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71.
Columnar apple is an important genetic resource for tree form breeding of apple. In this study, 106 individuals of the F1 population derived from 'Spur Fuji' (coco)x 'Telamon'(Coco) were used as plant materials for screening SSR markers linked to gene. By bulked segregating analysis (BSA), eight SSR markers from the tenth linkage group of apple genome were tested. Finally, three of them, COL, CH02a10 and CH03d11, were identified to be SSR markers of Co gene. Linkage analysis showed that the genetic distance of COL, CH02a10 and CH03d11 to Co locus was 15.3cM, 22.2cM and 3.9 cM, respectively. On the linkage map of these markers, Co gene was located between COL and CH03d11.  相似文献   
72.
环鸟苷酸对卵巢细胞功能的调控   总被引:4,自引:0,他引:4  
环鸟苷酸(cGMP)是一种具有广泛生物学活性的环核苷酸。尽管cGMP作为第二信使,在调控卵巢细胞功能中发挥着广泛而重要的作用早有报道,但直至近年,cGMP在生殖活动中的重要作用才受到人们的关注,而成为生殖科学研究领域的热点之一。卵巢是雌性动物的重要器官,而cGMP在卵巢细胞中起着多方面的调节作用。现对卵巢内cGMP的来源,cGMP在卵巢内抑制雌激素(E2)的合成、LH受体表达、卵泡闭锁的作用,以及cGMP的作用机制等方面的研究进展进行综述。  相似文献   
73.
Dilution and copepod addition incubations were conducted in the Yellow Sea (June) and the East China Sea (September) in 2003. Microzooplankton grazing rates were in the range of 0.37–0.83 d−1 in most of the experiments (except at Station A3). Correspondingly, 31–50% of the chlorophyll a (Chl a) stock and 81–179% of the Chl a production was grazed by microzooplankton. At the end of 24 h copepod addition incubations, Chl a concentrations were higher in the copepod-added bottles than in the control bottles. The Chl a growth rate in the bottles showed good linear relationship with added copepod abundance. The presence of copepods could enhance the Chl a growth at a rate (Z) of 0.03–0.25 (on average 0.0691) d−1 ind−1 l. This study, therefore parallels many others, which show that microzooplankton are the main grazers of primary production in the sea, whereas copepods appear to have little direct role in controlling phytoplankton.  相似文献   
74.
水培经济植物对污水中磷的吸收利用及去除效果   总被引:13,自引:0,他引:13  
对13种经济植物在污水水培条件下净化污水中磷的能力进行了研究。结果表明,黑麦草(Lolium multiflorum)、水芹(Oenanthe stolonifera)、莴苣(Lactuca sativavar.angustana)、酸模(Poly-gonum iapathifolium)、生菜(Lactuca sativa)、小葱(Allium ascalonicum)、五月慢青菜(Brassica chinen-sis)等品种具有较高的净化能力。在4个半月的水培中,TP的去除量分别达到10.27、10.35、6.5~6.896、.91、5.72、5.46和6.19 g.m-2;TP的去除率分别达到94.5%、95.2%、93.6%~99.3%、99.6%、99.5%、95%和89.2%。植物吸收作用是最主要的污水磷去除机制,沉淀在污水磷净化中的作用较小。污水中磷的去除与植物的生长期密切相关。黑麦草、水芹等7种植物适宜作为苏南地区冬季化粪池污水水培植物。  相似文献   
75.
近几年来,DNA疫苗以其高效、稳定等特点越来越受到各国研究者的重视,并在鱼类生产上做了很多试验研究,取得了一定的成果。就DNA疫苗的构建、作用原理、佐剂、接种方法、安全性、目前存在的问题及应用前景作一综述。  相似文献   
76.
STAT6 ASODN对哮喘小鼠脾淋巴细胞影响的实验研究   总被引:1,自引:0,他引:1  
目的研究STAT6反义寡核苷酸对哮喘小鼠脾淋巴细胞的影响作用。方法实验细胞分组:正常鼠空白组(A组)、正常鼠OVA组(B组)、哮喘空白组(C组)、哮喘OVA组(D组)、哮喘治疗组(E组)。正常设计并人工合成一段互补于小鼠STAT6 mRNA翻译起始区271-290的反义寡核苷酸片段,全链硫代修饰。用卵白蛋白和氢氧化铝复制哮喘模型,用淋巴细胞分离液分离脾淋巴细胞,进行体外培养并导入由阳离子脂质体转染剂Geneshuttle携带的反义寡核苷酸,观察反义寡核苷酸的转染对脾淋巴细胞STAT6蛋白表达水平及细胞培养上清中IL-4分泌水平的影响。免疫细胞化学观察脾淋巴细胞中STAT6蛋白的表达水平,同时采用酶联免疫吸附(ELISA)法测定脾细胞培养上清液中IL-4的浓度。结果D组细胞STAT6蛋白表达明显高于其余各组,均具有显著性差异(P均<0.01),STAT6 ASODN转染后,E组细胞该蛋白的表达量明显下降(P<0.01);D组脾淋巴细胞培养上清中IL-4分泌水平明显高于其余各组,均具有显著性差异(P均<0.01);STAT6 ASODN转染后,E组培养上清中IL-4分泌水平显著低于D组(P<0.01)。结论STAT6 ASODN可特异性抑制哮喘鼠脾淋巴细胞中STAT6蛋白的表达,并可特异性抑制脾淋巴细胞中IL-4的分泌,为反义基因技术治疗哮喘提供了依据。  相似文献   
77.
目的研究β-cat在新生儿细支气管中的表达情况,探讨β-cat在新生儿支气管发育中的作用。方法采用免疫组化(SP)法,检测22例尸检新生儿β-cat、GSK-3β在细支气管上皮细胞的表达,以12例儿童为对照。结果β-cat在新生儿组有6例出现细胞膜表达降低、3例出现胞质表达、2例胞核表达;对照组中2例胞膜表达减少,1例胞质表达。β-cat的平均光密度值在新生儿组为0·112±0·024,对照组为0·128±0·037。两组比较P>0·05,无显著性差异;GSK-3β平均光密度值在对照组为0·147±0·037,新生儿组为0·115±0·028,两组比较P<0·05,有显著性差异。结论β-cat在新生儿细支气管的异位表达,提示Wnt信号与支气管的发育成熟有关。  相似文献   
78.
浙江天童常绿阔叶林中11种常绿乔灌木叶片虫食状分析   总被引:3,自引:0,他引:3  
为探讨昆虫对植物叶片的取食行为和伤害方式,作者选择浙江天童常绿阔叶林内的11种常绿乔灌木为对象,对叶片虫食状类型和格局进行分析。结果如下:(1)共发现16种虫食状类型,每种植物叶片虫食状类型数在10–13种之间,每种虫食状出现频率在0.5–28.7%之间。缘食状出现频率最高(28.7%),虫瘿和泡状出现频率最低(0.5%)。(2)叶片虫食状分布格局可分为3种类型,即一种虫食状占绝对优势的单优格局,如马银花(Rhododendronovatum)和檵木(Loropetalumchinense);两种虫食状(缘食状和顶食状)共占优势的双优格局,仅有木荷(Schimasu-perba);3种及3种以上虫食状占优势的多优格局(其余8种植物)。(3)叶片虫食状多样性指数变化在1.57–2.23之间,最高为苦槠(Castanopsissclerophylla),最低为马银花;乔木的多样性指数(2.040)高于灌木(1.882),优势种多样性指数高于伴生种,但差异均不显著;多样性指数反映了虫食状类型和出现频率的综合差异。(4)16种虫食状类型中有8对显著正相关,4对显著负相关,可能反映出不同类型昆虫取食植物的趋同和差异。  相似文献   
79.
In vitro fertilization (IVF) of isolated male and female gametes of flowering plants was first accomplished in the last decade. Successful isolation of male and female gametes, and culturing of in vitro zygotes to form new plants, is a prelude to the use of IVF for research into the cellular and molecular control of fertilization in higher plants and its application as a tool in biotechnology. Genes unique to male and female gametes and zygotes of higher plants, although currently incompletely characterized, are expected to permit direct molecular dissection of fertilization. By applying IVF and microculture to zygotes and endosperm obtained by both in vivo and in vitro methods, newly activated fusion products may be observed and manipulated in media where they are directly accessible to the techniques of molecular cell biology. IVF and zygote culture may also offer potential for creating new hybrid plants by fusing isolated gametes from different species to produce unique zygotes and ultimately plants that would be impossible to obtain using typical crossing techniques. Transformation and regeneration frequencies using IVF may also be high enough to avoid the necessity of adding controversial antibiotic and herbicide resistant genes to screen transformed products. This review describes advances using IVF in plant sexual reproduction and discusses its potential in the genetic improvement of flowering plants.  相似文献   
80.
A superior novel recombinant strain, E. coli BL21(DE3)/pETNHM, containing the start codon mutation of the subunit, was constructed and selected as an overexpression and high efficient mutation platform for the genetic manipulation of the nitrile hydratase (NHase). Under optimal conditions, the specific activity of the recombinant strain reached as high as 452 U/mg dry cell. Enzymatic characteristics studies showed that the reaction activation energy of the recombinant NHaseM was 24.4 ± 0.5 kJ/mol, the suited pH range for catalysis was 5.5–7.5, and the Km value was 4.34 g/L (82 mM). To assess the feasibility of the NHase improvement by protein rational design using this E. coli, site-directed mutagenesis of S122A, S122C, S122D and βW47E of the NHaseM were carried out. The NHaseM (S122A) and NHaseM (S122D) mutants were entirely inactive due to the charge change of the side-chain group. The product tolerance of the NHaseM (S122C) mutant was enhanced while its activity decreased by 30%. The thermo-stability of the NHaseM (βW47E) mutant was significantly strengthened, while its activity reduced by nearly 50%. These results confirmed that the specific activity of the mutant NHase expressed by the recombinant E. coli BL21(DE3)/pETNHM can reasonably change with and without mutations. Therefore, this recombinant E. coli can be efficiently and confidently used for the further rational/random evolution of the NHase to simultaneously improve the activity, thermo-stability and product tolerance of the target NHase.  相似文献   
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