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Critical Assessment of Methods to Quantify Biofilm Growth and Evaluate Antibiofilm Activity of Host Defence Peptides

机译:评估生物膜生长和评估宿主防御肽抗生物膜活性的方法的关键评估

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摘要

Biofilms are multicellular communities of bacteria that can adhere to virtually any surface. Bacterial biofilms are clinically relevant, as they are responsible for up to two-thirds of hospital acquired infections and contribute to chronic infections. Troublingly, the bacteria within a biofilm are adaptively resistant to antibiotic treatment and it can take up to 1000 times more antibiotic to kill cells within a biofilm when compared to planktonic bacterial cells. Identifying and optimizing compounds that specifically target bacteria growing in biofilms is required to address this growing concern and the reported antibiofilm activity of natural and synthetic host defence peptides has garnered significant interest. However, a standardized assay to assess the activity of antibiofilm agents has not been established. In the present work, we describe two simple assays that can assess the inhibitory and eradication capacities of peptides towards biofilms that are formed by both Gram-positive and negative bacteria. These assays are suitable for high-throughput workflows in 96-well microplates and they use crystal violet staining to quantify adhered biofilm biomass as well as tetrazolium chloride dye to evaluate the metabolic activity of the biofilms. The effect of media composition on the readouts of these biofilm detection methods was assessed against two strains of Pseudomonas aeruginosa (PAO1 and PA14), as well as a methicillin resistant strain of Staphylococcus aureus. Our results demonstrate that media composition dramatically alters the staining patterns that were obtained with these dye-based methods, highlighting the importance of establishing appropriate biofilm growth conditions for each bacterial species to be evaluated. Confocal microscopy imaging of P. aeruginosa biofilms grown in flow cells revealed that this is likely due to altered biofilm architecture under specific growth conditions. The antibiofilm activity of several antibiotics and synthetic peptides were then evaluated under both inhibition and eradication conditions to illustrate the type of data that can be obtained using this experimental setup.
机译:生物膜是细菌的多细胞群落,几乎可以粘附于任何表面。细菌生物膜在临床上是相关的,因为它们可导致多达三分之二的医院获得性感染,并导致慢性感染。令人不安的是,生物膜中的细菌对抗生素治疗具有适应性抗性,与浮游细菌细胞相比,杀死生物膜中的细胞所需要的抗生素多达1000倍。为了解决这一日益增长的问题,需要鉴定和优化专门针对在生物膜中生长的细菌的化合物,并且已报道的天然和合成宿主防御肽的抗生物膜活性已引起广泛关注。但是,尚未建立评估抗生物膜剂活性的标准化测定法。在目前的工作中,我们描述了两个简单的测定方法,它们可以评估肽对革兰氏阳性和阴性细菌形成的生物膜的抑制和清除能力。这些测定法适用于96孔微孔板中的高通量工作流程,并且它们使用结晶紫染色来量化粘附的生物膜生物量以及氯化四唑鎓染料来评估生物膜的代谢活性。针对两种铜绿假单胞菌菌株(PAO1和PA14)以及耐甲氧西林的金黄色葡萄球菌菌株,评估了培养基组成对这些生物膜检测方法读数的影响。我们的结果表明,培养基成分会极大地改变使用这些基于染料的方法获得的染色模式,从而突出显示为每种待评估细菌建立适当的生物膜生长条件的重要性。在流通池中生长的铜绿假单胞菌生物膜的共聚焦显微镜成像显示,这可能是由于在特定生长条件下生物膜结构发生了变化。然后在抑制和消除条件下评估了几种抗生素和合成肽的抗生物膜活性,以说明使用该实验装置可获得的数据类型。

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