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91.
Calcium channels in the plasma membrane of root cells fulfill both nutritional and signaling roles. The permeability of these
channels to different cations determines the magnitude of their cation conductances, their effects on cell membrane potential
and their contribution to cation toxicities. The selectivity of the rca channel, a Ca2+-permeable channel from the plasma membrane of wheat (Triticum aestivum L.) roots, was studied following its incorporation into planar lipid bilayers. The permeation of K+, Na+, Ca2+ and Mg2+ through the pore of the rca channel was modeled. It was assumed that cations permeated in single file through a pore with three energy barriers and two
ion-binding sites. Differences in permeation between divalent and monovalent cations were attributed largely to the affinity
of the ion binding sites. The model suggested that significant negative surface charge was present in the vestibules to the
pore and that the pore could accommodate two cations simultaneously, which repelled each other strongly. The pore structure
of the rca channel appeared to differ from that of L-type calcium channels from animal cell membranes since its ion binding sites had
a lower affinity for divalent cations. The model adequately accounted for the diverse permeation phenomena observed for the
rca channel. It described the apparent submillimolar K
m
for the relationship between unitary conductance and Ca2+ activity, the differences in selectivity sequences obtained from measurements of conductance and permeability ratios, the
changes in relative cation permeabilities with solution ionic composition, and the complex effects of Ca2+ on K+ and Na+ currents through the channel. Having established the adequacy of the model, it was used to predict the unitary currents that
would be observed under the ionic conditions employed in patch-clamp experiments and to demonstrate the high selectivity of
the rca channel for Ca2+ influx under physiological conditions.
Received: 23 August 1999/Revised: 12 November 1999 相似文献
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Rupali M. Khadake Prabhakar K. Ranjekar Abhay M. Harsulkar 《Molecular biotechnology》2009,42(2):168-174
The Δ12 desaturase represents a diverse gene family in plants and is responsible for conversion of oleic acid (18:1) to linoleic
acid (18:2). Several members of this family are known from plants like Arabidopsis and Soybean. Using primers from conserved C- and N-terminal regions, we have cloned a novel Δ12 desaturase gene amplified
from flax genomic DNA, denoted as LuFAD2-2. This intron-less gene is 1,149-base pair long encoding 382 amino acids—putative membrane-bound Δ12 desaturase protein. Sequence
comparisons show that the novel sequence has 85% similarity with previously reported flax Δ12 desaturase at amino acid level
and shows typical features of membrane-bound desaturase such as three conserved histidine boxes along with four membrane-spanning
regions that are universally present among plant desaturases. The signature amino acid sequence ‘YNNKL’ was also found to
be present at the N terminus of the protein, which is necessary and sufficient for ER localization of enzyme. Neighbor-Joining
tree generated from the sequence alignment grouped LuFAD2-2 among the other FAD2 sequences from Ricinus, Hevea, Jatropha, and Vernicia. When LuFAD2-2 and LuFAD2 were expressed in Saccharomyces cerevisiae, they could convert the oleic acid to linoleic acid, with an average conversion rate of 5.25 and 8.85%, respectively. However,
exogenously supplied linoleic acid was feebly converted to linolenic acid suggesting that LuFAD2-2 encodes a functional FAD2 enzyme and has substrate specificity similar to LuFAD2. 相似文献
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98.
肉桂酰辅酶A还原酶(cinnamoyl-CoA reductase,CCR)是木质素合成代谢的关键酶。该研究以菊芋(Helianthus tuberosus L.)‘廊芋8号’为材料,克隆到1个菊芋的CCR基因,命名为HtCCR1(GenBank登录号为MN205540),其开放阅读框(ORF)长975bp,编码324个氨基酸,其中含有FR_SDR_e保守结构域。系统进化分析表明,HtCCR1与向日葵CCR蛋白(XP_021989763.1)共聚于一支,二者亲缘关系最近。实时定量PCR分析表明,HtCCR1基因在菊芋茎和叶中的表达量显著高于在根和块茎中;盐(150mmol·L-1 NaCl)胁迫处理6、12和24h后,处理组HtCCR1基因的表达量均显著高于对照组;干旱(20%PEG6000)胁迫6和12h后,处理组HtCCR1基因的表达较对照组均显著上调。成功构建pET-28a-HtCCR1原核表达载体,转化大肠杆菌BL21(DE3)并诱导出了符合预期大小的蛋白,表明HtCCR1重组蛋白已成功表达。该研究结果为进一步研究HtCCR1基因的功能及利用基因工程手段调节菊芋中木质素的生物合成奠定了基础。 相似文献
99.
100.
Víctor Faundes William G. Newman Laura Bernardini Natalie Canham Jill Clayton-Smith Bruno Dallapiccola Sally J. Davies Michelle K. Demos Amy Goldman Harinder Gill Rachel Horton Bronwyn Kerr Dhavendra Kumar Anna Lehman Shane McKee Jenny Morton Michael J. Parker Julia Rankin Siddharth Banka 《American journal of human genetics》2018,102(1):175-187