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用于测量微小隐孢子虫感染性的体外细胞培养与小鼠试验的比较。

Comparison of in vitro cell culture and a mouse assay for measuring infectivity of Cryptosporidium parvum.

作者信息

Rochelle Paul A, Marshall Marilyn M, Mead Jan R, Johnson Anne M, Korich Dick G, Rosen Jeffrey S, De Leon Ricardo

机构信息

Water Quality Laboratory, Metropolitan Water District of Southern California, La Verne, California 91750, USA.

出版信息

Appl Environ Microbiol. 2002 Aug;68(8):3809-17. doi: 10.1128/AEM.68.8.3809-3817.2002.

Abstract

In vitro cell cultures were compared to neonatal mice for measuring the infectivity of five genotype 2 isolates of Cryptosporidium parvum. Oocyst doses were enumerated by flow cytometry and delivered to animals and cell monolayers by using standardized procedures. Each dose of oocysts was inoculated into up to nine replicates of 9 to 12 mice or 6 to 10 cell culture wells. Infections were detected by hematoxylin and eosin staining in CD-1 mice, by reverse transcriptase PCR in HCT-8 and Caco-2 cells, and by immunofluorescence microscopy in Madin-Darby canine kidney (MDCK) cells. Infectivity was expressed as a logistic transformation of the proportion of animals or cell culture wells that developed infection at each dose. In most instances, the slopes of the dose-response curves were not significantly different when we compared the infectivity models for each isolate. The 50% infective doses for the different isolates varied depending on the method of calculation but were in the range from 16 to 347 oocysts for CD-1 mice and in the ranges from 27 to 106, 31 to 629, and 13 to 18 oocysts for HCT-8, Caco-2, and MDCK cells, respectively. The average standard deviations for the percentages of infectivity for all replicates of all isolates were 13.9, 11.5, 13.2, and 10.7% for CD-1 mice, HCT-8 cells, Caco-2 cells, and MDCK cells, respectively, demonstrating that the levels of variability were similar in all assays. There was a good correlation between the average infectivity for HCT-8 cells and the results for CD-1 mice across all isolates for untreated oocysts (r = 0.85, n = 25) and for oocysts exposed to ozone and UV light (r = 0.89, n = 29). This study demonstrated that in vitro cell culture was equivalent to the "gold standard," mouse infectivity, for measuring the infectivity of C. parvum and should therefore be considered a practical and accurate alternative for assessing oocyst infectivity and inactivation. However, the high levels of variability displayed by all assays indicated that infectivity and disinfection experiments should be limited to discerning relatively large differences.

摘要

为测定5株微小隐孢子虫2型分离株的感染性,对体外细胞培养和新生小鼠进行了比较。通过流式细胞术对卵囊剂量进行计数,并采用标准化程序将其接种到动物和细胞单层中。每剂卵囊接种到多达9个重复组中,每组包含9至12只小鼠或6至10个细胞培养孔。通过苏木精和伊红染色在CD-1小鼠中检测感染,通过逆转录聚合酶链反应在HCT-8和Caco-2细胞中检测感染,通过免疫荧光显微镜在Madin-Darby犬肾(MDCK)细胞中检测感染。感染性表示为在每个剂量下发生感染的动物或细胞培养孔比例的逻辑转换。在大多数情况下,当我们比较每种分离株的感染性模型时,剂量反应曲线的斜率没有显著差异。不同分离株的50%感染剂量因计算方法而异,但对于CD-1小鼠,其范围为16至347个卵囊,对于HCT-8、Caco-2和MDCK细胞,其范围分别为27至106、31至62并9和13至18个卵囊。所有分离株所有重复组感染性百分比的平均标准差,对于CD-1小鼠、HCT-8细胞、Caco-2细胞和MDCK细胞分别为13.9%、11.5%、13.2%和10.7%,表明所有试验中的变异性水平相似。在所有分离株中,未经处理的卵囊以及暴露于臭氧和紫外线的卵囊,HCT-8细胞的平均感染性与CD-1小鼠的结果之间存在良好的相关性(r = 0.85,n = 25)以及(r = 0.89,n = 29)。本研究表明,体外细胞培养等同于测量微小隐孢子虫感染性的“金标准”——小鼠感染性,因此应被视为评估卵囊感染性和灭活的一种实用且准确的替代方法。然而,所有试验显示的高变异性水平表明,感染性和消毒实验应限于辨别相对较大的差异。

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