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991.
Heat shock proteins are induced by stressful stimuli and have been shown to protect cells and organs from such stresses both in vitro and in vivo. This study examined the regulation of HSP70 mRNA expression and detected the effect of aging on RNA expression in hippocampus of rats. The stress models were built by using forced-swimming in 25 degrees C and 4 degrees C water, respectively. Two groups of male rats, 2-month-old and 16-month-old, respectively, were randomly divided into three subgroups: acute stress (AS) model, chronic habituation stress (CHS) model and chronic dishabituation stress (CDS) model. Observation of exploratory behavior in an open-field (OF) test indicated stress levels. The expression of HSP70 mRNA in hippocampus was measured by RT-PCR after 0, 30, 60, 180, and 360 min of stress, respectively. Results showed that the number of quadrant crossing in both aged CHS and young CHS groups decreased gradually with the process of stress, reflecting an adaptation to the stress condition. Repeated swimming in warm water resulted in habitual expression of HSP70 mRNA in both young and aged CHS group, indicating an adaptation to the stress. The RNA expression of young CHS group was significantly stronger than that of the aged CHS group at 30, 60, 180, and 360 min after stress (P < 0.05). Meanwhile, in an intensive stress level in which the rats swam in 4 degrees C water, a high expression level of HSP70 mRNA was achieved in CDS groups, producing a dishabituation that proved the habitual expression from the other side. These results showed that senescence dramatically affected both exploratory behavior and HSP70 mRNA expression in rats' hippocampus. The results also suggested that chronic stress could lead to the habituational expression of HSP70 mRNA, but high intensive stress could reverse the habituational state and lead to the dishabituational expression. Moreover, the duration of stimuli is one of the important factors that affect the level of HSP70 mRNA expression. 相似文献
992.
Xu F Ji J Li L Chen R Hu WC 《Biochemical and biophysical research communications》2007,352(3):681-688
The role of the adventitia in vascular function and vascular lesion formation has been largely ignored. This study observed the activation of the adventitia and specifically the fibroblasts in the development of atherosclerosis in the apoE(-/-) mouse. The results showed a gradual increase in expression of collagen types I and III after 2, 4, and 8 weeks of hyperlipidic diet. The earliest expression of monocyte chemoattractant protein-1 (MCP-1) protein and mRNA was detected in the adventitial fibroblast before the formation of intimal lesions. Proliferation, too, was first found in the adventitial fibroblasts. We hypothesize that the adventitial fibroblast is activated in the early stage of atherosclerosis. Adventitial inflammation may be an early event in the development of atherosclerotic lesions. 相似文献
993.
Athanasiou A Clarke AB Turner AE Kumaran NM Vakilpour S Smith PA Bagiokou D Bradshaw TD Westwell AD Fang L Lobo DN Constantinescu CS Calabrese V Loesch A Alexander SP Clothier RH Kendall DA Bates TE 《Biochemical and biophysical research communications》2007,364(1):131-137
Time-lapse microscopy of human lung cancer (H460) cells showed that the endogenous cannabinoid anandamide (AEA), the phyto-cannabinoid Δ-9-tetrahydrocannabinol (THC) and a synthetic cannabinoid HU 210 all caused morphological changes characteristic of apoptosis. Janus green assays of H460 cell viability showed that AEA and THC caused significant increases in OD 595 nm at lower concentrations (10-50 μM) and significant decreases at 100 μM, whilst HU 210 caused significant decreases at all concentrations. In rat heart mitochondria, all three ligands caused significant decreases in oxygen consumption and mitochondrial membrane potential. THC and HU 210 caused significant increases in mitochondrial hydrogen peroxide production, whereas AEA was without significant effect. All three ligands induced biphasic changes in either mitochondrial complex I activity and/or mitochondrial complex II-III activity. These data demonstrate that AEA, THC, and HU 210 are all able to cause changes in integrated mitochondrial function, directly, in the absence of cannabinoid receptors. 相似文献
994.
To determine the significance of the gamma2 calcium-binding site in fibrin polymerization, we synthesized the fibrinogen variant, gammaD298,301A. We expected these two alanine substitutions to prevent calcium binding in the gamma2 site. We examined the influence of calcium on the polymerization of gammaD298,301A fibrinogen, evaluated its plasmin susceptibility, and solved 2.7 and 2.4 A crystal structures of the variant with the peptide ligands Gly-Pro-Arg-Pro-amide (GPRP) and Gly-His-Arg-Pro-amide (GHRP), respectively. We found that thrombin-catalyzed polymerization of gammaD298,301A fibrinogen was modestly impaired, whereas batroxobin-catalyzed polymerization was significantly impaired relative to normal fibrinogen. Notably, the influence of calcium on polymerization was the same for the variant and for normal fibrinogen. Fibrinogen gammaD298,301A was more susceptible to plasmin proteolysis in the presence of GPRP. This finding suggests structural changes in the near-by "a" polymerization site. Comparisons of the structures revealed minor conformational changes in the gamma294-301 loop that are likely responsible for the weakened "a" site. When considered altogether, the data suggest that the gamma2 calcium-binding site does not significantly modulate polymerization. We cannot, however, rule out the possibility that the weakened "a" polymerization site masks an important role for the gamma2 calcium-binding site in normal polymerization. Somewhat unexpectedly, the structure data showed that GPRP bound to the "b" site and induced the same local conformational changes as GHRP to this site. This structure shows that "A:b" interactions can occur and suggests that these may participate in normal polymerization. 相似文献
995.
Yu F Jones GS Hung M Wagner AH MacArthur HL Liu X Leavitt S McDermott MJ Tsiang M 《Biochemistry》2007,46(10):2899-2908
LEDGF/p75 is known to enhance the integrase strand transfer activity in vitro, but the underlying mechanism is unclear. Using an integrase assay with a chemiluminescent readout adapted to a 96-well plate format, the effect of LEDGF/p75 on both the 3'-processing and strand transfer steps was analyzed. Integrase inhibitors of the strand transfer reaction remained active in the presence of LEDGF/p75, but displayed 3- to 7-fold higher IC50 values. Our analyses indicate that, in the presence of 150 nM LEDGF/p75, active integrase/donor DNA complexes were increased by 5.3-fold during the 3'-processing step. In addition, these integrase/donor DNA complexes showed a 4.5-fold greater affinity for the target DNA during the subsequent strand transfer step. We also observed a 3.7-fold increase in the rate constant of catalysis of the strand transfer step when 150 nM LEDGF/p75 was present during the 3'-processing step. In contrast, when LEDGF/p75 was added at the beginning of the strand transfer step, no increase in either the concentration of active integrase/donor DNA complex or its rate constant of strand transfer catalysis was observed. This observation suggested that the integrase/donor DNA formed in the absence of LEDGF/p75 became refractory to the stimulatory effect of LEDGF/p75. Instead, this LEDGF/p75 added at the start of the strand transfer step was able to promote the formation of a new cohort of active integrase/donor DNA complexes which became functional with a delay of 45 min after LEDGF/p75 addition. We propose a model whereby LEDGF/p75 can only bind integrase before the latter binds donor DNA whereas donor DNA can engage either free or LEDGF/p75-bound integrase. 相似文献
996.
The marcoalga Ulva pertusa was cultured under (20 ± 2)°C, (20 ± 4)°C, (20 ± 6)°C, (20 ± 8)°C and (20 ± 10)°C circadian rhythms of fluctuating temperature
conditions, and constant temperature of 20°C was used as the control. The growth rate of macroalga at (20 ± 2)°C, (20 ± 4)°C
and (20 ± 6)°C were significantly higher than that at constant temperature of 20°C, while growth rate at (20 ± 8)°C and (20
± 10)°C were significantly lower than that at constant temperature of 20°C. The growth rate of macroalga was a quadratic function
of the thermal amplitude. Such a growth model can be described by G = β
0 + β
1(TA) + β
2(TA)2, where G represents the relative growth rate, TA is thermal amplitude in degree Celsius, β
0 is the intercept on the G axis, and β
1 and β
2 are the regression coefficients. The optimal thermal amplitude for the growth of thallus at mean temperature of 20°C was
estimated to be ± 3.69°C. Analysis of biochemical composition at the final stages of thaulls growth revealed that diel fluctuating
temperature caused various influences (P < 0.05). The content of chlorophyll, protein and total solute carbohydrate at (20 ± 2)°C and (20 ± 4)°C were slightly higher
than those at constant temperature of 20°C, however no statistically significant differences were found among them (P > 0.05). While osmolytes (total solute carbohydrate and free proline) at (20 ± 10)°C were significantly higher than that at
20°C (P < 0.05). Therefore, more chlorophyll and carbohydrate production might account for the enhancement in the growth of macroalga
at the diel fluctuating temperatures in the present study.
Handling editor: S. M. Thomaz 相似文献
997.
998.
MalE of group A Streptococcus participates in the rapid transport of maltotriose and longer maltodextrins
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Shelburne SA Fang H Okorafor N Sumby P Sitkiewicz I Keith D Patel P Austin C Graviss EA Musser JM Chow DC 《Journal of bacteriology》2007,189(7):2610-2617
Study of the maltose/maltodextrin binding protein MalE in Escherichia coli has resulted in fundamental insights into the molecular mechanisms of microbial transport. Whether gram-positive bacteria employ a similar pathway for maltodextrin transport is unclear. The maltodextrin binding protein MalE has previously been shown to be key to the ability of group A Streptococcus (GAS) to colonize the oropharynx, the major site of GAS infection in humans. Here we used a multifaceted approach to elucidate the function and binding characteristics of GAS MalE. We found that GAS MalE is a central part of a highly efficient maltodextrin transport system capable of transporting linear maltodextrins that are up to at least seven glucose molecules long. Of the carbohydrates tested, GAS MalE had the highest affinity for maltotriose, a major breakdown product of starch in the human oropharynx. The thermodynamics and fluorescence changes induced by GAS MalE-maltodextrin binding were essentially opposite those reported for E. coli MalE. Moreover, unlike E. coli MalE, GAS MalE exhibited no specific binding of maltose or cyclic maltodextrins. Our data show that GAS developed a transport system optimized for linear maltodextrins longer than two glucose molecules that has several key differences from its well-studied E. coli counterpart. 相似文献
999.
1000.