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1.
Richard Frazee M.D. Glennon Einspanier D.O. Mitchell S. Wachtel M.D. Eldo E. Frezza M.D. M.B.A. F.A.C.S. 《Surgery for obesity and related diseases》2007,3(2):191-175
BACKGROUND: Gastric bypass is an established bariatric procedure that has undergone multiple modifications to improve its effectiveness. The side-to-side stapled technique is well recognized, but closure of the gastrotomy/enterotomy by the stapler can potentially narrow the Roux limb. Because of this, many surgeons will hand suture the closure of the gastrotomy/enterotomy. To obviate this difficulty, we inserted the linear stapler from the stomach's greater curvature, using a double-stapled anastomosis that minimized the need for hand suturing. METHODS: We performed a retrospective analysis of 307 patients undergoing this technique for laparoscopic gastric bypass. The weight loss and 30-day morbidity and mortality were tabulated and compared with those in other published series. RESULTS: Of the 307 patients, none died postoperatively. The overall 30-day morbidity rate was 15%. Two leaks from the gastrojejunostomy and 2 from the jejunojejunostomy (1.2%) developed. The mean percentage of excess weight loss was 34% at 3 months, 52% at 6 months, 73% at 1 year, 71% at 2 years, and 69% at 3 years. CONCLUSION: The greater curve approach avoids Roux limb obstruction, minimizes the need for hand suturing, and uses standard trocar incisions. Our short-term follow-up results are similar to those of series of other techniques. 相似文献
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辛伐他汀对人低密度脂蛋白氧化修饰影响的实验研究 总被引:2,自引:2,他引:0
目的研究辛伐他汀在体外对低密度脂蛋白氧化修饰的影响.方法以低密度脂蛋白氧化修饰为模型,以硫代巴比妥酸反应物质(TBARS)生成量及相对电泳迁移率(REM)为指标,研究了辛伐他汀对铜离子(Cu2 )诱导低密度脂蛋白氧化修饰的抑制作用.结果随辛伐他汀浓度从1~10μmol/L的增加,TBARS值分别减少67.3%,73.9%,81.9%,REM值减少48.3%,55.2%,58.6%,呈浓度及时间依赖关系.其中10μmol/L辛伐他汀可几乎完全抑制低密度脂蛋白氧化.结论辛伐他汀在体外能明显抑制Cu2 诱导的低密度脂蛋白氧化修饰. 相似文献
4.
通过溴化聚苯醚和格利雅试剂反应,将不饱和基团烯丙基引入聚苯醚中实现其热固性改性,由^1H-NMR和FTIR进行结构表征。确定了烯丙化聚苯醚的固化工艺,并对其固化产物性能进行测试。结果表明:按合成新工艺制备的热固性聚苯醚,其固化产物具有优异的介电性能(低介电常数、低介电损耗因子),良好的耐溶剂性能和低吸湿性。 相似文献
5.
I. Ibarrola M. L. Sanz† P. M. Gamboa‡ A. Mir§ D. Benahmed§ A. Ferrer¶ M. C. Arilla A. Martínez J. A. Asturias 《Clinical and experimental allergy》2004,34(2):303-309
BACKGROUND: Allergoids are widely used in specific immunotherapy (SIT) for the treatment of IgE-mediated allergic diseases, but all techniques for standardization of conventional allergic extracts may not be appropriate for standardization of a glutaraldehyde (GA)-modified extract because of the unique characteristics of these extracts. OBJECTIVE: To assess an accurate methodology for standardization of chemically modified extracts. METHODS: GA-modified extracts from Parietaria judaica pollen were purified by diafiltration. Biochemical properties were investigated by determination of amino groups, chromatography, and SDS-PAGE. The IgE-binding activity was determined by skin prick test, enzyme allergosorbent test inhibition, basophil activation, and histamine release tests. Peripheral blood mononuclear cells (PBMCs) from P. judaica pollen-allergic subjects were stimulated with either native or allergoid extracts, and proliferation was measured. RESULTS: Biochemical data indicated a high degree of allergen polymerization resulting in extract components higher than 100 kDa. IgE-binding activity, both in vivo and in vitro, was reduced by more than 99.8%. Both allergen and allergoid induced PBMC proliferation and synthesis of blocking IgG antibodies at similar rates. Moreover, no evidence of introduction of new determinants by chemical modification was found. CONCLUSIONS: The preparation of GA-modified extracts by diafiltration is faster and more reliable than previous chromatographic methods. These modified extracts have drastically reduced their allergenicity while maintaining their immunogenicity, and therefore they can be used in safer and shortened schedules of SIT. 相似文献
6.
A brief mechanical or electrical stimulus to peripheral nerve afferents from the upper and lower limbs elicited a small and inconsistent EMG response of the orbicularis oculi muscles. This response was facilitated when the stimuli were delivered at fixed leading time intervals, of 45–300 ms, with respect to a supraorbital nerve electrical stimulus. Also, the peripheral nerve stimulus modified the conventional blink reflex responses, inducing facilitation of R1 and inhibition of R2. These results suggest a complex processing of sensory inputs from the face and the limbs at the brainstem, where they are probably integrated in a network of interneurons influencing the excitability of facial motoneurons. 相似文献
7.
Leoncio Garrido Bettina Pfleiderer Bruce G. Jenkins Carol A. Hulka Daniel B. Kopans 《Magnetic resonance in medicine》1994,31(3):328-330
Studies using magnetic resonance spectroscopy in human volunteers to evaluate their livers in vivo and to analyze their blood in vitro suggest that there are measurable amounts of silicon compounds in the blood of some women with implants and that there is migration of silicone to other organs such as the liver. 相似文献
8.
BDNF基因修饰神经干细胞移植后大鼠脊髓损伤移植处的基因表达变化 总被引:5,自引:0,他引:5
目的:了解脑源性神经营养因子(Brain-derived neurotrophic factor,BDNF)基因修饰神经干细胞移植到大鼠脊髓损伤处后的基因表达变化,为脊髓损伤修复提供基础研究资料。方法:大鼠随机分为4组:正常对照组,手术对照组,神经干细胞(Neural stem cells,NSCs)移植组,BDNF-NSCs移植组,各组分4个时相点(7d、1个月、2个月、3个月),利用细胞移植、X-gal组化、免疫组化、原位杂交等方法,观察了移植处细胞的标记基因(LacZ)表达和BDNF、胶质纤维酸性蛋白(GFAP)、神经丝-200(NF-200)的表达。结果:大鼠脊髓损伤移植处细胞中,有标记基因阳性细胞,BDNF强烈表达,尤其是BDNF-NSCs移植组的移植后1周和1个月时。各组各时相点均有GFAP和NF-200免疫反应阳性细胞和纤维。结论:BDNF基因修饰神经干细胞能在脊髓损伤移植处存活,强烈表达BDNF,BDNF基因修饰神经干细胞可以作为脊髓损伤修复的移植材料。 相似文献
9.
单甲氧聚乙二醇化学修饰药物酶的研究进展 总被引:4,自引:0,他引:4
用单甲氧基聚乙二醉(1)化学修饰药物酶是生化药物研究开发的重要手段之一。本文综述了1化学修饰药物酶的一般方法及修饰后酶在生物和理化性质方面的变化,同时对1研究前景进行展望,并指出了尚待解决的问题。 相似文献
10.
George G. J. M. Kuiper Petra E. de Ruiter J. Anton Grootegoed Albert O. Brinkmann 《Molecular and cellular endocrinology》1991,80(1-3):65-73
Androgen receptor synthesis and modification were studied in the human LNCaP cell line. Immunoblotting with a specific polyclonal antibody showed that the androgen receptor migrated as a closely spaced 110–112 kDa doublet on sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) gels. Most of the receptor protein is present in the higher molecular mass form. Pulse labelling experiments with [35S]methionine showed that the androgen receptor is synthesized as a single 110 kDa protein which is rapidly converted to a 112 kDa protein. Alkaline phosphatase treatment of cytosols from [35S]methionine pulse labelled cells caused a gradual elimination of the 112 kDa isoform with a concomitant increase of the 110 kDa isoform. This indicates that the observed 110 to 112 kDa upshift of the newly synthesized androgen receptor reflects receptor phosphorylation. Both isoforms can bind hormone and can undergo a hormone dependent transformation to a tight nuclear binding form, indicating that the 110 to 112 kDa conversion is not an obligatory step for hormone binding or receptor transformation. 相似文献