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建立一种基于磁珠荧光显微镜免疫检测法的技术,用于检测和定量环境水样中的钩端螺旋体。

Development of a magnetic bead fluorescence microscopy immunoassay to detect and quantify Leptospira in environmental water samples.

机构信息

R&D Group of Biological and Environmental Physics, Department of Physics, Faculty of Science, Mahidol University, Bangkok 10400, Thailand.

出版信息

Acta Trop. 2012 Apr;122(1):119-25. doi: 10.1016/j.actatropica.2011.12.011. Epub 2012 Jan 5.

Abstract

Climate change, world population growth, and poverty have led to an increase in the incidence of leptospirosis. Leptospirosis is caused by pathogenic spirochaete bacteria that belong to the genus Leptospira. The bacteria are maintained in the renal tubules of the reservoir hosts (typically a rodent), then shed into the environment via the urine. Water is key for environmental survival and transmission, as leptospires can survive for several weeks in a moist environment. Therefore, environmental epidemiological studies are needed to study the contamination of environmental water sources. However, few such studies have been performed using cultivation of the isolates and PCR assays. But, leptospira cultivation can be easily contaminated by other organisms and takes usually several weeks. Moreover, PCR is a complex and costly analysis for the underdeveloped countries that have the highest incidence of leptospirosis. In this study, we describe two modifications of a fluorescence microscopy assay based on immuno-magnetic separation (IMS) to detect leptospires in environmental water samples that mainly differ in fluorescent dye staining. The first type uses acridine orange fluorescent dye staining combined with multiplexed IMS for sample screening. The detection limit ranged from 10(2) to 10(3) organisms per mL and largely depended on the capture efficiency (CE) of the immuno-magnetic particles. The second type uses serogroup-specific immuno-particles and direct fluorescence antibody staining (DFA) to detect leptospires; the detection limit of this second assay was approximately 10(1) cells per mL. Both assay types were applied to natural and experimentally infected water samples, which were also analysed with DFM and real-time PCR. Our data show that the fluorescent microscopy immunoassay successfully identified experimental leptospire contamination and was as sensitive as PCR. This modified immune-fluorescence assay may therefore enable epidemiological studies of leptospirosis.

摘要

气候变化、世界人口增长和贫困导致钩端螺旋体病的发病率上升。钩端螺旋体病是由属于钩端螺旋体属的致病性螺旋体细菌引起的。这些细菌存在于储存宿主(通常是啮齿动物)的肾小管中,然后通过尿液排放到环境中。水是环境生存和传播的关键,因为钩端螺旋体可以在潮湿的环境中存活数周。因此,需要进行环境流行病学研究来研究环境水源的污染情况。然而,使用培养分离物和 PCR 检测的此类研究很少。但是,钩端螺旋体的培养很容易被其他生物体污染,通常需要数周时间。此外,PCR 是一种复杂且昂贵的分析方法,对于钩端螺旋体发病率最高的发展中国家来说并不适用。在这项研究中,我们描述了两种基于免疫磁分离 (IMS) 的荧光显微镜检测法的修改,主要区别在于荧光染料染色。第一种方法使用吖啶橙荧光染料染色结合多重 IMS 进行样本筛选。检测限范围为 10(2)至 10(3)个生物体/毫升,主要取决于免疫磁性颗粒的捕获效率 (CE)。第二种方法使用血清群特异性免疫颗粒和直接荧光抗体染色 (DFA) 检测钩端螺旋体;第二种检测方法的检测限约为 10(1)个细胞/毫升。这两种检测方法都应用于天然和实验感染的水样,并用 DFM 和实时 PCR 进行了分析。我们的数据表明,荧光显微镜免疫检测法成功地识别了实验性钩端螺旋体污染,并且与 PCR 一样灵敏。因此,这种改良的免疫荧光检测法可能有助于钩端螺旋体病的流行病学研究。

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