首页> 美国卫生研究院文献>Journal of the American Association for Laboratory Animal Science : JAALAS >PCR Testing of IVC Filter Tops as a Method for Detecting Murine Pinworms and Fur Mites
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PCR Testing of IVC Filter Tops as a Method for Detecting Murine Pinworms and Fur Mites

机译:IVC滤嘴的PCR测试作为检测鼠科蠕虫和皮螨的方法

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摘要

We evaluated PCR testing of filter tops from cages maintained on an IVC system through which exhaust air is filtered at the cage level as a method for detecting parasite- infected and -infested cages. Cages containing 4 naïve Swiss Webster mice received 360 mL of uncontaminated aspen chip or α-cellulose bedding (n = 18 cages each) and 60 mL of the same type of bedding weekly from each of the following 4 groups of cages housing mice infected or infested with Syphacia obvelata (SO), Aspiculuris tetraptera (AT), Myocoptes musculinus (MC), or Myobia musculi (MB) and Radfordia affinis (RA; 240 mL bedding total). Detection rates were compared at 30, 60, and 90 d after initiating bedding exposure, by using PCR analysis of filter tops (media extract and swabs) and testing of mouse samples (fur swab [direct] PCR testing, fecal flotation, anal tape test, direct examination of intestinal contents, and skin scrape). PCR testing of filter media extract detected 100% of all parasites at 30 d (both bedding types) except for AT (α-cellulose bedding, 67% detection rate); identified more cages with fur mites (MB and MC) than direct PCR when cellulose bedding was used; and was better at detecting parasites than all nonmolecular methods evaluated. PCR analysis of filter media extract was superior to swab and direct PCR for all parasites cumulatively for each bedding type. Direct PCR more effectively detected MC and all parasites combined for aspen chip compared with cellulose bedding. PCR analysis of filter media extract for IVC systems in which exhaust air is filtered at the cage level was shown to be a highly effective environmental testing method.
机译:我们评估了在IVC系统上维护的笼子上的过滤器顶部的PCR测试,通过该系统在笼子水平上过滤废气,作为检测寄生虫感染和感染的笼子的方法。笼中有4只幼稚的Swiss Webster小鼠,每星期从以下4组笼中的360只未感染的白杨木屑或α-纤维素床上用品(每组18个笼子)和60 mL相同类型的床上用品中,每个笼子都感染或感染了小鼠包括Syphacia obvelata(SO),Aspiculuris tetraptera(AT),Myocoptes musculinus(MC)或Myobia musculi(MB)和Radfordia affinis(RA;共240 mL床上用品)。在开始铺垫暴露后的30、60和90天,通过使用滤纸条(培养基提取物和拭子)的PCR分析和小鼠样品的测试(毛皮拭子[直接] PCR测试,粪便浮选,肛门胶带测试)比较检测率,直接检查肠内容物和皮肤刮擦)。过滤介质提取物的PCR测试在30 d(两种垫层类型)上检测到所有寄生虫的100%,除AT(α-纤维素垫层,检出率67%)外;当使用纤维素被褥时,与直接PCR相比,发现有更多螨虫(MB和MC)的笼子;与所有评估的非分子方法相比,它在检测寄生虫方面更好。对于每种被褥类型,累积的所有寄生虫的过滤介质提取物的PCR分析均优于拭子和直接PCR。与纤维素垫层相比,直接PCR可以更有效地检测出MC和所有寄生虫组合在一起的白杨片。对于在笼级过滤废气的IVC系统,过滤介质提取物的PCR分析被证明是一种高效的环境测试方法。

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