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用于鉴定血吸虫病传播地点的分子方法的开发。

Development of molecular approaches for the identification of transmission sites of schistosomiasis.

作者信息

Melo Fábio L, Gomes Ana Lisa do Vale, Barbosa Constança S, Werkhauser Roberto P, Abath Frederico G C

机构信息

Departamento de Imunologia, Centro de Pesquisas Aggeu Magalhães-FIOCRUZ, Av. Prof. Moraes Rego s/n, Cidade Universitária, 50670-420, Recife, Brazil.

出版信息

Trans R Soc Trop Med Hyg. 2006 Nov;100(11):1049-55. doi: 10.1016/j.trstmh.2005.12.008. Epub 2006 Apr 18.

Abstract

Primers targeting the gene encoding the small subunit rRNA were designed to amplify DNA from Schistosoma mansoni with high specificity. Three PCR systems were developed: conventional PCR, two-step nested PCR (NPCR) and single-tube nested PCR (STNPCR). The limits of detection of parasite DNA for the conventional PCR, NPCR and STNPCR were 10 pg, 0.1 fg and 1 fg, respectively. The assays were highly specific for S. mansoni and did not recognise DNA from closely related non-schistosome trematodes. Using pools of Biomphalaria molluscs, PCR, NPCR and STNPCR were positive in 6/16 (37.5%), 15/16 (93.8%) and 13/16 (81.3%) of the tested samples, respectively, whereas the observation of cercariae shedding after exposure to light was able to detect S. mansoni infection in 6/16 (37.5%) of the pools. Thus, the molecular detection systems had a higher level of sensitivity than standard screening of intermediate hosts by cercarial shedding when DNA was purified from pools of snails collected from endemic areas. These PCR protocols have potential to be used as tools for monitoring of schistosome transmission.

摘要

设计了靶向编码小亚基rRNA基因的引物,以高特异性扩增曼氏血吸虫的DNA。开发了三种PCR系统:常规PCR、两步巢式PCR(NPCR)和单管巢式PCR(STNPCR)。常规PCR、NPCR和STNPCR检测寄生虫DNA的限度分别为10 pg、0.1 fg和1 fg。这些检测方法对曼氏血吸虫具有高度特异性,不识别来自密切相关的非血吸虫吸虫的DNA。使用双脐螺软体动物池,PCR、NPCR和STNPCR在分别6/16(37.5%)、15/16(93.8%)和13/16(81.3%)的测试样本中呈阳性,而暴露于光线下后观察尾蚴逸出能够在6/16(37.5%)的池中检测到曼氏血吸虫感染。因此,当从流行地区收集的蜗牛池中纯化DNA时,分子检测系统比通过尾蚴逸出对中间宿主进行标准筛查具有更高的灵敏度水平。这些PCR方案有潜力用作监测血吸虫传播的工具。

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