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101.
为提高甘蓝型油菜耐寒育种过程中的筛选效率,研究甘蓝型油菜耐低温机理,以8个不同抗寒性的甘蓝型油菜为材料,对低温条件下各材料的生物量、叶绿素、脯氨酸和相对电导率进行测定,发现在室外平均气温2.75℃时,抗性材料的生物量、叶绿素和脯氨酸的累积量都显著高于敏感材料,相对电导率没有显著差异;当平均气温7.52℃回升至12.39℃,抗性材料和敏感材料生物量的累积量无显著差异;在恒定低温10℃/4℃处理下抗性材料和敏感材料在处理前3周生物量均持续累积,但从第4周开始敏感材料新叶出现白斑,生物量减少,抗性材料老叶出现白斑,生物量维持不变。结果表明,耐低温材料在低温条件下叶绿素含量受到的影响较小,脯氨酸的积累量持续上升,具有较强的快速适应能力,在低温下具有显著的持续生长优势。  相似文献   
102.
Cycloastragenol (CA) is the genuine sapogenin of astragaloside IV (ASI). This study focuses on the preparation of CA from ASI. Five hydrolysis methods were compared including H2SO4 hydrolysis, HCl hydrolysis, two-phase acid hydrolysis, mild acid hydrolysis, and Smith degradation. Seven hydrolysis products were purified, and five of them were identified as new compounds. The results indicated that Smith degradation was the most effective approach to prepare CA. In contrast, mild acid hydrolysis produced CA at a low yield, accompanied with the artificial sapogenin astragenol. The other three acid hydrolysis methods mainly produced astragenol. Furthermore, the reaction conditions for Smith degradation were optimized as follows: ASI was dissolved in 60% MeOH–H2O solution, oxidized with 5 equiv. NaIO4 for 12 h, followed by reduction with 3 equiv. NaBH4 for 4 h, and finally acidified with 1 M H2SO4 at pH 2 for 24 h. Under the optimal conditions, CA could be prepared from ASI at a yield of 84.4%.  相似文献   
103.
[目的/意义]科技文献资源保存已纳入多个国家图书馆的战略规划,中国图书馆仍缺少对数字资源本地保存及服务方法,亟待明确其中的关键问题并建立工作策略。[方法/过程]针对当前国际知识产权形势以及机构对数字资源资产管理新要求,调研国内外文献保障机构的数字资源本地保存现状,梳理图书馆数字资源实现馆藏保存与服务中的关键问题,进而提出中国图书馆数字资源本地保存及服务方式。[结果/结论]数字资源本地保存涉及到知识产权保护、图书馆服务方式、保存工作持续性等问题,有必要从数字资源馆藏体系建设的角度,确定数字资源馆藏保护、本地保存、自主可控的原则,以国家协议、电子资源采购条款约定保存权益、国际合作、数字呈缴等方法来获取数字资源馆藏内容、服务权益,通过技术架构支持数字资源的“在线、近线、离线”服务策略。  相似文献   
104.
本试验旨在探讨单宁酸对生长猪胃、小肠仿生消化中消化酶活性及玉米-豆粕型饲粮干物质和粗蛋白消化率的影响,为评价单宁酸的生物学效应提供参考。试验一采用单因素完全随机设计,考察在无饲粮下2种单宁酸对猪模拟胃液、模拟小肠液消化酶活性的影响。设5个处理,单宁酸添加量分别为0 mg (胃液体积为20 mL,小肠液体积为22 mL);单宁酸1,10 mg;单宁酸1,20 mg;单宁酸2,10 mg;单宁酸2,20 mg。测定各处理的胃蛋白酶、淀粉酶、胰蛋白酶和糜蛋白酶的活性。试验二考察玉米-豆粕型饲粮添加单宁酸对猪仿生消化中胃、小肠阶段消化酶活性及养分消化率的影响。采用单因素完全随机设计,设5个处理,单宁酸在饲粮中的含量分别为0 mg·(2 g)-1;单宁酸1,10 mg·(2 g)-1;单宁酸1,20 mg·(2 g)-1;单宁酸2,10 mg·(2 g)-1;单宁酸2,20 mg·(2 g)-1。测定仿生消化中胃阶段0.5和4 h时胃蛋白酶活性,小肠阶段0.5、4和8 h时淀粉酶、胰蛋白酶和糜蛋白酶活性及生长猪胃-小肠仿生消化测定饲粮的干物质和粗蛋白消化率。结果表明:1)无饲粮的情况下,和空白对照组相比,2种单宁酸对模拟胃液中胃蛋白酶活性无显著影响(P>0.05),单宁酸1比单宁酸2更高地降低了模拟小肠液中淀粉酶、胰蛋白酶和糜蛋白酶的活性(P<0.05)。2)在饲粮进行仿生消化的胃消化0.5~4 h内,除4 h时10 mg·(2 g)-1添加量外,添加单宁酸1时胃蛋白酶的活性均显著高于添加单宁酸2时的相应值(P<0.05),除单宁酸2在消化0.5 h外,2种单宁酸在添加10 mg·(2 g)-1时胃蛋白酶活性均显著高于20 mg·(2 g)-1添加量的相应值(P<0.05)。在小肠仿生消化0.5 h时,饲粮中添加单宁酸1、2的2个水平对消化液中淀粉酶活性无显著影响(P>0.05),但均显著降低了糜蛋白酶的活性(P<0.05);单宁酸1的消化液中胰蛋白酶活性高于单宁酸2的相应值(P<0.05)。在小肠仿生消化4 h时,除添加水平为20 mg·(2 g)-1时的糜蛋白酶活性外,饲粮中添加单宁酸1消化液中淀粉酶、糜蛋白酶活性高于添加单宁酸2的相应值,而胰蛋白酶活性低于添加单宁酸2的相应值(P<0.05)。单宁酸1、2的两个添加量均降低了胰蛋白酶和糜蛋白酶的活性(P<0.05)。在小肠仿生消化8 h时,饲粮中单宁酸的添加量影响了淀粉酶的活性,但单宁酸1和单宁酸2各两个添加量在淀粉酶的平均活性上无显著差异(P>0.05)。单宁酸1、2的两个添加量均降低了胰蛋白酶、糜蛋白酶的活性(P<0.05)。3)与对照组相比,两种单宁酸在两种添加水平下均显著降低了饲料粗蛋白消化率(P<0.05),且单宁酸2比单宁酸1更多地降低了饲粮粗蛋白的消化率(P<0.05)。综上所述,在有、无饲粮条件下,单宁酸对消化酶活性呈现不一致影响。单宁酸影响饲粮粗蛋白的消化率可能主要与消化液中糜蛋白酶活性降低以及单宁酸与饲粮中的化学成分形成螯合物降低了小肠消化酶的水解效率有关。  相似文献   
105.
旨在对辽宁绒山羊和内蒙古绒山羊的基因组选择信号进行筛选。本研究利用Illumina 50K的山羊芯片,对内蒙古绒山羊、辽宁绒山羊和黄淮山羊进行基因型检测,质控后获得50 010个共同SNPs位点。通过群体分化系数Fst和XP-EHH,以黄淮山羊为参考群体分别对内蒙古绒山羊和辽宁绒山羊进行选择信号检测,Fst和XP-EHH值的top 5%作为阈值。结果,利用Fst在绒山羊基因组中筛选到501个候选基因,利用XP-EHH在绒山羊基因组中筛选到145个候选基因。其中有12个SNPs在绒山羊基因组中受到较强选择。通过基因注释筛选到21个候选基因,包括EXOC4、ASIC2、PCDH9、RHBDD1、IRS1和PDE10A等。这些基因主要富集在PI3K-Akt信号通路、蛋白质消化吸收和松弛素信号通路等。研究结果发现,绒山羊在驯化过程中其基因组很多与毛囊相关的基因受到了强烈的选择。这些发现也有助于更好地了解绒山羊的选择进展,为中国绒山羊品种的种质资源保护和利用提供重要参考。  相似文献   
106.
107.
【目的】 筛选不同温度下烟草花叶病毒(Tobacco mosaic virus,TMV)侵染后枯斑三生烟(Nicotiana tabacum var. Samsun NN)差异表达的长链非编码RNA(long non-coding RNA,lncRNA),研究lncRNA在枯斑三生烟抗性反应中的作用。【方法】 N基因的温度敏感性使枯斑三生烟在25℃时具备对TMV的抗性、在31℃抗性丧失,在这两个温度条件下对枯斑三生烟接种TMV和磷酸盐缓冲盐水(phosphate buffered saline,PBS),48 h后提取系统叶总RNA,构建链特异性文库后进行深度测序。对测序结果进行过滤后利用HTSeq将有效数据与近缘品种TN90(N. tabacum var. TN90)基因组比对,筛选得到lncRNA后利用FPKM法估计lncRNA的表达水平。通过edgeR筛选差异表达lncRNA(differentially expressed lncRNA,DElncRNA),并利用qRT-PCR技术对这一结果进行验证。通过共定位及共表达分析预测DElncRNA的靶基因,通过参考基因组注释、GO和KEGG富集分析研究靶基因的功能。【结果】 4个处理共12个样本经lncRNA-seq各测得约8 000万条clean reads,共获得4 737条已知lncRNA、40 169条新lncRNA。其中64个lncRNA在不同温度条件下TMV侵染后存在差异表达,qRT-PCR测定结果显示这些lncRNA的测序正确率在80%左右,表明本研究所得测序数据具备较高的可信度。对DElncRNA进行靶基因预测,发现一些基因同时被25℃下调和31℃上调的DElncRNA靶向。靶基因注释功能丰富,主要参与植物抗病、激素和代谢等生理过程。部分可能与激素通路相关的lncRNA,在25℃下TMV侵染时呈现下调趋势,而在31℃下TMV侵染则呈现上调趋势。GO富集分析显示靶基因主要参与构成膜、囊泡等组分,具备钙、钾离子通道抑制剂活性等分子功能,使相应离子得以转运引发随后的反应,同时也参与发病、抗原加工和呈现、细胞分裂素代谢等生理过程。KEGG分析发现靶基因显著富集在植物激素信号转导通路,25℃下调和31℃上调的DElncRNA靶基因同时富集在激素信号传导、ABC运输蛋白、苯丙烷类生物合成等通路。【结论】 不同温度(25℃和31℃)条件下TMV侵染枯斑三生烟后,长链非编码RNA差异表达,DElncRNA通过作用于激素信号传导、物质转运等过程参与寄主系统获得性抗性反应。研究结果可为揭示植物系统获得性抗性中lncRNA的调控功能以及新型抗病毒技术开发提供依据。  相似文献   
108.
Fungal N2O production results from a respiratory denitrification that reduces NO3/NO2 in response to the oxidation of an electron donor, often organic C. Despite similar heterotrophic nature, fungal denitrifiers may differ from bacterial ones in exploiting diverse resources. We hypothesized that complex C compounds and substances could favor the growth of fungi over bacteria, and thereby leading to fungal dominance for soil N2O emissions. Effects of substrate quality on fungal and bacterial N2O production were, therefore, examined in a 44-d incubation after soils were amended with four different substrates, i.e., glucose, cellulose, winter pea, and switchgrass at 2 mg C g−1 soil. During periodic measurements of soil N2O fluxes at 80% soil water-filled pore space and with the supply of KNO3, substrate treatments were further subjected to four antibiotic treatments, i.e., no antibiotics or soil addition of streptomycin, cycloheximide or both so that fungal and bacterial N2O production could be separated. Up to d 8 when antibiotic inhibition on substrate-induced microbial activity and/or growth was still detectable, bacterial N2O production was generally greater in glucose- than in cellulose-amended soils and also in winter pea- than in switchgrass-amended soils. In contrast, fungal N2O production was more enhanced in soils amended with cellulose than with glucose. Therefore, fungal-to-bacterial contribution ratios were greater in complex than in simple C substrates. These ratios were positively correlated with fungal-to-bacterial activity ratios, i.e., CO2 production ratios, suggesting that substrate-associated fungal or bacterial preferential activity and/or growth might be the cause. Considering substrate depletion over time and thereby becoming limited for microbial N2O production, measurements of soil N2O fluxes were also carried out with additional supply of glucose, irrespective of different substrate treatments. This measurement condition might lead to potentially high rates of fungal and bacterial N2O production. As expected, bacterial N2O production was greater with added glucose than with added cellulose on d 4 and d 8. However, this pattern was broken on d 28, with bacterial N2O production lower with added glucose than with added cellulose. In contrast, plant residue impacts on soil N2O fluxes were consistent over 44-d, with greater bacterial contribution, lower fungal contribution, and thus lower fungal-to-bacterial contribution ratios in winter pea- than in switchgrass-amended soils. Real-time PCR analysis also demonstrated that the ratios of 16S rDNA to ITS and the copy numbers of bacterial denitrifying genes were greater in winter pea- than in switchgrass-amended soils. Despite some inconsistency found on the impacts of cellulose versus glucose on fungal and bacterial leading roles for N2O production, the results generally supported the working hypothesis that complex substrates promoted fungal dominance for soil N2O emissions.  相似文献   
109.
Quantifying the amount of carbon (C) incorporated from decomposing residues into soil organic carbon (CS) requires knowing the rate of C stabilization (humification rate) into different soil organic matter pools. However, the differential humification rates of C derived from belowground and aboveground biomass into CS pools has been poorly quantified. We estimated the contribution of aboveground and belowground biomass to the formation of CS in four agricultural treatments by measuring changes in δ13C natural abundance in particulate organic matter (CPOM) associated with manipulations of C3 and C4 biomass. The treatments were (1) continuous corn cropping (C4 plant), (2) continuous soybean cropping (C3), and two stubble exchange treatments (3 and 4) where the aboveground biomass left after the grain harvest was exchanged between corn and soybean plots, allowing the separation of aboveground and belowground C inputs to CS based on the different δ13C signatures. After two growing seasons, CPOM was primarily derived from belowground C inputs, even though they represented only ∼10% of the total plant C inputs as residues. Belowground biomass contributed from 60% to almost 80% of the total new C present in the CPOM in the top 10 cm of soil. The humification rate of belowground C inputs into CPOM was 24% and 10%, while that of aboveground C inputs was only 0.5% and 1.0% for soybean and corn, respectively. Our results indicate that roots can play a disproportionately important role in the CPOM budget in soils. Keywords Particulate organic matter; root carbon inputs; carbon isotopes; humification rate; corn; soybean.  相似文献   
110.
Two novel diterpenoids, japodagricanones A (1) and B (2), along with their biogenetically related diterpenoid 15-epi-4E-jatrogrossidentadion (3), were isolated from the leaves and twigs of Jatropha podagrica. Japodagricanones A (1) and B (2) are the first C-5-nor lathyrane-type diterpenoids. Their structures were established using spectroscopic data, including MS, NMR and ECD data. A plausible biosynthetic pathway for their generation was also proposed.  相似文献   
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