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A real-time RT-PCR method to detect viable Giardia lamblia cysts in environmental waters

机译:一种实时RT-PCR方法检测环境水中可行的贾第鞭毛虫兰囊肿

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Currently, USEPA Method 1623 is the standard assay used for simultaneous detection of Giardia cysts and Cryptosporidium oocysts in various water matrices. However, the method is unable to distinguish between species, genotype, or to assess viability. Therefore, the objective of the present study was to address the shortcomings of USEPA Method 1623 by developing a novel molecular-based method that can assess viability of Giardia cysts in environmental waters and identify genotypes that pose a human health threat (assemblage groups A and B). Primers and TaqMan® probes were designed to target the beta-giardin gene in order to discriminate among species and assemblages. Viability was determined by detection of de-novo mRNA synthesis after heat induction. The beta-giardin primer/probe sets were able to detect and differentiate between Giardia lamblia assemblages A and B, and did not detect Giardia muris (mouse species) or G. lamblia assemblages C, D, E and F (non-human), with the exception of Probe A which did detect G. lamblia assemblage F DNA. Additionally, DNA or cDNA of other waterborne organisms were not detected, suggesting that the method is specific to Giardia assemblages. Assay applicability was demonstrated by detection of viable G. lamblia cysts in spiked (assemblage B) and unspiked (assemblage A and B) reclaimed water samples.
机译:当前,USEPA方法1623是用于同时检测各种水基质中的贾第鞭毛虫囊和隐孢子虫卵囊的标准检测方法。但是,该方法无法区分物种,基因型或评估生存力。因此,本研究的目的是通过开发一种新的基于分子的方法来解决USEPA方法1623的缺点,该方法可以评估贾第鞭毛虫囊肿在环境水中的生存力,并确定对人类健康构成威胁的基因型(A和B组) )。引物和TaqMan®探针设计用于靶向β-贾第蛋白基因,以区分物种和组合。通过检测热诱导后de-novo mRNA的合成来确定生存力。 β-贾第蛋白引物/探针组能够检测和区分贾第鞭毛虫兰氏菌组合A和B,而不能检测贾第鞭毛虫(小鼠)或贾第鞭毛虫兰氏菌组合C,D,E和F(非人类),除了探针A确实检测到了兰伯氏菌组合F DNA。此外,未检测到其他水生生物的DNA或cDNA,这表明该方法对贾第虫组合具有特异性。通过在加标(组合B)和未加标(组合A和B)的再生水样品中检测活的G. lamblia囊肿,证明了该方法的适用性。

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