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991.
Summary In the ovoviviparous fly, Sarcophaga bullata, vitellogenesis is cyclic; a process reflected in ultrastructural changes in the fat body cells and oenocytes. At eclosion the larval fat body has not yet completely disappeared. During vitellogenesis the fat body cells are specialized for intensive protein synthesis showing a very extensive RER and numerous invaginations of the plasma membrane. These features disappear when the eggs descend into the oviducts to complete embryogenesis. The predominant feature of the oenocytes is their very prominent SER. The fat body cells of the males are never as specialized for protein synthesis as those of the females. Feeding of ecdysterone to males for 3 or more days induces a rather extensive subcellular apparatus for protein synthesis, i.e., invaginations of the plasma membrane and an extensive RER. Juvenile hormone is completely ineffective in this respect. Both ecdysterone and juvenile hormone have pronounced but different effects on the oenocytes of males. 相似文献
992.
993.
994.
Input-output (I-O) relationships were studied in cercal “thread-hair” sensilla (THS) on Periplaneta americana L. by recording from individual axons of THS while displacing the corresponding hair with a galvanometric device. Sinusoidal analysis was attempted and pulse- and ramplike displacements were then tested. The effects of stimulus orientation were also investigated. THS were spontaneously active and purely phasic and did not respond to sustained displacements. With small sinusoidal displacements (<30°) they behaved as a linear, secondorder lead system sensitive to velocity. With larger amplitudes, however, they exhibited prominent nonlinear features with minimal consequences of displacements at the extremes. Responses to other waveforms indicated secondorder response components. THS were directionally sensitive. Phasic behavior and the nonlinearities may be due to mechanical properties at the base of the hair. The spike-firing threshold may also contribute. Resting activity appears to be due to neuronal factors since it was not abolished by preventing hair movements. Transducer operations were simulated in a digital computer. 相似文献
995.
A fluorescent photoaffinity label—8-azido-1-N6-etheno-adenosine 5′-triphosphate (8-N3ε ATP)—for ATP-binding proteins has been synthesized. The effectiveness of the label is demonstrated with F1ATPase from Micrococcus luteus. 8-N3ε ATP is a substrate for the enzyme in the presence of bivalent cations. Ultraviolet irradiation of F1ATPase in the presence of the label and Mg2+ ions inhibits the enzyme irreversibly. The fluorescent label is bound preferentially to the β subunit of the enzyme. Labeling and inactivation are decreased by protection with ATP or ADP. 相似文献
996.
M. Bornancin G. De Renzis J. Maetz 《Journal of comparative physiology. B, Biochemical, systemic, and environmental physiology》1977,117(3):313-322
Summary Freshwater eel gills are notorious for their limited ability to pump chloride. As a result there is a considerable discrepancy between the Na+ and Cl– plasma levels, and plasma HCO3
– and blood pH are relatively high in this species.When eels are kept in tanks aerated with pure oxygen, significant alterations in blood acid-base balance, an increase in plasma pCO2 and a decrease in blood pH, are observed. In fish studied after 3 weeks hyperoxia, the decrease in blood pH is compensated by an increase in plasma HCO3
–. Such fish exhibit a Cl– influx 5 times higher than that observed in normoxic fish. This Cl– influx is readily inhibited by addition of SCN– to the external medium.An anion-stimulated ATPase activated by HCO3
– and by Cl– and inhibited by SCN– was recently described in membrane fractions of the gills ofCarassius auratus, a fish noted for its high Cl– pumping rate. This enzyme is also found in the gills of the eel. While the maximal rates of enzyme activation by HCO3
– and by Cl– are similar inCarassius andAnguilla, the affinity of the enzyme for Cl– is 25 times higher inCarassius. In the microsomal fraction of the hyperoxic eel gills, the maximal anionstimulated ATPase activity remains unchanged but HCO3
– affinity decreases by 50%, while Cl– affinity increases 5 times. Thus some characteristics of this ATPase seem to be closely related to the Cl– pump activity exhibited by the gill in fresh water. 相似文献
997.
Antonio De Marco Harald Tschesche Gerhard Wagner Kurt Wüthrich 《European biophysics journal : EBJ》1977,3(3-4):303-315
In the 1H NMR spectra obtained at 360 MHz after digital resolution enhancement, the multiplet resonances of the methyl groups in the basic pancreatic trypsin inhibitor (BPTI) were resolved. With suitable double irradiation techniques the individual methyl resonances were assigned to the different types of aliphatic amino acid residues. Furthermore, from pH titration and comparison of the native protein with chemically modified BPTI, the resonance lines of Ala 16 in the active site and Ala 58 at the C-terminus were identified. Potential applications of the resolved methyl resonances as natural NMR probes for studies of the molecular conformations are discussed. 相似文献
998.
Inhibition of haem synthesis caused by cobalt in rat liver. Evidence for two different sites of action. 总被引:4,自引:3,他引:1 下载免费PDF全文
Cobalt inhibits liver haem synthesis in vivo by acting at least two different sites in the biosynthetic pathway: (1) synthesis of 5-aminolaevulinate and (2) conversion of 5-amino-laevulinate into haem. The first effect is largely, if not entirely, due to inhibition of the activity of 5-aminolaevulinate synthase, rather than to inhibition of the formation of the enzyme. The second effect results from diversion of 5-aminolaevulinate into an unidentified liver pool with solubility properties similar to those of cobalt protoporphyrin. 相似文献
999.
Loss of haem from cytochrome P-450 caused by lipid peroxidation and 2-allyl-2-isoprophylacetamide. An abnormal pathway not involving production of carbon monoxide. 总被引:6,自引:4,他引:2 下载免费PDF全文
1. Microsomal preparations undergoing lipid peroxidation produce CO and lose haem from cytochrome P-450. 2. The amount of CO produced does not correlate with the amount of haem lost and, after pre-labelling of microsomal haem in its bridges with 5-amino[5-14C]laevulinate, the radioactivity lost from haem is not recorved as CO. 3. Similarly, when pre-labelled microsomal haem is destroyed by the action of 2-allyl-2-isopropylacetamide, no radioactivity is recovered as CO. In clear contrast, on degradation of haem by the haem oxygenase system, CO is produced in an amount equimolar to the haem lost. 4. It is concluded that (a) the CO produced during lipid peroxidation originates from a source different from haem and (b) the degradations of haem caused by lipid peroxidation and 2-allyl-2-isopropylacetamide do not involve to any significant extent evolution of the methene-bridge carbon of haem as CO. 相似文献
1000.
A. J. M. Vermorken A. A. Groeneveld J. M. H. C. Hilderink R. De Waal H. Bloemendal 《Molecular biology reports》1977,3(5):371-378
Lens epithelial cells can be kept in their original differentiated state or brought to dedifferentiation depending on the culture conditions. The different stages of differentiation can be identified using specific markers, namely the activity of steroid metabolizing enzymes, and the synthesis of specific structural lens polypeptides. For this reason lens epithelial cells in tissue culture provide a unique system for the study of the regulation of RNA and protein biosynthesis.Abbreviations dehydroepiandrosterone (DHEA)=
3-hydroxy-5-androsten-17-one
- androstenediol (ADIOL)=
5-androstene-3, 17-diol
- androstenedione(ADION)=
4-androstene-3, 17-dione 相似文献