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221.
Stanley L Marks Elizabeth J Kather 《Veterinary Clinics of North America: Small Animal Practice》2003,33(5):1029-1060
The clinical documentation of enteropathogenic bacteria causing diarrhea in dogs is clouded by the presence of many of these organisms existing as normal constituents of the indigenous intestinal flora. The diagnosis of a putative bacterial enteropathogen(s) in dogs should be made based on a combination of parameters, including signalment and predisposing factors, clinical signs, serologic assays for toxins, fecal culture, and PCR. Relying on results of fecal culture alone is problematic, because C perfringens, C difficile, Campylobacter spp, and pathogenic and non-pathogenic E coli are commonly isolated from apparently healthy dogs [10,13,33]. Nevertheless, culture may be useful in procuring isolates for the application of molecular techniques, such as PCR, for detection of specific toxin genes or molecular typing of isolated strains to establish clonality in suspected outbreaks. The oversimplistic attempt to characterize bacterially associated diarrhea by anatomic localization of clinical signs should be discouraged, because most of the previously mentioned bacteria have been associated with small and large intestinal diarrhea. Accurate diagnosis of infections may require diagnostic laboratories to incorporate PCR-based assays using genus- and species-specific primers to facilitate detection of toxin genes and differentiation of species that appear phenotypically and biochemically similar. There has been tremendous interest in the application of microarray technology for the simultaneous detection of thousands of genes or target DNA sequences on one glass slide. This powerful tool could be used for detection of specific pathogenic bacterial strains in fecal specimens obtained from dogs in the future. 相似文献
222.
Regulation of Capacitation of Canine Spermatozoa during Co-culture with Heterologous Oviductal Epithelial Cells 总被引:2,自引:0,他引:2
AM Petrunkina K Simon A-R Günzel-Apel E Töpfer-Petersen 《Reproduction in domestic animals》2003,38(6):455-463
Progress of essential steps of the capacitation is coordinated in the oviductal isthmus, where sperm are stored in close contact with the epithelium. A crucial capacitational event is the phosphorylation of sperm membrane proteins. Regulation of the tyrosine phosphorylation by the oviduct has not been examined in dog sperm yet. The aim of this work was to study the effect of dog sperm binding to porcine oviductal epithelium on capacitation‐induced cellular and molecular changes. Epithelial cells were stripped from the oviducts of post‐puberal sows and cultured for 5–7 days at 39°C and 5% CO2 on Biomatrix‐covered Chamber slides. Sperm washed through Percoll was co‐incubated with the oviductal epithelium cell cultures in a bicarbonate Tyrode's medium. During co‐incubation, sperm membrane changes, the state of tyrosine phosphorylation and motility were determined after 3, 30, 90, 180, 240 and 360 min. Significant increases in the percentage of capacitated and dead cells were observed in unbound sperm, while bound sperm remained uncapacitated, live and motile. An increasing tyrosine phosphorylation of tail proteins in bound, unbound and control sperm suspensions and a subsequent phosphorylation of head proteins in unbound and control sperm suspensions were observed. A significant difference regarding head phosphorylation (p < 0.05) was found between sperm bound to oviductal epithelium and unbound sperm. Binding occurred mainly in sperm with non‐ phosphorylated heads, while higher proportions of phosphorylated cells were found in unbound populations. The head phosphorylation progressed significantly during incubation in unbound spermatozoa (p < 0.05); however, it was suppressed in population of sperm attached to oviductal epithelium. Significant correlations between motility parameters related to hyperactivation and tail phosphorylation were found in unbound sperm. These observations support the hypothesis that spermatozoa with non‐phosphorylated heads preferentially attach to epithelial cells. It can be concluded that tyrosine phosphorylation of head membrane proteins and capacitation are delayed in canine spermatozoa being in closed contact with oviductal epithelium. 相似文献
223.
Diagnosis of mastitis for therapy decisions. 总被引:2,自引:0,他引:2
Philip M Sears Kate K McCarthy 《Veterinary Clinics of North America: Food Animal Practice》2003,19(1):93-108, vi
Identifying specific groups of mastitis pathogens by their growth on selective agars can help identify the pathogens that are present in mastitic milk samples. This article addresses issues that are essential in making good use of diagnostic procedures to improve udder health on dairies. 相似文献
224.
鸭疫里氏杆菌各血清型在我国的分布 总被引:3,自引:1,他引:2
吕殿红 《广东畜牧兽医科技》2003,28(5):18-20
鸭疫里氏杆菌病(Riemerella anatipestifersis,RA)是家鸭、火鸡、鹅和多种其它鸟类的一种接触性传染病,能引起1~8周龄的鸭发生浆膜炎、心包炎、气囊炎和肝周炎等为特征的急性败血性传染病。我国近年来对该病病原的分离及其血清型的鉴定等方面进行了较多的研究,目前已证实我国有1、2、3、4、5、6、7、8、10、11、13、14、15、17等14种血清型的RA,另新发现4种新血清型(22、23、24、25型),多种血清型的存在是造成该病防制困难的重要原因。本文介绍了我国对RA血清型的研究,及各血清型在我国的分布,以期对综合防制该病有一定的启发和指导。 相似文献
225.
Guidi A. Iannone G. Castigliego L. Gianfaldoni D. 《Veterinary research communications》2004,28(1):193-196
Veterinary Research Communications - 相似文献
226.
Jennifer L Davis 《Veterinary Clinics of North America: Equine Practice》2003,19(3):765-778
In summary, peritonitis in the horse is a potentially life-threatening disease that must be treated promptly and aggressively. Therapy should be aimed at reducing systemic shock and hypovolemia, correction of the primary cause, antibiotic and anti-inflammatory therapy, and abdominal drainage and lavage. The prognosis depends on the ability to diagnose and treat the underlying cause and prevent the development of complications. Mortality rates can be as high as 59.7%, with horses developing postoperative peritonitis having a 56% mortality rate. Long-term complications like adhesion formation or internal abscesses may further reduce the survival rate. The prognosis is best determined by an early and quick response to aggressive treatment. 相似文献
227.
228.
Blomquist HL 《Science (New York, N.Y.)》1938,88(2272):59-60
229.
Kellogg VL 《Science (New York, N.Y.)》1913,38(982):601-602
230.