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941.
Summary A frequency-time domain 3D NMR technique has been developed for measurement of heteronuclear coupling constants in oligonucleotides employing a combination of COSY andJ-resolved techniques. The method employs frequency-selective excitation to generate the 1 axis and 2D FT to generate the 2 and 3 axes. The procedure yields high resolution, especially along the 1 axis. The technique is demonstrated on a dinucleotide.  相似文献   
942.
A group of 12 alkaloids were tested as inhibitors of photophosphorylation in spinach chloroplasts. Ajmaline, a dihydroindole alkaloid, was found to be the strongest inhibitor of both cyclic and non-cyclic photophosphorylation. Low concentrations of ajmaline also inhibited the dark and light ATPases, and the coupled electron flow from water to ferricyanide, measured either as ferrocyanide formed or as oxygen evolved, but not the uncoupled electron transport or the pH rise of illuminated unbuffered suspensions of chloroplasts. Higher concentrations of ajmaline stimulated, instead of inhibiting, photosynthetic electron transport or oxygen evolution and decreased the pH rise, thus behaving as an uncoupler, such as ammonia.Photophosphorylation was partially inhibited by 100 μM dihydrosanguinarine, 100 μM dihydrochelerythrine (benzophenanthridine alkaloids); 500 μM O,O'-dimethylmagnoflorine, 500 μM N-methylcorydine (aporphine alkaloids) and 1 mM julocrotine. They also inhibited coupled oxygen evolution and only partially (dihydrosanguinarine and dihydrochelerythrine) or not at all (the other alkaloids) uncoupled oxygen evolution.Spegazzinine (dihydroindole alkaloid), magnoflorine, N-methylisocorydine, coryneine (aporphine alkaloids), candicine and ribalinium chloride were without effect on photophosphorylation at 500 μM.  相似文献   
943.
Summary Colloidal ThO2 particles (diameter of 60 Å) were used as electron-opaque markers to trace the intracellular compartments continuous with the bulk interstitial fluid of guinea pig ventricular muscle. Beating and quiescent hearts in a Langendorff preparation were perfused for 30 min with oxygenated Ringer solution containing 1% ThO2. The hearts were immediately fixed by perfusing with glutaraldehyde solution. The colloidal ThO2 particles entered into many of the T tubules and into longitudinallyrunning tubules. No differences in distribution of ThO2 were observed in a heart which was not exposed to ThO2 until after it was fixed. Tracer did not penetrate into the intercalated disk clefts in the guinea pig hearts and one frog heart used for comparison. Tubular profiles filled with ThO2 were not seen in frog heart, an observation which confirms the absence of T tubules in this amphibian. It is concluded that, in mammalian cardiac muscle, the lumens of the longitudinal tubules are continuous with the lumens of the T tubules, forming an extensively interconnected T-L tubular system. Hence, every myofibril has close access to a fluid-filled space which is continuous with the interstitial fluid and which may be of similar cationic composition; such an arrangement should facilitate excitation-contraction coupling.Supported by grants from the American Heart Association and from the Public Health Service (HE-11155, HE-05815 and HE-10384). The authors wish to acknowledge the expert technical assistance of Mrs. Jan Redick and to thank Dr. James Smith of Marquette University for the supply of Thorotrast used in these studies.  相似文献   
944.
The relationship between the rate of electron flow, internal H+ concentration and the magnitude of the H+ concentration gradient (ΔpH) in chloroplasts illuminated at various light intensities has been examined. At an external pH of 7.0, the internal H+ concentration is a linear function of the rate of electron flow except at saturating light intensity. In contrast, at pH 8.1, this relationship between electron flow and internal H+ concentration holds only at values of ΔpH below about 2.8 – 2.9 units. At higher ΔpH values, the rate of electron flow increases much more dramatically than the internal H+ concentration. ATP (0.1 mM) prevents this increase. It is suggested that at pH 8.1 but not at pH 7.0, the conformation of coupling factor 1 is altered at high ΔpH values. Its altered conformation may result in an increased efflux of H+ from the chloroplasts. This notion is supported by the effects of ATP on electron flow and ΔpH as well as the effect of external pH and light intensity on the reactivity of coupling factor 1 to N-ethylmaleimide.  相似文献   
945.
Osmotically disrupted chloroplasts catalyze a rapid, light and AMP and ATP dependent 32Pi incorporation into ATP. Light does not stimulate [14C] AMP incorporation into ATP in this system. AMP in the presence of Pi inhibits electron flow in a manner analogous to ADP inhibition in the absence of Pi. The inhibition of AMP + Pi is reversed on addition of ADP.  相似文献   
946.
H. M. Behrens  D. Gradmann 《Planta》1985,163(4):453-462
Electrical transmembrane potential differences and resistances in different tissues of intact root tips of Lepidium sativum L. were investigated in a humid atmosphere by conventional glass-microelectrode techniques with the reference electrode at the surface (apoplast) of the root. The resting potential (inside negative) in cells of the root cap rose from-80 mV in external cell layers (secretion cells) to approx.-140 mV in central cells (statocytes). Measurements of the electric input resistance within the apoplast of the root tip (calyptra, meristem and elongation zone) yielded a preference for longitudinal contact (resistance per length of tissue approx. 3.4 GOhm m-1) compared with transversal contact (approx. 14 GOhm m-1). Similarly, the symplastic coupling expressed as the characteristic length (L) where a signal is reduced to 1/c compared with the origin yielded L y =390 m in the longitudinal (y) direction and L x =140 m in the transversal (x) direction. Cable analytical treatment of the symplastic input resistances (approx. 10 MOhm) resulted in low membrane resistances in the y-direction at the ends of cells compared with the membrane resistances in the x-direction (approx. 0.2 Ohm m2) of the lateral membranes in the approximately cylindrical cells. This anisotropy is discussed in terms of model calculations. The resistivity of the symplast was calculated to be about 2.5 Ohm m. The input current-voltage relationship displayed a slight curvature with increasing slope for the more negative membrane potential typical of membranes with electrogenic pumps. Even after massive electrical stimulation in the range from-50 to-150mV carried out to trace current-voltage curves, electrical excitations (action potentials) were not detected in the cells investigated.Abbreviations el voltage recording electrodes - R resistance - V r resting potential  相似文献   
947.
Summary Vascular endothelial cultures, derived from large vessels, retain many of the characteristics of theirin vivo counterparts. However, the observed reduction in size and complexity of intercellular gap and tight junctions in these cultured cells (Larson, D.M., and Sheridan, J.D., 1982,J. Cell Biol. 92:183) suggests that important functions, thought to be mediated by these structures, may be alteredin vitro. In our continuing studies on intercellular communication in vessel wall cells, we have quantitated the extent of junctional transfer of small molecular tracers (the fluorescent dye Lucifer Yellow CH and tritiated uridine nucleotides) in confluent cultures of calf aortic (BAEC) and umbilical vein (BVEC) endothelium. Both BAEC and BVEC show extensive (and quantitatively equivalent) dye and nucleotide transfer. As an analogue of intimal endothelium, we have also tested dye transfer in freshly isolated sheets of endothelium. Transfer in BAEC and BVEC sheets was more rapid, extensive and homogeneous than in the cultured cells, implying a reduction in molecular coupling as endothelium adapts to culture conditions. In addition, we have documented heterocellular nucleotide transfer between cultured endothelium and vascular smooth muscle cells, of particular interest considering the prevalence of myo-endothelial junctionsin vivo. These data yield further information on junctional transfer in cultured vascular endothelium and have broad implications for the functional integration of the vessel wall in the physiology and pathophysiology of the vasculature.  相似文献   
948.
The coupling mechanism of sarcoplasmic reticulum ATPase is based on the reciprocal influence of calcium binding and phosphorylation domains. Cooperative calcium binding activates the enzyme, permitting utilization of ATP by transfer of its terminal phosphate to the enzyme. Occupancy of the phosphorylation domain then produces internalization and dissociation of the bound calcium. Hydrolytic cleavage of Pi completes the catalytic and transport cycle. Conversely, the phosphorylated enzyme intermediate can be formed with Pi in the absence of Ca2+. This intermediate is then destabilized by calcium binding, permitting formation of ATP by phosphoryl transfer to ADP.  相似文献   
949.
The binding of various nucleotides to chloroplast coupling factor CF1 was studied by two dialysis techniques. It was found that the number of nucleoside diphosphate sites and their specificities for the base moiety is dependent on the magnesium concentration. In the presence of 50 μM added MgCl2, the protein has a single strong site/mol protein with Kd = 0.5 μM for ADP and high specificity (Kd > 20 μM for ?ADP, GDP, CDP). In the presence of 5 mM MgCl2, the protein has two independent tight ADP sites (Kd = 0.4 μM) of low specificity (Kd ≈ 0.8, 2, and 2 μrmM, respectively for ?ADP, GDP, and CDP). These results are compared with the specificity of the partial reactions for photophosphorylation.  相似文献   
950.
The kinetics of the hydrogen-deuterium exchange reaction in a stable ATPase (TF1) from a thermophilic bacterium PS3 was followed by infrared absorption measurements. The rates of the hydrogen-deuterium exchange reactions decreased in following order; free form, TF1·ADP, TF1·ATP and TF1·AMP-P(NH)P. TF1 does not dissociate into subunits even in the absence of nucleotides, thus differences in exchange likely reflect differences in conformations of subunits. These results indicate that the structure is most restricted when ATP or AMP-P(NH)P is bound to the enzyme.  相似文献   
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