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101.
102.
Interdigestive small bowel motility and duodenal bacterial overgrowth in experimental acute pancreatitis 总被引:10,自引:0,他引:10
I. D. Van felius L. M. A. akkermans K. bosscha A. Verheem W. Harmsen† M. R. Visser† & H. G. Gooszen 《Neurogastroenterology and motility》2003,15(3):267-276
The objective of this study is to investigate the effects of an acute necrotizing pancreatitis (ANP), without biliary obstruction, on the migrating motor complex (MMC), small bowel bacterial overgrowth (SBBO), bacterial translocation (BT) and infection of the pancreas simultaneously. Rats were divided into four groups: mild pancreatitis, control, ANP and sham operated control. Jejunal myoelectrodes were used to measure MMCs. Blood, peritoneal fluid, bile, and abdominal organs were harvested for microbial culturing 72 h after induction of pancreatitis. The splenic portion of the pancreas was taken for histology. During ANP the MMC cycle length was significantly increased from 14.1 +/- 0.2 to 22.4 +/- 1.9 min (P < 0.05). The duodenum of ANP rats was in contrast with the other groups characterized by Enterobacteriacae (> 3 log 10 CFU g-1 in seven of 12 rats, P < 0.05). A positive correlation (r = 0.78, P < 0.01) existed between duodenal Gram-negative and anaerobic flora and the MMC cycle. Correlation between MMC cycle length and BT to the pancreas was positive as well (r = 0.70, P < 0.01). A positive correlation (r = 0.85, P < 0.01) was found between the severity of pancreatitis and duodenal bacterial overgrowth. During ANP without biliary obstruction, the jejunal MMC is disturbed and consequently SBBO occurs. The correlation between the severity of pancreatitis, the disturbance of the MMC and SBBO suggests an important pathophysiological role of the proximal small bowel in the infection of pancreatic necrosis. 相似文献
103.
V. UMBRAIN J. D'HAESE M. ALAFANDY E. DE ROOVER A. SCHOUTENS B. VAN GANSBEKE A. ALBERT G. GOFFINET F. CAMU F. J. LEGROS 《Acta anaesthesiologica Scandinavica》1997,41(1):25-34
Background: Liposomes containing local anaesthetics have been administered intrathecally and in the epidural space. Poor attention has been given to the pharmacokinetics of liposomes as drug carriers. Therefore, we observed the biodistribution of liposomes after intrathecal injection in rats by scintigraphic imaging during 24 h.
Methods: We administered99 Tc-labeled multilamellar (MLV) and small unilamellar vesicles (SUV) of defined size and volume dispersities into the cerebrospinal fluid at the lumbar level. Those vesicles were free of contamination by radiolabeled colloids as visualized by light and electron microscopy and of neurotoxic products from phosphatidylcholine hydrolysis and peroxidation, both during the preparation process and after 24 h incubation in cerebrospinal fluid at 37°C in vitro.
Results: SUV immediately diffused from the lumbar site of injection to the head and were cleared between 1 and 24 h after injection. MLV were cleared more slowly from the spinal space and appeared in the head region 1 h after injection where they accumulated up to 24 h. These differences were explained in terms of vesicle sizes and volumes. SUV with 0.05 μm diameters were rapidly absorbed into the blood through the arachnoid granulations. In contrast, particles larger than the upper size limit of the arachnoid granulations permeability (±8 μm) could accumulate in the head with a slow elimination rate.
Conclusion: This difference in clearance from the intrathecal space outlines the importance of defining the size of the liposomes, the distribution of a tracer or a drug inside the liposomal preparation, the chemical stability and the absence of toxic degradation products of liposome formulations before clinical use. 相似文献
Methods: We administered
Results: SUV immediately diffused from the lumbar site of injection to the head and were cleared between 1 and 24 h after injection. MLV were cleared more slowly from the spinal space and appeared in the head region 1 h after injection where they accumulated up to 24 h. These differences were explained in terms of vesicle sizes and volumes. SUV with 0.05 μm diameters were rapidly absorbed into the blood through the arachnoid granulations. In contrast, particles larger than the upper size limit of the arachnoid granulations permeability (±8 μm) could accumulate in the head with a slow elimination rate.
Conclusion: This difference in clearance from the intrathecal space outlines the importance of defining the size of the liposomes, the distribution of a tracer or a drug inside the liposomal preparation, the chemical stability and the absence of toxic degradation products of liposome formulations before clinical use. 相似文献
104.
通过对补中益气汤及西药治疗慢性乙型肝炎临床疗效的对比研究,发现补中益气汤能较快改善慢性乙型肝炎的临床症状及体征,改善肝功能,促使乙型肝炎病毒血清学标志好转(HBsAg、HBeAg转阴或滴度下降,抗-HBe或抗-HBs转为阳性),与西药治疗对照组比较有显著性差异(P<0.05)。动物实验观察了补中益气汤对小鼠肝组织DNA、RNA、蛋白质合成的影响,结果表明,补中益气汤对三者的合成均有明显的促进作用。其抗肝炎的作用机制可能与该方增强肝脏蛋白质的合成,促进肝组织的修复,改善机体整体的抗病机能有关。 相似文献
105.
106.
男性不育症患者中YRRM2基因缺陷的研究 总被引:2,自引:1,他引:1
YRRM基因是控制精子生成与成熟的一个重要因素,一旦该基因缺陷,将会造成无精或少精。本研究对340例无精与少精患者的外周血标本进行了PCR基因扩增筛查,结果发现7例为该基因缺陷,占2%。证明YRRM2的缺陷也是造成中国人群男性不育的一个原因,从而可作为指导医生采用适当治疗方法的一个可靠指标。在实验过程中,采用直接加热白细胞提取基因组DNA,并以此作为模板对YRRM2基因进行扩增,既节省时间和经费,又保持良好的扩增效果,使之可用于临床医院作为常规检查。 相似文献
107.
目的:建立一种应用T7 RNA聚合酶体外转录合成大量siRNA的方法。方法:以萤火虫荧光素酶为靶标,应用T7 RNA聚合酶体外转录合成siRNA,脂质体转染法将其导入HepG2细胞中,通过测定荧光素酶的量,评价siRNA对萤火虫荧光素酶基因表达的抑制作用。结果:合成了以萤火虫荧光素酶为靶标的siRNA,合成的siRNA能特异性地抑制荧光素酶基因的表达,抑制率为80%。结论:建立了一种经济简便的体外合成siRNA的方法。 相似文献
108.
人正、反义转化生长因子beta1基因真核表达载体的构建 总被引:1,自引:0,他引:1
目的 :构建人转化生长因子beta 1(TGFβ1)正、反义基因真核表达载体。方法 :从人胎脑的cDNA文库中扩增出TGFβ1共 12 84bp长的DNA片段后 ,与T载体直接进行高效连接 ,并测序证实无突变。接着利用TGFβ1引物两端所设计的酶切位点将目的片段定向亚克隆到真核表达载体pcDNA3.1( )。构建的正反义表达重组体 (pcDNA3.1 TGFβ1和pcDNA3.1 antiTGFβ1)经限制性内切酶消化证实其中有目的片段完整插入。结果 :本实验成功构建了人正、反义TGFβ1基因真核表达载体。结论 :人正、反义TGFβ1基因真核表达载体的构建 ,为今后研究腹膜纤维化的防治奠定了实验基础。 相似文献
109.
Down-regulation amyloid β-protein 42 production by interfering with transcript of presenilin 1 gene with siRNA 总被引:2,自引:0,他引:2
Huan-min LUO Hui DENG Fei XIAO Qin GAO Wen WENG Pei-fen ZHANG Xiao-guang LI Neuropharmacological Research Laboratory College ofPharmacy Ji-nan University Guangzhou China 《Acta pharmacologica Sinica》2004,(12)
AIM:ToinvestigatethepathogenesisofAβ42yieldingandnewdrugtargetsaswellasthepossibilityofRNAinterference(RNAi)techniquefortreatmentofAlzheimerdisease(AD).METHODS:HumanADpresenilin1(PS1)cDNAsequencewasobtainedfromNCBIwebsite.ThethreesitesofRNAiactionandonemissensecontrolsitewereselectedinPS1cDNAthroughonlinedesignofAmbioncompany.Toconfirmspecificityofthesesites,weconductedaBLASTsearchoftheIMAGEESTlibrary.Thecorrespondingdouble-strandedDNAwasusedtoconstructpSilencer3.1-H1p… 相似文献
110.