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11.
The traditional culture-dependent plate counting and culture-independent small-subunit-ribosomal RNA gene-targeted molecular techniques, Single-Strand Conformation Polymorphism (SSCP) and ter-minal Restriction Fragment Length Polymorphism (tRFLP) combined with 16S rDNA clone library were adopted to investigate the impacts of secretion from Camptotheca acuminata (abbreviated to Ca) roots on the quantities and structure of eukaryotic microbes and bacteria in the rhizosphere, and the possi-bility that Ca controls exotic invasive plant Eupatorium adenophorum (Ea). The counting results indi-cated that the number of bacteria increased in turn in rhizospheres of Ea, Ca-Ea mixed culture and Ca, while that of eukaryotic microbes decreased. PCR-SSCP profiles showed eukaryotic microbial bands (corresponding to biodiversity) in rhizosphere of Ea were more complex than those of Ca and CE. Meristolohmannia sp., Termitomyces sp. and Rhodophyllus sp. were the dominant populations in the rhizosphere of Ca. Bacterial terminal restriction fragments (TRFs) profiles showed no difference among three kinds of rhizospheres, and the sequences of the 16S rDNA clone library from Ca rhizospheres were distributed in 10 known phyla, in which phylum Proteobacteria were the absolute dominant group and accounted for 24.71% of the cloned sequences (δ-Proteobacteria accounted for up to 17.65%), and phyla Acidobacteria and Bacteroidetes accounted for 16.47% and 10.59% of the cloned sequences, respectively. In addition, high performance liquid chromatography detected a trace amount of camp-tothecin and hydroxycamptothecin in the rhizospheric soil of Ca and CE, but examined neither camp-tothecin nor hydroxycamptothecin in rhizospheric soil of Ea. Therefore, invasion and diffusion of Ea evidently depended on distinguishing the eukaryotic community structure, but not on that of the bac-terial pattern. Ca was able to alter the eukaryotic community structure of invasive Ea by secreting camptothecin and hydroxycamptothecin into rhizospheres, and may benefit the control of overspread of Ea. This study provided theoretical evidence for rhizospheric microbial aspects on substituting Ca for Ea.  相似文献   
12.
喜树细胞悬浮培养中生理生化指标的测定   总被引:5,自引:0,他引:5  
以喜树(Camptotheca acuminata Decsne.)幼嫩叶片为材料,诱导和筛选愈伤组织,进行细胞悬浮培养。初步研究了液体培养条件下光照对喜树细胞生长和生理生化特性的影响。结果显示:在光照条件下培养细胞生长周期30d,在黑暗条件下培养细胞生长周期为27d,细胞的增殖曲线呈“S”形;在两种不同光照条件下,其培养液pH值先下降后回升;培养细胞中可溶性蛋白质含量及过氧化物酶活性均出现两个峰值,但出现的时间不同。  相似文献   
13.
To understand soil colonization by a root system, information is needed on the architecture of the root system. In monocotyledons, soil exploration is mainly due to the growth of adventitious primary roots. Primary root emergence in banana was quantified in relation to shoot and corm development. Root emergence kinetics were closely related to the development of aerial organs. Root position at emergence on the corm followed an asymptotic function of corm dry weight, so that the age of each root at a given time could be deduced from its position. Root diameter at emergence was related to the position of the roots on the corm, with younger roots being thicker than older ones. However, root diameters were not constant along a given root, but instead decreased with the distance to the base; roots appear to be conical in their basal and apical parts. Root growth directions at emergence were variable, but a high proportion of the primary roots emerged with a low angle to the horizontal. Further research is needed to evaluate whether these initial trajectories are conserved during root development. Results presented in this study are in good agreement with those reported for other monocotyledons such as maize and rice. They give quantitative information that will facilitate the development of models of root system architecture in banana.  相似文献   
14.
Fluorescent in situ hybridisation (FISH) was used to determine the number and distribution of the 18S-25S and 5S rDNA sites on mitotic chromosomes of 6 wild and 2 edible diploid (2n=22) accessions belonging to the two banana species, Musa acuminata and M. balbisiana. FISH with the 18S-25S probe resulted in signals on one pair of chromosomes, the position of signals corresponded to the secondary constriction at the end of a short arm. The intensity of labelling was different between the homologues and the larger site corresponded to a larger secondary constriction. This labelling pattern was observed consistently in all genotypes. On the other hand, differences in the number of 5S sites were observed between the accessions. While in some of the wild seeded species, the 5S rDNA was localised on two pairs of chromosomes, hybridisation signals appeared on three pairs of chromosomes in other wild accessions. Quite unexpectedly, only five sites of 5S rDNA were reproducibly observed in the two vegetatively propagated diploid edible cultivars, Pisang Mas and Niyarma Yik, evidence for structural heterozygosity. A dual colour FISH showed that in all accessions, the satellite chromosomes carrying the 18S-25S loci did not carry the 5S loci. The results demonstrate that molecular cytogenetics can be applied to Musa and that physical cytogenetic maps can be generated. This revised version was published online in July 2006 with corrections to the Cover Date.  相似文献   
15.
从香蕉cDNA文库中克隆到了一个香蕉(Musa acuminata AAA subgroup)乙二醛酶(glyoxalase,GLO)基因(MaGLO14)。构建了带有MaGLO14的酵母表达载体PYES2-MaGLO14,转化酿酒酵母(Saccharomyces cerevisiae)尿嘧啶营养缺陷型菌株INVSC1,挑取转化子进行PCR和酶切鉴定,证实获得了转基因菌株。通过比较转基因菌株和非转基因菌株在NaCl、高温、低温、干旱、UV胁迫下的生长状况,证明转基因菌株在以上非生物胁迫条件下的存活菌落数均高于非转基因菌株。利用酿酒酵母初步证明MaGLO14具有增强酵母菌对非生物胁迫抵抗力的功能。  相似文献   
16.
【背景】投加微生物菌剂是强化生物处理效能的重要手段,反硝化是污水脱氮除磷的关键步骤,但目前对于反硝化微生物菌剂相关的研究报道较少。【目的】驯化高效反硝化聚磷菌菌剂,并对系统进行生物强化。【方法】采用两阶段法快速富集反硝化聚磷菌,筛选高效脱氮除磷功能菌株NC1-1并进行鉴定,以NC1-1为菌种来源制备干粉菌剂,研究菌剂强化A2SBR系统污水处理效果。【结果】历经36 d后反硝化聚磷菌富集成功,菌株NC1-1经鉴定属于戈登氏菌属,其脱氮除磷率分别为89.46%和91.68%。麦麸、玉米粉配比为85%:15%、NC1-1投菌量为20 mL、发酵液用量20 mL的条件下成功制得干粉菌剂,干粉菌剂最佳投加量为10%的A2SBR系统总磷(total phosphorus,TP)和NO3--N去除率比未投加菌剂的A2SBR系统提高12.06%和11.52%。【结论】菌剂NC1-1的投加使A2SBR系统的污染物去除效能进一步提高,研究结果为进一步研究反硝化聚磷菌菌剂提供了...  相似文献   
17.
采用高效液相色谱法和生物量法,以四川种源的普通喜树为对照,对生长季内喜树新品系海喜1号不同冠层枝叶喜树碱产量进行了测定。结果表明:由于海喜1号枝叶喜树碱含量、生物量均高于普通喜树,其产量更加显著地高于普通喜树;虽然海喜1号幼嫩的上层枝叶喜树碱含量高于中层和下层,但由于生物量偏低,产量明显低于中下层枝叶;虽然基于喜树碱含量较高(即优质为目标时),采收期应确定为6月份,但为了达到持续产量,在6月份可采收上层枝叶,7~10月以适度透光为方法连续采收中下部枝叶,11月份,即生长季末采收冠层下部全部1/3枝叶。  相似文献   
18.
The deacylated phosphatidylinositol manno-oligosaccharides (dPIMs) from the glycosyl phosphatidylinositol (GPI) carbohydrate antigen anchor of Gordonia sputi were the known 2,6-di-O-alpha-mannopyranosyl-myo-inositol glycerophosphate (dPIM-2) and the illustrated novel compound (dPIM-8), which could not be separated from dPIM-7 and dPIM-6, these three compounds being present in the mixture in the molar ratios 1.0:0.65:0.4. dPIM-8 is an analogue of dPIM-2 (and also of dPIM-7 and dPIM-6) in having alpha-mannopyranose and an alpha-mannopyranosyl linked heptasaccharide bonded to O-2 and O-6, respectively, of the inositol. The dPIM-8 species has not been found previously. [structure: see text]  相似文献   
19.
利用PCR方法扩增香蕉红素氧还蛋白基因的保守结构域序列CdRD和开放性阅读框序列FRD,并在其上下游分别引入NdeⅠ和SalⅠ酶切位点,双酶切后与同样经NdeⅠ和SalⅠ双酶切的诱饵质粒载体pGBKT7连接,构建重组诱饵质粒pGBKT7-CdRD和pGBKT7-FRD,并将此两重组诱饵质粒转入酵母菌株AH109中进行营养缺陷型分析检测毒性及自激活。结果表明,成功构建了重组诱饵质粒pGBKT7-CdRD和pGBKT7-FRD,并且其无自激活报告基因作用,对酵母菌株也无毒性作用。这说明此两个重组诱饵质粒可用于酵母双杂交系统,为从香蕉叶片cDNA文库中筛选获得与香蕉红素氧还蛋白基因的保守结构域序列CdRD和开放性阅读框序列FRD相互作用的受体蛋白基因奠定了基础。  相似文献   
20.
不同种源喜树幼枝中喜树碱的含量   总被引:7,自引:0,他引:7  
通过HPLC测定了喜树(Camptotheca acuminata)不同器官及不同种源幼枝中喜树碱的含量.结果表明,喜树碱含量在叶、种子和幼枝(幼叶和幼茎)中较高,木质部中较少,髓中最低.不同种源的幼枝中,来自成都种源喜树的喜树碱含量最高.通过比较,两年生喜树各器官中喜树碱含量普遍比一年生高,幼枝中顶枝的喜树碱含量比侧枝高.  相似文献   
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