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101.
102.
The blue light dependent utilization of nitrate by green algae under common air and high irradiances, besides its assimilatory nature, is associated with the release of NO2 and NH4 + to the culture medium. If the CO2 content of the sparging air was increased up to 2%, previously excreted NO2 and NH4 + were rapidly assimilated. When under air and high irradiances the cell density in the culture reached values corresponding to 25 g Ch 1.ml-1, no further growth was observed and the highest values of NO3 consumption and NO2 and NH4 + release were attained. Besides low CO2 tensions, increasing NO3 concentrations in the medium stimulated the release of NO3 and NH4 +. Under CO2-free air the consumption of NO3 and the release of NO2 and NH4 + on a total N bases were almost stoichiometric and their rates saturated at much lower irradiances than under air. Under CO2-free air high rates of NO2 release were only observed under the blue radiations that were effectively absorbed by photosynthetically active pigments, i.e. 460 nm, but not under 404 and 630 nm radiations. However, the simultaneous illumination of the cells with 404 and 630 nm monochromatic light showed a remarkable synergistic effect on NO2 release.The results are discussed in terms of the close relationship between C and N metabolism, the photosynthetic reducing power required to convert NO inf3 sup± -N into R – NH2-N and the blue light activation of nitrate reductase.  相似文献   
103.
本文介绍一种能准确而迅速改变光刺激器光学参数(波长、强度等)的远距控制装置。将具有不同光学参数的滤光片(或孔径)置于转盘的不同位置,并对其编码。通过对编码值与预置值的比较,驱动步进马达带动转盘到所需的位置。仪器操作简便,有良好的重复性。  相似文献   
104.
The effect of mutations in the cistrons coding for the phage structural proteins has been studied by analyzing the phage-related structures accumulated after restrictive infection. Infection with susmutants in cistron 8, lacking both the major head and the fiber protein, does not produce any phage-related structure, suggesting a single route for the assembly of phage phi29; infection with ts mutants in this cistron produces isometric particles. Mutants is cistron 9, coding for the tail protein, TP1, produce DNA-free prolate heads with an internal core; these particles are abortive and contain the head proteins HPO, HP1 and HP3, the upper collar protein NP2 and the nonstructural proteins p7, p15 and p16. Mutants in cistron 10, coding for the upper collar protein, NP2, produce DNA-free isometric heads also with an internal core; they contain the head proteins and the nonstructural protein p7, suggesting that this protein forms the internal core. Mutants in cistrons 11 and 12, coding for the lower collar protein, NP3, and the neck appendages, NP1, respectively, give rise to the formation of DNA-containing normal capsids and DNA-free prolate particles, more rounded at the corners than the normal capsids and with an internal core; the DNA-containing 11-particles are formed by the head proteins and the upper collar protein; the DNA-free 11-particles contain, besides these proteins, the nonstructural protein p7 and a small amount of proteins p15 and 16. The DNA-containing 12-particles have all the normal phage structural proteins except the neck appendages, formed by protein NP1; the DNA-free particles are similar to the DNA-free 11-particles. After restricitive infection mutant sus14(1241) has a delayed lysis phenotype and produces a phage burst higher than normal, after artificial lysis. It produces DNA-containing particles, identical to wild-type phage, which have all the normal phage structural proteins, and DNA-free prolate particles, more rounded at the corners than the final phage particles and with an internal core; the last particles contain the same proteins as the DNA-free 11 or 12-particles. These particles could represent a prohead state, ready for DNA encapsulation. None of the DNA-containing particles have the nonstructural proteins p7, p15 or p16, suggesting that these proteins are released from the proheads upon DNA encapsulation.  相似文献   
105.
106.
Summary The metabolic cost of active sodium transport was determined in toad bladder at different gradients of transepithelial potential, , by continuous and simultaneous measurements of CO2 production and of transepithelial electric current. Amiloride was used to block active sodium transport in order to assess the nontransport-linked, basal, production of CO2 and the passive permeability of the tissue. From these determinations active sodium transport,J Na, and suprabasal CO2 production, , were calculated. Since large transients inJ Na and frequently accompanied any abrupt change in , steady state conditions were carefully defined.Some 20 to 40 min were required after a change in before steady state of transport activity and of CO2 production were achieved. The metabolic cost of sodium transport proved to be the same whether the bladder expended energy moving sodium against a transepithelial electrical potential grandient of +50 mV or whether sodium was being pulled through the active transport pathway by an electrical gradient of –50 mV. In both cases the value of the ratio averaged some 20 sodium ions transported per molecule of CO2 produced.When the Na pump was blocked by 10–2 m ouabain, the perturbations of the transepithelial electrical potential did not elicit changes ofJ Na nor, consequently, of .The independence of the ratio from over the range ±50 mV indicates a high degree of coupling between active sodium transport and metabolism.  相似文献   
107.
108.
Supernumerary chromosomes of two types have been observed in the grasshopper Eyprepocnemis plorans subsp. plorans. One of these (the B-type) is similar in size to an S autosome; the other is smaller (B-type). Both are telocentric and mitotically stable. The frequencies of individuals with the B-type supernumeraries in five natural populations were 56, 56, 70, 71 and 30 per cent respectively. The equivalent levels of the B-type supernumerary were 0, 0, 13, 3 and 0 per cent respectively. Because of the relative infrequency of the B-type only the B-type has been studied in detail. In males with 1B, anaphase I segregation of X and B was random in four populations but non-random in that from Otivar. Here the B was distinctive in having a secondary constriction near the centromere. A study of chiasma frequency among A-chromosomes revealed that the B-type supernumerary increases significantly both the mean chiasma frequency and the between-cell variance. A comparison of body morphometrics failed to reveal any effect of these B-chromosomes on the exophenotype.  相似文献   
109.
110.
Cytogenetic aspects of the cryptobranchid salamander Andrias davidianus of western China have been studied, including chromosome number and morphology, C-band patterns, meiosis, and the chromosomal localization of ribosomal 5S RNA genes. Our data regarding chromosome number (2n=60) and general chromosome morphology largely confirm the results of Morescalchi et al. (1977). The karyotype consists of 16 pairs of macrochromosomes that decrease gradually in relative length to 14 pairs of microchromosomes. Telocentric chromosomes are a conspicuous feature of the karyotype, representing more than half the genome. Differential staining reveals that all of the chromosomes, except four pairs of microchromosomes, have C-band heterochromatin in their centromeric regions, the amount varying irrespective of chromosome size. Faint bands of interstitial and telomeric C-band heterochromatin are found in mitotic chromosomes but are not seen in meiotic preparations. In C-banded mitotic preparations from a female, one of the smallest macrochromosome pairs is heteromorphic in respect to C-band heterochromatin and centromere position. In situ hybridization of an iodinated 5S RNA probe to meiotic chromosome preparations reveals that this repeated gene is clustered near the telomeric region of chromosome 7, a medium size telocentric, a location corresponding to a band of heterochromatin. Studies of spermatocytes indicate that the process of meiosis in A. davidianus closely resembles that of more advanced salamanders, and that the microchromosomes are meiotically stable. The significance of microchromosomes and chromosome morphology in the reorganization of salamander genomes during evolution is discussed on the basis of cytogenetic data available for A. davidianus and various other primitive and advanced salamanders.  相似文献   
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