评价联合高效 DNA 提取和实时 PCR 检测亚临床感染奶牛中的分枝杆菌副结核亚种:与粪便培养、乳实时 PCR 和乳 ELISA 的比较。
Evaluation of combined high-efficiency DNA extraction and real-time PCR for detection of Mycobacterium avium subsp. paratuberculosis in subclinically infected dairy cattle: comparison with faecal culture, milk real-time PCR and milk ELISA.
机构信息
Institute of Microbiology and Parasitology, Gerbičeva 60, Ljubljana, Slovenia.
出版信息
BMC Vet Res. 2012 May 2;8:49. doi: 10.1186/1746-6148-8-49.
BACKGROUND
Johne's disease is caused by Mycobacterium avium subsp. paratuberculosis (Map) and it is one of the most important diseases in cattle worldwide. Several laboratory tests for Map detection are available; however, these are limited by inadequate sensitivity and specificity when used in subclinically infected populations. To identify Map shedders in subclinically infected cattle, we used a new, high-yield method for DNA-extraction from Map in faeces combined with quantitative real-time PCR (qPCR) for amplification of the insertion sequence IS900 of Map (HYDEqPCR). Evaluation of HYDEqPCR was carried out in comparison with faecal culture, milk qPCR, and milk enzyme-linked immunosorbent assay (ELISA), on 141 faecal and 91 milk samples, from 141 subclinically infected dairy cattle.
RESULTS
The qPCR proved to be highly sensitive, with a detection limit of 2 IS900 DNA copies/μl in 67 % of the reactions. It also showed 100 % specificity, as determined from 50 Map and non-Map strains, and by the sequencing of qPCR amplicons. The detection limit of HYDEqPCR was 90 Map/g Map-spiked faeces, which corresponds to 2.4 colony forming units/g Map-spiked faeces, with an estimated efficiency of 85 % (±21 %). When tested on the field samples, HYDEqPCR showed 89 % of the samples as positive for Map, whereas faecal culture, milk qPCR, and milk ELISA detected 19 %, 36 % and 1 %, respectively. Fisher's exact tests only show statistical significance (p ≤0.05) for the correlation between HYDEqPCR and faecal culture. The agreement between HYDEqPCR and milk qPCR and milk ELISA was poor, slight, and non-significant.
CONCLUSIONS
This study highlights the advantages of HYDEqPCR for detection of Map in subclinically infected populations, in comparison with faecal culture, milk qPCR and milk ELISA. HYDEqPCR can detect low-level Map shedders that go undetected using these other methods, which will thus underestimate the proportions of Map-shedders in herds. Identification of these shedding animals is extremely important for prevention of the spread of Map infection in an animal population. Due to the relatively high sensitivity and specificity of HYDEqPCR, it can be applied to test for Map at the herd or individual level, regardless of animal age or production stage. HYDEqPCR will allow early detection and control of Map in any population at risk.
背景
约氏乳杆菌病由鸟分枝杆菌副结核亚种(Map)引起,是全球范围内牛群最重要的疾病之一。有几种用于检测 Map 的实验室检测方法,但在亚临床感染人群中使用时,这些方法的灵敏度和特异性有限。为了鉴定亚临床感染牛群中的 Map 排放者,我们使用了一种从粪便中提取 Map 的新型高产 DNA 提取方法,并结合了用于扩增 Map 插入序列 IS900 的定量实时 PCR(qPCR)(HYDEqPCR)。通过将 HYDEqPCR 与粪便培养、牛奶 qPCR 和牛奶酶联免疫吸附测定(ELISA)进行比较,对 141 份粪便和 91 份牛奶样本进行了评估,这些样本来自 141 头亚临床感染的奶牛。
结果
qPCR 被证明具有很高的灵敏度,在 67%的反应中检测到 2 IS900 DNA 拷贝/μl 的检测限。它还显示出 100%的特异性,这是从 50 株 Map 和非 Map 菌株以及 qPCR 扩增子的测序中确定的。HYDEqPCR 的检测限为 90 Map/g Map 接种粪便,相当于 2.4 个菌落形成单位/g Map 接种粪便,估计效率为 85%(±21%)。在现场样本中进行测试时,HYDEqPCR 显示 89%的样本为 Map 阳性,而粪便培养、牛奶 qPCR 和牛奶 ELISA 分别检测到 19%、36%和 1%。Fisher 确切检验仅显示 HYDEqPCR 与粪便培养之间相关性的统计学意义(p ≤0.05)。HYDEqPCR 与牛奶 qPCR 和牛奶 ELISA 的一致性较差、轻微且无统计学意义。
结论
与粪便培养、牛奶 qPCR 和牛奶 ELISA 相比,本研究突出了 HYDEqPCR 用于检测亚临床感染人群中 Map 的优势。HYDEqPCR 可以检测到其他方法无法检测到的低水平 Map 排放者,从而低估了牛群中 Map 排放者的比例。鉴定这些排放动物对于防止 Map 感染在动物种群中的传播至关重要。由于 HYDEqPCR 的灵敏度和特异性相对较高,因此可以应用于牛群或个体水平的 Map 检测,无论动物年龄或生产阶段如何。HYDEqPCR 将允许在任何有风险的人群中早期检测和控制 Map。
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