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通过重新利用依布硒啉来对抗粘质沙雷氏菌的浮游和生物膜生长。

Combating planktonic and biofilm growth of Serratia marcescens by repurposing ebselen.

机构信息

School of Chemical Sciences, UM DAE Centre for Excellence in Basic Sciences, University of Mumbai, Kalina Campus, Mumbai, India.

School of Biological Sciences, UM DAE Centre for Excellence in Basic Sciences, University of Mumbai, Kalina Campus, Mumbai, India.

出版信息

Int Microbiol. 2023 Nov;26(4):693-704. doi: 10.1007/s10123-022-00301-5. Epub 2022 Dec 12.

Abstract

AIM OF THE STUDY

The rising instances of multidrug-resistant pathogens are rapidly evolving into a global healthcare crisis. Identifying new ways of synthesis of antibiotics is both time-consuming and expensive. Repurposing existing drugs for the treatment of such antimicrobial-resistant pathogens has also been explored.

METHODS AND RESULTS

In the current study, ebselen was screened for antibacterial and antibiofilm activity against Serratia marcescens. Various antibacterial studies such as minimum inhibitory concentration (MIC), minimum bactericidal concentration (MBC), time-kill curves, intracellular reactive oxygen species (ROS) quantification, and colony-forming unit assays were performed. The antibiofilm potential was assayed by biofilm inhibition, cell surface hydrophobicity assay, eradication, quantification of extracellular DNA (eDNA), and extracellular polymeric substance (EPS) layer and scanning electron microscopy (SEM) analysis were performed. Anti-quorum sensing assay was validated by quantifying the virulence factors production. Further molecular docking of ebselen with two quorum sensing (QS) specific proteins was also carried out. Antibacterial susceptibility tests showed potent antimicrobial activity of ebselen against S. marcescens with MIC of 14 μg/mL. Ebselen's ability to disturb the redox environment by inducing significant ROS generation led to bacterial death. It also showed concentration-dependent bactericidal activity as indicated by reduced bacterial growth and colony-forming unit propagation. Ebselen was also found to prevent biofilm attachment by altering the cell surface hydrophobicity while also being effective against preformed biofilms as validated by scanning electron microscopy (SEM) analysis. Additionally, ebselen showed reduced virulence factors like urease enzyme activity and prodigiosin pigment production indicating its promising anti-quorum sensing potential. Molecular docking analysis validated the strong binding of ebselen with QS-specific proteins (1Joe and PigG) with binding energies of - 6.6 and - 8.1kj/mol through hydrogen bonds and aromatic interactions. These results show that ebselen has potent antibiofilm potential that can be explored to identify treatment against bacterial infections.

摘要

研究目的

多药耐药病原体的不断增加正在迅速演变成一场全球健康危机。寻找抗生素的新合成方法既耗时又昂贵。因此,人们也探索了将现有药物重新用于治疗此类抗微生物耐药病原体。

方法和结果

在本研究中,筛选了依布硒啉对粘质沙雷氏菌的抗菌和抗生物膜活性。进行了各种抗菌研究,如最低抑菌浓度(MIC)、最低杀菌浓度(MBC)、时间杀伤曲线、细胞内活性氧(ROS)定量和集落形成单位测定。通过生物膜抑制、细胞表面疏水性测定、清除、细胞外 DNA(eDNA)和细胞外聚合物质(EPS)层定量以及扫描电子显微镜(SEM)分析测定了抗生物膜潜力。通过定量测定毒力因子的产生来验证抗群体感应测定。还进行了依布硒啉与两种群体感应(QS)特异性蛋白的分子对接。抗菌药敏试验显示依布硒啉对粘质沙雷氏菌具有很强的抗菌活性,MIC 为 14μg/mL。依布硒啉通过诱导显著的 ROS 生成来扰乱氧化还原环境,导致细菌死亡。它还表现出浓度依赖性杀菌活性,表现为细菌生长和集落形成单位繁殖减少。通过改变细胞表面疏水性,依布硒啉还可以防止生物膜附着,并且通过扫描电子显微镜(SEM)分析验证了其对已形成的生物膜的有效性。此外,依布硒啉还显示出降低了脲酶酶活性和灵菌红素色素产生等毒力因子,表明其具有有前途的抗群体感应潜力。分子对接分析验证了依布硒啉与 QS 特异性蛋白(1Joe 和 PigG)的强结合,其结合能分别通过氢键和芳香相互作用为-6.6 和-8.1kJ/mol。这些结果表明,依布硒啉具有很强的抗生物膜潜力,可用于确定针对细菌感染的治疗方法。

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