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141.
Sbragaglia Valerio Espasandín Lucía Coco Salvatore Felici Alberto Correia Ricardo A. Coll Marta Arlinghaus Robert 《Reviews in Fish Biology and Fisheries》2022,32(2):687-700
Reviews in Fish Biology and Fisheries - Fisheries are among the human activities that are most strongly affected by ongoing climate-related changes in the presence and abundance of fish species... 相似文献
142.
Gorosbel Antonella Bernad Luca Muoz Sebastin D. Pedrana Julieta 《Biodiversity and Conservation》2022,31(3):949-970
Biodiversity and Conservation - Understanding the link between biodiversity, ecosystem services and human well-being is necessary to work towards a sustainable use of agroecosystems and the... 相似文献
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145.
Jorge Mansur Medina Juliany Cola Fernandes Rodrigues Otacilio C Moreira Geórgia Atella Wanderley de Souza Hector Barrabin 《Memórias do Instituto Oswaldo Cruz》2015,110(1):48-55
Phytomonas serpens are flagellates in the family Trypanosomatidae that parasitise the
tomato plant (Solanum lycopersicum L.), which results in fruits with low commercial
value. The tomato glycoalkaloid tomatine and its aglycone tomatidine inhibit the
growth of P. serpens in axenic cultures. Tomatine, like many other saponins, induces
permeabilisation of the cell membrane and a loss of cell content, including the
cytosolic enzyme pyruvate kinase. In contrast, tomatidine does not cause
permeabilisation of membranes, but instead provokes morphological changes, including
vacuolisation. Phytomonas treated with tomatidine show an increased accumulation of
labelled neutral lipids (BODYPY-palmitic), a notable decrease in the amount of
C24-alkylated sterols and an increase in zymosterol content. These
results are consistent with the inhibition of 24-sterol methyltransferase (SMT),
which is an important enzyme that is responsible for the methylation of sterols at
the 24 position. We propose that the main target of tomatidine is the sterols
biosynthetic pathway, specifically, inhibition of the 24-SMT. Altogether, the results
obtained in the present paper suggest a more general effect of alkaloids in
trypanosomatids, which opens potential therapeutic possibilities for the treatment of
the diseases caused by these pathogens. 相似文献
146.
147.
M. E. Stevenson A. P. Blaschke S. Toze J. P. S. Sidhu W. Ahmed I. H. van Driezum R. Sommer A. K. T. Kirschner S. Cervero-Aragó A. H. Farnleitner L. Pang 《Applied and environmental microbiology》2015,81(13):4277-4283
Members of the genus Cryptosporidium are waterborne protozoa of great health concern. Many studies have attempted to find appropriate surrogates for assessing Cryptosporidium filtration removal in porous media. In this study, we evaluated the filtration of Cryptosporidium parvum in granular limestone medium by the use of biotin- and glycoprotein-coated carboxylated polystyrene microspheres (CPMs) as surrogates. Column experiments were carried out with core material taken from a managed aquifer recharge site in Adelaide, Australia. For the experiments with injection of a single type of particle, we observed the total removal of the oocysts and glycoprotein-coated CPMs, a 4.6- to 6.3-log10 reduction of biotin-coated CPMs, and a 2.6-log10 reduction of unmodified CPMs. When two different types of particles were simultaneously injected, glycoprotein-coated CPMs showed a 5.3-log10 reduction, while the uncoated CPMs displayed a 3.7-log10 reduction, probably due to particle-particle interactions. Our results confirm that glycoprotein-coated CPMs are the most accurate surrogates for C. parvum; biotin-coated CPMs are slightly more conservative, while unmodified CPMs are markedly overly conservative for predicting C. parvum removal in granular limestone medium. The total removal of C. parvum observed in our study suggests that granular limestone medium is very effective for the filtration removal of C. parvum and could potentially be used for the pretreatment of drinking water and aquifer storage recovery of recycled water. 相似文献
148.
Leonardo E. Pelletán Laila Suhaiman Cintia C. Vaquer Matías A. Bustos Gerardo A. De Blas Nicolas Vitale Luis S. Mayorga Silvia A. Belmonte 《The Journal of biological chemistry》2015,290(15):9823-9841
Regulated secretion is a central issue for the specific function of many cells; for instance, mammalian sperm acrosomal exocytosis is essential for egg fertilization. ARF6 (ADP-ribosylation factor 6) is a small GTPase implicated in exocytosis, but its downstream effectors remain elusive in this process. We combined biochemical, functional, and microscopy-based methods to show that ARF6 is present in human sperm, localizes to the acrosomal region, and is required for calcium and diacylglycerol-induced exocytosis. Results from pulldown assays show that ARF6 exchanges GDP for GTP in sperm challenged with different exocytic stimuli. Myristoylated and guanosine 5′-3-O-(thio)triphosphate (GTPγS)-loaded ARF6 (active form) added to permeabilized sperm induces acrosome exocytosis even in the absence of extracellular calcium. We explore the ARF6 signaling cascade that promotes secretion. We demonstrate that ARF6 stimulates a sperm phospholipase D activity to produce phosphatidic acid and boosts the synthesis of phosphatidylinositol 4,5-bisphosphate. We present direct evidence showing that active ARF6 increases phospholipase C activity, causing phosphatidylinositol 4,5-bisphosphate hydrolysis and inositol 1,4,5-trisphosphate-dependent intra-acrosomal calcium release. We show that active ARF6 increases the exchange of GDP for GTP on Rab3A, a prerequisite for secretion. We propose that exocytic stimuli activate ARF6, which is required for acrosomal calcium efflux and the assembly of the membrane fusion machinery. This report highlights the physiological importance of ARF6 as a key factor for human sperm exocytosis and fertilization. 相似文献
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150.
Transient receptor potential melastatin 2 (TRPM2), a Ca2+-permeable cation channel implicated in postischemic neuronal cell death, leukocyte activation, and insulin secretion, is activated by intracellular ADP ribose (ADPR). In addition, the pyridine dinucleotides nicotinamide-adenine-dinucleotide (NAD), nicotinic acid–adenine-dinucleotide (NAAD), and NAAD-2′-phosphate (NAADP) have been shown to activate TRPM2, or to enhance its activation by ADPR, when dialyzed into cells. The precise subset of nucleotides that act directly on the TRPM2 protein, however, is unknown. Here, we use a heterologously expressed, affinity-purified–specific ADPR hydrolase to purify commercial preparations of pyridine dinucleotides from substantial contaminations by ADPR or ADPR-2′-phosphate (ADPRP). Direct application of purified NAD, NAAD, or NAADP to the cytosolic face of TRPM2 channels in inside-out patches demonstrated that none of them stimulates gating, or affects channel activation by ADPR, indicating that none of these dinucleotides directly binds to TRPM2. Instead, our experiments identify for the first time ADPRP as a true direct TRPM2 agonist of potential biological interest. 相似文献