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牛囊尾蚴病——实时 PCR 的发展增强了在肉品检验中疑似囊尾蚴的分类。

Bovine cysticercosis--development of a real-time PCR to enhance classification of suspect cysts identified at meat inspection.

机构信息

School of Veterinary Science, University of Queensland, Gatton, QLD 4343, Australia.

出版信息

Vet Parasitol. 2013 May 1;194(1):65-9. doi: 10.1016/j.vetpar.2013.02.018. Epub 2013 Feb 28.

DOI:10.1016/j.vetpar.2013.02.018
PMID:23499482
Abstract

Laboratory confirmation methods are important in bovine cysticerosis diagnosis as other pathologies can result in morphologically similar lesions resulting in false identifications. We developed a probe-based real-time PCR assay to identify Taenia saginata in suspect cysts encountered at meat inspection and compared its use with the traditional method of identification, histology, as well as a published nested PCR. The assay simultaneously detects T. saginata DNA and a bovine internal control using the cytochrome c oxidase subunit 1 gene of each species and shows specificity against parasites causing lesions morphologically similar to those of T. saginata. The assay was sufficiently sensitive to detect 1 fg (Ct 35.09 ± 0.95) of target DNA using serially-diluted plasmid DNA in reactions spiked with bovine DNA as well as in all viable and caseated positive control cysts. A loss in PCR sensitivity was observed with increasing cyst degeneration as seen in other molecular methods. In comparison to histology, the assay offered greater sensitivity and accuracy with 10/19 (53%) T. saginata positives detected by real-time PCR and none by histology. When the results were compared with the reference PCR, the assay was less sensitive but offered advantages of faster turnaround times and reduced contamination risk. Estimates of the assay's repeatability and reproducibility showed the assay is highly reliable with reliability coefficients greater than 0.94.

摘要

实验室确认方法在牛囊尾蚴病诊断中很重要,因为其他病理学变化可能导致形态相似的病变,从而导致错误识别。我们开发了一种基于探针的实时 PCR 检测方法,用于鉴定在肉类检查中遇到的疑似囊泡中的带绦虫,并用传统的鉴定方法、组织学以及已发表的巢式 PCR 对其进行了比较。该检测方法同时使用每个物种的细胞色素 c 氧化酶亚基 1 基因检测绦虫和牛内参的 DNA,并显示出对形态上与带绦虫相似的病变的寄生虫具有特异性。该检测方法足够灵敏,可使用牛 DNA 加标的系列稀释质粒 DNA 在反应中检测到 1 fg(Ct 35.09 ± 0.95)的靶 DNA,并且在所有有活力和干酪样阳性对照囊泡中均可检测到。与其他分子方法一样,随着囊泡变性的增加,PCR 敏感性会降低。与组织学相比,实时 PCR 检测到 10/19(53%)的带绦虫阳性,而组织学无一例阳性,检测的敏感性和准确性更高。当将结果与参考 PCR 进行比较时,该检测方法的敏感性较低,但具有周转时间更快和污染风险降低的优势。检测方法的重复性和再现性估计表明,该检测方法的可靠性很高,可靠性系数大于 0.94。

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