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141.
Toru Terachi 《Journal of plant research》1993,106(1):75-79
Recent advances in manipulating nucleic acids have opened a new research field called plant molecular systematics. This short
review provides an overview of molecular techniques which have been used in the analysis of DNA molecules for the study of
plant systematics, with a special emphasis on PCR. The early application of DNA analysis, DNA/DNA hybridization, has not become
popular with plant systematists, because of several disadvantages inherent in the method. The survey of restriction fragment
length polymorphisms (RFLPs), on the contrary, has become one of the preferred methods used by plant molecular systematists,
since the method is relatively easy to perform. Although unambiguous data can be obtained by both long-range restriction mapping
and nucleotide sequencing, these approaches may have limited use in plant molecular systematics because of their laborious
experimental procedures relying on conventional molecular cloning techniques. To date, PCR based analyses of the DNA molecule
seem to be the most suitable experimental approach for plant molecular systematics. Several advantages of the method have
changed both the quality and quantity of the DNA data. Further application of PCR to plant molecular systematics will open
up a new era in the field.
The present paper is based on the contribution which was read in a symposium entitled “Organellar DNA Variations in Higher
Plants and their Taxonomic Significance”, at the 50th Annual Meeting of the Botanical Society of Japan in Shizuoka on October
2, 1990, under the auspices of the Japan Society of Plant Taxonomists. 相似文献
142.
增强型绿色荧光蛋白(enhanced green fluorescent protein,EGFP)是一种优化的突变型GFP,DFL是从甘菊中分离出的LFY基因的同源序列。为了研究DFL基因的功能和表达模式,研究利用小片段克隆法将linker序列插入到EGFP基因5′端启始密码子前面,在pBI121载体的CaMV35S启动子的3′端后面插入一段多克隆位点,成功地构建了pBI-DFL-EGFP表达载体。通过设计特异引物,利用PCR技术扩增得了到拟南芥LFY基因的启动子序列,用粘性末端PCR技术将pBI-DFL-EGFP表达载体中CaMV35S启动子替换成LFY基因启动子,构建成了pLFY-DFL-EGFP表达载体。用含有pBI-DFL-EGFP和pLFY-DFL-EGFP质粒的农杆菌侵染洋葱表皮细胞,在荧光显微镜下分别用蓝光激发,均观测到了荧光。这一结果表明,融合蛋白DFL∷EGFP表达载体构建成功,同时还证明了通过PCR技术克隆到的LFY启动子序列具有启动子功能。 相似文献
143.
144.
Yang Ping He Yu-quan Zeng Hong Ni Jin-song Yun Qing-jun Huang Xiao-ping Li Shu-mei .Cadiovascular Department China-Japan Union Hospital of Jilin University Changchun P. R. China . Department of Pathdogy School of Basic Medical Sciences of Jilin University Changchun P. R. China . Cardiovascular Department Second Hospital of Jilin University Changchun P. R. China 《仿生工程学报(英文版)》2005,2(2):87-91
1Introduction Congestiveheartfailureisamultipleaetiology,high prevalence,cardiovasculardisorderwithpoorprognosis. Medicaltreatmentofdilatedcardiomyopathyisaimedat alleviatingthesymptomsofheartfailure.Diuretics,ACE inhibitorsandbeta blockershavefavourableeffectson symptoms,exercisecapacityandmortality[1-3].Growth hormone(GH)andinsulin likegrowthfactor(IGF) 1 areinvolvedinseveralphysiologicalprocessessuchas thecontrolofmusclemassandfunction,bodycomposi tionandtheregulationofnutrientmetaboli… 相似文献
145.
目的:克隆与表达辣根过氧化物酶同功酶C3(HRPC3)基因。方法:用PCR方法从辣根的总DNA中,扩增得到一种辣根过氧化物酶同功酶C3基因,将PCR产物连接到pMD18-T载体上,测序证明正确后,再将目的基因正确插入到巴斯德毕赤酶母表达载体pPIC9K中,含有目的基因的重组pPIC9K质粒在毕赤酶母中进行表达与分析。结果:应用毕赤酶母作为受体菌,成功表达了HRPC3基因,其活性为56IU/L。结论:毕赤酶母直接表达出了具有生物活性的辣根过氧化物酶同功酶C3。 相似文献
146.
A quantitative real-time PCR method for in planta monitoring of Phytophthora infestans growth 总被引:1,自引:0,他引:1
Llorente B Bravo-Almonacid F Cvitanich C Orlowska E Torres HN Flawiá MM Alonso GD 《Letters in applied microbiology》2010,51(6):603-610
Aim: To develop a real‐time PCR‐based strategy for the detection of Paenibacillus larvae vegetative cells and spores to improve the diagnosis and the screening of American foulbrood (AFB), the most harmful pathology of honeybee brood. Methods and Results: A real‐time PCR that allowed selective identification and quantification of P. larvae 16S rRNA sequence was developed. Using standard samples quantified by flow cytometry, detection limits of 37·5 vegetative cells ml?1 and 10 spores ml?1 were determined. Compared to spread plate method, this real‐time PCR‐based strategy allowed, in only 2 h, the detection of P. larvae in contaminated honeys. No false‐positive results were obtained. Moreover, its detection limit was 100 times lower than that of the culture method (2 vs 200 spores g?1 of honey). Conclusion: A rapid, selective, with low detection limit, sensitive and specific method to detect and quantify vegetative cells and spores of P. larvae is now available. Significance and Impact of Study: In addition to honey samples, this real‐time PCR‐based strategy may be also applied to confirm AFB diagnosis in honeybee brood and to screen other apiary supplies and products (bees, pollen, wax), thus broadening the control of AFB spreading. 相似文献
147.
Hidetaka Suzuki Seiko YamadaYoshiharu Toyama Shigeki Takeda 《Biochimica et Biophysica Acta - Proteins and Proteomics》2010,1804(9):1738-1742
The Mu phage virion contains tail-spike proteins beneath the baseplate, which it uses to adsorb to the outer membrane of Escherichia coli during the infection process. The tail spikes are composed of gene product 45 (gp45), which contains 197 amino acid residues. In this study, we purified and characterized both the full-length and the C-terminal domains of recombinant gp45 to identify the functional and structural domains. Limited proteolysis resulted in a Ser64-Gln197 sequence, which was composed of a stable C-terminal domain. Analytical ultracentrifugation of the recombinant C-terminal domain (gp45-C) indicated that the molecular weight of gp45-C was about 58 kDa and formed a trimeric protomer in solution. Coprecipitation experiments and a quartz crystal microbalance (QCM) demonstrated that gp45-C irreversibly binds to the E. coli membrane. These results indicate that gp45 shows behaviors similar to tail-spike proteins of other phages; however, gp45 did not show significant sequence homology with the other phage tail-spike structures that have been identified. 相似文献
148.
目的:制备黄热病病毒寡核苷酸检测微阵列.方法:根据黄热病病毒基因组序列,并应用生物信息学软件设计出寡核苷酸探针用于制备基因芯片,克隆于质粒上的黄热病病毒全长基因DNA经限制性显示技术扩增并标记,完成杂交后对芯片进行扫描和数据分析.结论:微阵列检测技术为检测黄热病病毒提供了一种早期、快速、可靠的方法,具有应用于临床检测的前景. 相似文献
149.
Tzyy‐Rong Jinn Suey‐Sheng Kao Yin‐Chin Tseng Ying‐Ju Chen Tzong‐Yuan Wu 《Biotechnology progress》2009,25(2):384-389
The baculovirus–insect expression system is a popular tool for recombinant protein production. The standard method for infecting insect larvae with recombinant baculovirus for protein production involves either feeding occlusion bodies or injecting budded virus into the cuticle. In this study, we showed that the recombinant Autographa californica multiple nucleopolyhedrovirus (AcMNPV) at titers >108 pfu/mL efficiently infected Trichoplusia ni (T. ni) larvae through aerosol inoculation of budded virus at a pressure of 5.5 × 104 Pa. The dipping T. ni larvae in virus‐containing solution efficiently infected them. These results indicate that surface contamination, either by aerosol or dipping, lead to infection via spiracles. The aerosol infection route for AcMNPV was restricted to T. ni and Plutella xylostella larvae, whereas Spodoptera litura and Helicoverpa armigera larvae were resistant to this inoculation process. The yields of the reporter proteins DsRed and EGFP from T. ni larvae following aerosol infection were nearly identical to those following oral feeding or injection. This alternative baculovirus infection strategy facilitates recombinant protein and virus production by insect larvae. © 2009 American Institute of Chemical Engineers Biotechnol. Prog., 2009 相似文献
150.