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一种超灵敏的微流控方法揭示了实验性肽类抗生素的物理化学和生物学活性之间的相关性。

An ultrasensitive microfluidic approach reveals correlations between the physico-chemical and biological activity of experimental peptide antibiotics.

机构信息

Living Systems Institute, University of Exeter, Stocker Road, Exeter, EX4 4QD, UK.

College of Engineering, Mathematics and Physical Sciences, University of Exeter, North Park Road, Exeter, EX4 4QF, UK.

出版信息

Sci Rep. 2022 Mar 7;12(1):4005. doi: 10.1038/s41598-022-07973-z.

Abstract

Antimicrobial resistance challenges the ability of modern medicine to contain infections. Given the dire need for new antimicrobials, polypeptide antibiotics hold particular promise. These agents hit multiple targets in bacteria starting with their most exposed regions-their membranes. However, suitable approaches to quantify the efficacy of polypeptide antibiotics at the membrane and cellular level have been lacking. Here, we employ two complementary microfluidic platforms to probe the structure-activity relationships of two experimental series of polypeptide antibiotics. We reveal strong correlations between each peptide's physicochemical activity at the membrane level and biological activity at the cellular level. We achieve this knowledge by assaying the membranolytic activities of the compounds on hundreds of individual giant lipid vesicles, and by quantifying phenotypic responses within clonal bacterial populations with single-cell resolution. Our strategy proved capable of detecting differential responses for peptides with single amino acid substitutions between them, and can accelerate the rational design and development of peptide antimicrobials.

摘要

抗菌药物耐药性挑战了现代医学控制感染的能力。鉴于对抗生素的迫切需求,多肽抗生素具有特殊的应用前景。这些药物以细菌最暴露的部位——细胞膜作为起始靶点,攻击多个目标。然而,目前尚缺乏适用于量化多肽抗生素在膜和细胞水平上的疗效的方法。在这里,我们使用两种互补的微流控平台来探究两个实验系列的多肽抗生素的结构-活性关系。我们揭示了每个肽在膜水平上的理化活性与其在细胞水平上的生物活性之间存在很强的相关性。我们通过在数百个单独的巨大脂质体上测定化合物的膜溶解活性,并通过单细胞分辨率量化克隆细菌群体内的表型反应来实现这一知识。我们的策略证明能够检测到氨基酸替换差异对肽的影响,并且能够加速对抗菌肽的合理设计和开发。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/345f/8901753/f83ca4d3a578/41598_2022_7973_Fig1_HTML.jpg

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