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51.
The genetic regulation of stomatal movement mainly depends on an efficient control system of gene expression, and guard cell-specific promoter is becoming the best choice. Here we combined the dehydration responsive element (DRE) with guard cell specific element (GCSE) to construct a novel promoter, DGP1. Histochemical assays in transgenic tobacco carryingβ-glucuronidase (gus) gene fused to DGP1 demonstrated that GUS activity was found to be highly inducible by drought treatment and specifically restricted to guard cells. No GUS activity was detected in roots, stems or flowers after treatment. Further quantitative analysis showed that GUS activity in the epidermal strips was apparently induced by dehydration and dramatically increased with the elongation of treatment. The GUS activity after 8 h treatment was 179 times that of those without treatment. Although GUS activity in roots, stems or mesophyll increased after treatment, no great changes were observed. These results suggested that DGP1 could drive target gene expressed in guard cells when plant is subjected to drought stress. And this gets us prepared to control opening and closing of stomata through plant gene engineering.  相似文献   
52.
To observe the binding of plasmid DNA to non-nuclear DNA binding proteins in sarcoplasmic reticulum (SR) and the effects of this binding on SR function, sarcoplasmic reticulum proteins in rat skeletal muscle were isolated by differential centrifuge and sucrose density-gradient centrifuge. The results showed that there are two sequence-independent DNA binding proteins in SR proteins, the molecular weights of which are 83 and 58 ku, respectively. Ca2+ uptake and release of SR were remarkably promoted by the binding of plasmid DNA to DNA binding proteins in SR, the mechanism is probably through increasing of Ca2+-ATPase activity in SR and changing of character of Ca2+ release channel ryanodine receptors induced by the binding. These results suggest that there exist DNA binding proteins in SR and its binding to DNA may affect Ca2+ transport of SR.  相似文献   
53.
Several genetically stable mutants blocked in nikkomycin biosynthesis were obtained after the slightly germinated spores ofStreptomyces ansochromogenes, a nikkomycin producer, were treated with ultra violet radiation. One of the mutants is the same in morpholotical differentiation as the wild type strain and is designated as NBB19. A DNA library was constructed using plasmid pIJ702 as cloning vector, NBB19 as cloning recipient. A 6 kb DNA fragment which can genetically complement NBB19 was cloned when screening the library for antifungal activity. Sequence analysis showed that the 3 kbBgl II -Sal I fragment contains one complete ORF (ORF1) and one partial ORF (ORF2). ORF1 is designated assanA. sanA is 1 365 bp, encoding a protein consisting of 454 amino acid residues. Database searching indicated thatsanA is homologous to the hypothetical methyltransferase inPyrococcus horikoshii with 25% identities and 41% positives. Disruptant ofsanA lost the ability to synthesize nikkomycin. It indicated thatsanA is a novel gene which is essential for nikkomycin biosynthesis.  相似文献   
54.
Abstract The repeat sequence primer‐PCR technique was used to determine DNA polymorphism of the aphid Aphis gossypii (Glover) collected from 8 different localites in China. Three primers were selected and used for similarity index (SI) and cluster analysis based on the data of Nei's genetic distance (D). We found that the populations in the north and northwest of China was linked before they were joined by those in southern China. A proposed explanation emphasizes the populations in the north and northwest of China were located near — 4 °C isotherm or lower in January with less than 200 frost‐free days per year, whereas populations in southern China were located near 0 °C isotherm or higher with more than 300 frost ‐ free days per year. So it may be the over‐winter host plants instead of the geographic distance or gene flow, exert pronounced influence on the geographic population differentiation of A. gossypii. Species on different over‐winter host plants may directly lead to the genetic differentiation of their summer offsprings.  相似文献   
55.
利用差速离心法从牛脊髓中分离神经丝 ,在电镜下观察了其形态 ;应用扫描隧道显微镜 (STM)研究了它的结构 ,发现神经丝具有长短 2种侧臂 ,二者相间排列 ,相邻长侧臂或相邻短侧臂的间距都是 2 0~ 2 2nm ;由此推测神经丝内部存在 3 /4分子交错 ;还研究了神经丝蛋白的体外组装 ,以胶体金标记的方法证明 ,中等分子量与高分子量的神经丝蛋白 ,都能同低分子量的神经丝蛋白共同装配成 10nm的纤维 ;同时发现 ,中等分子量与高分子量的神经丝蛋白能够组装成一种较细的纤维 ,不同于中间纤维 .  相似文献   
56.
克隆及测定了水稻黄矮病毒基因组RNA的 3′端leader区和 5′端trailer区的序列 .结果表明 ,RYSV的 3′leader长 2 0 3个核苷酸 ,5′trailer长 191个核苷酸 .两者末端的 9个核苷酸完全互补 ,可形成弹状病毒基因组RNA的典型的锅柄结构 .与其他弹状病毒的leader和trailer相比较 ,RYSV的leader和trailer较长 ,除leader的 3′末端和trailer的 5′末端序列具有一定的保守性外 ,其余的核苷酸序列无明显的同源性 .用 3′RACE方法在感染RYSV的水稻中检测出leader的转录物 ,并证明该leaderRNA具有polyA尾巴 .这是继苦苣菜黄脉病毒的leaderRNA后第 2例弹状病毒leaderRNA带polyA尾巴的报道 .用类似的方法没有检测到带polyA尾巴的trailer的正链转录物 .  相似文献   
57.
通过将AFLP聚丙烯酰胺变性胶切小、适当曝光过量、以聚丙烯酰胺凝胶电泳代替琼脂糖电泳检测克隆片段大小的方法 ,增加了回收克隆AFLP阳性带的准确性。该方法对于从变性和非变性大page胶上回收克隆目的片段具有普遍意义。  相似文献   
58.
扬麦5号旗叶光合功能衰退进程中光合膜特性的变化   总被引:4,自引:0,他引:4  
旗叶自然衰退过程中光合膜特性变化的结果表明,光合功能高值持续期类囊体膜电子传递活性均维持较高水平,多肽组分也维持相对稳定;进入光合功能的速降期后,活性呈快速下降趋势,类囊体膜小分子多肽等组分均出现不同降解。旗叶全展后叶绿体ATP含量在高值持续期维持一定水平;进入速降期后,对应于光合膜电子传递活性及P/O值,叶绿体ATP含量变化存在“滞后”的现象;强光逆境下,速降期类囊体电子传递活性受抑制程度比高值  相似文献   
59.
按季节测定了莼菜生长周期呵溶性蛋白质、可溶性糖、脯氨酸以及水分的含量,测定结果表明冬芽越冬阶段其体现人可溶性蛋白质、可溶性9糖以及水分的含量较高,而脯氨酸却是一年中最低。这说明冬芽冬越期间其抗寒性的维持可能与体内高浓度的可溶性蛋白质,可溶性糖以及水分有关,而与脯氨酸无直接的关系。  相似文献   
60.
目的和方法:将不同剂量三氯化镧LaCl3注射大鼠侧脑室,观察下丘脑腹内侧(VMN)放电频率和血清生长素(GH)含量,研究LaCl3对神经内分泌的影响。结果:小剂量(0.005μmol)注射后可使VMN中GH相关神经元放明显增加,并可引起血清中GH含量的增加;而大剂量LaCl3(0.5μmol)组,VMN放电呈抑制反应,此组动物血清中GH含量呈减少趋势,明显低于小剂量组(P〈0.01),但与生理盐水  相似文献   
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