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1.
切割取样对胚胎发育的影响   总被引:2,自引:0,他引:2  
体视显微镜下,采用徒手持金属刀片和自制的玻璃切割针分别对小鼠和牛胚胎进行切割取样,并对取样后的胚胎进行体外培养48h,其发育率分别为76.7%(46/60)和80%(16/20),两者差异不显著(P>0.05);奶牛新鲜胚胎切割取样后,胚胎移植妊娠率47.1%(8/17),比对照组妊娠率59.0%(23/39)差异显著(P<0.05)。冷冻-解冻胚胎切割取样后移植妊娠率42.9%(6/17)虽然也比对照组50%低,但是差异不显著(P>0.05)。  相似文献   
2.
给休情期性成熟母犬肌注 PGF2α(0 .5 m g/ kg) ,2 4 h后肌注 e CG(5 0 IU/ kg) ,再经 12 0 h后肌注 h CG(2 0 U/ kg) ,诱导其发情。将诱导发情的母犬与公犬交配 ,于交配后 16 d,摘取卵巢、子宫 ,观察其卵泡发育和胚胎着床情况。结果表明 ,药物处理可明显促使母犬提前结束休情期而进入发情期 (9/ 10 ) ,促进卵巢内卵泡发育 (P<0 .0 1) ,并使更多的胚胎着床 ,每只母犬子宫胚胎着床点为 (17.4± 2 .2 )个 ,提示 3种生殖激素联合应用可提高母犬繁殖率  相似文献   
3.
Metabolic disorder is a major health problem and is associated with a number of metabolic diseases. Due to native hyperglycaemia and resistance to exogenous insulin, chickens as a model had used in the studies of adipose tissue biology, metabolism and obesity. But no detailed information is available about the comprehensive changes of serum metabolites at different stages of chicken embryonic development. This study employed LC/MS‐QTOF to determine the changes of major functional metabolites at incubation day 14 (E14d), 19 (E19d) and hatching day 1 (H1d), and the associated pathways of differential metabolites during chicken embryonic development were analysed using Metabolite Set Enrichment Analysis method. Results showed that 39 metabolites were significantly changed from E14d to E19d and 68 metabolites were significantly altered from E19d to H1d in chicken embryos. Protein synthesis was promoted by increasing the concentrations of L‐glutamine and threonine, and gonadal development was promoted through increasing oestrone content from E14d to E19d in chicken embryos, which indicated that serum glutamine, threonine and oestrone contents may be considered as the candidate indicators for assessment of early embryonic development. 2‐oxoglutaric acid mainly contributed to enhancing the citric cycle, and it plays an important role in improving the growth of chicken embryos at the late development; the decreasing of L‐glutamine, L‐isoleucine and L‐leucine contents from E19d to H1d in chicken embryonic development implied their possible functions as the feed additive during early posthatch period of broiler chickens to satisfy the growth. These results provided insights into understand the roles of serum metabolites at different developmental stages of chicken embryos, it also provides available information for chicken as a model to study metabolic disease or human obesity.  相似文献   
4.
Japanese Balck cattle fetal fibroblasts (JBCFF) were induced with Xenopus leavis egg extracts and somatic cell nuclear transfer (SCNT) was carried out with the reprogrammed JBCFF as donor cells in order to investigate their effects on SCNT efficiency.Three samples of egg extracts were acquired from different Xenopus laevis.The protein contents and kinds in extracts were evaluated with BCA Protein Quantification Kit and SDS-PAGE.Concentration of Digitonin to permeabilize JBCFF was optimized and assessed with PI staining.Reprogrammed cells treated with egg extract were used as donor in SCNT.Additionally the reconstructed embryos were activated with ionomycin+6-DMAP and A23187+6-DMAP to compare their effects on the development competence.The protein contents of extracts samples were 56.2255,64.6570 and 71.2158 μg/mL,respectively,the each extract had the same composition about 40-55 and 70-100 ku.The optimal concentration of Digitonin was 7 μg/mL and the permeabilization rate was 55.44%.After extracts treatment and continuous culture for 6-7 d,JBCFF formed well-defined colony structures.No significant composition difference was found in rates of fusion (92.83% vs 96.04%),cleavage (89.64% vs 89.78%) and blastocyst formation (24.06% vs 23.12%) of cloned embryos when the colony cells and JBCFF without extracts treatment were used as donor cells (P>0.05).Similarly,the two activation methods had no significant effect on the developmental competence of cloned embryos (cleavage rate 92.16% vs 92.28%,blastocyst rate 23.21% vs 24.18%).Conclusively,Xenopus leavis,egg extracts could induce JBCFF reprogramming to a low differentiated state.However donor cells with reprogramming partially could not improve the development of cloned embryos and its mechanism requires further research.  相似文献   
5.
以白檀未成熟胚为试材,以改良MS为培养基,研究了白檀未成熟胚的器官发生和植株再生.结果表明:改良MS(mMS)能够很好的诱导愈伤组织,在添加了0.2 mg/L 6-BA+0.1 mg/L NAA的培养基中,诱导率高达92.5%;胚性愈伤组织分化最佳培养基为mMS+0.25 mg/L 6-BA+0.15 mg/L NAA,分化率为72.4%;分化出的胚性愈伤组织在空白mMS培养基上继代培养15 d,76.6%的组织分化出芽,再转入1/2mMS+ 1.5%蔗糖培养基上培养20 d,芽长至1.5 cm.  相似文献   
6.
冰草属植物组织培养再生体系的建立   总被引:10,自引:3,他引:10  
以适宜西北地区种植的优质牧草冰草属(AgropyronGaertn)中的三个不同种———蒙古冰草新品系(A.mongolicumKeng)、航道冰草(A.cristatumcv.Fairway)、诺丹冰草(A.desertorumcv.Nordan)和一个种间杂种冰草———蒙农杂种冰草(A.cristatum×A.desertorumcv.Mengnong)为材料,分别以幼穗为外植体建立了冰草组织培养再生体系。诱导愈伤组织的培养基为改良MS+2,4 D2.0mg/L,分化培养基为MS(无附加成分),在1/2MS培养基上生根后得到完整小植株。结果表明在本试验条件下,不同长度的幼穗在培养时,其愈伤组织发生的部位及其增殖速度不同;4种材料愈伤组织诱导率和分化率无明显差异,均可有效诱导愈伤组织并分化成再生植株,再生植株的产生主要通过直接器官发生途径。  相似文献   
7.
以3个普通小麦品种为材料,用^60Coγ射线辐照小麦幼胚愈伤组织,在MR1、MR2代中才观察到广泛变异,其后代在育性、株高、抽穗期、千粒重、株型、蛋白质含量等方面者发生了明显变异,这些变异较单纯用组织培养得到的无性系的后代的变异频率更大,变异范围也更为广泛,并且从MR2中得到了几个有较高利用价值的变异株系。  相似文献   
8.
以苜蓿雄性不育系Ms-4幼嫩茎段、叶片、叶柄为外植体,诱导苜蓿雄性不育系再生植株.结果表明:叶柄是诱导愈伤组织的良好外植体,体细胞胚诱导率为90%,再生率49%.苜蓿雄性不育系插条生根的最佳处理为接种前用水进行预处理0.5h,外植体为完整插条,培养基为A1、A2,其生根率为97%,生根系数为5.3.  相似文献   
9.
杏胚珠培养及幼胚子叶不定芽诱导研究   总被引:2,自引:1,他引:2  
以盛花后25、35、50、55、60d的凯特杏胚珠为外植体,研究胚珠培养的适宜条件;选择发育一致的幼胚子叶,研究不定芽的发生条件。结果表明,SH培养基是凯特杏胚珠培养的适宜培养基;盛花后25d的凯特杏胚珠(PF=0),仅采用生长培养不足以发育成可见胚,试验采用诱导方式获得了可见胚,诱导出胚率为80%;以MS为基本培养基,BA与NAA结合诱导能力强;但这种胚小且瘦弱,继续生长培养,利用幼胚子叶诱导不定芽。在幼胚子叶诱导不定芽方面,盛花后25、35d取样的凯特杏胚珠,培养后获得幼胚子叶,诱导不定芽的适宜TDZ质量浓度为1.25mg/L,诱导出芽率分别为85.00%、80.00%;盛花后50、55d取样的材料,适宜TDZ质量浓度为2.50mg/L,出芽率分别为65.00%、60.00%,而盛花后60d取样的材料,适宜TDZ质量浓度为5.0mg/L,出芽率为61.11%,不定芽主要发生在子叶的近轴面、胚轴连接处及子叶近轴端两侧;在相同培养基中,25℃进行21d暗培养,盛花后35、50、55、60d材料出芽率分别为72.22%、65.00%、60.00%、55.56%;4℃下28d暗培养,35、50、55、60d依次为59.09%,71.42%、77.78%、86.36%;对不定芽进行伸长、生根与快繁培养,获得了健康正常的植株。通过以上研究,建立了凯特杏幼胚4级培养体系,即(1)胚珠培养,获得可见胚(1级培养);(2)幼胚生长培养(胚培养),获得了健壮幼胚(2级培养);(3)幼胚子叶再生,获得不定芽(3级培养);(4)不定芽组培苗快繁(4级培养)。  相似文献   
10.
利用脂质体包裹含EGFP基因的质粒,并将之导入山羊乳腺上皮细胞,经G418筛选获得阳性细胞,以阳性细胞作为核供体,利用核移植技术构建转基因克隆胚。结果表明:用转基因山羊乳腺上皮细胞作为核供体,电融合法更适合构建转基因克隆胚。转基因山羊克隆胚体外培养最佳方案是用SOFaa培养液,在培养72 h后加入10%的正常山羊血清(Normal goat serum,NGS)。荧光显微镜下观察到转基因克隆胚中EGFP的表达,大部分克隆胚发育到8-16细胞以后的时期,绿色荧光蛋白才开始逐渐表达,随着发育时间的延长,绿色荧光蛋白的表达也逐渐增强。说明外源基因在胚胎早期发育阶段可以表达,EGFP可以作为报告基因来实现对外源基因整合及表达的监测。  相似文献   
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