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111.
Kołodziej Barbara Kochan Ewa Kazimierczak Jerzy Chmiel Aleksander 《Plant Growth Regulation》2006,48(1):13-19
American ginseng (Panax quinquefolium L.) is a perennial medicinal herb originally grown in Canada and USA, and recently also in China, Australia, Holland and
Poland. Several commercial preparations are produced from ginseng roots, that are known for their antifatigue, antitumor,
antistress and immune system stimulating functions. The medicinal properties are due mainly to the active components – ginsenosides.
In this work, the results of field cultivation experiments are presented that examine the effects of foliar application of
several growth regulators on quality parameters and ginsenoside content of P. quinuefolium roots. The growth regulators tested, i.e., kinetin, daminozide, mixture of gibberellic acid (GA3) with potassium salt of α-naphthalene acetic acid (kNAA) and new preparation – IPO-1 – benzimidazole derivative (obtained
from the Institute of Organic Industry in Warsaw – at present during the process of patent), were applied at a concentration
of 100 or 200 mg l−1 in the middle of June in the 2nd year of vegetation. After 4 years of cultivation, the roots were dug up and dried, and subsequently
the quantitative analysis of individual saponins (Rb1, Rb2, Rc, Rd, Re, Rg1) by HPLC was performed. Growth regulators significantly affected quality parameters, morphological features and accumulation
of individual and total ginsenosides in ginseng roots. Regardless of doses, the plant roots treated with growth regulators
had a higher content of total ginsenosides in comparison to the control. The growth regulators also affected individual ginsenosides
level and narrowed the ratio of Rb:Rg group. The application of kinetin, daminozide and benzimidazole derivative for foliar spray during 2nd year of American ginseng
vegetation caused a significant increase in air dry weight of roots and aboveground parts whereas the mixture of GA3 and kNAA showed a decreasing effect. An increase of roots size was observed using higher doses (200 mg l−1) of kinetin and daminozide while a decreasing tendency appeared with the application of the other preparations. 相似文献
112.
Jerzy Chelkowski Piotr Zajkowski Marcin Zawadzki Juliusz Perkowski 《Mycotoxin Research》1987,3(1):25-32
An isolated rat liver was perfused with deoxynivalenol (DON) at a dose of 3 mg in a recirculating perfusion system. To identify glucuronide conjugates equal amounts of bile samples, perfusate and liver homogenates were incubated with and without (control) a β-glucuronidase preparation and analyzed by thin layer chromatography and capillary gas liquid chromatography — chemical ionization mass spectrometry. A total of 40.4% of the administered dose of DON was found to be conjugated with glucuronic acid (perfusate 20.4%, bile 19.2%, liver 0.8%), while only 1.3% of the parent DON (perfusate 1.1%, bile 0.2%) was detected. The cleavage of DON-glucuronide was demonstrated by incubating DON-glucuronide containing bile samples with intestine contents under anaerobic conditions. 相似文献
113.
Compant S Kaplan H Sessitsch A Nowak J Ait Barka E Clément C 《FEMS microbiology ecology》2008,63(1):84-93
The colonization pattern of Vitis vinifera L. by Burkholderia phytofirmans strain PsJN was determined using grapevine fruiting cuttings with emphasis on putative inflorescence colonization under nonsterile conditions. Two-week-old rooted plants harbouring flower bud initials, grown in nonsterile soil, were inoculated with PsJN:gfp2x. Plant colonization was subsequently monitored at various times after inoculation with plate counts and epifluorescence and/or confocal microscopy. Strain PsJN was chronologically detected on the root surfaces, in the endorhiza, inside grape inflorescence stalks, not inside preflower buds and flowers but rather as an endophyte inside young berries. Data demonstrated low endophytic populations of strain PsJN in inflorescence organs, i.e. grape stalks and immature berries with inconsistency among plants for bacterial colonization of inflorescences. Nevertheless, endophytic colonization of inflorescences by strain PsJN was substantial for some plants. Microscopic analysis revealed PsJN as a thriving endophyte in inflorescence organs after the colonization process. Strain PsJN was visualized colonizing the root surface, entering the endorhiza and spreading to grape inflorescence stalks, pedicels and then to immature berries through xylem vessels. In parallel to these observations, a natural microbial communities was also detected on and inside plants, demonstrating the colonization of grapevine by strain PsJN in the presence of other microorganisms. 相似文献
114.
115.
Jerzy W. Jurka 《Journal of theoretical biology》1977,68(4):515-520
Some properties of transitions generated during an imprecise replication of nucleic acids are described here. A possible role of these transitions in the evolution of the genetic code with respect to the evolution of the tertiary structure of proteins is suggested. The data supporting this hypothesis are obtained from the analysis of certain regularities present in the genetic code and in the proportions of amino acid residues buried in the interior of globular proteins. 相似文献
116.
Construction of interleukin-1 alpha mutants using unequal contamination of synthetic oligonucleotides. 总被引:1,自引:2,他引:1
Proteins without readily available three-dimensional structural data present a difficult problem in the exploration of structure/function relationships. Saturation mutagenesis using contaminated oligonucleotides can identify potentially interesting regions of such a protein. This technique, in which synthesized oligonucleotides contain low-level base substitutions, allows random mutations to be placed throughout a gene sequence. Using double-stranded cassettes, a region of the human interleukin-1 alpha gene has been altered using such mutagenic oligonucleotides. However, instead of contaminating both strands of the gene sequence at the same level, each strand of the insert was contaminated at a different level. Several recombinants were sequenced and the effects of the mutations on the activity of the proteins were examined. Contaminating the two oligonucleotides at different levels produced a significantly different distribution of nucleotide changes from that seen if both strands were contaminated at the same level. The observed distribution followed the average of the distributions for each of the two contamination levels. This resulted in roughly equal frequencies of 1 to 5 nucleotide changes per clone with very few clones containing the wild-type nucleotide sequence. This helped overcome the redundancy in the genetic code, resulting in a high frequency of amino acid changes, and allowed changes at every amino acid to be sampled in a small number of mutants. This procedure can allow a gene sequence to be screened rapidly by removing most wild-type sequences from analysis while making sure that there are many amino acid changes in the resultant mutants. 相似文献
117.
118.
Waszkiewicz N Szajda SD Zalewska A Szulc A Kępka A Minarowska A Wojewódzka-Żelezniakowicz M Konarzewska B Chojnowska S Ladny JR Zwierz K 《Folia histochemica et cytobiologica / Polish Academy of Sciences, Polish Histochemical and Cytochemical Society》2012,50(1):1-11
The relationship between alcohol consumption and glycoconjugate metabolism is complex and multidimensional. This review summarizes the advances in basic and clinical research on the molecular and cellular events involved in the metabolic effects of alcohol on glycoconjugates (glycoproteins, glycolipids, and proteoglycans). We summarize the action of ethanol, acetaldehyde, reactive oxygen species (ROS), nonoxidative metabolite of alcohol--fatty acid ethyl esters (FAEEs), and the ethanol-water competition mechanism, on glycoconjugate biosynthesis, modification, transport and secretion, as well as on elimination and catabolism processes. As the majority of changes in the cellular metabolism of glycoconjugates are generally ascribed to alterations in synthesis, transport, glycosylation and secretion, the degradation and elimination processes, of which the former occurs also in extracellular matrix, seem to be underappreciated. The pathomechanisms are additionally complicated by the fact that the effect of alcohol intoxication on the glycoconjugate metabolism depends not only on the duration of ethanol exposure, but also demonstrates dose- and regional-sensitivity. Further research is needed to bridge the gap in transdisciplinary research and enhance our understanding of alcohol- and glycoconjugate-related diseases. 相似文献
119.
Shiina T Dijkstra JM Shimizu S Watanabe A Yanagiya K Kiryu I Fujiwara A Nishida-Umehara C Kaba Y Hirono I Yoshiura Y Aoki T Inoko H Kulski JK Ototake M 《Immunogenetics》2005,56(12):878-893
Salmonid fishes are among the few animal taxa with a probable recent tetraploid ancestor. The present study is the first to compare large (>100 kb) duplicated genomic sequence fragments in such species. Two contiguous stretches with major histocompatibility complex (MHC) class I genes were detected in a rainbow trout BAC library, mapped and sequenced. The MHC class I duplicated regions, mapped by fluorescence in situ hybridization (FISH), were shown to be located on different metaphase chromosomes, Chr 14 and 18. Gene organization in both duplications is similar to that in other fishes, in that the class I loci are tightly linked with the PSMB8, PSMB9, PSMB10 and ABCB3 genes. Whereas one region, Onmy-IA, has a classical MHC class I locus (UBA), Onmy-IB encodes only non-classical class Ib proteins. The nucleotide diversity between the Onmy-IA and Onmy-IB noncoding regions is about 14%. This suggests that the MHC class I duplication event has occurred about 60 mya close to the time of an hypothesized ancestral tetraploid event. The present article is the first convincing report on the co-existence of two closely related MHC class I core regions on two different chromosomes. The interchromosomal duplication and the homology levels are supportive of the tetraploid model.Nucleotide sequence data reported are available in the DDBJ/EMBL/GenBank database under the accession numbers AB162342, AB162343 and from AY525774 to AY525776. 相似文献
120.