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Cold Plasma Inactivation of Bacterial Biofilms and Reduction of Quorum Sensing Regulated Virulence Factors

机译:细菌生物膜的冷血浆失活和仲裁感调节毒力因子的减少。

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摘要

The main objectives of this work were to investigate the effect of atmospheric cold plasma (ACP) against a range of microbial biofilms commonly implicated in foodborne and healthcare associated human infections and against P. aeruginosa quorum sensing (QS)-regulated virulence factors, such as pyocyanin, elastase (Las B) and biofilm formation capacity post-ACP treatment. The effect of processing factors, namely treatment time and mode of plasma exposure on antimicrobial activity of ACP were also examined. Antibiofilm activity was assessed for E. coli, L. monocytogenes and S. aureus in terms of reduction of culturability and retention of metabolic activity using colony count and XTT assays, respectively. All samples were treated ‘inpack’ using sealed polypropylene containers with a high voltage dielectric barrier discharge ACP generated at 80 kV for 0, 60, 120 and 300 s and a post treatment storage time of 24 h. According to colony counts, ACP treatment for 60 s reduced populations of E. coli to undetectable levels, whereas 300 s was necessary to significantly reduce populations of L. monocytogenes and S. aureus biofilms. The results obtained from XTT assay indicated possible induction of viable but non culturable state of bacteria. With respect to P. aeruginosa QS-related virulence factors, the production of pyocyanin was significantly inhibited after short treatment times, but reduction of elastase was notable only after 300 s and no reduction in actual biofilm formation was achieved post-ACP treatment. Importantly, reduction of virulence factors was associated with reduction of the cytotoxic effects of the bacterial supernatant on CHO-K1 cells, regardless of mode and duration of treatment. The results of this study point to ACP technology as an effective strategy for inactivation of established biofilms and may play an important role in attenuation of virulence of pathogenic bacteria. Further investigation is warranted to propose direct evidence for the inhibition of QS and mechanisms by which this may occur.
机译:这项工作的主要目的是研究大气冷血浆(ACP)对一系列通常与食源性和医疗保健相关的人类感染相关的微生物生物膜以及铜绿假单胞菌群体感应(QS)调控的毒力因子(例如ACP处理后的花青素,弹性蛋白酶(Las B)和生物膜形成能力。还检查了处理因素(即处理时间和血浆暴露方式)对ACP抗菌活性的影响。分别通过菌落计数和XTT分析,就可培养性的降低和代谢活性的保留而言,评估了大肠杆菌,单核细胞增生李斯特菌和金黄色葡萄球菌的抗生物膜活性。使用密封的聚丙烯容器对所有样品进行“内装”处理,该容器具有80 kV电压下产生的0、60、120和300 s的高压电介质阻挡放电ACP,后处理时间为24 h。根据菌落计数,ACP处理60 s可将大肠杆菌种群降至无法检测的水平,而300 s则是显着减少单核细胞增生李斯特菌和金黄色葡萄球菌生物膜种群所必需的。从XTT分析获得的结果表明,可能诱导了细菌的存活但不可培养的状态。关于铜绿假单胞菌QS相关的毒力因子,在短时间处理后,绿脓素的产生被显着抑制,但是弹性蛋白酶的减少仅在300 s后才显着,ACP处理后实际生物膜的形成没有减少。重要的是,毒力因子的降低与细菌上清液对CHO-K1细胞的细胞毒性作用的降低有关,而与治疗的方式和持续时间无关。这项研究的结果指出,ACP技术是使已建立的生物膜失活的有效策略,并且可能在减轻病原细菌的毒力方面发挥重要作用。有必要进行进一步的研究,以提供直接证据证明抑制QS及其可能发生的机制。

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