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951.
Lin WH Song JS Chang TY Chang CY Fu YN Yeh CL Wu SH Huang YW Fang MY Lien TW Hsieh HP Chao YS Huang SF Tsai SF Wang LM Hsu JT Chen YR 《Analytical biochemistry》2008,377(1):89-94
Epidermal growth factor receptor (EGFR) is a valid drug target for development of target-based therapeutics against non-small-cell lung cancer. In this study, we established a high-throughput cell-based assay to screen for compounds that may inhibit EGFR activation and/or EGFR-mediated downstream signaling pathway. This drug screening platform is based on the characterization of an EGFR-transfected 32D cell line (32D-EGFR). The expression of EGFR in 32D cells allowed cell proliferation in the presence of either epidermal growth factor (EGF) or interleukin 3 (IL-3) and provided a system for both screening and counterscreening of EGFR pathway-inhibitory compounds. After the completion of primary and secondary screenings in which 32D-EGFR cells were grown under the stimulation of either EGF or IL-3, 9 of 20,000 compounds were found to selectively inhibit the EGF-dependent proliferation, but not the IL-3-dependent proliferation, of 32D-EGFR cells. Subsequent analysis showed that 3 compounds of the 9 initial hits directly inhibited the kinase activity of recombinant EGFR in vitro and the phosphorylation of EGFR in H1299 cells transfected with EGFR. Thus, this 32D-EGFR assay system provides a promising approach for identifying novel EGFR and EGFR signaling pathway inhibitors with potential antitumor activity. 相似文献
952.
ADP-ribosyl cyclase and NAD+ glycohydrolase (CD38, E.C.3.2.2.5) efficiently catalyze the exchange of the nicotinamidyl moiety of NAD+, nicotinamide adenine dinucleotide phosphate (NADP+) or nicotinamide mononucleotide (NMN+) with an alternative base. 4′-Pyridinyl drugs (amrinone, milrinone, dismerinone and pinacidil) were efficient alternative substrates (kcat/KM = 0.9-10 μM−1 s−1) in the exchange reaction with ADP-ribosyl cyclase. When CD38 was used as a catalyst the kcat/KM values for the exchange reaction were reduced two or more orders of magnitude (0.015-0.15 μM−1 s−1). The products of this reaction were novel dinucleotides. The values of the equilibrium constants for dinucleotide formation were determined for several drugs. These enzymes also efficiently catalyze the formation of novel mononucleotides in an exchange reaction with NMN+, kcat/KM = 0.05-0.4 μM−1 s−1. The kcat/KM values for the exchange reaction with NMN+ were generally similar (0.04-0.12 μM−1 s−1) with CD38 and ADP-ribosyl cyclase as catalysts. Several novel heterocyclic alternative substrates were identified as 2-isoquinolines, 1,6-naphthyridines and tricyclic bases. The kcat/KM values for the exchange reaction with these substrates varied over five orders of magnitude and approached the limit of diffusion with 1,6-naphthyridines. The exchange reaction could be used to synthesize novel mononucleotides or to identify novel reversible inhibitors of CD38. 相似文献
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955.
Qing-Yan Guo Long-Hua Zhang Chao Zuo Dong-Liang Huang Zhipeng A.Wang Ji-Shen Zheng Chang-Lin Tian 《蛋白质与细胞》2019,10(3):211-216
Dear Editor,It is known that most of lives on the earth compose of homochiral molecules of L-amino acids and D-ribose nucleic acids.However,little is known why and how the life's chirality in such a way.Studies on an artificial mirror-image life could strengthen our understanding of the question about the origin of life on the Earth and even elsewhere in the universe.Especially studies on mirror-image life would also have a plenty of vast application prospects in materials,energy and pharmaceutical sciences(Bohannon,2010). 相似文献
956.
非特异性脂质转移蛋白突变体的构建及在两种硫氧还蛋白表达载体中的表达比较 总被引:4,自引:0,他引:4
对水稻非特异性脂质转移蛋白(Nospecific lipid transfer protein,nsLTP) LTP110中结构重要的5个氨基酸位点进行了定点突变,测序结果证实了突变体构建成功。在尝试了多种大肠杆菌表达系统进行表达之后,发现硫氧还蛋白融合表达载体适合于LTP110野生型及突变体的表达。将编码野生型LTP110及突变体Y17A,P72L,R46A,D45A,C50A蛋白的cDNA顺序克隆进两种硫氧还蛋白表达载体并对其表达情况进行了比较:pTrxFus载体可以在宿主菌GI724中以较低水平表达野生型LTP110及突变体Y17A,P72L,R46A融合蛋白,但不能表达D45A和C50A融合蛋白;pET32a(+)载体可以在宿主菌BL21 (DE3) trxB-中以可溶蛋白的形式表达野生型及所有突变型融合蛋白,且表达量比在pTrxFus载体/GI724突主菌中表达量高。对pET32a(+)载体中表达的LTP110融合蛋白进行了纯化,并利用带有荧光标记的脂肪酸分子对其测活,结果表明表达的野生型LTP110分子具有结合脂质的活性。 相似文献
957.
赤链蛇染色体组型、C型和Ag—NORs的研究 总被引:1,自引:0,他引:1
以骨髓细胞为材料研究赤链蛇的染色体,结果表明该物种2n=46,由8对大型的和15对微小的染色体组成,AF=50。性染色体的大小介于3号和4号之间,为ZW;8大型染色体均显示着丝粒C带,1-6号还显示浅染端粒C带。W染色体为整条C带阳性,该物种一对NOR位于7号染色体近着丝粒区。不同地理分布群赤链蛇核型可能经历过Z与W染色体不等交换。 相似文献
958.
CREB Is One Component of the Binding Complex of the Ces-2/E2A-HLF Binding Element and Is an Integral Part of the Interleukin-3 Survival Signal
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Wannhsin Chen Yung-Luen Yu Shern-Fwu Lee Yun-Jung Chiang Jyh-Rong Chao Jin-Hwa Huang Jiao-How Chiong Chang-Jen Huang Ming-Zong Lai Hsin-Fang Yang-Yen Jeffrey J.-Y. Yen 《Molecular and cellular biology》2001,21(14):4636-4646
The Ces-2/E2A-HLF binding element (CBE) is recognized by Caenorhabditis elegans death specification gene product Ces-2 and human acute lymphocytic leukemia oncoprotein E2A-HLF. In an attempt to identify a cellular CBE-binding protein(s) that may be involved in apoptosis regulation in mammals, multiple nuclear binding complexes of CBE were identified in various mammalian cell lines and tissues by electrophoretic mobility shift assay. Cyclic AMP (cAMP)-responsive element (CRE)-binding protein (CREB) was present in one major CBE complex of Ba/F3 and TF-1 cells, and both in vitro-translated and Escherichia coli-synthesized CREB bound to CBE. Activation of CREB by cAMP-elevating chemicals or the catalytic subunit of protein kinase A (PKAc) resulted in induction of the CBE-driven reporter gene. Stimulation of Ba/F3 cells with interleukin-3 (IL-3) promptly induced phosphorylation of CREB at serine(133) partially via a PKA-dependent pathway. Consistently, Ba/F3 cell survival in the absence of IL-3 was prolonged by activation of PKA. Conversely, treatment of cells with a PKA inhibitor or expression of the dominant negative forms of the regulatory subunit type I of PKA and CREB overrode the survival activity of IL-3. Last, the bcl-2 gene was demonstrated to be one candidate cellular target of the CREB-containing CBE complex, as mutations in the CRE and CBE sites significantly reduced the IL-3 inducibility of the bcl-2 promoter. Together, our results suggest that CREB is one cellular counterpart of Ces-2/E2A-HLF and is part of IL-3 dependent apoptosis regulation in hematopoietic cells. 相似文献
959.
BACE蛋白的表达、纯化和活性测定 总被引:2,自引:0,他引:2
在大肠杆菌中表达、纯化并重新折叠以获得有活性的酸性蛋白水解酶 (BACE蛋白 )———一种与阿尔茨海默病 (AD)发病相关的蛋白水解酶。克隆BACE活性区的表达序列到原核表达载体 pET11a中 ,经E .coliBL2 1(DE3)表达 ,从包涵体中获取蛋白质 ,电泳鉴定后经梯度反向快速折叠法重新折叠 ,柱层析分离纯化 ,得到了表达的重组可溶性BACE蛋白 ;用高效液相色谱、质谱等方法检测其对人工合成多肽底物的水解作用 ;测定了BACE蛋白的酶促动力学常数。结果表明 ,得到的重组BACE蛋白具有水解人工合成小肽底物的活性。 相似文献
960.