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71.
Our objective was to correlate p16, p21cip1, p27kip1, and cyclin E protein expression with the degree of dysplasia on ThinPrep Papanicolaou (Pap) smears using a modified immunoperoxidase staining. Smears read as normal, atypical squamous cells of undetermined significance (ASC-US), low-grade squamous intraepithelial lesion (LSIL), or high-grade SIL (HSIL) were identified and tested for high-risk human papillomavirus (HR-HPV). Additional smears were processed for immunoperoxidase for p16, p21cip1, p27kip1, and cyclin E. Thirty-four smears were satisfactory for study. The p16 was positive in all nine HSIL, in four of nine LSIL, and in one of seven ASC-US. The p27kip1 was positive in all nine HSIL, in eight of nine LSIL, and in one of seven ASC-US. The p21cip1 was positive in all nine HSIL, in one of nine LSIL, and in one of seven ASC-US. Cyclin E was positive in seven of nine HSIL and in one of nine LSIL and in none of the ASC-US smears. Normal smears were negative for all the antigens. There was poor correlation of protein expression and HR-HPV infection. We concluded that p16, p21cip1, p27kip1, and cyclin E can be demonstrated on Pap smears and they are expressed differentially in dysplastic cells, with highest expression in HSIL. The p21cip1 and cyclin E showed the greatest correlation with HSIL.  相似文献   
72.
目的:DNA甲基化和组蛋白乙酰化是基因表达调控的主要形式。人类免疫缺陷病毒(HIV-1)可引起T淋巴细胞DNA甲基化酶上调。本文旨在明确HIV-1对细胞周期依赖刺激酶抑制剂p21^WAF1表达的影响。方法:建立HIV-1感染的Hut78细胞系;以RT-PCR和Westem blotting 分析p21^WAF1表达情况;以亚硫酸氢钠修饰DNA和基因测序,研究p21^WAF1基因启动子甲基化,以Western blot-ting 和染色体免疫测定探究总组蛋白和与p21^WAF1基因启动子相关的组蛋白乙酰化水平。并以GST pull-down和免疫沉淀分析HIV-1导致乙酰化及乙酰化引起p21^WAF1过表达的可能机理。结果:HIV-1感染后,其反式激活蛋白Tat与辅助转录因子P/CAF、hGCN5结合,共同刺激组蛋白H3乙酰化。尽管p21^WAF1启动子部分区域有甲基化发生,但p21^WAF1表达仍上调。这可能与E2A对p21^WAF1的作用有关。结论:HIV-1感染可引起T淋巴细胞p21^WAF1基因的甲基化和乙酰化紊乱,导致p21^WAF1表达增强。  相似文献   
73.
The embryonic chick is able to regenerate the retina after it has been removed. We have previously shown that proliferating stem/progenitor cells present in the ciliary body/ciliary marginal zone (CB/CMZ) of the chick eye are responsible for regeneration, which can be induced by ectopic fibroblast growth factor-2 (FGF2) or Sonic hedgehog (Shh). Here, we reveal the mechanisms showing how FGF2 and Shh signaling are interdependent during retina regeneration. If the FGF pathway is inhibited, regeneration stimulated by Shh is inhibited. Likewise, if the Hedgehog pathway is inhibited, regeneration stimulated by FGF2 is inhibited. We examined early signaling events in the CB/CMZ and found that FGF2 or Shh induced a robust Erk phosphorylation during the early stages of retina regeneration. Shh also up-regulated the expression of several members of the FGF signaling pathway. We show that ectopic FGF2 or Shh overexpression increased the number of phosphohistone 3 (PH3)-positive cells in the CB/CMZ and inhibition of either pathway decreased the number of PH3-positive cells. Additionally, both FGF and Hh signaling are required for cell survival in the CB/CMZ, whereas Hh and not FGF signaling plays a role in maintaining the identity of the retinal progenitor population in this region. Combined, our results support a model where the FGF and Hedgehog pathways work together to stimulate retina regeneration.  相似文献   
74.
双基因共表达在血管再狭窄研究中的应用   总被引:2,自引:0,他引:2  
目的 观察携带反义凝血酶受体(ATR)和p21的双基因载体共表达后对血管平滑肌细胞增殖的抑制作用,为再狭窄基因治疗寻求新途径。方法 以携带ATR或/和p21的单、双基因载体重组腺病毒伴随病毒(rAAV)感染培养的人主动脉平滑肌细胞(hASMC),用半定量RT-PCR检测各基因的整合与表达,MTT法测定病毒感染后不同时间点的细胞存活率。将携带AP双基因的rAAV导入WKY大鼠拉伤侧的颈总动脉,免疫组织化学法分别检测凝血酶受体(TR)和p21两基因在动脉壁中的表达。结果 RT-PCR结果显示,TR单基因的mRNA表达降低,p2l单基因表达升高,AP双基因得到了共表达;MTT法测定的生长曲线显示,双基因对hASMC增殖的抑制作用大于两个单基因;免疫组织化学证实,AP双基因导入后,TR基因的表达受到完全抑制,p2l基因的表达明显增加,血管新生内膜与平滑肌细胞的增殖受到了抑制。结论 ATR和p21双基因共表达在体外可明显抑制ASMC的增殖,在体内可明显抑制血管内膜新生和中膜的增生。  相似文献   
75.
The p53 tumour suppressor gene is a cell cycle regulator, able to induce cell cycle arrest to allow DNA repair or apoptosis. The molecular mechanisms underlying p53 action imply transactivation of p53 dependent genes such as WAF1 (for wild type p53 associated fragment 1) and the murine double minute (MDM2) gene. In some cases, inactivation of the p53 gene results from p53 gene mutations leading to p53 protein accumulation, but in others it may results from mechanisms other than mutation, such as interaction with viral or cellular proteins. The expression of p53 protein and p53 transactivated gene proteins p21/WAF1 and MDM2, combined with in situ detection of apoptosis, was studied in specimens of CMV-infected patients as an in vivo model of p53 alteration not due to point mutation. p53 positivity was found in CMV + cells in different tissues, in cells with typical inclusion bodies, and in in situ hybridization and immunohistochemistry CMV + cells without inclusions (hidden infection). Although this p53 reactivity was accompanied by the expression of MDM2 and p21/WAF1 proteins, the patterns of MDM2 and p21/WAF1 protein expression were mutually exclusive, and were associated with the presence or absence of inclusion bodies. Nuclei bearing inclusion bodies were usually MDM2 +, p21/WAF1?, while hidden infected cells were usually MDM2?, p21/WAF1 +. Apoptosis was not detected in any tissue section from CMV-infected patients. Two alternative patterns were found in CMV-infected tissues: p53 +, p21/WAF1 +, MDM2?, or p53 +, p21/WAF1?, MDM2 + protein expression. These may represent examples of p53 dependent alternative effects in the course of CMV infection. Early stages are represented by CMV + cells without inclusion bodies, which display p53 and p21/WAF1 expression, suggesting that p53 could be acting as a growth suppressor protein. Late CMV infection is represented by cells harbouring inclusion bodies. These cells showed a p53 +, p21/WAF1?, MDM2 + profile, consistent with MDM2 mediated p53 inactivation. The absence of p21/WAF1 expression and lack of apoptosis suggest that the p53 protein expressed by MDM2 + cells could be functionally inactivated in CMV-infected cells with inclusion bodies. Previous studies have suggested that p53 inactivation by MDM2 over-expression occurs in sarcomas and lymphomas. Our observations seem to indicate that this mechanism of MDM2 mediated p53 inactivation may play a role in the late phase of CMV infection.  相似文献   
76.
We have used 9 conventional RFLPs and 6 dinucleotide repeat polymorphisms on chromosome 21q to demonstrate that 17 of 19 cases of rea(21q21q) were consistent with isochromosomes i(21q) with the remaining 2 being true Robertsonian translocations. Eight of the 17 isochromosomes were of maternal origin and 9 cases were paternally derived. The 2 Robertsonian translocations were both maternally derived. Of the 17 isochromosomes, 7 were dicentric Wc(21q)I and 10 were monocentric M21q)l. Both rob(21q21q) were monocentric. Our findings agree with those made in 17 previously published cases of rea(21q21q). The parental origins of the i(21q) were equally divided between maternal (n = 17) and paternal (n = 15) origins. All 4 true rob(21q21q) reported to date are of maternal origin. Collectively, it appears that most homologous rearrangements of chromosome 21 are isochromosomes and only a small proportion are consistent with true Robertsonian translocations. © 1993 Wiley-Liss, Inc.  相似文献   
77.
Summary The oestrogenic component of oral contraceptives affects the activity of liver enzymes and the concentrations of plasma proteins implicated in steroid metabolism and transport. The present study was designed to determine these effects on the kinetics of prednisone and prednisolone. After an oral dose of prednisone, women on oral contraceptive steroids (n=10) had higher mean (±SD) area under the plasma concentration versus time curves of total (428±67 µg/ml/min vs 188±28 µg/ml/min, p<0.001) and unbound prednisolone (64±10 µg/ml/min vs 41±10 µg/ml/min, p<0.001) than women not taking oral contraceptive steroids (n=10). The differences were attributable to a lower non-renal clearance of prednisolone and to a higher apparent systemic availability of the drug in contraceptive users than in the controls. The affinity of albumin and transcortin for prednisolone was lower in women on oral contraceptives than in controls (p<0.001). Thus, altered kinetics and protein binding may account for the known increase in glucocorticoid efficacy by oestrogens.  相似文献   
78.
黄维清  纪萍  王海燕 《河北医学》2001,7(3):206-208
目的:研究同一胃癌中癌基因和抑癌基因蛋白产物的表达。方法;应用免疫组织化学SP方法检测10例正常胃粘膜、10例萎缩性胃炎、10例肠上皮化生的胃壁组织和145例胃癌组织中P21和P53蛋白的表达水平。结果:10例正常胃粘膜、10例萎缩性胃炎、10例肠上皮化生的胃壁组织中未发现P21和P53。145例胃癌组织中P21和 P53的阳性检出率分别为55.2%和51.2%。表达阳性的P53定位于肿瘤核内,P21定位于细胞膜或细胞浆上。P21和P53的阳性表达率与胃癌的分化程度呈正相关。结论;检测P21和P53有助于评估胃癌的预后。  相似文献   
79.
目的探讨D7S2 1位点在河北汉族人群分布的多态性 ,为DNA指纹数据库的构建及其法医学应用提供基础资料。方法应用MVR PCR方法和聚丙烯酰胺梯度凝胶电泳银染法对 12 4名河北汉族人群无关个体D7S2 1位点进行了快速检测 ,并进行数字编码。结果每一个体平均得到 3 6个数字编码 ,未发现任何两个无关个体所有编码相同 ,两无关个体 3 6个编码相同的机率为 3 .4 8× 10 -18。三种重复单位a 型、t 型和o 型出现的机率分别为 4 8.5 %、4 9.5 %和 2 .1%。该位点杂合度为 0 .9876,非父排除率为 0 .974 6,多态性信息含量为 0 .9872。结论D7S2 1位点在河北汉族人群中具有高度的多态性 ,聚丙烯酰胺梯度凝胶电泳银染法简便、快速 ,具有一定的实用价值  相似文献   
80.
肺癌诊断中CYFRA_(21-1)、CA_(50)、CEA联检的临床意义   总被引:9,自引:0,他引:9  
目的 :探讨血清CYFRA2 1- 1、CA50 、CEA变化对诊断肺癌的临床价值。方法 :应用放射免疫法对 186例肺癌患者进行血清CYFRA2 1- 1、CA50 、CEA联合检测。结果 :肺癌组患者血清CYFRA2 1- 1、CA50 、CEA检测水平明显高于正常对照组 (P <0 .0 1)、三项联合 (CYFRA2 1- 1+CA50 +CEA)检测的敏感性和准确性最高 ,分别为 :91.4 %、86.2 % ,优于二项和单项检测。结论 :三项肿瘤标志联合检测可提高肺癌的早期诊断率 ,在病情检测方面可为临床提供有价值的资料。  相似文献   
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