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61.
Mengjiao Fu Yuchen Liu Guannan Wang Peng Wang Jianing Zhang Chen Chen Mingliang Zhao Shan Zhang Jun Jiao Xuan Ouyang Yonghui Yu Bohai Wen Chengzhi He Jian Wang Dongsheng Zhou Xiaolu Xiong 《PLoS pathogens》2022,18(7)
Coxiella burnetii is the etiological agent of the zoonotic disease Q fever, which is featured by its ability to replicate in acid vacuoles resembling the lysosomal network. One key virulence determinant of C. burnetii is the Dot/Icm system that transfers more than 150 effector proteins into host cells. These effectors function to construct the lysosome-like compartment permissive for bacterial replication, but the functions of most of these effectors remain elusive. In this study, we used an affinity tag purification mass spectrometry (AP-MS) approach to generate a C. burnetii-human protein-protein interaction (PPI) map involving 53 C. burnetii effectors and 3480 host proteins. This PPI map revealed that the C. burnetii effector CBU0425 (designated CirB) interacts with most subunits of the 20S core proteasome. We found that ectopically expressed CirB inhibits hydrolytic activity of the proteasome. In addition, overexpression of CirB in C. burnetii caused dramatic inhibition of proteasome activity in host cells, while knocking down CirB expression alleviated such inhibitory effects. Moreover, we showed that a region of CirB that spans residues 91–120 binds to the proteasome subunit PSMB5 (beta 5). Finally, PSMB5 knockdown promotes C. burnetii virulence, highlighting the importance of proteasome activity modulation during the course of C. burnetii infection. 相似文献
62.
Yiwen Liu Jianfang Gao Min Xu Qianqian Zhou Zhongxiao Zhang Jiaxin Ye Rui Li 《Journal of cellular and molecular medicine》2022,26(13):3616
Congenital heart disease (CHD) is the most common birth defect, affecting approximately 1% of live births. Genetic and environmental factors are leading factors to CHD, but the mechanism of CHD pathogenesis remains unclear. Circular RNAs (circRNAs) are kinds of endogenous non‐coding RNAs (ncRNAs) involved in a variety of physiological and pathological processes, especially in heart diseases. In this study, three significant differently expressed circRNA between maternal embryonic day (E) E13 and E17 was found by microarray assay. Among them, the content of circ‐RCCD increases with the development of heart and was enriched in primary cardiomyocytes of different species, which arouses our attention. Functional experiments revealed that inhibition of circ‐RCCD dramatically suppressed the formation of beating cell clusters, the fluorescence intensity of cardiac differentiation marker MF20, and the expression of the myocardial‐specific markers CTnT, Mef2c, and GATA4. Next, we found that circ‐RCCD was involved in cardiomyocyte differentiation through negative regulation of MyD88 expression. Further experiments proved that circ‐RCCD inhibited MyD88 levels by recruiting YY1 to the promoter of MyD88; circ‐RCCD inhibited nuclear translocation of YY1. These results reported that circ‐RCCD promoted cardiomyocyte differentiation by recruiting YY1 to the promoter of MyD88. And, this study provided a potential role and molecular mechanism of circ‐RCCD as a target for the treatment of CHD. 相似文献
63.
Hong Lin Song Zhao Yuying Ye Lei Shao Nizhen Jiang Kun Yang 《The Korean journal of parasitology》2022,60(3):201
Babesia microti is one of the most common causative agents of babesiosis. A sensitive and rapid detection is necessary for screening potentially infected individuals. In this study, B. microti cytochrome c oxidase subunit I (cox1) was selected as the target gene, multiple primers were designed, and optimized by a recombinase-aided amplification (RAA) assay. The optimal primers and probe were labeled with fluorescein. The sensitivity of fluorescent RAA (fRAA) was evaluated using gradient diluents of the cox1 recombinant plasmid and genomic DNA extracted from whole blood of B. microti infected mice. The specificity of fRAA was assessed by other transfusion transmitted parasites. The analytical sensitivity of the fRAA assay was 10 copies of recombinant plasmid per reaction and 10 fg/μl B. microti genomic DNA. No cross-reaction with any other blood-transmitted parasites was observed. Our results demonstrated that the fRAA assay would be rapid, sensitive, and specific for the detection of B. microti. 相似文献
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65.
Aaron Mendez-Bermudez Liudmyla Lototska Melanie Pousse Florent Tessier Oliver Croce Chrysa
M Latrick Veronica Cherdyntseva Joe Nassour Jiang Xiaohua Yiming Lu Corinne Abbadie Sarantis Gagos Jing Ye Eric Gilson 《Nucleic acids research》2022,50(13):7493
Cellular senescence triggers various types of heterochromatin remodeling that contribute to aging. However, the age-related mechanisms that lead to these epigenetic alterations remain elusive. Here, we asked how two key aging hallmarks, telomere shortening and constitutive heterochromatin loss, are mechanistically connected during senescence. We show that, at the onset of senescence, pericentromeric heterochromatin is specifically dismantled consisting of chromatin decondensation, accumulation of DNA breakages, illegitimate recombination and loss of DNA. This process is caused by telomere shortening or genotoxic stress by a sequence of events starting from TP53-dependent downregulation of the telomere protective protein TRF2. The resulting loss of TRF2 at pericentromeres triggers DNA breaks activating ATM, which in turn leads to heterochromatin decondensation by releasing KAP1 and Lamin B1, recombination and satellite DNA excision found in the cytosol associated with cGAS. This TP53–TRF2 axis activates the interferon response and the formation of chromosome rearrangements when the cells escape the senescent growth arrest. Overall, these results reveal the role of TP53 as pericentromeric disassembler and define the basic principles of how a TP53-dependent senescence inducer hierarchically leads to selective pericentromeric dismantling through the downregulation of TRF2. 相似文献
66.
67.
发酵液内氨甲酰妥布拉霉素的定量测定 总被引:2,自引:2,他引:0
报道了应用一种以测量图象面积为指标的Zy-300A多功能抑菌圈测量仪,能够精确、稳定、快速地测定发酵液经薄层层析生物显迹后单组分氨甲酰妥布拉霉素的抑菌斑面积,然后从绘制的标准曲线中直接读取氨甲酸妥布拉霉素在发酵液中的含量,从而排除了其他组分对测定的干扰。试验证明,用Zy-300A多功能抑菌圈测量仪测定抗生素薄层层析生物显迹的抑菌斑,具有线性宽、精密度高、重复性强、操作简单方便等优点.本方法的建立为抗生素的纯品检定和多组分抗生素发酵、分离和纯化提供了准确的定量数据. 相似文献
68.
高通量测序技术的发展促进了组学技术在环境微生物研究中的广泛应用,而宏基因组学是目前最为关键和成熟的组学方法。生物信息学在微生物宏基因组学研究中具有至关重要的作用。它贯穿于宏基因组学的数据收集和存储、数据处理和分析等各个阶段,既是宏基因组学推广的最大瓶颈,也是目前宏基因组学研究发展的关键所在。本文主要介绍和归纳了目前在高通量宏基因组测序中常用的生物信息学分析平台及其重要的信息分析工具。未来几年之内,测序成本的下降和测序深度的增加将进一步增大宏基因组学研究在数据存储、数据处理和数据挖掘层面的难度,因此相应生物信息学技术与方法的研究和发展也势在必行。近期内我们应该首先加强基础性分析和存储平台的建设以方便普通环境微生物研究者使用,同时针对目前生物信息分析的瓶颈步骤和关键任务重点突破,逐步发展。 相似文献
69.
70.
【目的】系统比较两种不同保护剂冻干的仔猪副伤寒活疫苗(耐热苗和常规苗)质量指标,为科学评价两种疫苗质量提供参考。【方法】制备耐热苗和常规苗各3批,分别进行物理性状、纯粹性、活菌计数、安全性、剩余水分、真空度和保存期等参数测定和比较,同时比较冻干前后的活菌存活率及耐老化性能。任选耐热苗与常规苗1批,按3×109 CFU分别口服与肌肉注射仔猪各5头,设相同条件下不免疫对照5头,30 d后静脉注射致死量猪霍乱沙门氏菌,临床观察30 d后评估疫苗的效力。【结果】耐热苗及常规苗的物理性状、纯粹性、活菌计数、安全性、剩余水分、真空度均符合现行《中国兽药典》的要求。3批耐热苗冻干菌存活率分别为88.2%、83.1%和86.4%,耐老化试验后的活菌存活率为83.6%、82.9%和88.8%;然而3批常规苗冻干菌存活率分别为52.3%、56.2%和61.4%,耐老化活菌存活率分别为58.5%、60.2%和54.7%。经37°C、7 d耐老化试验结果显示,耐热苗物理性状良好,而常规苗原有团块表面凹陷1/4-1/2。保存期结果表明耐热苗4°C有效期可达24个月,常规苗仅为9个月。仔猪免疫攻毒结果表明,耐热苗肌肉注射及口服免疫均达100%(5/5)保护;常规苗肌肉注射达80%(4/5)保护,口服达100%(5/5)保护,不免疫对照0保护(5/5死亡)。【结论】耐热苗具有较高的冻干菌存活率和良好的耐老化性能,4°C可长期保存且不影响其免疫效力。 相似文献