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首页> 外文期刊>Journal of water and health >A review of technologies for rapid detection of bacteria in recreational waters
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A review of technologies for rapid detection of bacteria in recreational waters

机译:休闲水域细菌快速检测技术综述

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Monitoring of recreational beaches for fecal indicator bacteria is currently performed using culture-based technology that can require more than a day for laboratory analysis, during which time swimmers are at risk. Here we review new methods that have the potential to reduce the measurement period to less than an hour. These methods generally involve two steps. The first is target capture, in which the microbial group of interest (or some molecular/chemical/or biochemical signature of the group) is removed, tagged or amplified to differentiate it from the remaining material in the sample. We discuss three classes of capture methods: 1) Surface and whole-cell recognition methods, including immunoassay techniques and molecule-specific probes; 2) Nucleic acid methods, including polymerase chain reaction (PCR), quantitative PCR (Q-PCR), nucleic acid sequence based amplification (NASBA) and microarrays; and 3) Enzyme/substrate methods utilizing chromogenic or fluorogenic substrates. The second step is detection, in which optical, electrochemical or piezoelectric technologies are used to quantify the captured, tagged or amplified material. The biggest technological hurdle for all of these methods is sensitivity, as EPA'S recommended bathing water standard is less than one cell per ml and most detection technologies measure sample volumes less than 1 ml. This challenge is being overcome through addition of preconcentration or enrichment steps, which have the potential to boost sensitivity without the need to develop new detector technology. The second hurdle is demonstrating a relationship to health risk, since most new methods are based on measuring cell structure without assessing viability and may not relate to current water quality standards that were developed in epidemiology studies using culture-based methods. Enzyme/substrate methods may be the first rapid methods adopted because they are based on the same capture technology as currently-approved EPA methods and their relationship to health risk can be established by demonstrating equivalency to existing procedures. Demonstration of equivalency may also be possible for some surface and whole-cell recognition methods that capture bacteria in a potentially viable state. Nucleic acid technologies are the most versatile, but measure nonviable structure and will require inclusion in epidemiological studies to link their measurement with health risk.
机译:目前,休闲娱乐场所的粪便指示菌监测工作是通过基于文化的技术进行的,该技术可能需要一天以上的时间进行实验室分析,在此期间游泳者处于危险之中。在这里,我们回顾了有可能将测量周期缩短到不到一个小时的新方法。这些方法通常包括两个步骤。第一个是目标捕获,其中目标微生物组(或该组的某些分子/化学/或生化特征)被去除,标记或扩增,以使其与样品中的其余物质区分开。我们讨论了三类捕获方法:1)表面和全细胞识别方法,包括免疫测定技术和分子特异性探针; 2)核酸方法,包括聚合酶链反应(PCR),定量PCR(Q-PCR),基于核酸序列的扩增(NASBA)和微阵列; 3)利用发色或发荧光底物的酶/底物方法。第二步是检测,其中光学,电化学或压电技术用于量化捕获,标记或扩增的材料。所有这些方法的最大技术障碍是灵敏度,因为EPA推荐的沐浴水标准是每毫升少于一个细胞,并且大多数检测技术所测量的样本量都少于1毫升。通过添加预浓缩或富集步骤可克服这一挑战,无需开发新的检测器技术即可提高灵敏度。第二个障碍是证明与健康风险的关系,因为大多数新方法都基于在不评估生存能力的情况下测量细胞结构,并且可能与流行病学研究中使用基于培养物的方法制定的当前水质标准无关。酶/底物方法可能是最先采用的快速方法,因为它们基于与当前批准的EPA方法相同的捕获技术,并且可以通过证明与现有程序的等效性来建立它们与健康风险的关系。对于某些以潜在生存状态捕获细菌的表面和全细胞识别方法,也有可能证明其等效性。核酸技术用途最广泛,但只能测量不可行的结构,因此需要在流行病学研究中纳入以将其测量与健康风险联系起来。

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