Sippy Namrata, Luxton Richard, Lewis Roger J, Cowell David C
Faculty of Applied Sciences, Centre for Research in Biomedicine, University of the West of England, Coldharbour Lane, BS16 1QY, Bristol, UK.
Biosens Bioelectron. 2003 May;18(5-6):741-9. doi: 10.1016/s0956-5663(03)00023-x.
The rapid detection and identification of bacteria has application in a number of fields, e.g. the food industry, environmental monitoring and biomedicine. While in biomedicine the number of organisms present during infection is multiples of millions in the other fields it is the detection of low numbers of organisms that is important, e.g. an infective dose of Escherichia coli O157:H7 from contaminated food is less than 100 organisms. A rapid and sensitive technique has been developed to detect low numbers of the model organism E. coli O55, combining Lateral Flow Immunoassay (LFI) for capture and amperometry for sensitive detection. Nitrocellulose membranes were used as the solid phase for selective capture of the bacteria using antibodies to E. coli O55. Different concentrations of E. coli O55 in Ringers solution were applied to LFI strips and allowed to flow through the membrane to an absorbent pad. The capture region of the LFI strip was placed in close contact with the electrodes of a Clarke cell poised at +0.7 V for the detection of hydrogen peroxide. Earlier research identified that the consumption of hydrogen peroxide by bacterial catalase provided a sensitive indicator of aerobic and facultative anaerobic microorganisms numbers. Modification and application of this technique to the LFI strips demonstrated that the consumption of 8 mM hydrogen peroxide was correlated with the number of microorganisms presented to the LFI strips in the range of 2 x 10(1)-2 x 10(7) colony forming units (cfu). Capture efficiency was dependent on the number of organisms applied and varied from 71% at 2 x 10(2) cfu to 25% at 2 x 10(7) cfu. The procedure was completed in less than 10 min and could detect less than 10 cfu captured from a 200 microl sample applied to the LFI strip. The approached adopted provides proof of principle for the basis of a new technological approach to the rapid, quantitative and sensitive detection of bacteria that express catalase activity.
细菌的快速检测和鉴定在许多领域都有应用,如食品工业、环境监测和生物医学。在生物医学中,感染期间存在的生物体数量可达数百万倍,而在其他领域,检测少量生物体则很重要,例如,受污染食品中感染剂量的大肠杆菌O157:H7少于100个生物体。已经开发出一种快速灵敏的技术来检测少量的模式生物大肠杆菌O55,该技术结合了用于捕获的侧向流动免疫分析(LFI)和用于灵敏检测的安培法。使用硝酸纤维素膜作为固相,利用抗大肠杆菌O55抗体选择性捕获细菌。将林格氏溶液中不同浓度的大肠杆菌O55应用于LFI试纸条,并使其流过膜到达吸水垫。将LFI试纸条的捕获区域与置于+0.7 V的克拉克电池电极紧密接触,以检测过氧化氢。早期研究发现,细菌过氧化氢酶消耗过氧化氢可作为需氧和兼性厌氧微生物数量的灵敏指标。将该技术修改并应用于LFI试纸条表明,消耗8 mM过氧化氢与呈现给LFI试纸条的微生物数量在2×10¹-2×10⁷菌落形成单位(cfu)范围内相关。捕获效率取决于所应用的生物体数量,从2×10² cfu时的71%到2×10⁷ cfu时的25%不等。该过程在不到10分钟内完成,并且可以检测从应用于LFI试纸条的200微升样品中捕获的少于10 cfu的细菌。所采用的方法为一种新技术方法提供了原理证明,该方法用于快速、定量和灵敏地检测表达过氧化氢酶活性的细菌。
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