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Xi Lu Xinyi Yang Xue Li Yun Lu Zhitao Ren Longyin Zhao Xinxin Hu Jiandong Jiang Xuefu You 《PloS one》2013,8(7)
Background
Staphylococcus aureus can cause severe infections, including bacteremia and sepsis. The spread of methicillin-resistant Staphylococcus aureus (MRSA) highlights the need for novel treatment options. Sodium new houttuyfonate (SNH) is an analogue of houttuynin, the main antibacterial ingredient of Houttuynia cordata Thunb. The aim of this study was to evaluate in vitro activity of SNH and its potential for synergy with antibiotics against hospital-associated MRSA.Methodology
A total of 103 MRSA clinical isolates recovered in two hospitals in Beijing were evaluated for susceptibility to SNH, oxacillin, cephalothin, meropenem, vancomycin, levofloxacin, minocycline, netilmicin, and trimethoprim/sulfamethoxazole by broth microdilution. Ten isolates were evaluated for potential for synergy between SNH and the antibiotics above by checkerboard assay. Time-kill analysis was performed in three isolates to characterize the kill kinetics of SNH alone and in combination with the antibiotics that engendered synergy in checkerboard assays. Besides, two reference strains were included in all assays.Principal Findings
SNH inhibited all test strains with minimum inhibitory concentrations (MICs) ranging from 16 to 64 µg/mL in susceptibility tests, and displayed inhibition to bacterial growth in concentration-dependent manner in time-kill analysis. In synergy studies, the combinations of SNH-oxacillin, SNH-cephalothin, SNH-meropenem and SNH-netilmicin showed synergistic effects against 12 MRSA strains with median fractional inhibitory concentration (FIC) indices of 0.38, 0.38, 0.25 and 0.38 in checkerboard assays. In time-kill analysis, SNH at 1/2 MIC in combination with oxacillin at 1/128 to 1/64 MIC or netilmicin at 1/8 to 1/2 MIC decreased the viable colonies by ≥2log10 CFU/mL.Conclusions/Significance
SNH demonstrated in vitro antibacterial activity against 103 hospital-associated MRSA isolates. Combinations of sub-MIC levels of SNH and oxacillin or netilmicin significantly improved the in vitro antibacterial activity against MRSA compared with either drug alone. The SNH-based combinations showed promise in combating MRSA. 相似文献3.
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Yongjian Gong Weidong Xu Yang Chen Yun Liu Yuan Yang Beibei Wang Zhitao Lu Hung‐Chih Lin Xiaoyu Zhou Xiaoguang Zhou 《Journal of cellular and molecular medicine》2019,23(11):7664-7672
MicroRNA (miRNA) critically controls gene expression in many biological processes, including lung growth and pulmonary surfactant biosynthesis. The present study was conducted to investigate whether miR‐20a‐5p had such regulatory functions on alveolar type II (AT‐II) cells. To accomplish this, miR‐20a‐5p–overexpressed and miR‐20a‐5p–inhibited adenoviral vectors were constructed and transfected into cultured AT‐II cells that were isolated from rat foetal lungs of 19 days' gestation. Transfection efficiency was confirmed by observing the fluorescence of green fluorescent protein (GFP) carried by the viral vector, whereas miR‐20a‐5p levels were verified by real‐time PCR. The CCK‐8 assay was used to compare the proliferation ability of AT‐II cells that had over‐ or underexpressed miR‐20a‐5p. The expression of surfactant‐associated proteins (SPs) and phosphatase and tensin homolog (PTEN) was measured by real‐time PCR and Western blotting. In AT‐II cells, transfection resulted in over‐ or under‐regulation of miR‐20a‐5p. While overexpression of miR‐20a‐5p promoted pulmonary surfactant gene expression, its underexpression inhibited it. Consistent with its role in negatively regulating the pulmonary surfactant gene, an opposite pattern was observed for miR‐20a‐5p regulation of PTEN. As a result, when miR‐20a‐5p was rendered overexpressed, PTEN was down‐regulated. By contrast, when miR‐20a‐5p was underexpressed, PTEN was up‐regulated. Neither overexpression nor underexpression of miR‐20a‐5p altered the cell proliferation. miR‐20a‐5p plays no role in proliferation of foetal AT‐II cells but is a critical regulator of surfactant gene expression. The latter appears to be achieved through a regulatory process that implicates expression of PTEN. 相似文献
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以蒙古黄芪为试验材料,设置大田随机区组试验,研究苗期、开花期和根茎伸长期叶面喷施不同浓度硅(500、1000、2000和4000 mg/L)对蒙古黄芪生长发育、抗氧化酶活性、药材产量和品质的影响,并检测施硅对黄芪白粉病、根腐病的防治效果,以揭示硅对增强黄芪抗病性、提升品质和产量的影响机理,为生产中蒙古黄芪的高效栽培提供理论依据。结果表明:(1)在不同生育时期,喷施不同浓度硅能增加蒙古黄芪株高、茎粗、株幅和叶绿素含量,促进蒙古黄芪生长,并以2000 mg/L硅处理效果较佳。(2)不同生育时期喷施硅能提高蒙古黄芪叶片SOD、CAT、POD和APX等抗氧化酶活性,降低MDA含量,以开花期、根茎伸长期2000 mg/L硅处理较佳。(3)施硅能有效降低蒙古黄芪白粉病、根腐病的病情指数,当施硅浓度为2000 mg/L时防效均达到最高,并分别达到47.05%和39.08%。(4)施硅处理能有效提高蒙古黄芪单株干、鲜生物量、产量以及可溶性浸出物和黄芪甲苷含量等品质指标,并在2000 mg/L硅浓度处理下均达到最佳水平,此时可溶性浸出物和黄芪甲苷含量分别比对照显著提高了16.48%和31.96%。研究发现,叶面喷施适宜浓度硅可显著增强蒙古黄芪对白粉病、根腐病的抗性,促进植株生长,进而显著提高药材产量,改善药材品质,并以硅浓度为2000 mg/L时效果最佳。 相似文献
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组学分析技术的发展推动生物学逐渐成为一门以数据分析为中心的科学。依托生物数据在细胞整体系统水平建立数字细胞模型,对于理解细胞系统组织原理和生命产生进化规律,预测各种环境和基因扰动对细胞功能的影响并指导设计人工生命具有重要意义,因此数字细胞的构建模拟设计已成为合成生物学的核心研究内容与底层支撑技术。本文重点对天津工业生物技术研究所创立十年来在数字细胞研究方面的进展进行回顾介绍,重点包括基因组尺度代谢网络模型的构建、质控以及其在途径设计和指导菌种代谢工程改造方面的应用,进一步结合近年来细胞模型研究的前沿趋势,对整合多种约束的模型的构建和分析研究方面的最新成果进行了介绍,最后对数字细胞研究的未来发展方向进行展望。数字细胞技术将与基因组测序、合成和编辑等合成生物学前沿技术一起提升人们对生命进行读写改创的能力。 相似文献
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Seungwon Choi Kelsey P. Taylor Marios Chatzigeorgiou Zhitao Hu William R. Schafer Joshua M. Kaplan 《PLoS genetics》2015,11(7)
C. elegans undergoes periods of behavioral quiescence during larval molts (termed lethargus) and as adults. Little is known about the circuit mechanisms that establish these quiescent states. Lethargus and adult locomotion quiescence is dramatically reduced in mutants lacking the neuropeptide receptor NPR-1. Here, we show that the aroused locomotion of npr-1 mutants results from the exaggerated activity in multiple classes of sensory neurons, including nociceptive (ASH), touch sensitive (ALM and PLM), and stretch sensing (DVA) neurons. These sensory neurons accelerate locomotion via both neuropeptide and glutamate release. The relative contribution of these sensory neurons to arousal differs between larval molts and adults. Our results suggest that a broad network of sensory neurons dictates transitions between aroused and quiescent behavioral states. 相似文献
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对健康的日本沼虾(1.40±0.12)g分别肌肉注射0.6×10~6、2×10~6、4×10~6、6×10~6 CFU/mL的停乳链球菌茵液10μL、注射后3 h、6 h、9 h、12h、24h、5d、10d分别采集肝胰腺、肌肉和鳃组织,测定其中的总超氧化物歧化酶(T-SOD)活性,研究停乳链球菌时日本沼虾T-SOD活性的影响,研究结果显示,肝胰腺中T-SOD活性于注射5d后达到最大值(P0.05),10d后0.6×10~6、2×10~6和4×10~6 CFU/mL,组T-SOD活性下降并接近对照组水平,而最高浓度组(6×10~6 CFU/mL)T-SOD酶活性仅有对照组的46%。肌肉和鳃中T-SOD活性均在注射6 h后达到最大值,注射10 d后,4×10~6和6×10~6 CFU/mL组的肌肉和6×10~6 CFU/mL组的鳃组织中T-SOD活性均仅有对照组的50%左右。另外,肌肉组织中T-SOD的峰值远高于鳃和肝胰腺组织中的峰值。上述结果表明,停乳链球菌不仅影响日本沼虾机体T-SOD酶的活性。而且肌肉、鳃和肝胰腺组织中酶的活性应答时间不同,且组织内酶活性的应答与菌的感染方式有关,另外,注射高浓度停乳链球菌长时间后会降低其组织中T-SOD酶活性。 相似文献
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Two models have been proposed for endophilin function in synaptic vesicle (SV) endocytosis. The scaffolding model proposes that endophilin's SH3 domain recruits essential endocytic proteins, whereas the membrane-bending model proposes that the BAR domain induces positively curved membranes. We show that mutations disrupting the scaffolding function do not impair endocytosis, whereas those disrupting membrane bending cause significant defects. By anchoring endophilin to the plasma membrane, we show that endophilin acts prior to scission to promote endocytosis. Despite acting at the plasma membrane, the majority of endophilin is targeted to the SV pool. Photoactivation studies suggest that the soluble pool of endophilin at synapses is provided by unbinding from the adjacent SV pool and that the unbinding rate is regulated by exocytosis. Thus, endophilin participates in an association-dissociation cycle with SVs that parallels the cycle of exo- and endocytosis. This endophilin cycle may provide a mechanism for functionally coupling endocytosis and exocytosis. 相似文献