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将置于污染垫料中的介质进行 PCR 检测作为鼠群健康监测的一种方法。

PCR Testing of Media Placed in Soiled Bedding as a Method for Mouse Colony Health Surveillance.

机构信息

Division of Animal Resources, Emory University, Atlanta, Georgia;, Email:

Division of Animal Resources, Emory University, Atlanta, Georgia.

出版信息

J Am Assoc Lab Anim Sci. 2021 May 1;60(3):306-310. doi: 10.30802/AALAS-JAALAS-20-000096. Epub 2021 May 4.

Abstract

Rodent colony health surveillance has traditionally been accomplished by testing sentinel animals that have been exposed to soiled bedding from colony animals. Collecting samples from exhaust plenums on ventilated caging systems, followed by PCR analysis, has emerged as another promising method for health surveillance. However, environmental testing at the rack level is not effective for all ventilated rack designs. In this study, we tested whether media placed in soiled bedding is effective in detecting 3 adventitious agents: mouse norovirus (MNV), spp., and fur mites. Soiled bedding was collected from pathogen-positive colony mice and distributed to traditional sentinel mouse cages and mouse-free experimental cages every 1 to 2 wk for static and ventilated cages, respectively. Experimental cages contained 10 flocked swabs ('passive swabs') and 1 piece of filter media. After 90 d, fresh feces, pelage swabs, and blood were collected from the sentinel cages, and the passive swabs and filter media were collected from the experimental cages. Concurrently, 10 additional flocked swabs ('active swabs') were stirred through the cumulated soiled bedding of each experimental cage. Sentinel mice were positive for MNV and spp., but negative for fur mites by pelage swab PCR. All samples from experimental cages were positive for spp. and fur mites in both caging types. For MNV, passive swabs were most effective at detection (100%), followed by active swabs (80% to 100%) and filter media (60% to 80%). These findings suggest that testing media in pooled soiled bedding samples is more effective than traditional sentinel methods for colony health surveillance and is a viable option when sampling at the rack level is ineffective.

摘要

啮齿动物群体健康监测传统上是通过测试接触过受污染垫料的哨兵动物来完成的,这些垫料来自群体动物。从通风笼具的排气通道收集样本,然后进行 PCR 分析,已成为另一种有前途的健康监测方法。然而,对于所有通风架设计,在架级进行环境测试并不有效。在这项研究中,我们测试了放置在污染垫料中的介质是否能有效检测到 3 种偶然病原体:小鼠诺如病毒(MNV)、支原体和螨虫。从病原体阳性的群体小鼠中收集污染垫料,并每隔 1 至 2 周分别分配给传统的哨兵小鼠笼和无鼠实验笼(用于静态和通风笼)。实验笼中包含 10 个装有绒毛的拭子(“被动拭子”)和 1 个过滤介质。90 天后,从哨兵笼中收集新鲜粪便、皮毛拭子和血液,并从实验笼中收集被动拭子和过滤介质。同时,每个实验笼的累积污染垫料中搅拌 10 个额外的装有绒毛的拭子(“主动拭子”)。哨兵小鼠的 MNV 和支原体呈阳性,但皮毛拭子 PCR 检测为螨虫阴性。两种笼型的实验笼所有样本均检测到支原体和螨虫阳性。对于 MNV,被动拭子的检测效果最佳(100%),其次是主动拭子(80%至 100%)和过滤介质(60%至 80%)。这些发现表明,在污染垫料样本中测试介质比传统的哨兵方法更有效,并且当在架级采样无效时,是一种可行的选择。

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