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Evaluation of a Strategy for Toxoplasma gondii Oocyst Detection in Water

机译:水中弓形虫卵囊检测策略的评估

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Several recent outbreaks of toxoplasmosis were related to drinking water. We propose a strategy for Toxoplasma oocyst detection as part of an approach to detecting multiple waterborne parasites, including Giardia and Cryptosporidium spp., by the U.S. Environmental Protection Agency method with the same sample. Water samples are filtered to recover Toxoplasma oocysts and purified on a sucrose density gradient. Detection is based on PCR and mouse inoculation (bioassay) to determine the presence and infectivity of recovered oocysts. In an experimental seeding assay with 100 liters of deionized water, a parasite density of 1 oocyst/liter was successfully detected by PCR in 60% of cases and a density of 10 oocysts/liter was detected in 100% of cases. The sensitivity of the PCR assay varied from less than 10 to more than 1000 oocysts/liter, depending on the sample source. PCR was always more sensitive than mouse inoculation. This detection strategy was then applied to 139 environmental water samples collected over a 20-month period. Fifty-three samples contained PCR inhibitors, which were overcome in 39 cases by bovine serum albumin addition. Among 125 interpretable samples, we detected Toxoplasma DNA in 10 cases (8%). None of the samples were positive by mouse inoculation. This strategy efficiently detects Toxoplasma oocysts in water and may be suitable as a public health sentinel method.
机译:弓形虫病的最近几次爆发与饮用水有关。我们提出了一种检测弓形虫卵囊的策略,作为美国环境保护署对同一样本检测多种水生寄生虫(包括贾第虫和隐孢子虫)的方法的一部分。过滤水样以回收弓形虫卵囊,并在蔗糖密度梯度上纯化。检测基于PCR和小鼠接种(生物测定),以确定回收的卵囊的存在和感染性。在用100升去离子水进行的实验播种测定中,通过PCR成功地在60%的病例中检测到了1卵囊/升的寄生虫密度,在100%的情况下检测到了10卵囊/升的寄生虫密度。 PCR检测的灵敏度从小于10到大于1000卵囊/升不等,具体取决于样品来源。 PCR总是比小鼠接种更为敏感。然后,将这种检测策略应用于在20个月内收集的139个环境水样品。 53份样品中含有PCR抑制剂,在39例中通过添加牛血清白蛋白得以克服。在125个可解释样本中,我们检测了10例弓形虫DNA(8%)。小鼠接种后所有样品均无阳性。该策略可有效检测水中的弓形虫卵囊,可能适合作为公共卫生哨兵方法。

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