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21.
A detection method of dexamethasone sodium phosphate in houttuynia injection,bupleurum injection,vitamin C injection,lincomycin hydrochloride injection,and asragulus polysacharin injection was established by UPLC-PDA.The Waters ACQUITY UPLC® BEH C18 column(2.1 mm×50 mm,1.7 μm) was used,the mobile phase consisted of 0.75% triethylamine phosphatic liquor/solution (pH 3.0)-methyl alcohol-acetonitrile(50:45:5),the flow rate was 0.3 mL/min,the column temperature had remained 25℃,photodiode array detector wavelength range was 190 to 400 nm,the recorded wavelength was 242 nm,the injection volume was 10 μL.The linear range of dexamethasone sodium phosphatel was 10.0 to 200.0 mg/L (R2=0.9999),the mean recovery and RSD for dexamethasone sodium phosphate in houttuynia injection,bupleurum injection,vitamin C injection,lincomycin hydrochloride injection and asragulus polysacharin injection were 97.54% and 1.14%,101.59% and 0.19%,100.92% and 0.92%,99.82% and 0.73%,100.08% and 0.62%,respectively.This method was accurate,easy and fast,it was suitable for detection of dexamethasone sodium phosphatein houttuynia injection and other four kinds of injections.  相似文献   
22.
Forsyth, L.M.G., Jackson, L.A., Wilkie, G., Sanderson, A., Brown, C.G.D. and Preston, P.M., 1997. Bovine cells infected in vivo with Theileria annulata express CD11b, the C3bi complement receptor. Veterinary Research Communications, 21 (4), 249-263Bovine cells from cattle infected with Theileria annulata were phenotyped with monoclonal antibodies recognizing bovine leukocyte antigens. Macroschizont-infected, transformed cell lines prepared from peripheral blood mononuclear cells of cattle, infected with sporozoites, were assessed by flow cytometry; parasitized cells in tissues from infected cattle were examined by immunocytochemical techniques. Co-expression of markers for different cell lineages by the cell lines precluded a definite conclusion as to their phenotypic origins. For, while the pattern of leukocyte antigens expressed by these in vivo-derived schizont-infected cells, which included CD11b, was indicative of a myeloid origin, the possibility that they were NK cells could not be excluded. The monoclonal antibody (MAb) IL-A15, which recognizes CD11b, reacted with a high proportion of parasitized cells in sections of tissues from infected cattle at all stages of acute disease. Mononuclear cells infected with parasites at all stages of differentiation, from macroschizont to microschizont, expressed CD11b. Such parasitized cells occurred throughout the lymphoid tissues, being found in the thymus, spleen and lymph nodes, particularly the prescapular node draining the site of infection, the hepatic, mesenteric and precrural nodes, as well as in the reticulo-endothelial tissue of the liver, kidney, lung, abomasum, adrenal and pituitary glands. These observations provided the first evidence for a myeloid origin for the parasitized T. annulata cells found in infected bovine tissues and blood and suggested a mechanism whereby schizonts could transfer from cell to cell during mechanical infection with schizont-infected cells.  相似文献   
23.
目的揭示宣和猪PRKAG3基因外显子5多态性及其与肉质性状的关联。方法采用PCR产物直接测序法检测了120头宣和猪PRKAG3基因外显子5区域的SNP位点,借助最小二乘模型分析了各位点不同基因型及合并基因型对6个肉质性状的影响。结果宣和猪PRKAG3基因外显子5区域检出3个SNP位点,包括2个同义突变位点(T579C、T580C)和1个错义突变位点(G595A),分别以TT、TT、GA基因型和T、T、G等位基因的频率最高,且都处于Hardy-Weinberg平衡状态。T579C、T580C位点的TT和TC基因型可显著提高大理石纹(P<0.05)和降低失水率(P<0.01),分别呈显著的加性效应及加性—显性效应(P<0.05或P<0.01);G595A位点的AA基因型失水率最低(P<0.05)、熟肉率最高(P<0.05),呈显著的加性效应(P<0.05);3个位点的合并基因型TTTTGG、TCTCGG和TTTTAA分别具有最高的大理石纹、pH1和最低的失水率(P<0.05或P<0.01),CCCCGG基因型的大理石纹和pH1最低、失水率最高(P<0.05或P<0.01)。结论研究结果进一步确认宣和猪PRKAG3基因外显子5多态性与肌肉大理石纹、pH值和失水率显著关联,T579C、T580C位点的CC基因型和G595A位点的GG基因型具有协同降低猪肉品质的效应。  相似文献   
24.
本研究克隆了二化螟(Chilo suppressalis)、台湾稻螟(Cauricilius)、芦苞螟(C.luteellus)、甘蔗条螟(C.sac-chariphagus)、三化螟(Tryporyza incertulas)、亚洲玉米螟(Ostrinia furnacalis)、甘蔗红尾白螟(Scirpophaga ex-cerptalis)、黄纹髓草螟(Calamotrophapaludella)、桃蛀螟(Conogethes puncti eralis)、棘禾草螟(Chilo hyrax)和稻蛀茎夜蛾(Sesamia in.erens)11种常见蛀茎害虫102个个体的线粒体DNA细胞色素氧化酶亚基Ⅰ(COⅠ)基因片段.序列分析显示:该COⅠ基因片段长为709 bp,序列都未发生缺失或插入现象,碱基颠换率(55.42%)高于转换率(44.58%);种间遗传距离平均值为0.140(0.088~0.179),种内遗传距离平均值为0.004(0~0.015),两者之间没有重叠区域;聚类分析表明,不同种蛀茎害虫分别形成独立的进化分支,分支自展值均为100%.研究结果表明该COⅠ基因序列具有适宜的变异信息,种内相对保守,种间变异显著,适用于蛀茎害虫的物种识别,并为开发蛀茎害虫DNA条形码技术奠定了基础.  相似文献   
25.
26.
以马蔺(Iris lactea var.chinensis)和鸢尾(I. tectorum)2种耐性不同的鸢尾属植物为材料,采用溶液培养试验,研究了10、120 mg/L Cd胁迫下2种鸢尾幼苗膜透性、可溶性糖和蛋白以及根系生长等的生理耐性差异.结果表明:10 mg/L低Cd胁迫和120 mg/L高Cd胁迫均导致2种鸢尾幼苗叶片膜透性(CMP)增加;马蔺根系活力、可溶性糖和蛋白含量在低浓度Cd胁迫下增加,高浓度Cd胁迫下根系活力和可溶性糖含量出现下降趋势,而可溶性蛋白含量持续增加;鸢尾根系活力在低浓度和高浓度Cd胁迫下均呈下降趋势,可溶性糖和蛋白含量随Cd浓度增加表现为先增后降的趋势.  相似文献   
27.
旨在筛选并鉴定与鸭C4结合蛋白(C4b-binding protein,C4BP)互作的鸭疫里默氏菌(Riemerella anatipestifer,R.anatipestifer)外膜蛋白。本研究将保存的R.anatipestifer复苏培养,提取外膜蛋白,以鸭C4BPα作为诱饵蛋白进行His pull-down及LC-MS/MS蛋白质谱鉴定,筛选与鸭C4BP可能发生互作的候选外膜蛋白;将各候选蛋白进行克隆、原核表达,免疫小鼠制备多克隆抗体,利用Far-western blot验证与鸭C4BP发生相互作用的R.anatipestifer外膜蛋白;针对候选蛋白及C4BPα各功能结构域进行克隆及原核表达,利用Far-western blot鉴定候选蛋白及与C4BP的相互作用位点;利用ELISA对补体因子C3b、C4b及C4BP在R.anatipestifer表面沉积情况进行测定,验证候选蛋白的功能。结果显示,经His pull-down及LC-MS/MS蛋白质谱分析,共筛选出3个与鸭C4BP发生相互作用的R.anatipestifer外膜蛋白,即ECE-1、SODs和Omp62;成功获得3个外膜蛋白多克隆抗体,ELISA检测3种多克隆抗体效价均超过1∶6 400,Western blot检测3种多克隆抗体可以与重组蛋白发生特异性反应;Far-western blot结果显示,仅ECE-1能够与C4BP发生相互作用,并且只有ECE-1全长能与鸭C4BP相互作用,而鸭C4BP与ECE-1的相互作用区域位于C4BPα的SCR 2和SCR 3;当健康鸭血清稀释度为3.125%时,ECE-1抗体能够显著促进补体因子C3b、C4b在R.anatipestifer表面的沉积作用(P<0.05),当健康鸭血清稀释度为6.25%时,ECE-1抗体能够显著抑制C4BP在R.anatipestifer表面的沉积作用(P<0.05)。本研究成功筛选并鉴定出1个与C4BP互作的R.anatipestifer外膜蛋白ECE-1,为进一步阐明R.anatipestifer免疫逃逸机制奠定了基础。  相似文献   
28.
Sepsis is a frequent source of morbidity and mortality in critically ill patients. The goal of this case control study was to measure hemostatic changes in dogs with naturally occurring sepsis. Blood was collected within 24 hours of admission from 20 dogs that fulfilled the criteria for sepsis. Sepsis was defined as histologic or microbiological confirmation of infection and 2 or more of the following criteria: hypo- or hyperthermia, tachycardia, tachypnea, or leukopenia, leukocytosis, or > 3% bands. Culture and sensitivities were performed on appropriate samples from all septic dogs. Twenty-eight control dogs were enrolled on the basis of normal results of physical examination, CBC, serum biochemistry, and coagulation profile. Plasma samples were analyzed for prothrombin time (PT), partial thromboplastin time (PTT), fibrin(ogen) degradation products (FDP), D-dimer (DD) concentrations, antithrombin (AT) activity, and protein C (PC) activity. Data were compared between groups by chi-square or independent t-tests. PC (P < .001) and AT (P < .001) activities were significantly lower in dogs with sepsis compared to controls. Dogs with sepsis had significantly higher PT (P = .007), PTT (P = .005), D-dimer (P = .005), and FDP (P = .001) compared to controls. Platelet counts were not significantly different between groups. Ten of the 20 septic dogs (50%) died, but no association was identified between any of the measured variables and outcome. These findings are consistent with previous studies in animals with experimentally induced disease and in clinical studies of humans. On the basis of these results, further investigation of the role of AT and PC in canine sepsis is warranted.  相似文献   
29.
Akabane virus (AKAV), belonging to the genus Orthobunyavirus and family Peribunyaviridae, causes reproductive and congenital abnormalities in ruminants. Its envelope glycoprotein Gc is a neutralizing antigen, on which at least five distinct antigenic regions have been identified. We attempted to identify the domains using truncated recombinant AKAV Gc proteins expressed in Escherichia coli and monoclonal antibodies (mAbs) with AKAV-neutralizing activity. Dot blot analysis revealed that amino acid positions 1–97 and 189–397 (Gc1–97 and Gc189–397) in the truncated recombinant proteins reacted with the mAbs. Additionally, AKAV was neutralized by sera from mice immunized with these recombinant proteins. The results suggested that the two domains contain neutralizing epitopes and could be potential subunit vaccines against AKAV.  相似文献   
30.
扩增、克隆和表达了水肿病大肠杆菌的致病因子F18ab 菌毛的主要亚单位FedA全基因(包括信号肽序列),并与现有的另一致病因子志贺样毒素Ⅱ型变异体A亚单位基因(stx 2eA)连接,然后进行联合表达。同时用已制备的抗Stx 2eA 单克隆抗体和抗F18ab菌毛单克隆抗体对联合表达的融合蛋白质进行检测鉴定。  相似文献   
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