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Propidium iodide staining underestimates viability of adherent bacterial cells

机译:碘化丙啶染色低估了粘附细菌细胞的活力

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摘要

Combining membrane impermeable DNA-binding stain propidium iodide (PI) with membrane-permeable DNA-binding counterstains is a widely used approach for bacterial viability staining. In this paper we show that PI staining of adherent cells in biofilms may significantly underestimate bacterial viability due to the presence of extracellular nucleic acids (eNA). We demonstrate that gram-positive Staphylococcus epidermidis and gram-negative Escherichia coli 24-hour initial biofilms on glass consist of 76 and 96% PI-positive red cells in situ, respectively, even though 68% the cells of either species in these aggregates are metabolically active. Furthermore, 82% of E. coli and 89% S. epidermidis are cultivable after harvesting. Confocal laser scanning microscopy (CLSM) revealed that this false dead layer of red cells is due to a subpopulation of double-stained cells that have green interiors under red coating layer which hints at eNA being stained outside intact membranes. Therefore, viability staining results of adherent cells should always be validated by an alternative method for estimating viability, preferably by cultivation.
机译:膜不透性DNA结合染色碘化丙啶(PI)与膜可透性DNA结合复染的结合是细菌生存力染色的一种广泛使用的方法。在本文中,我们显示生物膜中粘附细胞的PI染色可能由于存在细胞外核酸(eNA)而大大低估了细菌的生存能力。我们证明革兰氏阳性表皮葡萄球菌和革兰氏阴性大肠杆菌在玻璃上的24小时初始生物膜分别由原位的76和96%PI阳性红细胞组成,即使这些聚集物中任一物种的细胞中有68%是代谢活跃。此外,收获后可培养82%的大肠杆菌和89%的表皮葡萄球菌。共聚焦激光扫描显微镜(CLSM)显示,这种红细胞假死层是由于双染色细胞的亚群所致,该细胞在红色涂层下具有绿色内部,暗示eNA被完整膜外染色。因此,粘附细胞的活力染色结果应始终通过另一种评估活力的方法来验证,最好是通过培养。

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