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基于生物膜亲水性的原位检测用于环境生物膜形成。

In-situ detection based on the biofilm hydrophilicity for environmental biofilm formation.

机构信息

RIKEN Center for Biosystems Dynamics Research, 1-3 Yamadaoka, Suita, Osaka, 565-0871, Japan.

National Institute of Technology (KOSEN), Suzuka College, Shiroko-cho, Suzuka, Mie, 510-0294, Japan.

出版信息

Sci Rep. 2019 May 30;9(1):8070. doi: 10.1038/s41598-019-44167-6.

Abstract

A biofilm has a unique structure composed of microorganisms, extracellular polymeric substances (EPSs), etc., and it is layered on a substrate in water. In material science, it is important to detect the biofilm formed on a surface to prevent biofouling. EPSs, the major component of the biofilm, mainly consist of polysaccharides, proteins, nucleic acids, and lipids. Because these biomolecules have a variety of hydrophilicities or hydrophobicities, the substrate covered with the biofilm shows different wettability from the initial state. To detect the biofilm formation, this study employed a liquid-squeezing-based wettability assessment method with a simple wettability index: the liquid-squeezed diameter of a smaller value indicates higher wettability. The method is based on the liquid-squeezing behaviour of a liquid that covers sample surfaces when an air-jet is applied. To form the biofilm, polystyrene surfaces were immersed and incubated in a water-circulated bioreactor that had collected microorganisms in ambient air. After the 14-d incubation, good formation of the biofilm on the surfaces was confirmed by staining with crystal violet. Although the contact angles of captive bubbles on the surfaces with the biofilm were unmeasurable, the liquid-squeezing method could distinguish between hydrophilic and hydrophobic initial surfaces with and without biofilm formation using the diameter of the liquid-squeezed area. The surface wettability is expected to be a promising property for in-situ detection of biofilm formation on a macroscopic scale.

摘要

生物膜具有独特的结构,由微生物、细胞外聚合物(EPS)等组成,并在水中分层在基质上。在材料科学中,检测表面形成的生物膜以防止生物污垢非常重要。EPS 是生物膜的主要成分,主要由多糖、蛋白质、核酸和脂质组成。由于这些生物分子具有各种亲水性或疏水性,因此覆盖有生物膜的基质的润湿性与初始状态不同。为了检测生物膜的形成,本研究采用了基于液体挤压的润湿性评估方法,使用简单的润湿性指数:较小值的液体挤压直径表示更高的润湿性。该方法基于当喷射空气时覆盖样品表面的液体的液体挤压行为。为了形成生物膜,将聚苯乙烯表面浸入并在循环水生物反应器中孵育,该生物反应器在环境空气中收集了微生物。孵育 14 天后,通过结晶紫染色确认了表面上生物膜的良好形成。尽管生物膜表面上的俘获气泡的接触角无法测量,但使用挤压区域的直径,液体挤压方法可以区分具有和不具有生物膜形成的亲水性和疏水性初始表面。表面润湿性有望成为在宏观尺度上原位检测生物膜形成的有前途的特性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/edd2/6542837/19db1d7e47fc/41598_2019_44167_Fig1_HTML.jpg

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