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871.
Toxoplasma gondii is a major zoonotic agent infecting a wide range of mammals, including wild felids. Like domestic cats, wild felids are involved in the complete infective cycle of T. gondii, as they can host in their gastrointestinal tract sexually mature parasites and shed infective oocysts in their feces. In order to evaluate the importance of this wildlife reservoir, 438 serum samples collected between 1984 and 1999 from 438 pumas (Felis concolor) and from 58 bobcats (Lynx rufus) from North America, Central America and South America were screened for antibodies to T. gondii. The overall prevalence of T. gondii antibodies was 22.4% in pumas and 51.7% in bobcats, with regional variations. Adults were more likely to be seropositive than juveniles and kittens (prevalence ratio (PR) = 2.61; confidence interval (CI) = 1.15, 4.04). In the US, pumas from the southwestern states (Arizona, California and New Mexico) were more likely to be seropositive for T. gondii ( PR = 2.61; 95% CI = 1.32-5.18 ) than pumas from the northwestern and mountain states (Colorado, Idaho, Oregon, Utah and Wyoming). Male pumas from the US were more likely to be seropositive than females (PR = 2.08; 95% CI = 1.11-3.92), whereas female pumas from Mexico, Central America and South America were more likely to be seropositive than female pumas from Canada and the US (PR = 2.49; 95% CI = 1.09-5.69). Captive pumas were also more likely to be seropositive (21.7%, 29/92) for T. gondii than free-ranging animals (19.9%, 69/346) (PR = 1.85; 95% CI = 1.06, 3.17).  相似文献   
872.
ABSTRACT To characterize host genes required for a compatible interaction, we identified a novel recessive Arabidopsis thaliana mutant, nws1 (no wilt symptoms), that failed to develop wilt symptoms in response to virulent strains of the phytopathogenic bacterium, Ralstonia solanacearum. The absence of wilting in nws1 plants was not correlated with a cell death phenotype or a constitutive expression of salicylic acid-, jasmonic acid- or ethylene-associated genes. In addition, this mutation, which conferred a symptomless phenotype in response to all the R. solanacearum strains tested, was highly specific to this pathogen, because nws1 responses to other plant pathogens, including oomycetes, nematodes, viruses, and other bacteria, were identical to those of wild-type Col-5 plants. Finally, the lack of disease development was shown to be different than RRS1-R-mediated resistance. The identification of mutants such as nws1, that are unable to develop disease, should lead to the isolation of target host factors required for pathogen growth or fitness, or of factors modified by the invading microorganism to avoid or inactivate plant defense mechanisms, and should bring a better understanding of bacterial wilt diseases.  相似文献   
873.
A Neospora caninum IgG avidity ELISA was carried out on the basis of a somatic N. caninum tachyzoite antigen. The test was validated using experimentally infected calves, where a clear maturation of the IgG avidity over time could be demonstrated. At a maximum of 82 days after infection (d.p.i.), all animals showed antibody avidities ranging above 35%, and respective sera were thus defined as highly avid.Sera of 103 naturally infected seropositive cows with abortion (N. caninum association was provided by a N. caninum PCR-positivity of the fetus in 40 cases) and 139 seropositive animals without abortion history were concurrently examined. Significantly lower avidities were observed in aborting cows when compared to animals without abortion problems (P<0.01). While the avidity of sera collected before abortion remained practically constant until abortion, a significant increase of avidity could be observed in samples collected weeks to months after abortion (P<0.01).The avidities of non-aborting animals from farms with or without abortion problems did not differ significantly with time and were mainly located in the high avidity area. These data indicate that low avidities are not necessarily linked to recent N. caninum infection but can also be an indicator for increased abortion risk in cattle.  相似文献   
874.
OBJECTIVE: To report clinical outcome after use of an interlocking nail (veterinary interlocking nail [VIN]) for stabilization of diaphyseal fractures in dogs and cats. STUDY DESIGN: Retrospective study. Animals: Seventy-eight dogs and 43 cats with diaphyseal fractures of the femur (n = 96), tibia (n = 14), or humerus (n = 11). METHODS: Interlocking nails (4 mm diameter [n = 72], 6 mm [n = 25] or 8 mm [n = 24]), were used in static (n = 106) or dynamic (n = 15) fixation mode. Cerclage wires also were used in 63 (52%) cases. Data about the patient (species, breed, weight, age), characteristics of the fracture, and details of the surgery and perioperative complications were recorded. The surgeon evaluated functional outcome, and fracture healing was quantified 6 weeks (W6) and 3 months (M3) after surgery with a radiographic index. RESULTS: Twelve cases had been unsuccessfully treated by another technique. Of 106 comminuted fractures, 60 were classified as unstable. Only 112 animals were evaluated at W6; 86 (77%) healed without complication and had a functional outcome considered excellent (n = 80, 93%), good (n = 5, 4%), or fair (n = 1). Twenty-six complications were noted: 16 (14%) patients did not require additional surgery and had a good or excellent outcome, whereas 10 (8%) patients needed surgical intervention to CONCLUSIONS: VINs can be used to repair diaphyseal fractures of the femur, tibia, and humerus in dogs and cats provided the implants are appropriately sized for the fractured bone. The high healing rate (even with unstable fractures), associated with a functional outcome, and low complication rate support the use of VINs for these fracture types. However, a period of training and the application of basic principles are necessary to ensure successful results. CLINICAL RELEVANCE: VINs should be considered as alternative technique for management of selected diaphyseal fractures of the femur, tibia, and humerus in dogs and cats.  相似文献   
875.
Bartonella henselae has been identified and characterized for the first time in Italy. A strain, designed Pavia-1, was isolated from the blood of a cat whose owner developed cat scratch disease (CSD). Pavia-1 and two American B. henselae strains (Houston-1, ATCC 49882, type I and strain 269608, UC Davis, type II) were compared by whole-cell fatty analysis (CFA), sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) for protein profiles, Western immunoblotting (WB) for reactivity with polyclonal antibodies, polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP), type-specific 16S rRNA PCRs, and pulsed-field gel electrophoresis (PFGE). Bartonella clarridgeiae (ATCC 51734) was also included for comparison. Pavia-1 was identified as a B. henselae type I. PFGE allowed differentiation between B. clarridgeiae and B. henselae and furthermore, between all the B. henselae strains. The fingerprints of PFGE observed for Pavia-1 were distinct from those of B. henselae type II and also of Houston-1, suggesting that the two type I strains derived from two different clones. These results show the capability of B. henselae to develop genotypic variability between genetically related strains.  相似文献   
876.
A total of 1253 ixodid ticks (254 tick pools) collected between the end of 1995 and the spring of 1997 from six California counties (El Dorado, Los Angeles, Orange, Santa Cruz, Shasta and Sonoma) were examined for the presence of Bartonella DNA by PCR of the citrate synthase gene. Of 1,119 adult Ixodes pacificus ticks tested, 26 (11.6%) of 224 pools, each containing five ticks, were positive (minimum percentage of ticks harboring detectable Bartonella DNA, 2.3%). Bartonella PCR-positive ticks were identified in five counties but none of the ticks from Los Angeles County was positive. Among 47 nymphal I. pacificus ticks collected in Sonoma County, one (10%) positive pool out of 10 pools was identified (minimum percentage of ticks harboring detectable Bartonella DNA, 2.1%). Among the 54 Dermacentor occidentalis grouped in 12 pools from Orange County, one pool (8.3%) was PCR positive for Bartonella and similarly one pool (14.3%) was positive among the 30 Dermacentor variabilis ticks grouped in seven pools. None of the three D. occidentalis from El Dorado County were positive. None of the nine tick pools positive for Ehrlichia phagocytophila were positive for Bartonella. Following our previous findings of Bartonella PCR-positive adult I. pacificus ticks in central coastal California, this is the first preliminary report of the presence of Bartonella DNA in I. pacificus nymphs and in Dermacentor sp. ticks. Distribution of Bartonella among ixodid ticks appears widespread in California.  相似文献   
877.
The intestinal mucosal immune system can discriminate actively between harmful pathogenic agents and harmless food antigens resulting in different immune responses namely IgA production and oral tolerance, respectively. Recently, a pig model has been developed for studying intestinal mucosal immune responses in which F4 fimbrial antigens of enterotoxigenic Escherichia coli (F4 ETEC) are used as oral antigens. A unique feature of this model is that soluble F4 antigens can be administered to pigs which have a receptor for this fimbriae (F4R(+)) on their small intestinal villous enterocytes and pigs which do not have this receptor (F4R(-)). Oral administration of F4 to the F4R(+) pigs results in an intestinal mucosal immune response that completely protects the pigs against a challenge infection. In F4R(-) pigs such an intestinal mucosal immune response does not occur. However, a priming of the systemic immune system can be seen similar to the priming in pigs fed with the same dose of a food antigen, suggesting that F4 in F4R(-) pigs behaves as a food antigen. The fact that different mucosal immune responses can be induced with soluble F4, makes it an interesting model to study mucosal immune mechanisms in the pig.  相似文献   
878.
Collaborative work was financed by the EU to develop and assess new diagnostic tools that can differentiate between bovine brucellosis and bovine infections due to Yersinia enterocolitica O:9 either in conjunction with, or as an alternative to, the classical serological, bacteriological or allergic skin tests. Sixteen heifers were experimentally infected with Brucella abortus biovar 1 (five heifers), Brucella suis biovar 2 (two heifers), Y. enterocolitica O:9 (six heifers) and Y. enterocolitica O:3 (three heifers). Four heifers, naturally infected with Y. enterocolitica O:9 that presented aspecific brucellosis serological reactions were also included in the experiment. A self-limited infection was induced in cattle by B. suis biovar 2. All the brucellosis serological tests used, i.e. the slow agglutination test (SAW), the Rose Bengal test (RB), the complement fixation test (CFT), indirect and competitive ELISA’s, lacked specificity when used to analyze sera from Y. enterocolitica O:9 infected animals. A Yersinia outer membrane proteins (YOPs)-ELISA was also used and although the test is able to detect a Yersinia group infection, it provided no evidence of whether or not there is a possible brucellosis infection when dual infections are present. The brucellergen IFN-γ test showed a lack of specificity also. The only test that was proven to be specific is the brucellergen skin test. All brucellosis serological tests, except the indirect ELISA, were limited in their ability to detect B. abortus persistently infected animals.

Based on these experimental studies, a strategy was implemented as part of the year 2001 Belgian Brucellosis Eradication Program to substantiate the eradication of bovine brucellosis. Epidemiological inquiries have identified risk factors associated with aspecific serological reactions, possible transmission and infection of cattle by B. suis biovar 2 from infected wild boars; and both legal and administrative measures taken by the veterinary services. No cases of bovine brucellosis have been confirmed in Belgium since March 2000.  相似文献   

879.
Some recreational activities in urban forests can cause extensive damage to soil and vegetation. In Switzerland, forest visitors frequently build fires outside picnic sites for barbecuing. This indicates that the existing picnic sites are either not attractive enough for these visitors, or that there are not enough sites for all the visitors during peak days. We used an on-site survey to assess the requirements of picnickers in two forest areas in the vicinity of Basle. Results showed that the existing picnic sites do not meet the requirements of some visitor groups, causing the respective visitors to make their own fires in locations that suit them better. There was a preference for sites near streams, away from forest roads and close to open spaces. Furthermore, while some visitors highly appreciated the well-equipped official sites, others preferred more natural infrastructure with pieces of stones forming a fire ring rather than concrete rims, and logs to sit on instead of benches. Picnic sites that are closer to the requirements of visitors who normally steer away from official sites might reduce the number of self-made fire rings. The study shows that understanding visitor behaviour is a prerequisite for the implementation of measures to reduce ecological impacts.  相似文献   
880.
AIM: The manner in which a cell responds to and influences its environment is ultimately determined by the genes that are expressed.To better understand cellular functions,the isolation of single cells and subsequent quantification of the expressed genes is essential.METHODS: Normal liver tissue was obtained from operation,snap-frozen in liquid nitrogen and sectioned in crystat.Individual hepatocytes were microdissected.RNA was extracted,then reverse transcribed and amplified using real-time quantitative polymerase chain reaction (PCR).RESULTS: Single hepatocytes were dissected by laser beam and catapulted to the microcentrifuge cap which was put above the slide.In this way,cells were collected,RNA was extracted,reverse transcribed to cDNA and used for analysis of RNA expression by real-time quantitative PCR.The amplification results showed that quantitation of the RNA inside the cell was compatible with the number of cells.CONCLUSION: The expression of RNA in single cells can be quantitated successfully by using laser microdissection and real-time PCR.These techniques provide an opportunity to monitor in vivo gene expression levels in single hepatocytes.  相似文献   
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