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1.
以云南、四川主栽的4个葡萄品种为试材,在常规用药方式基础上辅以微生态制剂,测定其对葡萄酸腐病和黑曲霉病防控效果及对果实品质的影响,以期为有效防控葡萄酸腐病和黑曲霉病的发生,解决生产实践中的具体问题提供科学参考依据。结果表明:微生态制剂能提高葡萄果粒大小和百粒质量,同时增加糖酸比。在传统用药基础上使用绿康威,对葡萄酸腐病和黑曲霉病的防效最佳,分别达52.3%和42.4%;在传统用药基础上使用绿地康3号,其防效为31.3%和21.9%,均表现出良好的防效;前期使用化学药剂,后期单独使用微生态制剂对酸腐病的防效不太明显。  相似文献   
2.
糖槭叶枯病 Phyllosticta negundinis病菌孢子放散开始期和高峰期与每年的温、湿度变化有关。病害发生严重程度与降雨量关系密切 ,降雨早且量大时病害严重。病菌以分生孢子器和分生孢子在病叶上越冬 ,通过气流传播成为翌年初侵染源。喷洒 70 %甲基托布津可湿性粉剂 10 0 0倍液和 75%百菌清可湿性粉剂 80 0倍液均能收到较好的效果  相似文献   
3.
Monokaryotic strains of Helicobasidium mompa were used as vectors of a mycovirus between various H. mompa isolates to examine the transmissibility of one of the mycoviruses, totivirus (HmTV1–17 virus) in the hypovirulent isolate V17 of H. mompa. The isolates that acquired HmTV1–17 virus were also examined for any alteration in the virulence. Twelve dikaryotic isolates of H. mompa, belonging to 11 mycelial compatibility groups (MCGs) and being mycelially incompatible with isolate V17, were used as recipients of HmTV1–17 virus. Two monokaryotic isolates that were mycelially incompatible with isolate V17 and all of the recipients were also used as vectors of HmTV1-17 virus between isolate V17 and the recipients. When isolate V17 and recipients were directly paired on plate media, HmTV1-17 virus was transmitted from isolate V17 into 2 of the 12 recipients (i.e., 2 of the 11 MCGs). Two monokaryotic strains were paired with isolate V17, and the monokaryotic strains that acquired HmTV1-17 virus were then used as new virus donors. When the monokaryotic strains containing HmTV1-17 virus were paired with the 12 recipients, HmTV1-17 virus was transmitted into 7 of the 12 recipients from the monokaryotic strains (i.e., 7 of 11 MCGs). Based on these results, we concluded that monokaryotic strains could act as vectors to transmit HmTV1-17 virus into H. mompa isolates. When four of the H. mompa isolates that acquired HmTV1-17 virus were used to inoculate apple rootstock Malus prunifolia, the virulence of all of the isolates was attenuated from that of their parental isolates. Moreover, because the DNA fingerprints of the fungal isolates that acquired HmTV1-17 virus were the same as those of their parental isolates, the infection with HmTV1-17 virus is considered the cause of virulence attenuation of H. mompa.  相似文献   
4.
Fusarium oxysporum对苗期大豆具有较强的致病作用。病原菌自伤口或直接侵入大豆幼苗根部的皮层组织,随着病原菌的侵入和扩展,细胞出现坏死,组织发生崩解,根部组织表现红褐色病斑。环境因素对病原菌的侵染时期和在大豆体内潜育时间的长短有着明显的影响。侵染时期主要受病原菌侵入前自身所处状态和寄主的影响,侵入后潜育时间的长短则受植株状态的影响。土壤环境条件直接影响着病原菌的侵入和寄主的抗病性,间接影响着病原菌在大豆植株体内的扩展和病症的表现。  相似文献   
5.
室内药效试验表明:麦根宁1号、敌力脱对小麦根腐病菌的生长均有良好的抑制作用。麦根宁Ⅰ号稀释300倍时,平均抑菌圈直径最大;敌力脱稀释800倍时,平均抑菌圈直径最大。同时,麦根宁Ⅰ号、敌力脱Ⅱ号,粉锈宁对小麦全蚀病菌生长也有明显的抑制作用。粉锈宁,麦根宁Ⅰ,Ⅱ号在稀释10000倍时,抑菌率均达100%;敌力脱在稀释15000倍时,平均抑菌率仍达89.7%。  相似文献   
6.
用全薯块吸头刺伤接种法测定时,较理想的测定条件为:每接种点接种0.1ml浓度为10~2~10~5CFU/ml菌悬液,随后在21±5℃~31±5℃(依所用菌株而定)下保持2~3天,以接种点腐烂斑的最大直径作记载标准。用新鲜薯片法测定时,除接种浓度为10~2~10~3CFU/ml,保持时间为1~2天及以侵染限值作评价标准外,其余条件和全薯块吸头刺伤接种法相同。当用皮孔浸渍法接种时,薯块在10_6CFU/ml菌悬液中浸5分钟,然后使薯块表面保持连续水膜,3~5天后测量薯块表面腐烂面积。上述3种方法都必须有20个以上重复,并使用大小一致、无伤无病的成熟薯块。  相似文献   
7.
一次防治大豆灰斑病籽粒灰斑   总被引:1,自引:1,他引:0  
通过室内及田间大豆不同生育期接种试验证明,籽粒感染灰斑病的关键时期是R3-R5期.R2期以前侵染不造成籽粒斑驳,据此提出一次防治大豆籽粒灰斑病的关键时期为R2-R4期.  相似文献   
8.
Blackspot, caused by Diplocarpon rosae , is the most severe and ubiquitous disease of garden roses, but information is lacking about genotype-specific forms of resistance and susceptibility of the host. Macro- and microscopic analyses of 34 rose genotypes with a defined monoconidial culture black spot inoculum identified susceptible and resistant rose genotypes and further genotype-specific subdivisions, indicating the presence of partial forms of resistance and different resistance mechanisms. In total, eight interaction types were characterized, five representing compatible (types 1–5) and three representing incompatible interactions (types 6–8). The incompatible interactions were characterized by the lack of any visible fungal structures beneath the cuticle (type 8), single-cell necroses (type 7) or necroses of larger cell clusters (type 6), the latter two types with penetration hyphae and haustoria in epidermal cells.  相似文献   
9.
Two viruses, detected frequently in the Netherlands in pelargonium, were identified by serology and test plant reactions. Antisera were prepared and an ELISA procedure was developed to detect the viruses in pelargonium.One of the viruses, PFBV-N, proved to be pelargonium flower-break virus. With the antiserum to PFBV-N, it could be detected reliably throughout the year inPelargonium zonale Springtime Irene.The other virus, PLPV-N, was serologically closely related to pelargonium line pattern virus (PLPV) and to pelargonium ring pattern virus (PRPV), as were an old virus isolate from Saturnus, collected in the Netherlands in 1971 (L128), and PLPV isolates from Yugoslavia (PLPV-Y) and Denmark (PLPV-D). There were only minor differences in host-plant reactions between the virus isolates. Based on these tests, PLPV and PRPV are considered as isolates of the same virus, for which, for practical reasons, the name pelargonium line pattern virus is proposed.PLPV could be reliably detected by ELISA inP. zonale Springtime Irene and Amanda throughout the year with only a few exceptions. InPelargonium peltatum Tavira, however, reslts were erratic due to uneven distribution of virus in the plant. Best results were obtained when petioles of fully expanded leaves were tested.  相似文献   
10.
One hundred and sixteen isolates of Fusarium oxysporum f. sp. lactucae obtained from 85 fields in three crisphead lettuce-producing areas in Nagano Prefecture, Japan were typed for races using differential cultivars Patriot, Banchu Red Fire and Costa Rica No. 4. They were also grouped into vegetative compatibility groups (VCGs) using complementation tests with nitrate non-utilizing (nit) mutants. Two California strains reported as F. oxysporum f. sp. lactucum, a type culture of F. oxysporum f. sp. lactucae, and 28 avirulent isolates of F. oxysporum obtained from crisphead lettuce were included for comparison. Among Nagano isolates, 66 isolates were identified as race 1, and 50 as race 2. Race 1 strains derived from Shiojiri and Komoro cities and race 2 from Kawakami village and Komoro city. All isolates of race 2 were biotin auxotrophs, and the race could be distinguished based on its requirement for biotin on minimal nitrate agar medium (MM). Pathogenic isolates were classified into two VCGs and three heterokaryon self-incompatible isolates. Strong correlations were found between race and VCG. All the race 1 strains were assigned to VCG 1 except self-incompatible isolates, and all the race 2 strains to VCG 2. The 28 avirulent isolates of F. oxysporum were incompatible with VCG 1 and VCG 2. California strains was vegetatively compatible with VCG 1, and they were assigned to race 1. Based on vegetative compatibility, these two races of F. oxysporum f. sp. lactucae may be genetically distinct, and F. oxysporum f. sp. lactucae race 1 is identical to F. oxysporum f. sp. lactucum. Received 7 May 2002/ Accepted in revised form 6 September 2002  相似文献   
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