice has differentiated into indica and japonica subspecies.An effective method is required to identify rice germplasm for its indica and japonica features,which is essential in rice genetic improvements.We developed a protocol that combined DNA extraction from a single rice seed and the insertion/deletion(InDel) molecular fingerprint to determine the indica and japonica features of rice germplasm.We analyzed a set of rice germplasm,including 166 Asian rice varieties,two African rice varieties,30 accessions of wild rice species,and 42 weedy rice accessions,using the single-seeded InDel fingerprints(SSIF).The results show that the SSIF method can efficiently determine the indica and japonica features of the rice germplasm.Further analyses revealed significant indica and japonica differentiation in most Asian rice varieties and weedy rice accessions.In contrast,African rice varieties and nearly all the wild rice accessions did not exhibit such differentiation.The pattern of cultivated and wild rice samples illustrated by the SSIF supports our previous hypothesis that indica and japonica differentiation occurred after rice domestication under different agroecological conditions.In addition,the divergent pattern of rice cultivars and weedy rice accessions suggests the possibility of an endoferal origin(from crop)of the weedy rice included in the present study. 相似文献
319.
Ohmori K Umeda M Tanaka N Takagi H Yoshimura I Sasaki K Asasda S Sakai A Araki H Asakura M Baba H Fushiwaki Y Hamada S Kitou N Nakamura T Nakamura Y Oishi H Sasaki S Shimada S Tsuchiya T Uno Y Washizuka M Yajima S Yamamoto Y Yamamura E Yatsushiro T;Non-Genotoxic Carcinogen Study Group in the Environmental Mutagen Society of Japan 《Alternatives to laboratory animals : ATLA》2005,33(6):619-639
The Bhas promotion assay is a cell culture transformation assay designed as a sensitive and economical method for detecting the tumour-promoting activities of chemicals. In order to validate the transferability and applicability of this assay, an inter-laboratory collaborative study was conducted with the participation of 14 laboratories. After confirmation that these laboratories could obtain positive results with two tumour promoters, 12-O-tetradecanoylphorbol-13-acetate (TPA) and lithocholic acid (LCA), 12 coded chemicals were assayed. Each chemical was tested in four laboratories. For eight chemicals, all four laboratories obtained consistent results, and for two of the other four chemicals, only one of the four laboratories showed inconsistent results. Thus, the rate of consistency was high. During the study, several issues were raised, each of which were analysed step-by-step, leading to revision of the protocol of the original assay. Among these issues were the importance of careful maintenance of mother cultures and the adoption of test concentrations for toxic chemicals. In addition, it is suggested that three different types of chemicals show positive promoting activity in the assay. Those designated as T-type induced extreme growth enhancement, and included TPA, mezerein, PDD and insulin. LCA and okadaic acid belonged to the L-type category, in which transformed foci were induced at concentrations showing growth-inhibition. In contrast, M-type chemicals, progesterone, catechol and sodium saccharin, induced foci at concentrations with little or slight growth inhibition. The fact that different types of chemicals similarly induce transformed foci in the Bhas promotion assay may provide clues for elucidating mechanisms of tumour promotion. 相似文献
320.