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991.
Preparation of o-palmitoyl alkyl lactates with methyl, ethyl, propyl, isopropyl and butyl lactates were attempted in a complex esterification reaction using lipases as catalysts. Compared to lactic acid, alkyl lactates were found to be less inhibitory in nature as they resulted in slightly better yields at shake-flask level. Of the alkyl lactates tested, butyl lactate showed better esterification. Porcine pancreas lipase gave higher yields of esters than Rhizomucor miehei lipase (Lipozyme IM20).  相似文献   
992.
不同海拔地区种植的水稻次库碳水化合物含量的比较   总被引:2,自引:2,他引:0  
在品种、土壤、底肥和追肥等一致的情况下,对三个不同海拔地区种植的水稻的次库(茎+叶鞘)中碳水化合物含量作了比较,结果表明:齐穗和黄熟期次库中总糖或淀粉含量均随海拔增高而增加。但在黄熟期,高海拔地区次库的总糖或淀粉含量比齐穗期的增加,而低海拔地区次库的总糖或淀粉含量则比齐穗期的降低。 齐穗期时,次库的淀粉含量随施用的氮素肥量的增加而降低。在黄熟期,温凉稻作区水稻次库的淀粉含量均随氮素底肥施用量的增加而增加,低熟地区水稻次库的淀粉含量则趋于一致,不过不同地区相比各处理次库的淀粉含量均因海拔增高而增加。 不同时期的氮素追肥使齐穗期次库淀粉含量因追肥时间推迟而增加,唯元江晚穗肥处理的低于中穗肥处理的。黄熟期因追肥时间提早而次库的淀粉含量增加,但元江以早穗肥处理的次库淀粉含量最低。与齐穗期相比时,低海拔地区的各个处理,其次库的淀粉含量均减低,但高海拔的昆明温凉稻作区,施早和中穗肥的水稻,在黄熟期次库的淀粉含量反而增高。还可以看出水稻种植地海拔越高,其次库淀粉含量对追肥时间越敏感。 基于水稻次库中淀粉含量对氮素肥料的反应,就三地气候条件讨论了上述的差异。  相似文献   
993.
Three forms of the normal human plasma fibrinogen γ-chain which differ in molecular weight have been purified. Plasma fibrinogen was separated by ion exchange chromatography on DEAE-Sephacel into three populations of molecules, each with a unique γ-chain composition. Following reduction and S-carboxymethylation, the fibrinogen polypeptide chains in each chromatographic peak were separated by ion exchange chromatography on DEAE-Sephacel and identified following sodium dodecyl sulfate-polyacrylamide gel electrophoresis. The Aα, Bβ and smallest γ-chain (γ50) eluted at progressively higher ionic strengths, but the elution positions of Aα, Bβ and γ50 chains were identifcal for fibrinogen from each of the three different chromatographic fractions. The unique γ chain of fibrinogen in the second chromatographic peak (γ55) eluted at an ionic strength higher than that of the γ50 chain, while the largest γ-chain (γ57.5), which was contained only in the third chromatographic peak of fibrinogen, eluted at the highest ionic strength. The higher ionic strengths needed to elute fibrinogen in the second and third peaks was paralleled by the higher ionic strengths needed to elute the γ-chains unique to them, suggesting that the γ-chain composition of the three fibrinogen fractions accounted for their differential binding to the ion exchange resin. Following desialation with neuraminidase, the differences in electrophoretic mobilities between the three γ-chain forms was maintained, indicating that differential migration on SDS-polyacrylamide gel electrophoresis was not due to variation in sialic acid content.  相似文献   
994.
Abstract. The decline of deciduous woodland populations of Anemone hepatica L. in southern Sweden is documented and possible causes are discussed. The study was based on (1) re‐investigations of 6.25 km2 grid‐squares first studied in 1938–1970, (2) distribution of A. hepatica in woodland sites with well‐known soil chemical properties and (3) a detailed study over 12 consecutive years into the relationships between biological characteristics of the species (number of individuals, vegetative development, flowering frequency) and environmental variables (temperature, precipitation), soil chemistry and time. There was a close relationship between soil acidity (pH, solubility of Al3+) and both distribution and biological characteristics. The biological variables declined significantly over time but were not related to climatic variability. Increasing soil acidity and Al3+ solubility are concluded to be the main factors responsible for the decline of A. hepatica in S. Swedish deciduous woodlands.  相似文献   
995.
UDPgalactose:sn-glycerol-3-phosphate α-D-galactosyltransferase (IFP-synthase, EC 2.4.1.96) shows low activity in extracts prepared from standard volume cells of Poterioochromonals malhamensis under certain conditions. This inactive enzyme has been partially purified by chromatography on DEAE-cellulose, Sephadex G-150 and α-lactalbumin-agarose. It can be activated by an auxiliary enzyme which can be eluted from membranes and which has been purified to homogeneity by chromatography on DEAE-Sephacel and immobilized hemoglobin and fetuin. The activating enzyme is inhibited by chymostatin, antipain and diisopropylfluorophosphate and does not require divalent ions. It consists of a single peptide chain of molecular weight 46 000, can split certain proteins and appears to be a serine proteinase operating around a pH of 6.0. The activating proteinase is irreversibly generated in the crude homogenates on addition of Ca2+ and also shows increased activity shortly after cell shrinkage. This might indicate that it represents one of the possibilities to render the galactosyltransferase active as a result of the physiological stimulus.  相似文献   
996.
997.
Hydroxyl radicals induce hinge cleavage in a human IgG1 molecule via initial radical formation at the first hinge Cys231 followed by electron transfer to the upper hinge residues. To enable engineering of a stable monoclonal antibody hinge, we investigated the role of the hinge His229 residue using structure modeling and site-directed mutagenesis. Direct involvement of His229 in the reaction mechanism is suggested by a 75–85% reduction of the hinge cleavage for variants in which His229 was substituted with either Gln, Ser, or Ala. In contrast, mutation of Lys227 to Gln, Ser, or Ala increased hinge cleavage. However, the H229S/K227S double mutant shows hinge cleavage levels similar to that of the single H229S variant, further revealing the importance of His229. Examination of the hinge structure shows that His229 is capable of forming hydrogen bonds with surrounding residues. These observations led us to hypothesize that the imidazole ring of His229 may function to facilitate the cleavage by forming a transient radical center that is capable of extracting a proton from neighboring residues. The work presented here suggests the feasibility of engineering a new generation of monoclonal antibodies capable of resisting hinge cleavage to improve product stability and efficacy.  相似文献   
998.
999.
Rat liver cytosol extracts catalyzed the formation of monoacetylspermidine when incubated with acetyl-CoA and spermidine.This activity was enhanced 15-fold by administration of thioacetamide (150 mg/kg). The peak of activity occurred 18–24 h after treatment with the drug and then declined reaching control levels by 76 h. Previous studies have shown that ornithine decarboxylase activity was also greatly increased over this time period. Putrescine content in the liver was increased 80–90-fold at 18–24 h and then declined. Spermidine levels were decreased significantly over the period 12–24 h after thioacetamide treatment and then increased substantially at later times. These results are consistent with the hypothesis that, at early times after administration of thioacetamide, the increase in putrescine content is brought about both by decarboxylation of ornithine and by degradation of monoacetylspermidine.Spermidine acetylase activity was also measured in liver extracts prepared after two other physiological stimuli known to enhance ornithine decarboxylase activity were used. Both growth hormone treatment and partial hepatectomy produced an early 2–3-fold increase in the cytosolic spermidine acetylase activity.  相似文献   
1000.
All-trans [11-3H]4,4-difluororetinyl acetate was synthesized by treating methyl all-trans [11-3H]4-oxoretinoate with diethylaminosulfurtrifluoride, followed by reduction and acetylation of the product. After oral administration of the radioactive difluoro analog in oil to rats, difluororetinol, difluororetinyl palmitate and related esters, 4-oxoretinol, 4-oxoretinoic acid and polar conjugated derivatives were identified in the intestine, liver, kidney and / or blood. The major metabolic products were difluororetinyl palmitate and related esters, which were stored in the liver. The presence of the difluoro analog in liver oil from treated rats was confirmed by 19F-NMR spectroscopy. Neither retinol nor retinyl esters were detected as products of the metabolism of the difluoro analog. Nonetheless, all-trans difluororetinyl acetate showed 26 ± 12% of the biological activity of all-trans retinyl acetate in the rat growth assay. Presumably, the difluoro analog is active per se in growth rather than by conversion to retinol or to one of its known growth-promoting metabolites. In general, however, the difluoro analog was metabolized in a manner very similar to vitamin A. The vitamin A moiety of administered difluororetinyl acetate and retinyl acetate was poorly stored (1.8–3.3%) in the liver of vitamin A-depleted rats, confirming and extending past reports that the liver storage mechanism is severely impaired when initial liver stores are very low.  相似文献   
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