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101.
薛煜  邵力平 《植物研究》1995,15(2):189-190
采到骨状拟夏孢锈(Uredinopsis ossiformis Kamei)为中国新记录种。  相似文献   
102.
钙调素对细胞周期的调节   总被引:1,自引:0,他引:1  
RC3细胞是一种用真核表达载体1~(CaM)转染NIH 3T3细胞建成的可调钙凋素(Calmodulin,CaM)高表达细胞模型。通过分子杂交及蛋白免疫印迹方法证实在地塞米松(Dexamethasome,DXM)作用下,RC3细胞可高表达CaM。CaM的过表达使G_1期细胞减少,S期细胞增加;CaM拮抗剂三氟拉嗪(trifluoperazine,TFP)则使G_1期细胞增加,S期细胞减少。高表达CaM使细胞分裂指数提高,G_2期细胞减少,有丝分裂前期细胞增加,M中期细胞比例下降。而TFP处理则使分裂指数下降,G_2期细胞增加,M前期细胞减少,M中期细胞增加。实验结果表明CaM在G_1/S、G_2/M和M中期/M后期3个位点上对细胞周期进行调控;通过加速G_1至S期,G_2至M期和M中期至M后期的进程,使细胞倍增时间缩短,促进细胞增殖。本工作表明,RC3细胞作为CaM表达可调细胞模型,是研究细胞周期调控的有力工具。  相似文献   
103.
在长白山地区以红皮云杉、樟子松为材料,研究其冬季光合能力的变化,探讨了除红松外的其它针叶树是否在冬季也存在光合抑制以及遮荫是否可减轻抑制等问题,结果表明,红皮云杉、樟子松有与红松相似的冬季光合抑制,但程度较轻;遮荫对减轻光合抑制非常有效,可以推测,在长白山地区或冬季气候与之相似的地区,常绿针叶树在冬季均可能表现光合抑制,遭受冬季光氧化伤害,并且其释放的CO2(光越强,释放量越大)是空气中CO2含量  相似文献   
104.
A组轮状病毒SA11VP6基因的克隆和表达   总被引:4,自引:0,他引:4  
晋圣瑾  方肇寅 《病毒学报》1995,11(2):119-123
从SA11VP6基因全序列克隆开始,设计一对两端带有酶切位点的引物,逆转录PCR扩增出VP6全基因CDNA。经酶切后插入PUC19,构建了VP6全基因克隆PRA6。再经酶切后插入痘苗病毒载休质凿PJSA1175中。利用Lipofectin导入TK143细胞,利用TK基因和Lac基因作为重组病毒的筛选标记。表达产物用单克隆抗体ELISA法检测,发现细胞培养上清和细胞裂解液都是阳性。Western b  相似文献   
105.
在我国腹泻患儿中发现诺瓦克样病霉感染   总被引:6,自引:0,他引:6  
诺瓦克病毒是引起无菌性急性胃肠炎爆发的重要病原。1990年10月至1991年1月从河南省急性腹泻门诊患儿便样中发现了诺瓦克样病毒。经电镜观察,病毒直径约为28nm,病毒壳似由有结构的亚单位组成,进一步用诺瓦克病毒特异的寡核苷酸引物做逆转录一聚合酶链式反应(RT-PCR),检定为阳性。由PCR产物测得的核苷酸序列与诺瓦克病毒原型株相应序列比较,同源性为72%。以上结果证实,在我国腹泻病人中有诺瓦克样病毒感染。这对我国病毒性胃肠炎流行的防治研究具有重要意义。  相似文献   
106.
新疆呼图壁盐化草甸群落的DCA, CCA及DCCA分析   总被引:15,自引:1,他引:14       下载免费PDF全文
 本文应用DCA、CCA及DCCA排序技术对新疆呼图壁盐化草甸群落进行了分析。分析中选取了地下水位、粘土层出现深度、粘土层厚度、地下水pH值及地下水矿化度5个环境因子;同时为了分析空间格局对植被分异影响的大小,建立了样地空间坐标矩阵。结果表明:地下水位和地下水的pH值是引起植被分异的两个主要因素,空间格局对植被分异的影响大于环境因子对植被分异的影响。  相似文献   
107.
温度对黄粉虫成虫繁殖的影响   总被引:2,自引:0,他引:2  
黄粉虫是多种小型经济动物的常用优良饵料,本试验在20.1℃,24.0℃、28.5℃、31.7℃和36.5五种恒温下饲养该成虫结果,成虫寿命平均分别为63.0、54.2、38.8、38.0和26.1天;每雌平均产卵量则分别为200.3、207.3、122.3、115.8和81.2粒,成虫平均生产1g卵消耗麸皮量分别为2.66、2.00、2.19、2.14和4.15g。结果说明人工繁殖黄粉虫的成虫期温度以24℃为最适宜。  相似文献   
108.
A uniparental mitochondrial (mt) transmission pattern has been previously observed in laboratory matings of the cultivated mushroom Agaricus bisporus on petri dishes. In this study, four sets of specific matings were further examined by taking mycelial plugs from the confluent zone of mated homokaryons and inoculating these plugs into rye grain for laboratory fruiting and for fruiting under industrial conditions. Examination of the mt genotype of each individual fruit body for mt-specific restriction fragment length polymorphisms further confirmed that the mt genome was inherited uniparentally. The vegetative radial growth and the fruiting activity of two pairs of intraspecific heterokaryons, each pair carrying the same combination of nuclear genomes but different mt genotypes, were compared. Our results suggested that the mt genotype did not appreciably affect radial growth or fruiting activity. The failure to recover both heterokaryons, each carrying either parental mt genotype in any given cross, therefore clearly indicated that in matings of A. bisporus, the mt genome from one of the parental homokaryons is either selectively excluded in the newly formed heterokaryon or selectively eliminated in the immediate heterokaryotic mitotic progeny of the newly formed heterokaryon.  相似文献   
109.
The ability of 2-n-propyl-4-pentenoic acid (Δ4-VPA) and 2-n-propyl-2(E)-pentenoic acid ([E]-Δ2-VPA), two unsaturated metabolites of valproic acid (VPA), to form reactive intermediates, deplete hepatic glutathione (GSH) and cause accumulation of liver triglycerides was investigated in the rat. With the aid of ionspray liquid chromatography-tandem mass spectrometry (LC-MS/MS), three GSH adducts were detected in the bile of Δ4-VPA-treated animals and were identified as 4-hydroxy-5-glutathion-S-yl-VPA-γ-lactone, 5-glutathion-S-yl-(E)-Δ3-VPA and 3-oxo-5-glutathion-S-yl-VPA. A fourth conjugate was identified tentatively as 4-glutathion-S-yl-5-hydroxy-VPA. Quantitative analysis of the corresponding N-acetylcysteine (NAC) conjugates in urine indicated that metabolism of Δ4-VPA via the GSH-dependent pathways accounted for approximately 20% of an acute dose (100 mg kg−1 i.p.). In contrast, when rats were given an equivalent dose of (E)-Δ2-VPA, only one GSH adduct (5-glutathion-S-yl-(E)-Δ3-VPA) was detected at low concentrations in bile. In vitro experiments with rat liver mitochondria demonstrated that Δ4-VPA undergoes coenzyme A- and ATP-dependent metabolic activation in this organelle via the β-oxidation pathway to intermediates which bind covalently to proteins. When liver homogenates and hepatic mitochondria from rats injected with Δ4-VPA, (E)-Δ2-VPA or VPA were analyzed for GSH content, it was found that only Δ4-VPA depleted GSH pools significantly. Treatment of rats with Δ4-VPA and (to a lesser extent) VPA led to an accumulation of liver triglycerides, whereas (E)-Δ2-VPA had no measurable effect. It is concluded that Δ4-VPA undergoes metabolic activation by both microsomal cytochrome P-450-dependent and mitochondrial coenzyme A-dependent processes, and that the resulting electrophilic intermediates, which are trapped in part by GSH, may mediate the hepatotoxic effects of this compound. In contrast, (E)-Δ2-VPA is not transformed to any appreciable extent to reactive metabolites, which thus accounts for the apparent lack of hepatotoxicity of this positional isomer in the rat.  相似文献   
110.
The nucleotide sequence was determined of the region upstream of the mukB gene of Escherichia coli. Two new genes were found, designated kicA and kicB (killing of cell); the gene order is kicB-kicA-mukB. Promoter activities were detected in the regions immediately upstream of kicB and kicA, but not in front of mukB. Gene disruption experiments revealed that the kicA disruptant was nonviable, but the kicB-disrupted mutant and the mutant lacking both the kicB and kicA genes were able to grow. When kicA disruptant cells bearing a temperature-sensitive replication plasmid carrying the kicA + gene were grown at 30° C and then transferred to 42° C, the mutant cells gradually lost colony-forming ability, even in the presence of a mukB + plasmid. Rates of protein synthesis, but not of RNA or DNA synthesis, fell dramatically during incubation at 42° C. These results suggested that the kicB gene encodes a killing factor and the kicA gene codes for a protein that suppresses the killing function of the kicB gene product. It was also demonstrated that KicA and KicB can function as a post-segregational killing system, when the genes are transferred from the E. coli chromosome onto a plasmid.  相似文献   
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